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THERAPEUTIC COMBINATION OF GALNAC-OLIGONUCLEOTIDE CONJUGATE AND SAPONIN, AND USES THEREOF

20230293562 · 2023-09-21

    Inventors

    Cpc classification

    International classification

    Abstract

    The invention relates to a pharmaceutical combination comprising: a conjugate of an effector molecule and a ligand for ASGPR, wherein the ligand for ASGPR comprises at least one GalNAc moiety; and a saponin of the monodesmosidic or bidesmosidic triterpene glycoside type. The invention also relates to a pharmaceutical composition comprising the conjugate and the saponin. In addition, the invention relates to a pharmaceutical combination or composition of the invention, for use as a medicament, or for use in the treatment or prophylaxis of a disease or health problem in which an expression product is involved of any one or more of genes: apoB, TTR, PCSK9, ALAS 1, ATS, GO, CCS, X gene of HBV, S gene of HBV, AAT and LDH, and/or for use in the treatment or prophylaxis of a cancer, an infectious disease, a viral infection, hypercholesterolemia, primary hyperoxaluria, haemophilia A, haemophilia B, AAT related liver disease, acute hepatic porphyria, TTR-mediated amyloidosis, hereditary TTR amyloidosis (hATTR), complement-mediated disease, hepatitis B infection, or an auto-immune disease. Furthermore, the invention relates to an in vitro or ex vivo method for transferring an effector molecule of the invention from outside a cell to inside said cell, preferably into the cytosol of said cell. The invention also relates to an in vitro or ex vivo method for transferring the conjugate of the invention from outside a cell to inside said cell.

    Claims

    1. Pharmaceutical combination comprising: a conjugate of an effector molecule and a ligand for asialoglycoprotein receptor (ASGPR), wherein the ligand for ASGPR comprises at least one N-acetylgalactosamine (GalNAc) moiety, preferably three or four GalNAc moieties, more preferably the ligand for ASGPR comprises or consists of (GalNAc).sub.3Tris; and a saponin, wherein the saponin is a monodesmosidic triterpene glycoside or a bidesmosidic triterpene glycoside, and optionally comprising a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent.

    2. Pharmaceutical combination of claim 1 in the form of at least two pharmaceutical compositions comprising: a first pharmaceutical composition comprising the conjugate and optionally comprising a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent; and a second pharmaceutical composition comprising the saponin and optionally comprising a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent.

    3. Pharmaceutical combination of claim 1 in the form of a single pharmaceutical composition comprising the conjugate, the saponin and optionally a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent.

    4. Pharmaceutical combination of any one of claims 1-3, wherein the effector molecule comprises or consists of at least one of a small molecule such as a drug molecule, a toxin such as a protein toxin, an oligonucleotide such as a BNA, a xeno nucleic acid or an siRNA, an enzyme, a peptide, a protein, or any combination thereof, preferably, the effector molecule is a toxin, an enzyme or an oligonucleotide.

    5. Pharmaceutical combination of any one of the previous claims, wherein the ligand for ASGPR and the effector molecule, preferably a toxin or an oligonucleotide, are conjugated via a covalent bond, preferably via at least one linker.

    6. Pharmaceutical combination of any one of the previous claims, wherein the effector molecule is an oligonucleotide selected from any one or more of a(n): short interfering RNA (siRNA), short hairpin RNA (shRNA), anti-hairpin-shaped microRNA (miRNA), single-stranded RNA, aptamer RNA, doublestranded RNA (dsRNA), anti-microRNA (anti-miRNA, anti-miR), antisense oligonucleotide (ASO), mRNA, DNA, antisense DNA, locked nucleic acid (LNA), bridged nucleic acid (BNA), 2′-O,4′-aminoethylene bridged nucleic Acid (BNA.sup.NC), BNA-based siRNA, and BNA-based antisense oligonucleotide (BNA-AON).

    7. Pharmaceutical combination of any one of the previous claims, wherein the effector molecule is an oligonucleotide selected from any one of an anti-miRNA, a BNA-AON or an siRNA, such as BNA-based siRNA, preferably selected from chemically modified siRNA, metabolically stable siRNA and chemically modified, metabolically stable siRNA.

    8. Pharmaceutical combination of any one of the previous claims, wherein the effector molecule is an oligonucleotide that is capable of silencing any one of genes: HSP27, apolipoprotein B (apoB), transthyretin (TTR), proprotein convertase subtilisin/kexin type 9 (PCSK9), delta-aminolevulinate synthase 1 (ALAS1), antithrombin 3 (AT3), glycolate oxidase (GO), complement component C5 (CC5), X gene of hepatitis B virus (HBV), S gene of HBV, alpha-1 antitrypsin (AAT) and lactate dehydrogenase (LDH), and/or is capable of targeting an aberrant miRNA.

    9. Pharmaceutical combination of any one of the previous claims, wherein the effector molecule is an oligonucleotide that, for example when present inside a mammalian cell, is capable of targeting an mRNA involved in expression of any one of proteins: HSP27, apoB, TTR, PCSK9, ALAS1, AT3, GO, CC5, expression product of X gene of HBV, expression product of S gene of HBV, AAT and LDH, or is capable of antagonizing or restoring an miRNA function such as inhibiting an oncogenic miRNA (onco-miR) or suppression of expression of an onco-miR, for example when present inside a mammalian cell.

    10. Pharmaceutical combination of any one of the claims 1-5, wherein the effector molecule is a toxin which comprises or consists of at least one proteinaceous molecule, preferably selected from any one or more of a peptide, a protein, an enzyme such as urease and Cre-recombinase, a proteinaceous toxin, a ribosome-inactivating protein, a protein toxin selected from Table A5 and/or a bacterial toxin, a plant toxin, more preferably selected from any one or more of a viral toxin such as apoptin; a bacterial toxin such as Shiga toxin, Shiga-like toxin, Pseudomonas aeruginosa exotoxin (PE) or exotoxin A of PE, full-length or truncated diphtheria toxin (DT), cholera toxin; a fungal toxin such as alpha-sarcin; a plant toxin including ribosome-inactivating proteins and the A chain of type 2 ribosome-inactivating proteins such as dianthin e.g. dianthin-30 or dianthin-32, saporin e.g. saporin-S3 or saporin-S6, bouganin or de-immunized derivative debouganin of bouganin, shiga-like toxin A, pokeweed antiviral protein, ricin, ricin A chain, modeccin, modeccin A chain, abrin, abrin A chain, volkensin, volkensin A chain, viscumin, viscumin A chain; or an animal or human toxin such as frog RNase, or granzyme B or angiogenin from humans, or any fragment or derivative thereof; preferably the protein toxin is dianthin and/or saporin, and/or comprises or consists of at least one of a toxin targeting ribosome, a toxin targeting elongation factor, a toxin targeting tubulin, a toxin targeting DNA and a toxin targeting RNA, more preferably any one or more of emtansine, pasudotox, maytansinoid derivative DM1, maytansinoid derivative DM4, monomethyl auristatin E (MMAE, vedotin), monomethyl auristatin F (MMAF, mafodotin), a Calicheamicin, N-Acetyl-γ-calicheamicin, a pyrrolobenzodiazepine (PBD) dimer, a benzodiazepine, a CC-1065 analogue, a duocarmycin, Doxorubicin, paclitaxel, docetaxel, cisplatin, cyclophosphamide, etoposide, docetaxel, 5-fluorouracyl (5-FU), mitoxantrone, a tubulysin, an indolinobenzodiazepine, AZ13599185, a cryptophycin, rhizoxin, methotrexate, an anthracycline, a camptothecin analogue, SN-38, DX-8951f, exatecan mesylate, truncated form of Pseudomonas aeruginosa exotoxin (PE38), a Duocarmycin derivative, an amanitin, α-amanitin, a spliceostatin, a thailanstatin, ozogamicin, tesirine, Amberstatin269 and soravtansine, or a derivative thereof.

    11. Pharmaceutical combination of any one of the previous claims, wherein the saponin comprises an aglycone core structure selected from the group consisting of: 2alpha-hydroxy oleanolic acid; 16alpha-hydroxy oleanolic acid; hederagenin (23-hydroxy oleanolic acid); 16alpha,23-dihydroxy oleanolic acid; gypsogenin; quillaic acid; protoaescigenin-21 (2-methylbut-2-enoate)-22-acetate; 23-oxo-barringtogenol C-21,22-bis(2-methylbut-2-enoate); 23-oxo-barringtogenol C-21(2-methylbut-2-enoate)-16,22-diacetate; digitogenin; 3,16,28-trihydroxy oleanan-12-en; gypsogenic acid, and derivatives thereof, preferably the saponin comprises an aglycone core structure selected from quillaic acid and gypsogenin or derivatives thereof, more preferably the saponin aglycone core structure is quillaic acid or a derivative thereof.

    12. Pharmaceutical combination of any one of the previous claims, wherein • the saponin comprises a saccharide chain bound to the aglycone core structure, which is selected from group A: GlcA-, Glc-, Gal-, Rha-(1.fwdarw.2)-Ara-, Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA-, Glc-(1.fwdarw.2)-[Glc-(1.fwdarw.4)]-GlcA-, Glc-(1.fwdarw.2)-Ara-(1.fwdarw.3)-[Gal-(1.fwdarw.2)]-GlcA-, Xyl-(1.fwdarw.2)-Ara-(1.fwdarw.3)-[Gal-(1.fwdarw.2)]-GlcA-, Glc-(1 .fwdarw.3)-Gal-(1 .fwdarw.2)-[Xyl-(1 .fwdarw.3)]-Glc-(1 .fwdarw.4)-Gal-, Rha-(1 .fwdarw.2)-Gal-(1 .fwdarw.3)-[Glc-(1 .fwdarw.2)]-GlcA-, Ara-(1 .fwdarw.4)-Rha-(1 .fwdarw.2)-Glc-(1 .fwdarw.2)-Rha-(1 .fwdarw.2)-GlcA-, Ara-(1 .fwdarw.4)-Fuc-(1 .fwdarw.2)-Glc-(1 .fwdarw.2)-Rha-(1 .fwdarw.2)-GlcA-, Ara-(1 .fwdarw.4)-Rha-(1 .fwdarw.2)-Gal-(1 .fwdarw.2)-Rha-(1 .fwdarw.2)-GlcA-, Ara-(1 .fwdarw.4)-Fuc-(1 .fwdarw.2)-Gal-(1 .fwdarw.2)-Rha-(1 .fwdarw.2)-GlcA-, Ara-(1 .fwdarw.4)-Rha-(1 .fwdarw.2)-Glc-(1 .fwdarw.2)-Fuc-(1 .fwdarw.2)-GlcA-, Ara-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, Ara-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, Ara-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, and derivatives thereof, or • the saponin comprises a saccharide chain bound to the aglycone core structure, which is selected from group B: Glc-, Gal-, Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.4)]-Rha-, Rha-(1.fwdarw.2)-[Ara-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha-, Ara-, Xyl-, Xyl-(1 .fwdarw.4)-Rha-(1 .fwdarw.2)-[R1-(.fwdarw.4)]-Fuc- wherein R1 is 4E-Methoxycinnamic acid, Xyl-(1 .fwdarw.4)-Rha-(1 .fwdarw.2)-[R2-(.fwdarw.4)]-Fuc- wherein R2 is 4Z-Methoxycinnamic acid, Xyl-(1.fwdarw.4)-[Gal-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-4-OAc-Fuc-, Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-3,4-di-OAc-Fuc-, Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R3-(.fwdarw.4)]-3-OAc-Fuc- wherein R3 is 4E-Methoxycinnamic acid, Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-4-OAc-Fuc-, Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-4-OAc-Fuc-, (Ara- or Xyl-)(1.fwdarw.3)-(Ara- or Xyl-)(1.fwdarw.4)-(Rha- or Fuc-)(1.fwdarw.2)-[4-OAc-(Rha- or Fuc-)(1.fwdarw.4)]-(Rha- or Fuc-), Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc-, Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc-, Xyl-(1.fwdarw.4)-[Gal-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc-, Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc-, Ara/Xyl-(1.fwdarw.4)-Rha/Fuc-(1.fwdarw.4)-[Glc/Gal-(1.fwdarw.2)]-Fuc-, Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R4-(.fwdarw.4)]-Fuc- wherein R4 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R5-(.fwdarw.4)]-Fuc- wherein R5 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4-OAc-Fuc-, Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4-OAc-Fuc-, 6-OAc-Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3-OAc-Rha-(1.fwdarw.3)]-Fuc-, Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3-OAc--Rha-(1.fwdarw.3)]-Fuc-, Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc-, Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc-, Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc-, Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3,4-di-OAc-Qui-(1.fwdarw.4)]-Fuc-, Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc-, 6-OAc-Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc-, Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc-, Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc-, Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4OAc-Fuc-, Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4OAc-Fuc-, Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R6-(.fwdarw.4)]-Fuc- wherein R6 is 5-O-[5-O-Rha-(1.fwdarw.2)-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R7-(.fwdarw.4)]-Fuc- wherein R7 is 5-O-[5O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R8-(.fwdarw.4)]-Fuc- wherein R8 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R9-(.fwdarw.4)]-Fuc- wherein R9 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R10-(.fwdarw.4)]-Fuc- wherein R10 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R11-(.fwdarw.3)]-Fuc- wherein R11 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R12-(.fwdarw.3)]-Fuc- wherein R12 is 5-O-5O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) Glc-(1.fwdarw.3)-[Glc-(1.fwdarw.6)]-Gal-, and derivatives thereof, or • the saponin is a bidesmosidic triterpene glycoside comprising a first saccharide chain selected from the group A bound to the aglycone core structure and comprising a second saccharide chain selected from the group B bound to the aglycone core structure.

    13. Pharmaceutical combination of any one of the previous claims, wherein the saponin is selected from the group consisting of: Quillaja bark saponin, dipsacoside B, saikosaponin A, saikosaponin D, macranthoidin A, esculentoside A, phytolaccagenin, aescinate, AS6.2, NP-005236, AMA-1, AMR, alpha-Hederin, NP-012672, NP-017777, NP-017778, NP-017774, NP-018110, NP-017772, NP-018109, NP-017888, NP-017889, NP-018108, SA1641, AE X55, NP-017674, NP-017810, AG1, NP-003881, NP-017676, NP-017677, NP-017706, NP-017705, NP-017773, NP-017775, SA1657, AG2, SO1861, GE1741, SO1542, SO1584, SO1658, SO1674, S01832, S01862, SO1904, QS-7, QS1861, QS-7 api, QS1862, QS-17, QS-18, QS-21 A-apio, QS-21 A-xylo, QS-21 B-apio, QS-21 B-xylo, beta-Aescin, Aescin la, Teaseed saponin I, Teaseedsaponin J, Assamsaponin F, Digitonin, Primula acid 1 and AS64R, stereoisomers thereof, derivatives thereof, and combinations thereof, preferably the saponin is selected from the group consisting of QS-21, a QS-21 derivative, SO1861, a SO1861 derivative, SA1641, a SA1641 derivative, GE1741,a GE1741 derivative and combinations thereof, more preferably the saponin is selected from the group consisting of a QS-21 derivative, a SO1861 derivative and combinations thereof, most preferably the saponin is a SO1861 derivative.

    14. Pharmaceutical combination of any one of the previous claims, wherein the saponin is a saponin derivative wherein either: i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised; or ii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A as defined in claim 12, the saccharide chain comprising a carboxyl group which has been derivatised; or iii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group B as defined in claim 12, the saccharide chain comprising an acetoxy (Me(CO)O-) group which has been derivatised; or iv. any combination of derivatisations i., ii. and iii. is present, optionally any combination of two derivatisations of derivatisations i., ii. and iii.

    15. Pharmaceutical combination of any one of the previous claims, wherein the saponin is selected from the group consisting of: SO1861, SA1657, GE1741, SA1641, QS-21, QS-21A, QS-21 A-api, QS-21 A-xyl, QS-21 B, QS-21 B-api, QS-21 B-xyl, QS-7-xyl, QS-7-api, QS-17-api, QS-17-xyl, QS1861, QS1862, Quillajasaponin, Saponinum album, QS-18, Quil-A, Gyp1, gypsoside A, AG1, AG2, SO1542, SO1584, SO1658, SO1674, SO1832, SO1904, stereoisomers thereof, derivatives thereof and combinations thereof, preferably the saponin is selected from the group consisting of QS-21, a QS-21 derivative, SO1861, a SO1861 derivative, SA1641, a SA1641 derivative, GE1741, a GE1741 derivative and combinations thereof, more preferably the saponin is selected from the group consisting of a QS-21 derivative, a SO1861 derivative and combinations thereof, most preferably the saponin is a SO1861 derivative.

    16. Pharmaceutical combination of any one of the previous claims, wherein the saponin is a saponin derivative of the quillaic acid or gypsogenin saponin of claim 11 and represented by Molecule 1: ##STR00023## wherein A.sub.1 represents hydrogen, a monosaccharide or a linear or branched oligosaccharide, preferably A.sub.1 represents a saccharide chain selected from group A as defined in claim 12, more preferably A.sub.1 represents a saccharide chain selected from group A as defined in claim 12 and A.sub.1 comprises or consists of a glucuronic acid moiety; A.sub.2 represents hydrogen, a monosaccharide or a linear or branched oligosaccharide, preferably A.sub.2 represents a saccharide chain selected from group B as defined in claim 12, more preferably A.sub.2 represents a saccharide chain selected from group B as defined in claim 12 and A.sub.2 comprises at least one acetoxy (Me(CO)O-) group, such as one, two, three or four acetoxy groups, wherein at least one of A.sub.1 and A.sub.2 is not hydrogen, preferably both A.sub.1 and A.sub.2 are an oligosaccharide chain; and R is hydrogen in gypsogenin or hydroxyl in quillaic acid; wherein the saponin derivative corresponds to the saponin represented by Molecule 1 wherein at least one of the following derivatisations is present: i. the aldehyde group at position C.sub.23 of the quillaic acid or gypsogenin has been derivatised; ii. the carboxyl group of a glucuronic acid moiety of A.sub.1, when A.sub.1 represents a saccharide chain selected from group A as defined in claim 12 and A.sub.1 comprises or consists of a glucuronic acid moiety, has been derivatised; and iii. one or more, preferably all, of acetoxy group(s) of one saccharide moiety or of two or more saccharide moieties of A.sub.2, when A.sub.2 represents a saccharide chain selected from group B as defined in claim 12 and A.sub.2 comprises at least one acetoxy group, has/have been derivatised.

    17. Pharmaceutical combination of claim 16, wherein A.sub.1 represents a saccharide chain selected from group A as defined in claim 12 and comprises or consists of a glucuronic acid moiety and wherein the carboxyl group of a glucuronic acid moiety of A.sub.1 has been derivatised and/or wherein A.sub.2 represents a saccharide chain selected from group B as defined in claim 12 and A.sub.2 comprises at least one acetoxy group and wherein at least one acetoxy group of A.sub.2 has been derivatised.

    18. Pharmaceutical combination of claim 16 or 17, wherein the saponin represented by Molecule 1 is a bidesmosidic triterpene saponin.

    19. Pharmaceutical combination of any one of the claims 16-18, wherein the saponin derivative corresponds to the saponin represented by Molecule 1 wherein at least one of the following derivatisations is present: i. the aldehyde group at position C.sub.23 of the quillaic acid or gypsogenin has been derivatised by; reduction to an alcohol; or transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or transformation into a hydrazone bond through reaction with N-[ß-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or transformation into a hydrazone bond through reaction with N-[k-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; ii. the carboxyl group of a glucuronic acid moiety of A.sub.1, when A.sub.1 represents a saccharide chain selected from group A as defined in claim 12 and A.sub.1 comprises or consists of a glucuronic acid moiety, has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu-AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; and iii. one or more, preferably all, of acetoxy group(s) of one saccharide moiety or of two or more saccharide moieties of A.sub.2, when A.sub.2 represents a saccharide chain selected from group B as defined in claim 12 and A.sub.2 comprises at least one acetoxy group, has/have been derivatised by transformation into a hydroxyl group (HO-) by deacetylation.

    20. Pharmaceutical combination of any one of the claims 16-19, wherein A.sub.1 is Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA and/or A.sub.2 is Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc, preferably the saponin represented by Molecule 1 is 3-O-beta-D-galactopyranosyl-(1.fwdarw.2)-[beta-D-xylopyranosyl-(1.fwdarw.3)]-beta-D-glucuronopyranosyl quillaic acid 28-O-beta-D-glucopyranosyl-(1.fwdarw.3)-beta-D-xylopyranosyl-(1.fwdarw.4)- alpha-L-rhamnopyranosyl-(1.fwdarw.2)-[beta-D-xylopyranosyl-(1.fwdarw.3)-4OAc-beta-D-quinovopyranosyl-(1.fwdarw.4)]-beta-D-fucopyranoside, more preferably SO1861, GE1741, SA1641 and/or QS-21, or a derivative thereof, most preferably SO1861 or a derivative thereof.

    21. Pharmaceutical combination of any one of the claims 14-20, wherein the saponin is a saponin derivative wherein either: i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised by: reduction to an alcohol; or transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or transformation into a hydrazon bond through reaction with N-[ß-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or transformation into a hydrazon bond through reaction with N-[κ-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or ii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A as defined in claim 12, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety which has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu- AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; or iii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group B as defined in claim 12, the saccharide chain comprising an acetoxy (Me(CO)O-) group which has been derivatised by transformation into a hydroxyl group (HO-) by deacetylation; or iv. the saponin derivative comprises any combination of derivatisations i., ii. and iii., optionally any combination of two derivatisations i., ii. and iii.; preferably, the saponin derivative comprises an aglycone core structure wherein the aglycone core structure comprises an aldehyde group which has been derivatised by transformation into a hydrazone bond through reaction with EMCH wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol.

    22. Pharmaceutical combination of claim 21 wherein the saponin is a saponin derivative wherein either: i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised by transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH; or ii. the saponin comprises a saccharide chain, preferably a saccharide chain selected from group A as defined in claim 12, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety which has been derivatised by transformation into an amide bond through reaction with N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; or iii. the saponin derivative comprises a combination of derivatisations i. and ii.

    23. Pharmaceutical combination of claim 21, wherein the saponin derivative comprises an aglycone core structure wherein the aglycone core structure comprises an aldehyde group and wherein the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A as defined in claim 12, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety, which glucuronic acid moiety has been derivatised by transformation into an amide bond through reaction with N-(2-aminoethyl)maleimide (AEM).

    24. Pharmaceutical combination of any one of claims 1-21, wherein the saponin is a saponin derivative represented by Molecule 2: ##STR00024## or wherein the saponin derivative is the saponin derivative represented by Molecule 3 ##STR00025## .

    25. Pharmaceutical combination of any one of the previous claims for use as a medicament.

    26. Pharmaceutical combination of any one of the claims 1-9 or 11-24 in so far dependent on any one of the claims 1-9, for use in the treatment or prophylaxis of a disease or health problem in which an expression product is involved of any one or more of genes: apoB, HSP27, TTR, PCSK9, ALAS1, AT3, GO, CC5, X gene of HBV, S gene of HBV, AAT and LDH.

    27. Pharmaceutical combination of any one of the claims 1-9 or 11-24 in so far dependent on any one of the claims 1-9, or pharmaceutical combination for use of claim 25, for use in the treatment or prophylaxis of a cancer, an infectious disease, a viral infection, hypercholesterolemia, primary hyperoxaluria, haemophilia A, haemophilia B, AAT related liver disease, acute hepatic porphyria, TTR-mediated amyloidosis, hereditary TTR amyloidosis (hATTR), complement-mediated disease, hepatitis B infection, a disease or disorder relating to HSP27 expression, or an auto-immune disease.

    28. Pharmaceutical combination for use according to any one of the claims 25-27, wherein the pharmaceutical combination is as described in any one of the claims 19-24.

    29. In vitro or ex vivo method for transferring the effector molecule of any one of the claims 1 and 5-10 from outside a cell to inside said cell, preferably into the cytosol of said cell, comprising the steps of: a) providing a cell which expresses ASGPR, preferably ASGPR1, on its surface, preferably selected from a liver cell, a virally infected cell and a cancer cell; b) providing the conjugate of any one of claims 1-24, the conjugate comprising the effector molecule to be transferred; c) providing the saponin of any one of claims 1-24; d) contacting the cell of step a) in vitro or ex vivo with the conjugate of step b) and the saponin of step c), therewith effecting the transfer of said conjugate comprising the effector molecule from outside the cell to inside said cell, and by effecting the transfer of said conjugate effecting the transfer of the effector molecule from outside the cell to inside said cell, preferably into the cytosol of said cell.

    30. In vitro or ex vivo method for transferring the conjugate of any one of the claims 1-24 from outside a cell to inside said cell, preferably into the cytosol of said cell, comprising the steps of: a) providing a cell which expresses ASGPR, preferably ASGPR1, on its surface, preferably selected from a liver cell, a virally infected cell and a cancer cell; b) providing the conjugate of any one of claims 1-24; c) providing the saponin of any one of claims 1-24; d) contacting the cell of step a) in vitro or ex vivo with the conjugate of step b) and the saponin of step c), therewith effecting the transfer of the conjugate from outside the cell inside said cell.

    31. The method of claim 29 or 30, wherein the ligand for ASGPR comprises at least one N-acetylgalactosamine (GalNAc) moiety, preferably three or four GalNAc moieties, more preferably the ligand for ASGPR comprises or consists of (GalNAc).sub.3Tris and/or wherein the effector molecule is an oligonucleotide selected from any one of an anti-miRNA, a BNA-AON or an siRNA, such as BNA-based siRNA, preferably selected from chemically modified siRNA, metabolically stable siRNA and chemically modified, metabolically stable siRNA.

    32. The method of claim 29 or 30, wherein the effector molecule comprises or consists of at least one of a small molecule such as a drug molecule, a toxin such as a protein toxin, an oligonucleotide such as a BNA, a xeno nucleic acid or an siRNA, an enzyme, a peptide, a protein, or any combination thereof, preferably, the effector molecule is a toxin, an enzyme or an oligonucleotide, preferably the toxin is saporin or dianthin.

    33. The method of any one of the claims 29-32, wherein the saponin is derivatised SO1861 and/or derivatised QS-21, preferably SO1861-Glu-AEM or SO1861-Ald-EMCH or QS-21-Glu-AEM or QS-21-Ald-EMCH according to claim 19.

    34. The method of any one of the claims 29-33, wherein the effector molecule is an oligonucleotide which, for example when present inside a mammalian cell, is capable of silencing any one of genes: apolipoprotein B (apoB), HSP27, transthyretin (TTR), proprotein convertase subtilisin/kexin type 9 (PCSK9), delta-aminolevulinate synthase 1 (ALAS1), antithrombin 3 (AT3), glycolate oxidase (GO), complement component C5 (CC5), X gene of hepatitis B virus (HBV), S gene of HBV, alpha-1 antitrypsin (AAT) and lactate dehydrogenase (LDH), and/or, for example when present inside a mammalian cell, is capable of targeting an aberrant miRNA and/or, for example when present inside a mammalian cell, wherein the oligonucleotide is capable of targeting an mRNA involved in expression of any one of proteins: HSP27, apoB, TTR, PCSK9, ALAS1, AT3, GO, CC5, expression product of X gene of HBV, expression product of S gene of HBV, AAT and LDH, or, for example when present inside a mammalian cell, is capable of antagonizing or restoring an miRNA function such as inhibiting an oncogenic miRNA (onco-miR) or suppression of expression of an onco-miR.

    35. Kit of parts, comprising the pharmaceutical combination of any one of the claims 1-24 or the second pharmaceutical composition of any one of the claims 2, 4-24, and instructions for use of said pharmaceutical combination or second pharmaceutical composition according to any one of claims 25-28 or for use in a method according to any one of claims 29-34.

    Description

    BRIEF DESCRIPTION OF THE DRAWINGS

    [0066] FIG. 1: synthesis of trivalent-GalNAc.

    [0067] FIG. 2: synthesis of SO1861-DBCO.

    [0068] FIG. 3: synthesis of monovalent-GalNAc-SO1861.

    [0069] FIG. 4: synthesis of trivalent-GalNAc-SO1861.

    [0070] FIG. 5: synthesis of monovalent-GalNAc-BNA.

    [0071] FIG. 6: synthesis of trivalent-GalNAc-BNA.

    [0072] FIG. 7: synthesis of trivalent-GalNAc-BNA.

    [0073] FIGS. 8A and 8B: synthesis of trivalent GalNAc.

    [0074] FIGS. 9A and 9B: Cell viability (MTS) of GalNAc-SO1861 and trivalent-GalNAc-SO1861 on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 9B also applies for FIG. 9A.

    [0075] FIGS. 10A and 10B: Cell viability assay (MTS) HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 10B also applies for FIG. 10A.

    [0076] FIGS. 11A and 11B: Gene expression analysis on HepG2 (A) and Huh7 (B) cell lines.

    [0077] FIGS. 12A and 12B: Gene expression analysis on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 12B also applies for FIG. 12A.

    [0078] FIGS. 13A and 13B: Cell viability assay on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 13B also applies for FIG. 13A.

    [0079] FIGS. 14A and B: Gene expression analysis on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 14B also applies for FIG. 14A.

    [0080] FIGS. 15A and B: Cell viability assay on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 15B also applies for FIG. 15A.

    [0081] FIGS. 16A and B: Gene expression analysis on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 16B also applies for FIG. 16A.

    [0082] FIGS. 17A and B: Gene expression analysis on HepG2 (A) and Huh7 (B) cell lines. The legend displayed next to FIG. 17B also applies for FIG. 17A.

    [0083] FIGS. 18A and B: ApoB RNA expression analysis and cell viability assay on human primary hepatocytes.

    [0084] FIGS. 19A and B: ApoB RNA expression analysis and cell viability assay on human primary hepatocytes.

    [0085] FIGS. 20A and B: ApoB RNA expression analysis assay on mouse primary hepatocytes.

    [0086] FIG. 21: (GaINAc)3-Ls-SO1 861 synthesis, intermediate 22, 23.

    [0087] FIG. 22: (GalNAc)3-Ls-BNA synthesis, intermediate 25, 26.

    [0088] FIG. 23: (GalNAc)3-Ls-BNA synthesis.

    DETAILED DESCRIPTION

    [0089] It is a first goal of the present invention to provide an improved therapeutic combination or an improved pharmaceutical composition for delivery of an effector molecule coupled to a ligand for ASGPR, in particular ASGPR1, such as a GalNAc comprising ligand, when for example the delivery from outside a target cell into said cell is considered, or more in particular when the delivery of the effector molecule in the cytosol of said target cell is considered. It is a second goal of the present invention to provide an improved method of treatment of a (human) patient suffering from a disease to be treated with a conjugate comprising an effector molecule and a ligand for ASGPR.

    [0090] It is an objective of the current invention to provide a therapeutic composition or a therapeutic combination of e.g. two therapeutic compositions, comprising a conjugate of a ligand for ASGPR covalently linked to an effector molecule that is capable of exerting a biological effect once delivered inside a target cell which comprises the molecular target for the effector molecule, which conjugate, when administered to a (human) patient in need thereof, bearing the target cell, has an improved therapeutic effect or a sufficient effect at a lower dose than the currently required dose for the conjugate. This way, the therapeutic window of the conjugate is widened effectively.

    [0091] At least one of the above objectives is achieved by providing the therapeutic combination of at least two pharmaceutical compositions or the pharmaceutical composition of the invention.

    [0092] The present invention will be described with respect to particular embodiments but the invention is not limited thereto but only by the claims.

    [0093] A first aspect of the invention relates to a pharmaceutical combination comprising: [0094] a conjugate of an effector molecule and a ligand for asialoglycoprotein receptor (ASGPR), wherein the ligand for ASGPR comprises at least one N-acetylgalactosamine (GalNAc) moiety, preferably three or four GalNAc moieties, more preferably the ligand for ASGPR comprises or consists of (GaINAc).sub.3 Tris; and [0095] a saponin, wherein the saponin is a monodesmosidic triterpene glycoside or a bidesmosidic triterpene glycoside,and optionally comprising a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent.

    [0096] An embodiment is the pharmaceutical combination of the invention in the form of at least two pharmaceutical compositions comprising: [0097] a first pharmaceutical composition comprising the conjugate and optionally comprising a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent; and [0098] a second pharmaceutical composition comprising the saponin and optionally comprising a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent.

    [0099] An embodiment is the pharmaceutical combination of the invention in the form of a single pharmaceutical composition comprising the conjugate, the saponin and optionally a pharmaceutically acceptable excipient and/or pharmaceutically acceptable diluent.

    [0100] The inventors surprisingly found that cells which express ASGPR, in particular ASGPR1 at their surface, exhibit improved uptake of a conjugate comprising a ligand for ASGPR and an effector molecule, when said cells are contacted with both the conjugate and a saponin of the triterpene glycoside type, typically a bidesmosidic terpenoid type of saponin. For example, GalNAc based ligands for ASGPR1, such as a (GaINAc).sub.3Tris conjugate, covalently conjugated with an oligonucleotide, such as a gene silencing BNA, for example for silencing HSP27 exhibit such improved uptake in the presence of a saponin. Herewith, the inventors now provide a solution for the long-felt need for improving the efficacy of delivery of e.g. oligonucleotides from outside a target cell to be treated with such an oligonucleotide, to inside said cell, in particular for improving the intracellularly delivery into the cytosol of a target cell that expresses ASGPR1 on its surface, of an oligonucleotide such as a BNA and/or an siRNA. The applied saponins according to the invention are known for their ability to enhance the endosomal escape of e.g. protein toxins once a target cell is contacted with such a saponin and the toxin, wherein the toxin is for example part of an antibody-drug conjugate (ADC). The inventors now also established that certain derivatives of such saponins maintain their capability of enhancing the escape of effector molecules from endosomes and lysosomes into the cytosol, when the saponins and the effector molecule co-localize inside the cell, i.e. in the endosome. Surprisingly, such saponin derivatives are capable of enhancing the delivery of the effector molecule comprised by the conjugate into a target cell bearing the ASGPR1, while the cytotoxicity and the haemolytic activity of such saponin derivates are lower than observed for the (naturally occurring) non-modified saponin. Such saponin derivatives are described in more detail herein.

    Conjugate - Introduction

    [0101] The pharmaceutical combination and certain pharmaceutical compositions of the present invention comprise a conjugate of an effector molecule and a ligand for asialoglycoprotein receptor (ASGPR) such as ASGPR1, and preferably ASGPR1. When the effector molecule is bound to the remainder of the conjugate it is referred to herein as an “effector moiety”. The ASGPR ligand comprises at least one N-acetylgalactosamine (GalNAc) moiety. In accordance with embodiments of the present invention each GalNAc moiety is bound to the remainder of the ASGPR ligand or - in case an ASGPR ligand consists of a single GaINAc moiety - to the effector moiety, via a covalent bond to the oxygen on position “1” as indicated in formula (I):

    ##STR00001##

    [0102] As shown in formula (II), the ASGPR ligand consists of a single GaINAc moiety bound to the effector moiety E, preferably via an effector moiety linker L.sub.E.

    ##STR00002##

    [0103] The ASGPR ligand may comprise more than one GalNAc moiety, such as 2, 3, 4, 5 or 6 GaINAc moieties, preferably 3 or 4 GaINAc moieties, more preferably 3 GalNAc moieties. In such case, it is preferred that the GalNAc moieties are each separately covalently bound via the oxygen on position “1” to a central bridging moiety B, which effectively forms a bridge between the GalNAc moieties and the effector moiety, preferably via an effector moiety linker L.sub.E.The GalNAc moieties may be directly bound to the bridging moiety B as shown in formula (III):

    ##STR00003##

    [0104] wherein n is an integer larger than or equal to 3 or 4, preferably n is 3, L.sub.E is an effector moiety linker and E is the effector moiety. More preferably, the GalNAc moieties are bound to the bridging moiety B via GalNAc linkers L.sub.GAL as shown in formula (IV): [0105] wherein n is an integer larger than or equal to 3 or 4, preferably n is 3, L.sub.E is an effector moiety linker and E is the effector moiety. While each occurrence of L.sub.GAL may be independently chosen, the skilled person will appreciate that the synthesis of the conjugate is simplified in case each occurrence of L.sub.GAL represents the same moiety.

    Conjugate - Linker L.SUB.E

    [0106] The effector moiety linker L.sub.E represents any chemical moiety suitable for covalently binding an effector moiety to GalNAc as in formula (II) or to the bridging moiety B as in formula (III) and (IV). The identity and size of the linker is not particularly limited and covalently binding an effector molecule to GalNAc as in formula (II) or to the bridging moiety B as in formula (III) and (IV) may be effected by means of a ‘regular’ chemical functional group (e.g. an ether bond) as well as through “click-chemistry” type linkers which typically have a long chain length, resulting in a linker E.sub.L comprising e.g. more than 10 or more than 20 carbon atoms. Suitable effector moiety linkers L.sub.E and associated coupling reactions are described in the handbook Hermanson, Greg T. Bioconjugate techniques. Academic press, 2013.

    [0107] As will be understood by the skilled person, the effector moiety linker L.sub.E will typically be the result of a coupling reaction (e.g. “click-chemistry” type) between at least a first precursor L.sub.E1 covalently bound to GalNAc or the bridging moiety B and a second precursor L.sub.E2 covalently bound to the effector moiety. This principle is illustrated in the following reaction scheme for the compound of formula (II):

    ##STR00005##

    wherein L.sub.E is an effector moiety linker, L.sub.E1 is a precursor of the effector moiety linker L.sub.E which is covalently bound to GalNAc and L.sub.E2 is a precursor of the effector moiety linker L.sub.E which is covalently bound to the effector moiety and E is the effector moiety.

    [0108] The corresponding reaction scheme for the compound of formula (III) is as follows:

    ##STR00006##

    wherein L.sub.E is an effector moiety linker, L.sub.E1 is a precursor of the effector moiety linker L.sub.E which is covalently bound to GalNAc and L.sub.E2 is a precursor of the effector moiety linker L.sub.E which is covalently bound to the effector moiety, n is an integer larger than or equal to 3 or 4, preferably n is 3, B is a bridging moiety and E is the effector moiety.

    [0109] The corresponding reaction scheme for the compound of formula (IV) is as follows:

    ##STR00007##

    wherein L.sub.E is an effector moiety linker, L.sub.E1 is a precursor of the effector moiety linker L.sub.E which is covalently bound to GalNAc and L.sub.E2 is a precursor of the effector moiety linker L.sub.E which is covalently bound to the effector moiety, n is an integer larger than or equal to 3 or 4, preferably n is 3, E is the effector moiety, and L.sub.GAL is a GalNAc linker and B is a bridging moiety.

    [0110] The effector moiety linker L.sub.E can be the result of a coupling reaction between at least a first precursor L.sub.E1 covalently bound to GalNAc or the bridging moiety and a second precursor L.sub.E2 covalently bound to the effector moiety, wherein the coupling reaction is for example an azide-alkyne cycloaddition, a thiol maleimide coupling, a staudinger reaction, a nucleophilic ring-opening of strained heterocyclic electrophiles (such as aziridines, epoxides, cyclic sulfates, aziridinium ions, episulfonium ions), a carbonyl reaction of the non-aldol type (such as urea, thiourea, hydrazon, oxime ether, amide or aromatic heterocycle formation) or an addition to a carbon-carbon double bond (such as epoxidation, aziridination, dihydroxylation, sulfentyl halide addition, nitrosyl halide addition or micheal addition), preferably wherein the coupling reaction is an azide-alkyne cycloaddition, a thiol maleimide coupling, a staudinger reaction, a nucleophilic ring-opening of strained heterocyclic electrophiles, more preferably wherein the coupling reaction is an azide-alkyne cycloaddition or a thiol maleimide coupling.

    [0111] In accordance with some embodiments of the invention, the effector moiety linker L.sub.E comprises a succinimide thioether moiety. Such a succinimide thioether is e.g. the result of a thiol maleimide coupling between an N-substituted maleimide and a thiol or sulfhydryl containing compound. This thiol maleimide coupling is a commonly known ‘click′-chemistry tool in the field of bioconjugation and is for example described in Hermanson, Greg T. Bioconjugate techniques. Academic press, 2013 page 289. Consequently, it is preferred that the effector moiety linker L.sub.E is the result of a coupling reaction between a first precursor L.sub.E1 covalently bound to GalNAc or the bridging moiety, the first precursor L.sub.E1 comprising an N-substituted maleimide; and a second precursor L.sub.E2 covalently bound to the effector moiety, the second precursor L.sub.E2 comprising a thiol or a precursor thereof. A suitable thiol precursor is a disulfide, which may be cleaved (e.g. in-situ) via reduction to the corresponding thiol.

    [0112] A preferred structure for the precursor L.sub.E1 present in the compounds of formula (V), (VII) or (VIII) is the following terminal N-substituted maleimide:

    ##STR00008##

    wherein X represents any linker suitable for covalently bonding the terminal N-substituted maleimide to GalNAc or the bridging moiety B. As will be understood by the skilled person, X may be the result of a coupling reaction between a first moiety covalently bound to GalNAc or the bridging moiety and a second moiety covalently bound to the maleimide. X can comprise a hydrazone and/or a 1, 2, 3-triazole. Whenever reference is made to a 1, 2, 3-triazole in the context of the linkers of the present application, this preferably means a 1H-1, 2, 3-triazole.

    [0113] Embodiments of the structure for the precursor L.sub.E1 present in the compounds of formula (V), (VII) or (VIII) are the following terminal N-substituted maleimides:

    ##STR00009##

    [0114] wherein a and b each independently represent an integer larger than or equal to 0, preferably a and b each independently represent an integer selected from 0, 1, 2, and 3, more preferably a and b represent 2, and wherein L.sub.E1a represents a hydrazone and/or a 1, 2, 3-triazole, preferably a 1, 2, 3-triazole and wherein L.sub.E1b represents a hydrazone and/or a 1, 2, 3-triazole, preferably a hydrazone; [0115] wherein b and c each independently represent an integer larger than or equal to 0, preferably b represents an integer selected from 0, 1, 2, and 3 and c represents an integer in the range of 5-15, more preferably b represents 2, and c represents 9, wherein L.sub.E1a represents a hydrazone and/or a 1, 2, 3-triazole, preferably a 1, 2, 3-triazole and wherein L.sub.E1b represents a hydrazone and/or a 1, 2, 3-triazole, preferably a hydrazone; and [0116] wherein c represents an integer larger than or equal to 0, preferably c represents an integer in the range of 5-15, more preferably c represents 9, wherein L.sub.E1c represents a hydrazone and/or a 1, 2, 3-triazole, preferably a 1, 2, 3-triazole.

    [0117] L.sub.E1a, L.sub.E1b and L.sub.E1c each preferably comprise less than 20 carbon atoms, more preferably L.sub.E1a, L.sub.E1b and L.sub.E1c each independently represent a moiety according to formula (XIII), (XIV) or (XV), preferably L.sub.E1a is the 1,2,3-triazole of formula (XIII), L.sub.E1b is the hydrazone of formula (XIV) and L.sub.E1c is the 1,2,3-triazole of formula (XV) :

    ##STR00012##

    ##STR00013##

    ##STR00014##

    [0118] Hence, in some embodiments the conjugate is a compound of formula (II), (III) or (IV) as described herein, wherein the effector moiety linker L.sub.E is the result of a coupling reaction between a compound of formula (V), (VII) or (VIII) with a compound of formula (VI), wherein the first precursor L.sub.E1 is a terminal N-substituted maleimide of formula (X), (XI) or (XII), wherein L.sub.E1a is for example the 1,2,3-triazole of formula (XIII), L.sub.E1b is for example the hydrazone of formula (XIV) and L.sub.E1c is for example the 1,2,3-triazole of formula (XV).

    Conjugate - Bridging Moiety B

    [0119] The bridging moiety B present in compounds of formula (III) or (IV) represents any moiety suitable for covalently binding 2 or more GalNAc moieties, preferably 3 GalNac moieties, and the effector moiety linker L.sub.E.

    [0120] According to preferred embodiments, the bridging moiety B is a compound of formula (XV):

    ##STR00015##

    wherein the oxygen atoms of the compound of formula (XV) are bound to GalNAc (corresponding to compounds of formula (III)) or to the GalNAc linkers L.sub.GAL (corresponding to compounds of formula (IV)), and the nitrogen atom of the compound of formula (XV) is bound to the effector moiety linker L.sub.E.

    [0121] The skilled person will understand that these compounds of formula (III) or (IV) wherein the bridging moiety B is a compound of formula (XV) correspond to conjugates wherein the ASGPR ligand consists of (GaINAc).sub.3Tris.

    Conjugate - Linker L.SUB.GAL

    [0122] The GalNAc linkers L.sub.GAL represent any chemical moiety suitable for covalently binding GalNAc to the bridging moiety as in formula (IV). The identity and size of the linker is not particularly limited.

    [0123] According to embodiments, the GalNAc linkers L.sub.GAL each comprise 2-25 carbon atoms, preferably 7-15 carbon atoms, more preferably 11 carbon atoms. Preferably the GalNAc linkers L.sub.GAL comprise at least one, preferably two amide moieties. A particularly preferred GalNAc linker L.sub.GAL is a compound according to formula (XVI):

    ##STR00016##

    Conjugate - Effector Moiety

    [0124] An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule comprises or consists of at least one of a small molecule such as a drug molecule, a toxin such as a protein toxin, an oligonucleotide such as a BNA, a xeno nucleic acid or an siRNA, an enzyme, a peptide, a protein, or any combination thereof, preferably, the effector molecule is a toxin, an enzyme or an oligonucleotide. According to the invention, the effector molecule is a molecule capable of exerting a biological effect inside a cell that expresses the ASGPR on its surface and that comprises the binding partner for the effector molecule inside the cell, e.g. in the cytosol of said cell, such that the effector molecule can exert its intracellular biological effect once delivered inside the cell and preferably inside the cytosol, i.e. at the location inside the cell where the target for the effector molecule resides.

    [0125] An embodiment is the pharmaceutical combination of the invention, wherein the ligand for ASGPR, in particular a ligand for ASGPR1, and the effector molecule, preferably a toxin or an oligonucleotide, are conjugated via a covalent bond, preferably via at least one linker. Such linkers suitable for coupling of the ligand for ASGPR, such as (GaINAc).sub.3Tris, to an effector molecule, such as a BNA or an siRNA or a protein toxin, etc., are detailed here above.

    [0126] An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule is an oligonucleotide selected from any one or more of a(n): short interfering RNA (siRNA), short hairpin RNA (shRNA), anti-hairpin-shaped microRNA (miRNA), single-stranded RNA, aptamer RNA, double-stranded RNA (dsRNA), anti-microRNA (anti-miRNA, anti-miR), antisense oligonucleotide (ASO), mRNA, DNA, antisense DNA, locked nucleic acid (LNA), bridged nucleic acid (BNA), 2′-O,4′-aminoethylene bridged nucleic Acid (BNA.sup.NC), BNA-based siRNA, and BNA-based antisense oligonucleotide (BNA-AON). As said, any effector molecule for which the target binding partner is present inside a cell that expresses the receptor for the ligand comprised by the conjugate of the invention, i.e. ASGPR, is suitably selected for incorporation in the conjugate of the invention. Thus, for example an ASO, an siRNA or a BNA capable for targeting a gene, mRNA, etc., present in the cell which exposes ASGPR at its surface, are suitable candidates for incorporation in the conjugate of the invention.

    [0127] An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule is an oligonucleotide selected from any one of: an anti-miRNA, a BNA-AON or an siRNA, such as BNA-based siRNA, preferably selected from chemically modified siRNA, metabolically stable siRNA and chemically modified, metabolically stable siRNA. Such chemically modified and/or metabolically stable siRNA moieties are known in the art, and are suitable for coupling to a ligand for ASGPR.

    [0128] An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule is an oligonucleotide that is capable of silencing any one of genes: HSP27, apolipoprotein B (apoB), transthyretin (TTR), proprotein convertase subtilisin/kexin type 9 (PCSK9), delta-aminolevulinate synthase 1 (ALAS1), antithrombin 3 (AT3), glycolate oxidase (GO), complement component C5 (CC5), X gene of hepatitis B virus (HBV), S gene of HBV, alpha-1 antitrypsin (AAT) and lactate dehydrogenase (LDH), and/or is capable of targeting an aberrant miRNA. An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule, when present inside a cell, is an oligonucleotide that is capable of silencing any one of genes: apolipoprotein B (apoB), transthyretin (TTR), proprotein convertase subtilisin/kexin type 9 (PCSK9), delta-aminolevulinate synthase 1 (ALAS1), antithrombin 3 (AT3), glycolate oxidase (GO), complement component C5 (CC5), X gene of hepatitis B virus (HBV), S gene of HBV, alpha-1 antitrypsin (AAT) and lactate dehydrogenase (LDH), and/or wherein the effector molecule, when present inside a cell, is capable of targeting an aberrant miRNA. According to the invention, any gene or mRNA present in a cell that expresses ASGPR at its cell surface can effectively be targeted by an effector molecule comprised by the conjugate of the invention, wherein the effector molecule is e.g. a BNA, an siRNA, an ASO, etc., when for example co-administered together with a saponin according to the invention, to a subject in need of modification of e.g. a gene, (level of) mRNA expression, silencing of a gene, etc. Under influence of the saponin, the therapeutic window of the conjugate comprising the effector molecule and the ligand for ASGPR is widened, resulting in a stronger biological effect of the effector molecule inside the target cell, and/or resulting in a biological effect of the effector molecule at a lower effective dose than what would be achieved when the target cells are exposed to the conjugate in the absence of the saponin or the saponin derivative. According to the invention, contacting the target cell which expresses ASGPR with a conjugate comprising a ligand for ASGPR and an effector molecule together with a saponin or a saponin derivative, can result in overcoming a threshold with regard to intracellular activity of the effector molecule. A dose of the conjugate that for example would be required for reaching a sufficiently high amount of effector molecule in the cytosol of a target cell in the absence of saponin, could be too high for safe administration to a patient in need of such treatment with the effector molecule. In the presence of the saponin, the effector molecule already can exert its biological effect in the cytosol of a target cell expressing the ASGPR at lower dose, which lower dose would not exert any effect inside the cell when target cells are exposed to such lower dose in the absence of saponin. For example, BNA for silencing HSP27 in (liver) cells did not silence HSP27 inside ASGPR bearing cells when a conjugate of GalNAc ligand for ASGPR and the BNA was contacted with ASGPR bearing cells, whereas when the same cells were contacted with the same or lower dose of the conjugate in the presence of saponin or saponin derivative such as a saponin with linker EMCH conjugated to the aldehyde group in the aglycone of the saponin, HSP27 was effectively silenced in the target cell (as shown in the appended example 2 and FIG. 11). Thus, the inventors now provide molecules, pharmaceutical combinations, pharmaceutical compositions and a method for treating a (human) subject with such molecules, combinations and compositions, such that effector molecules can be administered to a patient in need thereof at lower dose, or such that effector molecules with an improved therapeutic window can be administered, resulting in an improved therapeutic effect once the effector molecule reaches its intracellular target in a target cell for the conjugates according to the invention.

    [0129] An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule is an oligonucleotide that, for example when present inside a mammalian cell, is capable of targeting an mRNA involved in expression of any one of proteins: HSP27, apoB, TTR, PCSK9, ALAS1, AT3, GO, CC5, expression product of X gene of HBV, expression product of S gene of HBV, AAT and LDH, or is capable of antagonizing or restoring an miRNA function such as inhibiting an oncogenic miRNA (onco-miR) or suppression of expression of an onco-miR, for example when present inside a mammalian cell. Such proteins are typically involved in diseases for which e.g. silencing of the gene involved in expression of such a protein would result in relief from disease or disease symptoms to the benefit of the patient treated with the combination of the saponin and the conjugate comprising the ligand for ASGPR and the effector molecule capable of targeting mRNA involved in expression of any one of these proteins. Thus, it is part of the invention that the combinations and compositions of the invention, comprising saponin, are suitable for including in RNAi based treatment regimens. RNAi enables target gene silencing by cleaving mRNA or repressing mRNA translation. The saponin aids in potentiating the gene silencing effector molecule by improving the cytosolic delivery of the effector molecule, when a target cell selected for RNAi therapy and expressing the ASGPR is contacted with both the saponin and the conjugate as described herein.

    [0130] An embodiment is the pharmaceutical combination of the invention, wherein the effector molecule is a toxin which comprises or consists of at least one proteinaceous molecule, preferably selected from any one or more of a peptide, a protein, an enzyme such as urease and Cre-recombinase, a proteinaceous toxin, a ribosome-inactivating protein, a protein toxin selected from Table A5 and/or a bacterial toxin, a plant toxin, more preferably selected from any one or more of a viral toxin such as apoptin; a bacterial toxin such as Shiga toxin, Shiga-like toxin, Pseudomonas aeruginosa exotoxin (PE) or exotoxin A of PE, full-length or truncated diphtheria toxin (DT), cholera toxin; a fungal toxin such as alpha-sarcin; a plant toxin including ribosome-inactivating proteins and the A chain of type 2 ribosome-inactivating proteins such as dianthin e.g. dianthin-30 or dianthin-32, saporin e.g. saporin-S3 or saporin-S6, bouganin or de-immunized derivative debouganin of bouganin, shiga-like toxin A, pokeweed antiviral protein, ricin, ricin A chain, modeccin, modeccin A chain, abrin, abrin A chain, volkensin, volkensin A chain, viscumin, viscumin A chain; or an animal or human toxin such as frog RNase, or granzyme B or angiogenin from humans, or any fragment or derivative thereof; preferably the protein toxin is dianthin and/or saporin, and/or comprises or consists of at least one of a toxin targeting ribosome, a toxin targeting elongation factor, a toxin targeting tubulin, a toxin targeting DNA and a toxin targeting RNA, more preferably any one or more of emtansine, pasudotox, maytansinoid derivative DM1, maytansinoid derivative DM4, monomethyl auristatin E (MMAE, vedotin), monomethyl auristatin F (MMAF, mafodotin), a Calicheamicin, N-Acetyl-.sub.Y-calicheamicin, a pyrrolobenzodiazepine (PBD) dimer, a benzodiazepine, a CC-1065 analogue, a duocarmycin, Doxorubicin, paclitaxel, docetaxel, cisplatin, cyclophosphamide, etoposide, docetaxel, 5-fluorouracyl (5-FU), mitoxantrone, a tubulysin, an indolinobenzodiazepine, AZ13599185, a cryptophycin, rhizoxin, methotrexate, an anthracycline, a camptothecin analogue, SN-38, DX-8951f, exatecan mesylate, truncated form of Pseudomonas aeruginosa exotoxin (PE38), a Duocarmycin derivative, an amanitin, α-amanitin, a spliceostatin, a thailanstatin, ozogamicin, tesirine, Amberstatin269 and soravtansine, or a derivative thereof. The inventors established that the combination of the invention and the compositions of the invention are equally suitable for improved delivery of nucleic acid based effector molecules, when comprised by the conjugate of the ASGPR ligand and the effector molecule, as for cytosolic delivery of effector molecules such as peptides and proteins, when such an effector molecule as part of the conjugate is contacted with target cell expressing the ASGPR, in the presence of saponin or a saponin derivative. For example, the therapeutic window for protein toxins is widened when contacting target cells with the conjugate comprising the effector molecule, i.e. the protein toxin, and the ligand for ASGPR, and with the saponin, according to the invention. The toxin exerts its intracellular effect to a higher extent or at a lower dose, when the target cells are exposed to the saponin and to the conjugate comprising the toxin, compared to the intracellular effect achieved at the same toxin dose or at the same lower toxin dose in the absence of the saponin, or a saponin derivative.

    Saponin

    [0131] An embodiment is the pharmaceutical combination of the invention, wherein the saponin comprises an aglycone core structure selected from the group (here referred to as ‘Group C’) consisting of: [0132] 2alpha-hydroxy oleanolic acid; [0133] 16alpha-hydroxy oleanolic acid; [0134] hederagenin (23-hydroxy oleanolic acid); [0135] 16alpha,23-dihydroxy oleanolic acid; [0136] gypsogenin; [0137] quillaic acid; [0138] protoaescigenin-21 (2-methylbut-2-enoate)-22-acetate; [0139] 23-oxo-barringtogenol C-21,22-bis(2-methylbut-2-enoate); [0140] 23-oxo-barringtogenol C-21(2-methylbut-2-enoate)-16,22-diacetate; [0141] digitogenin; [0142] 3,16,28-trihydroxy oleanan-12-en; [0143] gypsogenic acid, and [0144] derivatives thereof,preferably the saponin comprises an aglycone core structure selected from quillaic acid and gypsogenin or derivatives thereof, more preferably the saponin aglycone core structure is quillaic acid or a derivative thereof. Such preferred aglycones comprise an aldehyde group at the C-4 atom. Without wishing to be bound by any theory, such an aldehyde group, or a derivative thereof as described herein elsewhere, contributes to the endosomal escape enhancing activity of saponins of the triterpene glycoside type, comprising an aglycone selected from Group C, especially quillajic acid and gypsogenin.

    [0145] An embodiment is the saponin conjugate of the invention, wherein the at least one saponin is a monodesmosidic or bi-desmosidic triterpene saponin belonging to the type of a 12,13-dehydrooleanane with the aldehyde group in position C-4 and optionally comprising a glucuronic acid group in a carbohydrate substituent at the C-3beta-OH group of the saponin, preferably a bi-desmosidic triterpene saponin belonging to the type of a 12,13-dehydrooleanane with the aldehyde group in position C-4 and comprising a glucuronic acid group in a carbohydrate substituent at the C-3beta-OH group of the saponin.

    [0146] An embodiment is the pharmaceutical combination of the invention, wherein [0147] the saponin comprises a saccharide chain bound to the aglycone core structure, which is selected from group A: [0148] GlcA-, [0149] Glc-, [0150] Gal-, [0151] Rha-(1---->2)-Ara-, [0152] Gal-(1---->2)-[Xyl-(1---->3)]-GlcA-, [0153] Glc-(1---->2)-[Glc-(1---->4)]-GlcA-, [0154] Glc-(1---->2)-Ara-(1---->3)-[Gal-(1---->2)]-GlcA-, [0155] Xyl-(1---->2)-Ara-(1---->3)-[Gal-(1---->2)]-GlcA-, [0156] Glc-(1---->3)-Gal-(1---->2)-[Xyl-(1---->3)]-Glc-(1---->4)-Gal-, [0157] Rha-(1---->2)-Gal-(1---->3)-[Glc-(1--->2)]-GlcA-, [0158] Ara-(1---->4)-Rha-(1---->2)-Glc-(1---->2)-Rha-(1---->2)-GlcA-, [0159] Ara-(1---->4)-Fuc-(1---->2)-Glc-(1---->2)-Rha-(1---->2)-GlcA-, [0160] Ara-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, [0161] Ara-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, [0162] Ara-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0163] Ara-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0164] Ara-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0165] Ara-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0166] Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, [0167] Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, [0168] Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, [0169] Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Rha-(1.fwdarw.2)-GlcA-, [0170] Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0171] Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Glc-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0172] Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, [0173] Xyl-(1.fwdarw.4)-Fuc-(1.fwdarw.2)-Gal-(1.fwdarw.2)-Fuc-(1.fwdarw.2)-GlcA-, and [0174] derivatives thereof, or [0175] the saponin comprises a saccharide chain bound to the aglycone core structure, which is selected from group B: [0176] Glc-, [0177] Gal-, [0178] Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.4)]-Rha-, [0179] Rha-(1.fwdarw.2)-[Ara-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha-, [0180] Ara-, [0181] Xyl-, [0182] Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R1-(.fwdarw.4)]-Fuc- wherein R1 is 4E-Methoxycinnamic acid, [0183] Xyl-(1 .fwdarw.4)-Rha-(1 .fwdarw.2)-[R2-(.fwdarw.4)]-Fuc- wherein R2 is 4Z-Methoxycinnamic acid, [0184] Xyl-(1.fwdarw.4)-[Gal-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-4-OAc-Fuc-, [0185] Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-3,4-di-OAc-Fuc-, [0186] Xyl-(1.fwdarw.4)-[GIc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R3-(.fwdarw.4)]-3-OAc-Fuc- wherein R3 is 4E-Methoxycinnamic acid, [0187] Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-4-OAc-Fuc-, [0188] Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-4-OAc-Fuc-, [0189] (Ara- or Xyl-)(1.fwdarw.3)-(Ara- or Xyl-)(1.fwdarw.4)-(Rha- or Fuc-)(1.fwdarw.2)-[4-OAc-(Rha- or Fuc-)(1.fwdarw.4)]-(Rha- or Fuc-), [0190] Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc-, [0191] Api-(1---->3)-Xyl-(1---->4)-[Glc-(1---->3)]-Rha-(1---->2)-Fuc-, [0192] Xyl-(1.fwdarw.4)-[Gal-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc-, [0193] Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc-, [0194] Ara/Xyl-(1.fwdarw.4)-Rha/Fuc-(1.fwdarw.4)-[Glc/Gal-(1.fwdarw.2)]-Fuc-, [0195] Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R4-(.fwdarw.4)]-Fuc- wherein R4 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0196] Api-(1---->3)-Xyl-(1--->4)-Rha-(1---->2)-[R5-(---->4)]-Fuc- wherein R5 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0197] Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4-OAc-Fuc-, [0198] Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4-OAc-Fuc-, [0199] 6-OAc-GIc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3-OAc-Rha-(1.fwdarw.3)]-Fuc-, [0200] Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3-OAc--Rha-(1.fwdarw.3)]-Fuc-, [0201] Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc-, [0202] Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc-, [0203] Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc-, [0204] Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3,4-di-OAc-Qui-(1.fwdarw.4)]-Fuc-, [0205] Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc-, [0206] 6-OAc-Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc-, [0207] lc-(1.fwdarw.3)-[Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc-, [0208] Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc-, [0209] Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[GIc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4OAc-Fuc-, [0210] Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[GIc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4OAc-Fuc-, [0211] Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R6-(.fwdarw.4)]-Fuc- wherein R6 is 5-O-[5-O-Rha-(1.fwdarw.2)-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0212] Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R7-(.fwdarw.4)]-Fuc- wherein R7 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0213] Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R8-(.fwdarw.4)]-Fuc- wherein R8 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0214] .Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R9-(.fwdarw.4)]-Fuc- wherein R9 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0215] Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R10-(.fwdarw.4)]-Fuc- wherein R10 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0216] Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R11-(.fwdarw.3)]-Fuc- wherein R11 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid), [0217] Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R12-(.fwdarw.3)]-Fuc- wherein R12 is 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) [0218] Glc-(1.fwdarw.3)-[Glc-(1.fwdarw.6)]-Gal-, and [0219] derivatives thereof, or [0220] the saponin is a bidesmosidic triterpene glycoside comprising a first saccharide chain selected from the group A bound to the aglycone core structure and comprising a second saccharide chain selected from the group B bound to the aglycone core structure.

    [0221] Such saponins display the typical endosomal escape enhancing effect when a target cell is contacted with the saponin and an effector molecule, such as an effector molecule that is part of the conjugate according to the invention, comprising the effector molecule and the ligand for ASGPR1, e.g. a (GalNAc).sub.3Tris. Under influence of such a selected saponin comprising the one or two saccharides selected from Group C, the effector molecule in the conjugate reaches an intracellular threshold level such that the biological activity of the effector molecule inside a target cell is either established, or is increased, or the activity of the effector molecule can be established at a lower dose than the dose required for the same level of activity in the absence of saponin. In Table 1, saponins with such endosomal escape enhancing activity are summarized. These saponins comprise the listed aglycone core structures of Group C and comprise the monosaccharides or polysaccharides of Group A and/or Group B, and have been shown to potentiate effector molecules when target cells are exposed to both the effector molecule and the saponin, or have high structural similarity with saponins for which such endosomal escape enhancing activity has been determined.

    [0222] Therefore, an embodiment is the pharmaceutical combination of the invention, wherein the saponin is selected from the group consisting of: Quillaja bark saponin, dipsacoside B, saikosaponin A, saikosaponin D, macranthoidin A, esculentoside A, phytolaccagenin, aescinate, AS6.2, NP-005236, AMA-1, AMR, alpha-Hederin, NP-012672, NP-017777, NP-017778, NP-017774, NP-018110, NP-017772, NP-018109, NP-017888, NP-017889, NP-018108, SA1641, AE X55, NP-017674, NP-017810, AG1, NP-003881, NP-017676, NP-017677, NP-017706, NP-017705, NP-017773, NP-017775, SA1657, AG2, SO1861, GE1741, SO1542, SO1584, SO1658, SO1674, SO1832, SO1862, SO1904, QS-7, QS1861, QS-7 api, QS1862, QS-17, QS-18, QS-21 A-apio, QS-21 A-xylo, QS-21 B-apio, QS-21 B-xylo, beta-Aescin, Aescin la, Teaseed saponin I, Teaseedsaponin J, Assamsaponin F, Digitonin, Primula acid 1 and AS64R, stereoisomers thereof, derivatives thereof, and combinations thereof, preferably the saponin is selected from the group consisting of QS-21, a QS-21 derivative, SO1861, a SO1861 derivative, SA1641, a SA1641 derivative, GE1741,a GE1741 derivative and combinations thereof, more preferably the saponin is selected from the group consisting of a QS-21 derivative, a SO1861 derivative and combinations thereof, most preferably the saponin is a SO1861 derivative. The present inventors have found that these derivatives have improved potentiating effects when employed in conjunction with a conjugate comprising an effector molecule as described herein. That is to say, the derivatives lead to comparable endosomal escape enhancing effects as the non-derivatised saponins, while displaying lower cytotoxicity and lower haemolytic activity. More structural details of saponin derivatives suitable in the context of the present invention are provided below.

    [0223] An embodiment is the pharmaceutical combination of the invention, wherein the saponin is a saponin derivative wherein either: [0224] i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised; or [0225] ii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A as defined here above, the saccharide chain comprising a carboxyl group which has been derivatised; or [0226] iii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group B as defined here above, the saccharide chain comprising an acetoxy (Me(CO)O-) group which has been derivatised; or [0227] iv. any combination of derivatisations i., ii. and iii. is present, optionally any combination of two derivatisations of derivatisations i., ii. and iii.

    [0228] The inventors established that in particular saponins which have been derivatised with regard to a single chemical group present in the naturally occurring saponin or with regard to two of such chemical groups, maintain sufficient effector molecule potentiating activity, while both cytotoxicity and haemolytic activity of such mono-derivatised and bi-derivatised saponins is strongly reduced compared to cytotoxicity and haemolytic activity of the naturally occurring non-modified counterparts of such saponin derivatives. Also suitable according to the invention are the naturally occurring saponins for which the effector molecule potentiating effect is established when the saponin and the conjugate comprising the effector molecule are both contacted with a target cell exposing ASGPR1 at its surface.

    [0229] An embodiment is the pharmaceutical combination of the invention, wherein the saponin is selected from the group consisting of: SO1861, SA1657, GE1741, SA1641, QS-21, QS-21A, QS-21 A-api, QS-21 A-xyl, QS-21B, QS-21 B-api, QS-21 B-xyl, QS-7-xyl, QS-7-api, QS-17-api, QS-17-xyl, QS1861, QS1862, Quillajasaponin, Saponinum album, QS-18, Quil-A, Gyp1, gypsoside A, AG1, AG2, SO1542, SO1584, SO1658, SO1674, SO1832, SO1904, stereoisomers thereof, derivatives thereof and combinations thereof, preferably the saponin is selected from the group consisting of QS-21, a QS-21 derivative, SO1861, a SO1861 derivative, SA1641, a SA1641 derivative, GE1741, a GE1741 derivative and combinations thereof, more preferably the saponin is selected from the group consisting of a QS-21 derivative, a SO1861 derivative and combinations thereof, most preferably the saponin is a SO1861 derivative.

    [0230] An embodiment is the pharmaceutical combination of the invention, wherein the saponin is a saponin derivative of the quillaic acid or gypsogenin saponin of Group C as listed here above and represented by Molecule 1:

    ##STR00017##

    wherein [0231] A.sub.1 represents hydrogen, a monosaccharide or a linear or branched oligosaccharide, preferably A.sub.1 represents a saccharide chain selected from group A as defined here above, more preferably A.sub.1 represents a saccharide chain selected from group A as defined here above and A.sub.1 comprises or consists of a glucuronic acid moiety; [0232] A.sub.2 represents hydrogen, a monosaccharide or a linear or branched oligosaccharide, preferably A.sub.2 represents a saccharide chain selected from group B as defined here above, more preferably A.sub.2 represents a saccharide chain selected from group B as defined here above and A.sub.2 comprises at least one acetoxy (Me(CO)O-) group, such as one, two, three or four acetoxy groups, wherein at least one of A.sub.1 and A.sub.2 is not hydrogen, preferably both A.sub.1 and A.sub.2 are an oligosaccharide chain; [0233] and R is hydrogen in gypsogenin or hydroxyl in quillaic acid;wherein the saponin derivative corresponds to the saponin represented by Molecule 1 wherein at least one of the following derivatisations is present: [0234] i. the aldehyde group at position C.sub.23 of the quillaic acid or gypsogenin has been derivatised; [0235] ii. the carboxyl group of a glucuronic acid moiety of A.sub.1, when A.sub.1 represents a saccharide chain selected from group A as defined here above and A.sub.1 comprises or consists of a glucuronic acid moiety, has been derivatised; and [0236] iii. one or more, preferably all, of acetoxy group(s) of one saccharide moiety or of two or more saccharide moieties of A.sub.2, when A.sub.2 represents a saccharide chain selected from group B as defined here above and A.sub.2 comprises at least one acetoxy group, has/have been derivatised.

    [0237] An embodiment is the pharmaceutical combination of the invention, wherein A.sub.1 represents a saccharide chain selected from group A as defined here above and comprises or consists of a glucuronic acid moiety and wherein the carboxyl group of a glucuronic acid moiety of A.sub.1 has been derivatised and/or wherein A.sub.2 represents a saccharide chain selected from group B as defined here above and A.sub.2 comprises at least one acetoxy group and wherein at least one acetoxy group of A.sub.2 has been derivatised.

    [0238] An embodiment is the pharmaceutical combination of the invention, wherein the saponin represented by Molecule 1 is a bidesmosidic triterpene saponin, i.e. a saponin of the bidesmosidic triterpene glycoside type.

    [0239] An embodiment is the pharmaceutical combination of the invention, wherein the saponin derivative corresponds to the saponin represented by Molecule 1 wherein at least one of the following derivatisations is present: [0240] i. the aldehyde group at position C.sub.23 of the quillaic acid or gypsogenin has been derivatised by; [0241] reduction to an alcohol; or [0242] transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0243] transformation into a hydrazone bond through reaction with N-[β-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0244] transformation into a hydrazone bond through reaction with N-[ĸ-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; [0245] ii. the carboxyl group of a glucuronic acid moiety of A.sub.1, when A.sub.1 represents a saccharide chain selected from group A as defined here above and A.sub.1 comprises or consists of a glucuronic acid moiety, has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu-AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; and [0246] iii. one or more, preferably all, of acetoxy group(s) of one saccharide moiety or of two or more saccharide moieties of A.sub.2, when A.sub.2 represents a saccharide chain selected from group B as defined here above and A.sub.2 comprises at least one acetoxy group, has/have been derivatised by transformation into a hydroxyl group (HO—) by deacetylation.

    [0247] An embodiment is the pharmaceutical combination of the invention, wherein A.sub.1 is Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA and/or A.sub.2 is Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc, preferably the saponin represented by Molecule 1 is 3-O-beta-D-galactopyranosyl-(1.fwdarw.2)-[beta-D-xylopyranosyl-(1.fwdarw.3)]-beta-D-glucuronopyranosyl quillaic acid 28-O-beta-D-glucopyranosyl-(1.fwdarw.3)-beta-D-xylopyranosyl-(1.fwdarw.4)- alpha-L-rhamnopyranosyl-(1.fwdarw.2)-[beta-D-xylopyranosyl-(143)-4OAc-beta-D-quinovopyranosyl-(1.fwdarw.4)]-beta-D-fucopyranoside, more preferably SO1861, GE1741, SA1641 and/or QS-21, or a derivative thereof, most preferably SO1861 or a derivative thereof.

    [0248] An embodiment is the pharmaceutical combination of the invention, wherein the saponin is a saponin derivative wherein either: [0249] i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised by: [0250] reduction to an alcohol; or [0251] transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0252] transformation into a hydrazon bond through reaction with N-[β-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0253] transformation into a hydrazon bond through reaction with N-[ĸ-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0254] ii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A as defined here above, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety which has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu- AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; or [0255] iii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group B as defined here above, the saccharide chain comprising an acetoxy (Me(CO)O—) group which has been derivatised by transformation into a hydroxyl group (HO—) by deacetylation; or [0256] iv. the saponin derivative comprises any combination of derivatisations i., ii. and iii., optionally any combination of two derivatisations i., ii. and iii;preferably, the saponin derivative comprises an aglycone core structure wherein the aglycone core structure comprises an aldehyde group which has been derivatised by transformation into a hydrazone bond through reaction with EMCH wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol.

    [0257] An embodiment is the pharmaceutical combination of the invention, wherein the saponin is a saponin derivative wherein either: [0258] i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised by transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH; or [0259] ii. the saponin comprises a saccharide chain, preferably a saccharide chain selected from group A as defined here above, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety which has been derivatised by transformation into an amide bond through reaction with N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; or [0260] iii. the saponin derivative comprises a combination of derivatisations i. and ii.

    [0261] An embodiment is the pharmaceutical combination of the invention, wherein the saponin derivative comprises an aglycone core structure wherein the aglycone core structure comprises an aldehyde group and wherein the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A as defined here above, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety, which glucuronic acid moiety has been derivatised by transformation into an amide bond through reaction with N-(2-aminoethyl)maleimide (AEM).

    [0262] An embodiment is the pharmaceutical combination of the invention, wherein the saponin is a saponin derivative represented by Molecule 2:

    ##STR00018##

    or wherein the saponin derivative is the saponin derivative represented by Molecule 3

    ##STR00019##

    TABLE-US-00001 Saponins displaying (late) endosomal/lysosomal escape enhancing activity, and saponins comprising a structure reminiscent to such saponins displaying (late) endosomal/lysosomal escape enhancing activity Saponin Name Aglycone core Carbohydrate substituent at the C-3beta-OH group Carbohydrate substituent at the C-28-OH group NP-005236 2alpha-Hydroxyoleanolic acid GlcA- Glc/Gal- AMA-1 16alpha-Hydroxyoleanolic acid Glc- Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.4)]-Rha- AMR 16alpha-Hydroxyoleanolic acid Glc- Rha-(1.fwdarw.2)-[Ara-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha- alpha-Hederin Hederagenin (23-Hydroxyoleanolic acid) Rha-(1.fwdarw.2)-Ara- - NP-012672 16alpha,23-Dihydroxyoleanolic acid Ara/Xyl-(1.fwdarw.4)-Rha/Fuc-(1.fwdarw.2)-Glc/Gal-(1.fwdarw.2)-Rha/Fuc-(1.fwdarw.2)-GlcA- Ara/Xyl- NP-017777 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc- (R = 4E-Methoxycinnamic acid) NP-017778 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc- (R = 4Z-Methoxycinnamic acid) NP-017774 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-[Gal-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-4-OAc-Fuc- N P-018110.sup.c NP-017772.sup.d Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-3,4-di-OAc-Fuc- NP-018109 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-3-OAc-Fuc- (R = 4E-Methoxycinnamic acid) NP-017888 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-4-OAc-Fuc- NP-017889 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-4-OAc-Fuc- NP-018108 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Ara/Xyl-(1.fwdarw.3)-Ara/Xyl-(1.fwdarw.4)-Rha/Fuc-(1.fwdarw.2)-[4-OAc-Rha/Fuc-(1 .fwdarw.4)]-Rha/Fuc- SA1641.sup.a, AE X55.sup.b Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc- NP-017674 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc- NP-017810 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-[Gal-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc- AG1 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-Fuc- NP-003881 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Ara/Xyl-(1.fwdarw.4)-Rha/Fuc-(1.fwdarw.4)-[Glc/Gal-(1.fwdarw.2)]-Fuc- NP-017676 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) NP-017677 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-( .fwdarw.4)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) NP-017706 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4-OAc-Fuc- NP-017705 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4-OAc-Fuc- NP-017773 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- 6-OAc-Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3-OAc-Rha-(1.fwdarw.3)]-Fuc- NP-017775 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3-OAc--Rha-(1.fwdarw.3)]-Fuc- SA1657 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc- AG2 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-[Qui-(1.fwdarw.4)]-Fuc- SO1861 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc- GE1741 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[3,4-di-OAc-Qui-(1.fwdarw.4)]-Fuc- SO1542 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc- SO1584 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- 6-OAc-Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc- SO1658 Gypsogenin Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc- SO1674 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Glc-(1.fwdarw.3)-[Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)]-Rha-(1.fwdarw.2)-Fuc- SO1832 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc- QS-7 (also referred to as QS1861) Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4OAc-Fuc- QS-7 api (also referred to as QS1862) Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[Rha-(1.fwdarw.3)]-4OAc-Fuc- QS-17 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc-(R = 5-O-[5-O-Rha-(1.fwdarw.2)-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) QS-18 Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api/Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-[Glc-(1.fwdarw.3)]-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) QS-21 A-apio Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) QS-21 A-xylo Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-(.fwdarw.4)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) QS-21 B-apio Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Api-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-(.fwdarw.3)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) QS-21 B-xylo Quillaic acid Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA- Xyl-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[R-(.fwdarw.3)]-Fuc-(R = 5-O-[5-O-Ara/Api-3,5-dihydroxy-6-methyl-octanoyl]-3,5-dihydroxy-6-methyl-octanoic acid) beta-Aescin (described: Aescin Ia) Protoaescigenin-21(2-methylbut-2-enoate)-22-acetat Glc-(1.fwdarw.2)-[Glc-(1.fwdarw.4)]-GlcA- - Teaseed saponin I 23-Oxo-barringtogenol C -21,22-bis(2-methylbut-2-enoate) Glc-(1.fwdarw.2)-Ara-(1.fwdarw.3)-[Gal-(1.fwdarw.2)]-GlcA- - Teaseedsaponin J 23-Oxo-barringtogenol C -21,22-bis(2-methylbut-2-enoate) Xyl-(1.fwdarw.2)-Ara-(1.fwdarw.3)-[Gal-(1.fwdarw.2)]-GlcA- - Assamsaponin F 23-Oxo-barringtogenol C -21(2-methylbut-2-enoate)-16,22-diacetat Glc-(1.fwdarw.2)-Ara-(1.fwdarw.3)-[Gal-(1.fwdarw.2)]-GlcA- - Digitonin Digitogenin Glc-(1.fwdarw.3)-Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-Glc-(1.fwdarw.4)-Gal- - Primula acid 1 3,16,28-Trihydroxyoleanan-12-en Rha-(1.fwdarw.2)-Gal-(1.fwdarw.3)-[Glc-(1.fwdarw.2)]-GlcA- - AS64R Gypsogenic acid - Glc-(1.fwdarw.3)-[Glc-(1.fwdarw.6)]-Gal- Carbohydrate substituent at the C-23-OH group AS6.2 Gypsogenic acid Gal- Glc-(1.fwdarw.3)-[Glc-(1.fwdarw.6)]-Gal- a, b: Different names refer to different isolates of the same structure c, d: Different names refer to different isolates of the same structure

    [0263] A second aspect of the invention relates to the pharmaceutical combination of the invention for use as a medicament. To the knowledge of the inventors they are the first to provide the pharmaceutical combination of the invention for improving the efficacy of e.g. siRNA or BNA based therapies. Use of the pharmaceutical combination of the invention potentiates the intracellular effect of the effector molecule comprised by the conjugate comprising the ligand for ASGPR1. The medicament is particularly suitable for treatment of diseases or abberancies involving aberrant liver cells which express ASGPR1. Aberrant liver cells are cells of patients who suffer for example from any disease or health problem in which an expression product is involved of any one or more of genes: HSP27, apoB, TTR, PCSK9, ALAS1, AT3, GO, CC5, X gene of HBV, S gene of HBV, AAT and LDH. Such diseases are for example any of a cancer, an infectious disease, a viral infection, hypercholesterolemia, primary hyperoxaluria, haemophilia A, haemophilia B, AAT related liver disease, acute hepatic porphyria, TTR-mediated amyloidosis, hereditary TTR amyloidosis (hATTR), complement-mediated disease, hepatitis B infection, a disease or disorder relating to HSP27 expression, or an auto-immune disease.

    [0264] A third aspect of the invention relates to the pharmaceutical combination of the invention, for use in the treatment or prophylaxis of a disease or health problem in which an expression product is involved of any one or more of genes: HSP27, apoB, TTR, PCSK9, ALAS1, AT3, GO, CC5, X gene of HBV, S gene of HBV, AAT and LDH.

    [0265] An embodiment is the pharmaceutical combination of the invention, or the pharmaceutical combination for use of the invention, for use in the treatment or prophylaxis of a cancer, an infectious disease, a viral infection, hypercholesterolemia, primary hyperoxaluria, haemophilia A, haemophilia B, AAT related liver disease, acute hepatic porphyria, TTR-mediated amyloidosis, hereditary TTR amyloidosis (hATTR), complement-mediated disease, hepatitis B infection, a disease or disorder relating to HSP27 expression, or an auto-immune disease.

    [0266] An embodiment is the pharmaceutical combination for use according to the invention, wherein the pharmaceutical combination comprises: [0267] a saponin derivative, wherein the saponin derivative corresponds to the saponin represented by Molecule 1 wherein at least one of the following derivatisations is present: [0268] i. the aldehyde group at position C.sub.23 of the quillaic acid or gypsogenin has been derivatised by; [0269] reduction to an alcohol; or [0270] transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0271] transformation into a hydrazone bond through reaction with N-[β-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0272] transformation into a hydrazone bond through reaction with N-[κ-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; [0273] ii. the carboxyl group of a glucuronic acid moiety of A.sub.1, when A.sub.1 represents a saccharide chain selected from group A and A.sub.1 comprises or consists of a glucuronic acid moiety, has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu-AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; and [0274] iii. one or more, optionally all, of acetoxy group(s) of one saccharide moiety or of two or more saccharide moieties of A.sub.2, when A.sub.2 represents a saccharide chain selected from group B and A.sub.2 comprises at least one acetoxy group, has/have been derivatised by transformation into a hydroxyl group (HO—) by deacetylation; or [0275] a saponin according to Molecule 1, wherein A.sub.1 is Gal-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)]-GlcA and/or A.sub.2 is Glc-(1.fwdarw.3)-Xyl-(1.fwdarw.4)-Rha-(1.fwdarw.2)-[Xyl-(1.fwdarw.3)-4-OAc-Qui-(1.fwdarw.4)]-Fuc, preferably the saponin represented by Molecule 1 is 3-O-beta-D-galactopyranosyl-(1.fwdarw.2)-[beta-D-xylopyranosyl-(1.fwdarw.3)]-beta-D-glucuronopyranosyl quillaic acid 28-O-beta-D-glucopyranosyl-(1.fwdarw.3)-beta-D-xylopyranosyl-(1.fwdarw.4)- alpha-L-rhamnopyranosyl-(1.fwdarw.2)-[beta-D-xylopyranosyl-(1.fwdarw.3)-4OAc-beta-D-quinovopyranosyl-(1.fwdarw.4)]-beta-D-fucopyranoside, more preferably SO1861, GE1741, SA1641 and/or QS-21, or a derivative thereof, most preferably SO1861 or a derivative thereof; or [0276] a saponin derivative whereinpreferably, the saponin derivative comprises an aglycone core structure wherein the aglycone core structure comprises an aldehyde group which has been derivatised by transformation into a hydrazone bond through reaction with EMCH wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0277] i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised by: [0278] reduction to an alcohol; or [0279] transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0280] transformation into a hydrazon bond through reaction with N-[β-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0281] transformation into a hydrazon bond through reaction with N-[κ-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; [0282] ii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety which has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu- AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; [0283] iii. the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group B, the saccharide chain comprising an acetoxy (Me(CO)O—) group which has been derivatised by transformation into a hydroxyl group (HO—) by deacetylation; or [0284] iv. the saponin derivative comprises any combination of derivatisations i., ii. and iii., optionally any combination of two derivatisations i., ii. and iii.; [0285] a saponin derivative wherein [0286] i. the saponin derivative comprises an aglycone core structure comprising an aldehyde group which has been derivatised by transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH; [0287] ii. the saponin comprises a saccharide chain, preferably a saccharide chain selected from group A, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety which has been derivatised by transformation into an amide bond through reaction with N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; or [0288] iii. the saponin derivative comprises a combination of derivatisations i. and ii.; or [0289] a saponin derivative that comprises an aglycone core structure wherein the aglycone core structure comprises an aldehyde group and wherein the saponin derivative comprises a saccharide chain, preferably a saccharide chain selected from group A, the saccharide chain comprising a carboxyl group, preferably a carboxyl group of a glucuronic acid moiety, which glucuronic acid moiety has been derivatised by transformation into an amide bond through reaction with N-(2-aminoethyl)maleimide (AEM); or [0290] a saponin derivative represented by Molecule 2: or a saponin derivative represented by Molecule 3:

    [0291] A fourth aspect of the invention relates to an in vitro or ex vivo method for transferring the effector molecule comprised by the conjugate comprising the ligand for ASGPR according to the invention, from outside a cell to inside said cell, preferably into the cytosol of said cell, comprising the steps of: [0292] a) providing a cell which expresses ASGPR, preferably ASGPR1, on its surface, preferably selected from a liver cell, a virally infected cell and a cancer cell; [0293] b) providing the conjugate of the invention, the conjugate comprising the effector molecule to be transferred; [0294] c) providing the saponin according to the invention; [0295] d) contacting the cell of step a) in vitro or ex vivo with the conjugate of step b) and the saponin of step c), therewith effecting the transfer of said conjugate comprising the effector molecule from outside the cell to inside said cell, and by effecting the transfer of said conjugate effecting the transfer of the effector molecule from outside the cell to inside said cell, preferably into the cytosol of said cell.

    [0296] A fifth aspect of the invention relates to an in vitro or ex vivo method for transferring the conjugate of the invention from outside a cell to inside said cell, comprising the steps of: [0297] a) providing a cell which expresses ASGPR, preferably ASGPR1, on its surface, preferably selected from a liver cell, a virally infected cell and a cancer cell; [0298] b) providing the conjugate of the invention; [0299] c) providing the saponin of the invention; [0300] d) contacting the cell of step a) in vitro or ex vivo with the conjugate of step b) and the saponin of step c), therewith effecting the transfer of the conjugate from outside the cell to inside said cell.

    [0301] An embodiment is any of the two methods of the invention, wherein the ligand for ASGPR comprises at least one N-acetylgalactosamine (GalNAc) moiety, preferably three or four GalNAc moieties, more preferably the ligand for ASGPR comprises or consists of (GalNAc).sub.3Tris and/or wherein the effector molecule is an oligonucleotide selected from any one of an anti-miRNA, a BNA-AON or an siRNA, such as BNA-based siRNA, preferably selected from chemically modified siRNA, metabolically stable siRNA and chemically modified, metabolically stable siRNA.

    [0302] An embodiment is any of the two methods of the invention, wherein the effector molecule comprises or consists of at least one of a small molecule such as a drug molecule, a toxin such as a protein toxin, an oligonucleotide such as a BNA, a xeno nucleic acid or an siRNA, an enzyme, a peptide, a protein, or any combination thereof, preferably, the effector molecule is a toxin, an enzyme or an oligonucleotide, preferably the toxin is saporin or dianthin.

    [0303] An embodiment is any of the two methods of the invention, wherein the saponin is derivatised SO1861 and/or derivatised QS-21, preferably SO1861-Glu-AEM or SO1861-Ald-EMCH or QS-21-Glu-AEM or QS-21-Ald-EMCH according to previous embodiments of the invention.

    [0304] An embodiment is any of the two methods of the invention, wherein the saponin is a saponin derivative corresponding to the saponin represented by Molecule 1 wherein at least one of the following derivatisations is present: [0305] i. the aldehyde group at position C.sub.23 of the quillaic acid or gypsogenin has been derivatised by; [0306] reduction to an alcohol; or [0307] transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing a saponin-Ald-EMCH such as a SO1861-Ald-EMCH or a QS-21-Ald-EMCH, wherein the maleimide group of the EMCH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0308] transformation into a hydrazone bond through reaction with N-[β-maleimidopropionic acid] hydrazide (BMPH) wherein the maleimide group of the BMPH is optionally derivatised by formation of a thioether bond with mercaptoethanol; or [0309] transformation into a hydrazone bond through reaction with N-[κ-maleimidoundecanoic acid] hydrazide (KMUH) wherein the maleimide group of the KMUH is optionally derivatised by formation of a thioether bond with mercaptoethanol; [0310] ii. the carboxyl group of a glucuronic acid moiety of A.sub.1, when A.sub.1 represents a saccharide chain selected from group A and A.sub.1 comprises or consists of a glucuronic acid moiety, has been derivatised by transformation into an amide bond through reaction with 2-amino-2-methyl-1,3-propanediol (AMPD) or N-(2-aminoethyl)maleimide (AEM), therewith providing a saponin-Glu-AMPD such as a QS-21-Glu-AMPD or a SO1861-Glu-AMPD or a saponin-Glu-AEM such as a QS-21-Glu-AEM or a SO1861-Glu-AEM; and [0311] iii. one or more, preferably all, of acetoxy group(s) of one saccharide moiety or of two or more saccharide moieties of A.sub.2, when A.sub.2 represents a saccharide chain selected from group B and A.sub.2 comprises at least one acetoxy group, has/have been derivatised by transformation into a hydroxyl group (HO—) by deacetylation.

    [0312] An embodiment is any of the two methods of the invention, wherein the effector molecule is an oligonucleotide which, for example when present inside a mammalian cell, can silence any one of genes: apolipoprotein B (apoB), transthyretin (TTR), proprotein convertase subtilisin/kexin type 9 (PCSK9), delta-aminolevulinate synthase 1 (ALAS1), antithrombin 3 (AT3), glycolate oxidase (GO), complement component C5 (CC5), X gene of hepatitis B virus (HBV), S gene of HBV, alpha-1 antitrypsin (AAT) and lactate dehydrogenase (LDH), and/or, for example when present inside a mammalian cell, can target an aberrant miRNA and/or, for example when present inside a mammalian cell, wherein the oligonucleotide can target an mRNA involved in expression of any one of proteins: apoB, TTR, PCSK9, ALAS1, AT3, GO, CC5, expression product of X gene of HBV, expression product of S gene of HBV, AAT and LDH, or, for example when present inside a mammalian cell, can antagonize or restore an miRNA function such as inhibiting an oncogenic miRNA (onco-miR) or suppression of expression of an onco-miR.

    [0313] A sixth aspect of the invention relates to a kit of parts, comprising the pharmaceutical combination of the invention or the second pharmaceutical composition of the invention, and instructions for use of said pharmaceutical combination or second pharmaceutical composition according to the invention or for use in a method according to the invention.

    [0314] While the invention has been described in terms of several embodiments, it is contemplated that alternatives, modifications, permutations and equivalents thereof will become apparent to one having ordinary skill in the art upon reading the specification and upon study of the drawings. The invention is not limited in any way to the illustrated embodiments. Changes can be made without departing from the scope which is defined by the appended claims.

    [0315] The present invention has been described above with reference to a number of exemplary embodiments. Modifications are possible, and are included in the scope of protection as defined in the appended claims. The invention is further illustrated by the following examples, which should not be interpreted as limiting the present invention in any way.

    EXAMPLES AND EXEMPLARY EMBODIMENTS

    Example 1. CD71-Saporin + 4000 nM Trivalent GalNAc-L-SO1861

    [0316] Trivalent-GalNAc is a targeting ligand that recognizes and binds the ASGPR1 receptor on hepatocytes. Trivalent GalNAC was produced (FIG. 1 and FIG. 8) and SO1861-EMCH was conjugated (labile, in a similar manner as described in FIG. 2 and FIG. 4 for underivatised SO1861, wherein SPT001 is synonymous to SO1861) to trivalent-GalNAc, with a DAR = 1 for the bound SO1861, (trivalent-GalNAc-SO1861), also referred to as (GalNAc)3-SO1861). SO1861-EMCH refers to SO1861 wherein the aldehyde group is derivatised by transformation into a hydrazone bond through reaction with N-ε-maleimidocaproic acid hydrazide (EMCH), therewith providing SO1861-Ald-EMCH. The ‘trivalent-GalNAc’ as depicted in FIGS. 1 and 8 is a typical (GalNAc).sub.3Tris conjugate suitable for coupling to an effector molecule or to saponin. As a control SO1861-EMCH was also conjugated (labile) to monovalent-GalNAc (FIG. 3), with a DAR = 1 for the bound SO1861, (GalNAc-SO1861). HepG2 (ASGPR1.sup.+; CD71.sup.+, Table A3) and Huh7 (ASGPR1.sup.+/-; CD71.sup.+, Table A3) cells were treated with a concentration range of trivalent-GalNAc-L-SO1861 and GalNAc-L-SO1861 in the presence and absence of 10 pM CD71-saporin (monoclonal antibody OKT-9 targeting CD71 conjugated to the protein toxin saporin). Cell treatment in absence of CD71-saporin show that the trivalent-GalNAc-L-SO1861 (or trivalent-GalNAc, also referred to as (GalNAc)3) as single compound is not toxic up to 15000 nM (FIG. 9).

    [0317] HepG2 and Huh7 cells were also treated with a range of concentrations of CD71-saporin, also referred to as CD71-SPRN, in combination with a fixed concentration of 1000 nM or 4000 nM trivalent-GalNAc-SO1861 (DAR = 1 for the bound SO1861), also referred to as (GalNAc)3-SPT. Targeted protein toxin mediated cell killing of ASGPR1/CD71 expressing cells (HepG2 and Huh7) was determined. This revealed strong cell killing at low concentrations of CD71-saporin (IC50 = 1 pM) in both cell lines, whereas equivalent concentrations CD71-saporin, CD71-saporin + 1000 nM trivalent-GalNAc or CD71-saporin + 4000 nM trivalent-GalNAc could only induce cell killing at high concentrations CD71-saporin (IC50 = 100 pM) in both cell lines (FIG. 10).

    [0318] All this shows that trivalent-GalNAc-SO1861 in combination with low concentrations of CD71-saporin effectively induce cell killing in ASGPR1/CD71 expressing cells. Thus trivalent-GalNAc-SO1861 effectively induces endosomal escape of a protein toxin in ASGPR1 expressing cells.

    Example 2 Trivalent-GalNAc-L/S-BNA + SO1861-EMCH

    [0319] HSP27BNA was conjugated to trivalent-GalNAc (FIGS. 6-7) and HepG2 (ASGPR1.sup.+) cells or Huh7 (ASPGR1.sup.+/-) were treated with a range of concentrations of trivalent-GalNAc-L-HSP27BNA (labile conjugation, FIG. 6) or trivalent-GalNAc-S-HSP27BNA (stable conjugation, FIG. 7) in combination with a fixed concentration of 4000 nM SO1861-EMCH, also referred to as SPT-EMCH. HSP27 gene silencing in HepG2 and Huh7 cells was determined. Only in combination with 4000 nM SO1861-EMCH effective gene silencing was observed at low concentrations of trivalent-GalNAc-L-HSP27BNA (HepG2: IC50 = 0,1 nM; Huh7: IC50 = 3 nM) or trivalent-GalNAc-S-HSP27BNA (HepG2: IC50 = 0,1 nM; Huh7: IC50 = 3 nM) in both HEPG2 and Huh7 cells, whereas equivalent concentrations trivalent-GalNAc-L-HSP27BNA (HepG2/Huh7: IC50> 2000 nM) or trivalent-GalNAc-S-HSP27BNA (HepG2/Huh7: IC50> 2000 nM) did not show gene silencing activity in HepG2 and Huh7 cell lines (FIG. 11).

    [0320] Next, ApoBBNA was conjugated in a similar manner (FIGS. 6-7) to trivalent-GalNAc and HepG2 (ASGPR1.sup.+) cells or Huh7 (ASPGR1.sup.+/-) were treated with a range of concentrations of trivalent-GalNAc-L-ApoBBNA (labile conjugation, FIG. 6, FIG. 12, FIG. 13) or trivalent GaINAc-S-ApoBBNA (stable conjugation, FIG. 7, FIG. 14, FIG. 15) or a trivalent GalNAc-L-ApoB.sub.scrambledBNA or trivalent GalNAc-S-ApoB.sub.scrambledBNA (where the scrambled ApoBBNA is an antisense scrambled oligo sequence that does not bind the ApoB mRNA; off-target control BNA) in combination with a fixed concentration of 4000 nM SO1861-EMCH. ApoB gene silencing in HepG2 (ASGPR1.sup.+) cells or Huh7 (ASPGR1.sup.+/-) was determined. Only in combination with 4000 nM SO1861-EMCH effective gene silencing was observed at low concentrations of trivalent-GalNAc-L-ApoBBNA (IC50 = 10 nM) or trivalent-GalNAc-S-ApoBBNA (IC50 = 10 nM) in HepG2 cells, whereas equivalent concentrations trivalent-GalNAc-L-ApoBBNA (IC50 > 2000 nM) or trivalent-GalNAc-S-ApoBBNA (IC50 > 2000 nM) did not show gene silencing activity in HepG2 cells (FIG. 12, FIG. 14). The treatments did not affect the viability of the cell lines (FIG. 13, FIG. 15). The ‘L’ refers to a ‘labile’ linker, which indicates that the linker is cleaved in the cell, i.e. at pH as apparent in the endosome and the lysosome. In contrast, the ‘S’ refers to a ‘stable’ linker, which indicates that the linker is not cleaved in the cell, i.e. at pH as apparent in the endosome and the lysosome. Thus, a conjugate comprising a labile bond between any two molecules forming the conjugate or comprised by the conjugate, will be cleaved at a position in the labile linker, therewith dissociating the two linked or bound molecules. An example is the cleavage of a hydrazone bond under acidic conditions as apparent in the endosome and lysosome of mammalian cells such as human cells.

    [0321] All this shows that SO1861-EMCH can enhance endosomal escape and target gene silencing of trivalent-GalNAc-L-BNA or trivalent-GalNAc-S-BNA for two independent gene targets. The gene silencing is more efficient in HepG2 cells compared to Huh7 cells, suggesting that higher levels of ASGPR1 expression at the plasma membrane of the cell facilitates increased uptake of the GalNAc-BNA conjugates.

    Example 3 Trivalent-GalNAc-L/S-BNA + Trivalent-GalNAc-L-SO1861

    [0322] SO1861-EMCH was conjugated (labile, in a similar manner as described in FIG. 2 and FIG. 4 for underivatised SO1861) to trivalent-GalNAc, with a DAR = 1 for the bound SO1861, (trivalent-GalNac-SO1861). HepG2 (ASGPR1.sup.+) cells or Huh7 (ASPGR1.sup.+/-) cells were treated with a range of concentrations of trivalent-GalNAc-L-ApoBBNA (labile conjugation FIG. 16), trivalent-GalNAc-S-ApoBBNA (stable conjugation (FIG. 17) or the scrambled off-target control conjugates (trivalent-GalNAc-L-ApoB.sub.scrambledBNA or trivalent-GalNAc-S-ApoB.sub.scrambledBNA) in combination with a fixed concentration of 4000 nM trivalent-GalNAc-L-SO1861 (DAR = 1 for the bound SO1861). ApoB gene silencing HepG2 (ASGPR1.sup.+) cells and Huh7 (ASPGR1.sup.+/-) cells was determined. Only in combination with 4000 nM trivalent-GalNAc-L-SO1861 effective gene silencing was observed at low concentrations of trivalent-GalNAc-L-ApoBBNA (IC50 = 50 nM) or trivalent-GalNAc-S-ApoBBNA (IC50 = 50 nM) in HepG2 cells (ASGPR1.sup.+). Both combination treatments in Huh7 cells (ASGPR1.sup.+/-) showed less effective gene silencing (trivalent-GalNAc-L-ApoBBNA: IC50 = 700 nM; trivalent-GalNAc-S-ApoBBNA: IC50 = 700 nM). Equivalent concentrations of trivalent-GalNAc-L-ApoBBNA (HepG2/Huh7: IC50> 1000 nM) or trivalent-GalNAc-S-ApoBBNA (HepG2/Huh7: IC50 > 1000 nM) did not show gene silencing activity in HepG2 and Huh7 cell lines, nor did 4000 nM trivalent-GalNAc-L-SO1861 induce/enhance gene silencing of scrambled trivalent-GalNAc-L-ApoB.sub.scrambledBNA (HepG2/Huh7: IC50 > 1000 nM) or scrambled trivalent-GalNAc-S-ApoB.sub.scrambledBNA (HepG2/Huh7: IC50 > 1000 nM) (FIG. 16). The treatments did not affect the viability of both cell lines (FIG. 17).

    [0323] All this shows that in combination with trivalent-GalNAc-L-SO1861, very low concentrations of trivalent-GalNAc-L-HSP27BNA or trivalent-GalNAc-S-HSP27BNA effectively induce gene silencing in ASGPR1 expressing cells, and again stronger effects are seen in cells with a higher ASGPR1 expression.

    Example 4 (GalNAc)3-BNA + SO1861-EMCH in Human Primary Hepatocytes

    [0324] ApoBBNA (ApoBBNA#01, targeting human ApoB mRNA) was conjugated to trivalent-GalNAc ((GalNAc)3) (FIG. 6) and primary hepatocytes (ASGPR1.sup.+) cells were treated with a range of concentrations of (GalNAc)3-ApoBBNA#01 with and without addition of 2000 nM SO1861. ApoB gene silencing in primary hepatocytes (ASGPR1.sup.+) cells was determined. Only in combination with 2000 nM, SO1861-EMCH effective gene silencing was observed at low concentrations of (GalNAc)3-ApoBBNA#01 (IC50 = 8 nM) in primary hepatocytes, whereas (GalNAc)3-ApoBBNA#01 alone revealed an IC50> 1000 nM (FIG. 18A). Next the effect on cell viability of these treatments was determined and this revealed, (GalNAc)3-ApoBBNA#01: IC50> 10000 nM and (GalNAc)3-ApoBBNA + SO1861-EMCH: IC50 ca 500 nM (FIG. 18B). All this shows that SO1861-EMCH can strongly enhance (GalNAc)3-targeted delivery of an oligonucleotide payload in human primary hepatocytes.

    Example 5 (GalNAc)3-BNA + SO1861-EMCH in Human Primary Hepatocytes

    [0325] An ApoB-sequence (targeting both, mouse and human ApoB RNA) BNA, more specifically ApoB#02 BNA.sup.NC, or ApoB#02 or ApoBBNA#02 or thiol13-ApoB BNA, was conjugated to a linker (‘Ls’) revealing (GalNAc)3-ApoB#02 with a DAR = 1 with respect to bound ApoB#02 (FIGS. 21-23).

    [0326] Human primary hepatocytes (ASGPR1.sup.+) were treated with a range of concentrations (GalNAc)3-ApoB#02 BNA with and without 2000 nM SO1861-EMCH. ApoB gene silencing in primary hepatocytes (ASGPR1.sup.+) cells was determined. Only in combination with 2000 nM SO1861-EMCH effective gene silencing was observed at very low concentrations of (GalNAc)3-ApoBBNA#02 (IC50 < 0.01 nM), whereas equivalent concentrations ApoBBNA#02 (IC50 = 200 nM), (GalNAc)3-ApoBBNA#02 (IC50 = 5 nM), or ApoBBNA#02 RNAiMAX transfection (IC50 = 5 nM) where less potent (FIG. 19A). The dotted line in the ApoBBNA#02 RNAiMAX indicates concentrations at which toxicity and cell death occurs. Next the effect on cell viability of these treatments was determined and this revealed, ApoBBNA#02: IC50 > 10000; (GalNAc)3-ApoBBNA#02: IC50 > 10000 nM; (GalNAc)3-ApoBBNA#02 + SO1861-EMCH: IC50 = 5000 nM; ApoBBNA#02 + RNAiMAX: IC50 = 100 nM (FIG. 19B). All this shows that SO1861-EMCH can strongly enhance (GalNAc)3-targeted delivery of an oligonucleotide payload in human primary hepatocytes.

    Example 6 (GalNAc)3-BNA + SO1861-EMCH in Primary Mouse Hepatocytes

    [0327] A murine ApoB-sequence targeting BNA, more specifically ApoB#02 BNA.sup.NC, or ApoB#02 or ApoBBNA#02 or thiol13-ApoB BNA, was conjugated to a linker (‘Ls’) revealing (GalNAc)3-ApoB#02 with a DAR = 1 with respect to bound ApoB#02 (FIGS. 21-23).

    [0328] Primary mouse hepatocytes were treated with a range of concentrations of either ApoB#02 BNA, (GalNAc)3-ApoB#02, or (GalNAc)3-ApoB#02 + 2000 nM SO1861-EMCH and ApoB RNA expression was determined by qPCR after 72 hrs incubation. Gene expression inhibition, was observed at low concentrations of (GalNAc)3-ApoB#02 BNA (IC50 ca 0.03 nM) in combination with 2000 nM SO1861-EMCH (FIG. 20). Treatment with ApoB#02 alone was approximately 100 - 667-fold less potent in ApoB RNA downmodulation (ApoB#02: IC50 = 20 nM), while (GalNAc)3-ApoB#02 with an ApoB#02 IC50 of ca. 2 nM was about 10 - 67-fold less potent (FIG. 20).

    [0329] This shows that only in combination with (GalNAc)3-SO1861 or SO1861-EMCH, very low concentrations of (GalNAc)3-ApoB#02 BNA are effectively inducing ApoB RNA downmodulation, i.e., gene silencing in murine primary hepatocytes.

    Materials and Methods

    [0330] TABLE-US-00002 Abbreviations AEM N-(2-Aminoethyl)maleimide trifluoroacetate salt AMPD 2-Amino-2-methyl-1,3-propanediol BOP (Benzotriazol-1-yloxy)tris(dimethylamino)phosphonium hexafluorophosphate DIPEA N,N-diisopropylethylamine DMF N,N-dimethylformamide EDCI.HCl 3-((Ethylimino)methyleneamino)-N,N-dimethylpropan-1-aminium chloride EMCH.TFA N-(ε-maleimidocaproic acid) hydrazide, trifluoroacetic acid salt HATU 1-[Bis(dimethylamino)methylene]-1H-1,2,3-triazolo[4,5-b]pyridinium 3-oxid hexafluorophosphate min minutes NMM 4-Methylmorpholine r.t. retention time TCEP tris(2-carboxyethyl)phosphine hydrochloride Temp temperature TFA trifluoroacetic acid

    Analytical Methods

    LC-MS Method 1

    [0331] Apparatus: Waters IClass; Bin. Pump: UPIBSM, SM: UPISMFTN with SO; UPCMA, PDA: UPPDATC, 210-320 nm, SQD: ACQ-SQD2 ESI, mass ranges depending on the molecular weight of the product: neg or neg/pos within in a range of 1500-2400 or 2000-3000; ELSD: gaspressure 40 psi, drift tube temp: 50° C.; column: Acquity C18, 50×2.1 mm, 1.7 .Math.m Temp: 60ºC, Flow: 0.6 mL/min, lin. Gradient depending on the polarity of the product: [0332] .sup.At.sub.0 = 2% A, t.sub.5.0 min = 50% A, t.sub.6.0 min = 98% A [0333] .sup.Bt.sub.0 = 2% A, t.sub.5.0 min = 98% A, t.sub.6.0 min = 98% A [0334] Posttime: 1.0 min, Eluent A: acetonitrile, Eluent B: 10 mM ammonium bicarbonate in water (pH=9.5).

    LC-MS Method 2

    [0335] Apparatus: Waters IClass; Bin. Pump: UPIBSM, SM: UPISMFTN with SO; UPCMA, PDA: UPPDATC, 210-320 nm, SQD: ACQ-SQD2 ESI, mass ranges depending on the molecular weight of the product: pos/neg 100-800 or neg 2000-3000; ELSD: gaspressure 40 psi, drift tube temp: 50° C.; column: Waters XSelect™ CSH C18, 50×2.1 mm, 2.5 .Math.m, Temp: 25° C., Flow: 0.5 mL/min, Gradient: t.sub.0min = 5% A, t.sub.2.0 min = 98% A, t.sub.2.7 min = 98% A, Posttime: 0.3 min, Eluent A: acetonitrile, Eluent B: 10 mM ammonium bicarbonate in water (pH=9.5).

    LC-MS Method 3

    [0336] Apparatus: Waters IClass; Bin. Pump: UPIBSM, SM: UPISMFTN with SO; UPCMA, PDA: UPPDATC, 210-320 nm, SQD: ACQ-SQD2 ESI, mass ranges depending on the molecular weight of the product pos/neg 105-800, 500-1200 or 1500-2500; ELSD: gaspressure 40 psi, drift tube temp: 50° C.; column: Waters XSelect™ CSH C18, 50×2.1 mm, 2.5 .Math.m, Temp: 40° C., Flow: 0.5 mL/min, Gradient: t.sub.0min = 5% A, t.sub.2.0 min = 98% A, t.sub.2.7 min = 98% A, Posttime: 0.3 min, Eluent A: 0.1% formic acid in acetonitrile, Eluent B: 0.1% formic acid in water.

    LC-MS Method 4

    [0337] Apparatus: Waters IClass; Bin. Pump: UPIBSM, SM: UPISMFTN with SO; UPCMA, PDA: UPPDATC, 210-320 nm, SQD: ACQ-SQD2 ESI, mass ranges depending on the molecular weight of the product: pos/neg 100-800 or neg 2000-3000; ELSD: gaspressure 40 psi, drift tube temp: 50° C. column: Waters Acquity Shield RP18, 50×2.1 mm, 1.7 .Math.m, Temp: 25° C., Flow: 0.5 mL/min, Gradient: t.sub.0min = 5% A, t.sub.2.0 min = 98% A, t.sub.2.7 min = 98% A, Posttime: 0.3 min, Eluent A: acetonitrile, Eluent B: 10 mM ammonium bicarbonate in water (pH=9.5).

    Preparative Methods

    Preparative MP-LC Method 1

    [0338] Instrument type: Reveleris™ prep MPLC; column: Waters XSelect™ CSH C18 (145×25 mm, 10 .Math.m); Flow: 40 mL/min; Column temp: room temperature; Eluent A: 10 mM ammoniumbicarbonate in water pH = 9.0); Eluent B: 99% acetonitrile + 1% 10 mM ammoniumbicarbonate in water; Gradient: [0339] .sup.At.sub.0min = 5% B, t.sub.1min = 5% B, t.sub.2min = 10% B, t.sub.17min = 50% B, t.sub.18min = 100% B, t.sub.23min = 100% B [0340] .sup.At.sub.0min = 5% B, t.sub.1min = 5% B, t.sub.2min = 20% B, t.sub.17min = 60% B, t.sub.18min = 100% B, t.sub.23min = 100% B [0341] ; Detection UV: 210, 235, 254 nm and ELSD.

    Preparative MP-LC Method 2

    [0342] Instrument type: Reveleris™ prep MPLC; Column: Phenomenex LUNA C18(3) (150×25 mm, 10 .Math.m); Flow: 40 mL/min; Column temp: room temperature; Eluent A: 0.1% (v/v) Formic acid in water, Eluent B: 0.1% (v/v) Formic acid in acetonitrile; Gradient: [0343] .sup.At.sub.0min = 5% B, t.sub.1min = 5% B, t.sub.2min = 20% B, t.sub.17min = 60% B, t.sub.18min = 100% B, t.sub.23min = 100% B [0344] .sup.Bt.sub.0min = 2% B, t.sub.1min = 2% B, t.sub.2min = 2% B, t.sub.17min = 30% B, t.sub.18min = 100% B, t.sub.23min = 100% B [0345] .sup.Ct.sub.0min = 5% B, t.sub.1min = 5% B, t.sub.2min = 10% B, t.sub.17min = 50% B, t.sub.18min = 100% B, t.sub.23min = 100% B [0346] .sup.Dt.sub.0min = 5% B, t.sub.1min = 5% B, t.sub.2min = 5% B, t.sub.17min = 40% B, t.sub.18min = 100% B, t.sub.23min = 100% B [0347] ; Detection UV : 210, 235, 254 nm and ELSD.

    Preparative LC-MS Method 3

    [0348] MS instrument type: Agilent Technologies G6130B Quadrupole; HPLC instrument type: Agilent Technologies 1290 preparative LC; Column: Waters XSelect™ CSH (C18, 150×19 mm, 10 .Math.m); Flow: 25 ml/min; Column temp: room temperature; Eluent A: 100% acetonitrile; Eluent B: 10 mM ammonium bicarbonate in water pH = 9.0; Gradient: [0349] .sup.At.sub.0 = 20% A, t.sub.2.5 min = 20% A, t.sub.11min = 60% A, t.sub.13min = 100% A, t.sub.17min = 100% A [0350] .sup.Bt.sub.0 = 5% A, t.sub.2.5 min = 5% A, t.sub.11min = 40% A, t.sub.13min = 100% A, t.sub.17min = 100% A [0351] ; Detection: DAD (210 nm); Detection: MSD (ESI pos/neg) mass range: 100 - 800; Fraction collection based on DAD.

    Preparative LC-MS Method 4

    [0352] MS instrument type: Agilent Technologies G6130B Quadrupole; HPLC instrument type: Agilent Technologies 1290 preparative LC; Column: Waters XBridge Protein (C4, 150×19 mm, 10 .Math.m); Flow: 25 ml/min; Column temp: room temperature; Eluent A: 100% acetonitrile; Eluent B: 10 mM ammonium bicarbonate in water pH=9.0; Gradient: [0353] .sup.At.sub.0 = 2% A, t.sub.2.5 min = 2% A, t.sub.11 min = 30% A, t.sub.13 min = 100% A, t.sub.17 min = 100% A [0354] .sup.Bt.sub.0 = 10% A, t.sub.2.5 min = 10% A, t.sub.11 min = 50% A, t.sub.13 min = 100% A, t.sub.17 min = 100% A [0355] .sup.Ct.sub.0 = 5% A, t.sub.2.5 min = 5% A, t.sub.11 min = 40% A, t.sub.13 min = 100% A, t.sub.17 min = 100% A [0356] ; Detection: DAD (210 nm); Detection: MSD (ESI pos/neg) mass range: 100 - 800; Fraction collection based on DAD

    Flash Chromatography

    [0357] Grace Reveleris X2® C-815 Flash; Solvent delivery system: 3-piston pump with auto-priming, 4 independent channels with up to 4 solvents in a single run, auto-switches lines when solvent depletes; maximum pump flow rate 250 mL/min; maximum pressure 50 bar (725 psi); Detection: UV 200-400 nm, combination of up to 4 UV signals and scan of entire UV range, ELSD; Column sizes: 4-330 g on instrument, luer type, 750 g up to 3000 g with optional holder.

    SO1861-EMCH Synthesis (SO1861-EMCH is Also Referred to as SO1861-Ald-EMCH)

    [0358] To SO1861 (121 mg, 0.065 mmol) and EMCH.TFA (110 mg, 0.325 mmol) was added methanol (extra dry, 3.00 mL) and TFA (0.020 mL, 0.260 mmol). The reaction mixture stirred at room temperature. After 1.5 hours the reaction mixture was subjected to preparative MP-LC. Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (120 mg, 90%) as a white fluffy solid. Purity based on LC-MS 96%. [0359] LRMS (m/z): 2069 [M-1].sup.1- [0360] LC-MS r.t. (min): 1.08.sup.4

    S01861-EMCH-Mercaptoethanol (SO1861-EMCH (Blocked))

    [0361] To SO1861-EMCH (0.1 mg, 48 nmol) 200 .Math.L mercaptoethanol (18 mg, 230 .Math.mol) was added and the solution was shaken for 1 h at 800 rpm and room temperature on a ThermoMixer C (Eppendorf). After shaking for 1 h, the solution was diluted with methanol and dialyzed extensively for 4 h against methanol using regenerated cellulose membrane tubes (Spectra/Por 7) with a MWCO of 1 kDa. After dialysis, an aliquot was taken out and analyzed via MALDI-TOF-MS.

    [0362] MALDI-TOF-MS (RP mode): m/z 2193 Da ([M+K].sup.+, SO1861-EMCH-mercaptoethanol), m/z 2185 Da ([M+K].sup.+, SO1861-EMCH-mercaptoethanol), m/z 2170 Da ([M+Na].sup.+, SO1861-EMCH-mercaptoethanol).

    Trivalent GalNAc-Azide Synthesis

    Intermediate 1:

    Tert-Butyl 1-Azido-17,17-bis((3-(Tert-Butoxy)-3-Oxopropoxy)Methyl)-15-Oxo-3,6,9,12,19-Pentaoxa-16-Azadocosan-22-Oate

    [0363] To di-tert-butyl 3,3′-((2-amino-2-((3-(tert-butoxy)-3-oxopropoxy)methyl)propane-1,3-diyl)bis(oxy))dipropionate (1.27 g, 2.51 mmol) was added a solution of 3-Azido(peg4)propionic acid N-hydroxysuccinimide ester (977 mg, 2.51 mmol) in DMF (10 mL). Next, DIPEA (657 .Math.L, 3.77 mmol) was added and the reaction mixture was stirred overnight at room temperature. The reaction mixture was evaporated in vacuo and the residue was dissolved in ethyl acetate (100 mL). The resulting solution was washed with 0.5 N potassium bisulphate solution (2 × 100 mL) and brine (100 mL), dried over Na.sub.2SO.sub.4, filtered and evaporated in vacuo. The residue was purified by flash chromatography (DCM -10% methanol in DCM (v/v) gradient 100:0 rising to 0:100) to give the title compound (1.27 g, 65%) as a colorless oil. Purity based on LC-MS 100% (ELSD). [0364] LRMS (m/z): 780 [M+1].sup.1+ [0365] LC-MS r.t. (min): 2.10.sup.2

    Intermediate 2:

    1-Azido-17,17-bis((2-Carboxyethoxy)Methyl)-15-Oxo-3,6,9,12,19-Pentaoxa-16-Azadocosan-22-oic acid

    [0366] To a solution of tert-butyl 1-azido-17,17-bis((3-(tert-butoxy)-3-oxopropoxy)methyl)-15-oxo-3,6,9,12,19-pentaoxa-16-azadocosan-22-oate (1.27 g, 1.63 mmol) in DCM (5.0 mL) was added TFA (5.0 mL, 65 mmol). The reaction mixture was stirred at room temperature. After 1.5 hours the reaction mixture was evaporated in vacuo, co-evaporated with toluene (3 × 10 mL) and DCM (3 × 10 mL) to give the crude title product as a colorless oil.

    [0367] LRMS (m/z): 611 [M+1].sup.1+

    Intermediate 3:

    Di-tert-butyl (10-(1-azido-3,6,9,12-Tetraoxapentadecan-15-Amido)-10-(13,13-Dimethyl-5,11-dioxo-2,12-Dioxa-6,10-Diazatetradecyl)-5,15-Dioxo-8,12-Dioxa-4,16-Diazanonadecane-1,19-diyl)Dicarbamate

    [0368] 1-azido-17,17-bis((2-carboxyethoxy)methyl)-15-oxo-3,6,9,12,19-pentaoxa-16-azadocosan-22-oic acid (997 mg, 1.63 mmol), Oxyma Pure (1.04 g, 7.35 mmol) and EDCl.HCl (1.17 g, 6.12 mmol) were dissolved in DMF (10.0 mL). Next, DIPEA (1.99 mL, 11.4 mmol) was added, followed directly by the addition of a solution of N-BOC-1,3-propanediamine (1.07 g, 6.12 mmol) in DMF (10.0 mL). The reaction mixture was stirred overnight at room temperature. The reaction mixture was evaporated in vacuo and the residue was dissolved in ethyl acetate (100 mL). The resulting solution was washed with 0.5 N potassium bisulphate solution (100 mL), saturated sodium bicarbonate solution (2 × 100 mL) and brine (100 mL), dried over Na.sub.2SO.sub.4, filtered and evaporated in vacuo. The residue was purified by flash chromatography (DCM - 10% methanol in DCM (v/v) gradient 0:100 rising to 100:0, staying at 100:0 until the product eluted) to give the title compound (1.16 g, 66%) as a yellowish viscous oil. LC-MS 99% (ELSD). [0369] LRMS (m/z): 1080 [M+1].sup.1+ [0370] LC-MS r.t. (min): 1.51.sup.3

    Intermediate 4:

    3,3′-(((3-((3-Aminopropyl)Amino)-3-Oxopropoxy)Methyl)-2-(1-Azido-3,6,9,12-Tetraoxapentadecan-15-Amido)Propane-1,3-diyl)bis(oxy))bis(N-(3-Aminopropyl)Propanamide) tris(2,2,2-Trifluoroacetate) Synthesis

    [0371] To a solution of di-tert-butyl (10-(1-azido-3,6,9,12-tetraoxapentadecan-15-amido)-10-(13,13-dimethyl-5,11-dioxo-2,12-dioxa-6,10-diazatetradecyl)-5,15-dioxo-8,12-dioxa-4,16-diazanonadecane-1,19-diyl)dicarbamate (1.16 g, 1.08 mmol) in DCM (10 mL) was added TFA (10 mL, 131 mmol). The reaction mixture was stirred at room temperature. After 2 hours the reaction mixture was evaporated in vacuo, co-evaporated with toluene (3 × 10 mL) and DCM (3 × 10 mL) to give the crude title product as a yellowish viscous oil.

    [0372] LRMS (m/z): 260 [M+3].sup.3+, 390 [M+2].sup.2+, 780 [M+1].sup.1+,

    Intermediate 5:

    (2R,3R,4R,5R,6R)-5-Acetamido-2-(Acetoxymethyl)-6-((5-((2,5-Dioxopyrrolidin-1-yl)Oxy)-5-Oxopentyl)Oxy)Tetrahydro-2H-Pyran-3,4-diyl Diacetate

    [0373] 5-(((2R,3R,4R,5R,6R)-3-acetamido-4,5-diacetoxy-6-(acetoxymethyl)tetrahydro-2H-pyran-2-yl)oxy)pentanoic acid (obtain according J. Am. Chem Soc., 2014, 136, 16958-16961, 3.00 g, 6.70 mmol) and N-Hydroxysuccinimide (926 mg, 8.05 mmol) were dissolved in DCM (50 mL). Next, EDCl.HCl (1.54 g, 8.05 mmol) and 4-(Dimethylamino)pyridine (82 mg, 0.67 mmol) were added and the reaction mixture was stirred overnight at room temperature. The reaction mixture was diluted with DCM and the resulting solution was washed with 0.5 N potassium bisulphate solution (150 mL), saturated sodium bicarbonate solution (150 mL) and brine (150 mL), dried over Na.sub.2SO.sub.4, filtered and evaporated in vacuo to give the title compound (3.60 g, 99%) as a white foam. Purity based on LC-MS 99% (ELSD). [0374] LRMS (m/z): 545 [M+1].sup.1+ [0375] LC-MS r.t. (min): 1.07.sup.3

    Intermediate 6:

    [(3R,6R)-3,4-bis(Acetyloxy)-6-{4-[(3-{3-[2-(1-Azido-3,6,9,12-Tetraoxapentadecan-15-Amido)-3-(2-{[3-(5-{[(2R,5R)-4,5-bis(Acetyloxy)-6-[(Acetyloxy)methyl]-3-Acetamidooxan-2-yl]oxy}Pentanamido)Propyl]Carbamoyl]ethoxy)-2-[(2-{[3-(5-{[(2R,5R)-4,5-bis(Acetyloxy)-6-[(Acetyloxy)Methyl]-3-Acetamidooxan-2-yl]oxy}Pentanamido)Propyl]Carbamoyl}Ethoxy)Methyl]Propoxy]Propanamido}Propyl)Carbamoyl ]Butoxy}-5-Acetamidooxan-2-yl]Methyl Acetate

    [0376] 3,3′-(((3-((3-aminopropyl)amino)-3-oxopropoxy)methyl)-2-(1-azido-3,6,9,12-tetraoxapentadecan-15-amido)propane-1,3-diyl)bis(oxy))bis(N-(3-aminopropyl)propanamide) tris(2,2,2-trifluoroacetate) (1.21 g, 1.08 mmol) was dissolved in a mixture of DMF (10 mL) and DIPEA (1.69 mL, 9.70 mmol). Next, (2R,3R,4R,5R,6R)-5-acetamido-2-(acetoxymethyl)-6-((5-((2,5-dioxopyrrolidin-1-yl)oxy)-5-oxopentyl)oxy)tetrahydro-2H-pyran-3,4-diyl diacetate (2.20 g, 4.04 mmol) was added and the reaction mixture was stirred over the weekend at room temperature. Next, the reaction mixture was evaporated in vacuo and the residue was purified by flash chromatography (DCM - 30% methanol in DCM (v/v) gradient 0:100 rising to 100:0) to give the title compound (1.84 g, 83%) as a yellowish foam. LC-MS 95% (ELSD). [0377] LRMS (m/z): 2068 [M+1].sup.1+ [0378] LC-MS r.t. (min): 1.18.sup.3

    Intermediate 7:

    Trivalent GalNAc-Azide

    [0379] [(3R,6R)-3,4-bis(acetyloxy)-6-{4-[(3-{3-[2-(1-azido-3,6,9,12-tetraoxapentadecan-15-amido)-3-(2-{[3-(5-{[(2R,5R)-4,5-bis(acetyloxy)-6-[(acetyloxy)methyl]-3-acetamidooxan-2-yl]oxy}pentanamido)propyl]carbamoyl}ethoxy)-2-[(2-{[3-(5-{[(2R,5R)-4,5-bis(acetyloxy)-6-[(acetyloxy)methyl]-3-acetamidooxan-2-yl]oxy}pentanamido)propyl]carbamoyl}ethoxy)methyl]propoxy]propanamido}propyl)carbamoyl]butoxy}-5-acetamidooxan-2-yl]methyl acetate (300 mg, 0.145 mmol) was dissolved in a mixture of triethylamine (2.00 mL, 14.4 mmol), methanol (2.00 mL) and water (2.00 mL) and the reaction mixture was stirred at room temperature. After 2 hours the reaction mixture was evaporated in vacuo. The residue was purified by preparative MP-LC..sup.2B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (164 mg, 67%) as a white solid. Purity based on LC-MS 97%. [0380] LRMS (m/z): 1688 [M-1].sup.1- [0381] LC-MS r.t. (min): 1.99.sup.1A

    Trivalent-GalNAc-SO1861 and GalNAc-SO1861 Synthesis (FIGS. 2, 4)

    Intermediate 8:

    SO1861-NH.SUB.2

    [0382] SO1861-azide (6.89 mg, 3.20 .Math.mol) was dissolved in mixture of 32 mM potassium carbonate (150 .Math.L, 4.80 .Math.mol) and acetonitrile (150 .Math.L). Directly afterwards, a 1.0 M trimethylphosphine solution in THF (32 .Math.L, 32 .Math.mol) was added and the resulting mixture was shaken for 1 min and left standing at room temperature. After 30 min. the reaction mixture was subjected to preparative MP-LC. Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (5.30 mg, 78%) as a white fluffy solid. Purity based on LC-MS 94%. [0383] LRMS (m/z): 1062 [M-2].sup.2- [0384] LC-MS r.t. (min): 2.51.sup.1B

    Intermediate 9:

    SO1861-DBCO

    [0385] To SO1861-amine (48.6 mg, 22.9 .Math.mol) and DBCO-NHS (13.0 mg, 32.4 .Math.mol) was added to a solution of DIPEA (5.98 .Math.L, 34.3 .Math.mol) and DMF (2.0 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 4 hours the reaction mixture was diluted with a solution of 50 mM sodium bicarbonate (1.00 mL, 50 .Math.mol). The resulting mixture was shaken for 1 min and left standing at room temperature. After 30 min the reaction mixture was subjected to preparative MP-LC..sup.1B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (16.9 mg, 31%) as a white fluffy solid. Purity based on LC-MS 94%. [0386] LRMS (m/z): 2412 [M-1].sup.1- [0387] LC-MS r.t. (min): 2.45.sup.1B

    SO1861-L-Trivalent GalNAc Synthesis

    [0388] SO1861-DBCO (7.50 mg, 3.11 .Math.mol) and trivalent GalNAc-azide (5.31 mg, 3.14 .Math.mol) were dissolved in a mixture of water/acetonitrile (2:1, v/v, 0.90 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative LC-MS..sup.3B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (9.60 mg, 75%) as a white fluffy solid. Purity based on LC-MS 99%. [0389] LRMS (m/z): 2050 [M-2].sup.2- [0390] LC-MS r.t. (min): 2.04.sup.1B

    SO1861-L-GalNAc Synthesis

    [0391] SO1861-DBCO (1.75 mg, 0.73 .Math.mol) and GalNAc-PEG3-azide (0.82 mg, 2.18 .Math.mol) were dissolved in a mixture of water/acetonitrile (1:1, v/v, 1.00 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative LC-MS..sup.3B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (1.63 mg, 81%) as a white fluffy solid. Purity based on LC-MS 100%. [0392] LRMS (m/z): 2790 [M-1].sup.1- [0393] LC-MS r.t. (min): 2.15.sup.1B

    Trivalent GalNAc-BNA Oligo Synthesis (FIGS. 6, 7)

    Intermediate 10:

    4-{2-aZatricyclo[10.4.0.0.SUP.4,9.]Hexadeca-1(12),4(9),5,7,13,15-Hexaen-10-yn-2-yl}-N-[2-(2-{2-[2-({4-[(E)-{[6-(2,5-Dioxo-2,5-Dihydro-1H-Pyrrol-1-yl)Hexanamido]Imino}Methyl]Phenyl}Formamido)Ethoxy]Ethoxy}Ethoxy)etHyl]-4-Oxobutanamide

    [0394] 4-{2-azatricyclo[10.4.0.0.sup.4,9]hexadeca-1(12),4(9),5,7,13,15-hexaen-10-yn-2-yl}-N-{2-[2-(2-{2-[(4-formylphenyl)formamido]ethoxy}ethoxy)ethoxy]ethyl}-4-oxobutanamide (25.0 mg, 40.9 .Math.mol) and EMCH.TFA (20.8 mg, 61.3 .Math.mol) were dissolved in methanol (extra dry, 2.00 mL). Next, TFA (9.39 .Math.L, 123 .Math.mol) was added. The reaction mixture was shaken for 1 min and left standing overnight at room. The reaction mixture was subjected to preparative MP-LC..sup.1B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (16.2 mg, 48%) as a white solid. Purity based on LC-MS 91%. [0395] LRMS (m/z): 410.2 [M+2].sup.2+ [0396] LC-MS r.t. (min): 1.41.sup.2

    Intermediate 11:

    Trivalent GalNAc-L-Maleimide

    [0397] Trivalent GalNAc-azide (20.3 mg, 12.0 .Math.mol) and 4-{2-azatricyclo[10.4.0.0.sup.4,9]hexadeca-1(12),4(9),5,7,13,15-hexaen-10-yn-2-yl}-N-[2-(2-{2-[2-({4-[(E)-{[6-(2,5-dioxo-2,5-dihydro-1H-pyrrol-1-yl)hexanamido]imino}methyl]phenyl}formamido)ethoxy]ethoxy}ethoxy)ethyl]-4-oxobutanamide (11.8 mg, 14.4 .Math.mol) were dissolved in a mixture of water/acetonitrile (2:1, v/v, 0.90 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative MP-LC..sup.2C Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (25.6 mg, 85%) as a white solid. Purity based on LC-MS 88%. [0398] LRMS (m/z): 2101 [M-405].sup.1-, 2304 [M-202].sup.1-, 2507 [M-1].sup.1- [0399] LC-MS r.t. (min): 1.90.sup.1B (double peaks due to isomers)

    Intermediate 12:

    Trivalent GalNAc-S-Maleimide

    [0400] Trivalent GalNAc-azide (20.3 mg, 12.0 .Math.mol) and DBCO-maleimide (10.3 mg, 24.0 .Math.mol) were dissolved in a mixture of water/acetonitrile (2:1, v/v, 0.90 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative MP-LC..sup.2D Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (22.2 mg, 87%) as a white solid. Purity based on LC-MS 85%. Contains 10% of the hydrolysed maleimide. [0401] LRMS (m/z): 2115 [M-1].sup.1- [0402] LC-MS r.t. (min): 1.60.sup.1B (double peaks due to isomers)

    Trivalent GalNAc-S-AzpoB (or HSP27) BNA Oligo Synthesis

    [0403] To ApoB BNA oligo disulfide (5.00 mg, 0.686 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (1.00 mL, 2.5 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 2 × 0.50 mL). Next, the residue solution was washed twice with a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (0.50 mL), each time filtered under the same conditions described above. As next, the residue solution was diluted with 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL) and the resulting solution was directly added to trivalent GalNAc-S-maleimide (3.02 mg, 1.43 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1.5 hours the reaction mixture was subjected to preparative LC-MS..sup.4A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (6.75 mg, quant.) as a white fluffy solid. Purity based on LC-MS 94% (very broad peak). [0404] LRMS (m/z): 2318 [M-4].sup.4- [0405] LC-MS r.t. (min): 1.65.sup.1A

    Trivalent GalNAc-S-ApoB (or HSP27) Scrambled BNA Oligo Synthesis

    [0406] To ApoB scrambled BNA oligo disulfide (5.00 mg, 0.688 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (1.00 mL, 2.5 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 2 × 0.50 mL ). Next, the residue solution was washed twice with a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (0.50 mL), each time filtered under the same conditions described above. As next, the residue solution was diluted with 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL) and the resulting solution was directly added to trivalent GalNAc-S-maleimide (3.09 mg, 1.46 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1.5 hours the reaction mixture was subjected to preparative LC-MS..sup.4A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (5.91 mg, 93%) as a white fluffy solid. Purity based on LC-MS 88% (very broad peak). [0407] LRMS (m/z): 2311 [M-4].sup.4- [0408] LC-MS r.t. (min): 1.60.sup.1A

    Trivalent GalNAc-L-ApoB (or HSP27) BNA Oligo Synthesis

    [0409] To ApoB BNA oligo disulfide (5.00 mg, 0.686 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (1.00 mL, 2.5 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 2 × 0.50 mL). Next, the residue solution was washed twice with a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (0.50 mL), each time filtered under the same conditions described above. As next, the residue solution was diluted with 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL) and the resulting solution was directly added to trivalent GalNAc-L-maleimide (3.63 mg, 1.45 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1.5 hours the reaction mixture was subjected to preparative LC-MS..sup.4A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (6.68 mg, quant.) as a white fluffy solid. Purity based on LC-MS 99% (very broad peak). [0410] LRMS (m/z): 2416 [M-4].sup.4- [0411] LC-MS r.t. (min): 1.97.sup.1A

    Trivalent GalNAc-L-ApoB (or HSP27) Scrambled BNA Oligo Synthesis

    [0412] To ApoB scrambled BNA oligo disulfide (5.00 mg, 0.688 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (1.00 mL, 2.5 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 2 × 0.50 mL). Next, the residue solution was washed twice with a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (0.50 mL), each time filtered under the same conditions described above. As next, the residue solution was diluted with 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL) and the resulting solution was directly added to trivalent GalNAc-L-maleimide (3.68 mg, 1.47 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1.5 hours the reaction mixture was subjected to preparative LC-MS..sup.4A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (4.71 mg, 71%) as a white fluffy solid. Purity based on LC-MS 96% (very broad peak). [0413] LRMS (m/z): 2409 [M-4].sup.4- [0414] LC-MS r.t. (min): 1.93.sup.1A

    Dendron(-L-SO1861).SUB.4.-Trivalent GalNAc and Dendron(-L-SO1861).SUB.8.-Trivalent GalNAc Synthesis

    Intermediate 13:

    Trivalent GalNAc-Amine Formate

    [0415] Trivalent GalNAc-azide (36.5 mg, 21.6 .Math.mol) was dissolved in a solution of potassium carbonate (5.97 mg, 43.2 .Math.mol) in water (1.00 mL) and acetonitrile (1.00 mL). Next, a 1.0 M trimethylphosphine solution in THF (216 .Math.L, 216 .Math.mol) was added and the resulting mixture was shaken for 1 min and left standing at room temperature. After 45 min the reaction mixture was evaporated in vacuo and the residue was dissolved in water/acetonitrile (9:1, v/v, 1 mL). The resulting solution was directly subjected to preparative MP-LC..sup.2B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (36.1 mg, 98%) as a white solid. Purity based on LC-MS 100%. [0416] LRMS (m/z): 1662 [M-1].sup.1- [0417] LC-MS r.t. (min): 1.62.sup.1A

    Intermediate 14:

    Trivalent GalNAc-DBCO

    [0418] Trivalent GalNAc-amine formate (17.4 mg, 10.2 .Math.mol) and DBCO-NHS (6.14 mg, 15.3 .Math.mol) were dissolved in a solution of NMM (2.24 .Math.L, 20.3 .Math.mol) in DMF (0.50 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was evaporated in vacuo and the residue was dissolved in water/acetonitrile (8:2, v/v, 1 mL). The resulting solution was directly subjected to preparative MP-LC..sup.2C Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (14.2 mg, 72%) as a white solid. Purity based on LC-MS 96%. [0419] LRMS (m/z): 1950 [M-1].sup.1 [0420] LC-MS r.t. (min): 1.86.sup.1B

    Intermediate 15:

    Dendron(-L-SO1861).SUB.8.-Azide

    [0421] Dendron(-L-SO1861).sub.8-amine (19.6 mg, 1.08 .Math.mol) and 2,5-dioxopyrrolidin-1-yl 1-azido-3,6,9,12-tetraoxapentadecan-15-oate (4.17 mg, 10.8 .Math.mol) were dissolved in DMF (1.50 mL). Next, DIPEA (1.87 .Math.L, 10.8 .Math.mol) was added and the mixture was shaken for 1 min and left standing overnight at room temperature. The reaction mixture was subjected to preparative LC-MS..sup.4B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (11.7 mg, 59%) as a white fluffy solid. Purity based on LC-MS 92% (very broad peak). [0422] LRMS (m/z): 2316 [M-8].sup.8-,): 2647 [M-7].sup.7- [0423] LC-MS r.t. (min): 4.29.sup.1A

    Dendron(-L-SO1861).SUB.4.-Trivalent GalNAc Synthesis

    [0424] Dendron(-L-SO1861).sub.4-azide (2.50 mg, 0.266 .Math.mol) and trivalent GalNAc-DBCO (1.56 mg, 0.799 .Math.mol) were dissolved in a mixture of water/acetonitrile (3:1, v/v, 1.00 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative LC-MS..sup.4B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (2.74 mg, 91%) as a white fluffy solid. Purity based on LC-MS 86% (very broad peak). [0425] LRMS (m/z): 2832 [M-4].sup.4- [0426] LC-MS r.t. (min): 4.07.sup.1A

    Dendron(-L-SO1861).SUB.8.-Trivalent GalNAc Synthesis

    [0427] Dendron(-L-SO1861).sub.8-azide (2.50 mg, 0.135 .Math.mol) and trivalent GalNAc-DBCO (0.79 mg, 0.405 .Math.mol) were dissolved in a mixture of water/acetonitrile (3:1, v/v, 1.00 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative LC-MS..sup.4B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (2.03 mg, 74%) as a white fluffy solid. Purity based on LC-MS 100% (very broad peak). [0428] LRMS (m/z): 2559 [M-8].sup.8-, 2925 [M-7].sup.7- [0429] LC-MS r.t. (min): 4.18.sup.1A

    Intermediate 16:

    Trivalent GalNAc-Thioacetate

    [0430] Trivalent GalNAc-amine formate (18.7 mg, 11.0 .Math.mol) and 4-nitrophenyl 3-(acetylthio)propanoate (5.90 mg, 21.9 .Math.mol) were dissolved in a solution of NMM (2.41 .Math.L, 21.9 .Math.mol) in DMF (0.50 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was evaporated in vacuo and the residue was dissolved in a mixture of 0.1% formic acid in water and 0.1% formic acid in acetonitrile (9:1, v/v, 1 mL). The resulting solution was directly subjected to preparative MP-LC..sup.2B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (13.0 mg, 66%) as a white solid. Purity based on LC-MS 100%. [0431] LRMS (m/z): 1749 [M-43].sup.1-, 1792 [M-1].sup.1 [0432] LC-MS r.t. (min): 1.24.sup.1B

    Intermediate 17:

    DBCO-TCO-Trivalent GalNAc

    [0433] Trivalent GalNAc-thioacetate (13.0 mg, 7.25 .Math.mol) was dissolved in methanol (0.50 mL). Next, a 1 M solution of sodium hydroxide (7.98 .Math.L, 7.98 .Math.mol) was added. The reaction mixture was shaken for 1 min and left standing at room temperature. After 30 min the reaction mixture was added to a freshly prepared solution of trifunctional linker (Ls-t) (i.e., is an example of a saponin moiety linker Ls) (7.39 mg, 6.13 .Math.mol) in 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 2.00 mL).

    [0434] The trifunctional linker has the IUPAC name: 5,8,11,18,21,24,27-Heptaoxa-2,14,30-triazatritriacontanoic acid, 14-[16-(11,12-didehydrodibenz[b,f]azocin-5(6H)-yl)-13,16-dioxo-3,6,9-trioxa-12-azahexadec-1-yl]-33-(2,5-dihydro-2,5-dioxo-1H-pyrrol-1-yl)-15,31-dioxo-, (1R,4E)-4-cycloocten-1-yl ester. The trifunctional linker has the following formula (XVII):

    ##STR00022##

    [0435] The resulting mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative MP-LC..sup.2A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (3.83 mg, 21%) as a white solid. Purity based on LC-MS 89%. [0436] LRMS (m/z): 2409 [M-546].sup.1-, 2955 [M-1].sup.1- [0437] LC-MS r.t. (min): 2.66.sup.1B

    Intermediate 18:

    Methyltetrazine-L-ApoB BNA Oligo

    [0438] To ApoB BNA oligo disulfide (5.00 mg, 0.686 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (1.00 mL, 2.5 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 2 × 0.50 mL). Next, the residue solution was washed twice with a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (0.50 mL), each time filtered under the same conditions described above. As next, the residue solution was diluted with 20 mM ammonium bicarbonate (1.50 mL) and the resulting mixture was directly added to a solution of (E)-1-(4-((2-(6-(2,5-dioxo-2,5-dihydro-1H-pyrrol-1-yl)hexanoyl)hydrazineylidene)methyl)benzamido)-N-(4-(6-methyl-1,2,4,5-tetrazin-3-yl)benzyl)-3,6,9,12-tetraoxapentadecan-15-amide

    [0439] (1.36 mg, 1.73 .Math.mol) in acetonitrile (0.5 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 30 min the reaction mixture was frozen and lyophilized overnight to yield the crude title product as a pink fluffy solid. To the crude product was added a solution of 20 mM ammonium bicarbonate (1.50 mL) and the resulting suspension was filtered over a 0.45 .Math.m syringe filter. The filtrate was lyophilized overnight to yield the title product (5.44 mg, quant) as a pink fluffy solid. Purity based on LC-MS 90% (very broad peak). [0440] LRMS (m/z): 2648 [M-3].sup.3- [0441] LC-MS r.t. (min): 0.62.sup.4

    Intermediate 19:

    Methyltetrazine-L-ApoB Scrambled BNA Oligo

    [0442] To ApoB scrambled BNA oligo disulfide (5.00 mg, 0.688 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (1.00 mL, 2.5 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 2 × 0.50 mL). Next, the residue solution was washed twice with a solution of 20 mM ammonium bicarbonate with 2.5 mM TCEP (0.50 mL), each time filtered under the same conditions described above. As next, the residue solution was diluted with 20 mM ammonium bicarbonate (1.50 mL) and the resulting mixture was directly added to a solution of (E)-1-(4-((2-(6-(2,5-dioxo-2,5-dihydro-1H-pyrrol-1-yl)hexanoyl)hydrazineylidene)methyl)benzamido)-N-(4-(6-methyl-1,2,4,5-tetrazin-3-yl)benzyl)-3,6,9,12-tetraoxapentadecan-15-amide (1.34 mg, 1.70 .Math.mol) in acetonitrile (0.5 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 30 min the reaction mixture was frozen and lyophilized overnight to yield the crude title product as a pink fluffy solid. To the crude product was added a solution of 20 mM ammonium bicarbonate (1.50 mL) and the resulting suspension was filtered over a 0.45 .Math.m syringe filter. The filtrate was lyophilized overnight to yield the title product (5.48 mg, quant) as a pink fluffy solid. Purity based on LC-MS 84% (very broad peak). [0443] LRMS (m/z): 2639 [M-3].sup.3- [0444] LC-MS r.t. (min): 0.58.sup.4

    Intermediate 20:

    DBCO-L-ApoB BNA Oligo-Trivalent GalNAc

    [0445] To methyltetrazine-L-ApoB BNA oligo (5.44 mg, 0.684 .Math.mol) and DBCO-TCO-trivalent GalNAc (2.03 mg, 0.687 .Math.mol) was added 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative LC-MS..sup.4C Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (2.87 mg, 39%) as a white fluffy solid. LC-MS shows multiple broad peaks with the correct m/z values. [0446] LRMS (m/z): 2175 [M-5].sup.5-, 2718 [M-6].sup.4- [0447] LC-MS r.t. (min): 2.60-3.00.sup.1A

    Intermediate 21:

    DBCO-L-ApoB Scrambled BNA Oligo-Trivalent GalNAc

    [0448] To methyltetrazine-L-ApoB scrambled BNA oligo (5.48 mg, 0.692 .Math.mol) and DBCO-TCO-trivalent GalNAc (1.80 mg, 0.609 .Math.mol) was added 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was subjected to preparative LC-MS..sup.4C Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (2.15 mg, 33%) as a white fluffy solid. LC-MS shows multiple broad peaks with the correct m/z values. [0449] LRMS (m/z): 2169 [M-5].sup.5-, 2711 [M-6].sup.4- [0450] LC-MS r.t. (min): 2.58-3.20.sup.1A

    Intermediate 22 (FIG. 21)

    Trivalent GalNAc-Thiol

    [0451] Trivalent GalNAc-thioacetate (16.2 mg, 9.02 .Math.mol) was dissolved in methanol (500 .Math.L). Next, a 1.00 M solution of sodium hydroxide (11.0 .Math.L, 11.0 .Math.mol) was added. The reaction mixture was shaken for 1 min and left standing at room temperature. After 30 min the reaction mixture was submitted to preparative MP-LC..sup.1A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (13.1 mg, 83%) as a white solid. Purity based on LC-MS 98%. [0452] LRMS (m/z): 1748 [M-H].sup.1- [0453] LC-MS r.t. (min): 1.78.sup.1A

    Intermediate 23: (FIG. 21)

    DBCO-TCO-Trivalent GalNAc

    [0454] Trifunctional linker (Ls) (15.0 mg, 12.4 .Math.mol) was dissolved in acetonitrile (0.50 mL). Next, a solution of 20 mM ammonium bicarbonate (1.50 mL) was added and the resulting solution was directly transferred to trivalent GalNAc-thiol (22.7 mg, 13.0 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was frozen and lyophilized overnight to yield the crude title product as a white solid. Purity based on LC-MS 84%. [0455] LRMS (m/z): 2409 [M-546].sup.1-, 2955 [M-1].sup.1- [0456] LC-MS r.t. (min): 2.63.sup.1B

    Intermediate 25 (FIG. 22):

    Methyltetrazine-BNA Oligo

    [0457] To Thiol-13-ApoB BNA oligo disulfide (20 mg, 4.17 .Math.mol) was added a solution of 20 mM ammonium bicarbonate with 5.0 mM TCEP (2.00 mL, 10.0 .Math.mol). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was filtered by using a centrifugal filter with a molecular weight cut-off of 3000 Da (5000 × g for 30 min, 4× 0.50 mL). Next, the residue solution was diluted with 20 mM ammonium bicarbonate (3.00 mL) and the resulting mixture was directly added to a solution of (E)-1-(4-((2-(6-(2,5-dioxo-2,5-dihydro-1H-pyrrol-1-yl)hexanoyl)hydrazineylidene)methyl)benzamido)-N-(4-(6-methyl-1,2,4,5-tetrazin-3-yl)benzyl)-,6,9,12-tetraoxapentadecan-15-amide (7.22 mg, 9.16 .Math.mol) in acetonitrile (1.0 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 1 hour the reaction mixture was frozen and lyophilized overnight to yield the crude title product as a pink fluffy solid. To the crude product was added a 20 mM ammonium bicarbonate/acetonitrile (2:1, v/v, 2.00 mL) and the resulting solution was subjected to preparative LC-MS..sup.1A Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (20.3 mg, 89%) as a pink fluffy solid. Purity based on LC-MS 93% (broad peak). [0458] LRMS (m/z): 1817 [M-3].sup.3- [0459] LC-MS r.t. (min): 0.59.sup.3

    Intermediate 26 (FIG. 22):

    (Blocked DBCO)-TCO-Trivalent GalNAc

    [0460] A solution of 1-azido-3,6,9-trioxaundecane-11-ol (2.17 mg, 9.88 .Math.mol) in DMF (0.50 mL) was added to DBCO-TCO-trivalent GalNAc (14.6 mg, 4.94 .Math.mol. The reaction mixture was shaken for 1 min and left standing at room temperature. After 2 hours the reaction mixture was submitted to preparative MP-LC..sup.1C Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (10.00 mg, 64%) as a white solid. Purity based on LC-MS 98%. [0461] LRMS (m/z): 1750 [fragment] [0462] LC-MS r.t. (min): 2.33.sup.1B

    Ls-(Blocked DBCO)-BNA Oligo-Trivalent GalNAc (FIG. 23)

    [0463] (blocked DBCO)-TCO-trivalent GalNAc (10.0 mg, 3.15 .Math.mol) and Methyltetrazine-BNA oligo (10.0 mg, 1.83 .Math.mol) were dissolved in a solution of 20 mM ammonium bicarbonate/acetonitrile (3:1, v/v, 1.00 mL). The reaction mixture was shaken for 1 min and left standing at room temperature. After 3 hours the reaction mixture was frozen and lyophilized overnight. The crude product was dissolved in 20 mM ammonium bicarbonate (1 mL) and the resulting solution was directly subjected to preparative LC-MS..sup.1B Fractions corresponding to the product were immediately pooled together, frozen and lyophilized overnight to give the title compound (GalNAc)3-Ls-BNA) ((11.3 mg, 72%) as a white fluffy solid. Purity based on LC-MS 95% (multiple (broad) peaks due to regioisomers). [0464] LRMS (m/z): 2149 [M-4].sup.4-, 2866 [M-3].sup.3- [0465] LC-MS r.t. (min): 2.92.sup.1A

    Anticd71-Saporin Synthesis

    [0466] Custom CD71mab-saporin conjugate was produced and purchased from Advanced Targeting Systems (San Diego, CA). CD71 antibody (anti-CD71, clone OKT-9, InVivoMab) was purchased from BioXCell.

    HSP27BNA, ApoB and ApoB.SUB.scrambled Oligo Sequences

    [0467] HSP27 (5′-GGCacagccagtgGCG-3′) [SEQ ID NO: 1] (The antisense BNA (HSP27) was BNA, more specifically BNA.sup.NC, with oligo nucleic acid sequence 5′-GGCacagccagtgGCG-3′ according to Zhang et al. (2011) [Y Zhang, Z Qu, S Kim, V Shi, B Liao1, P Kraft, R Bandaru, Y Wu, LM Greenberger and ID Horak, Down-modulation of cancer targets using locked nucleic acid (LNA)-based antisense oligonucleotides without transfection, Gene Therapy (2011) 18, 326-333]), ApoB, also referred to as ApoB#01 (5′-GCCTCagtctgcttcGCACC-3′) [SEQ ID NO: 2] and ApoB.sub.scrambled (5′-GGCCTctctacaccgCTCGT-3′) [SEQ ID NO: 3] BNA oligos, and murine and human sequence-compatible ApoB#02 (5′-GCattggtatTCA-3′) [SEQ ID NO: 12] BNA.sup.NC oligonucleotides were ordered with 5′-Thiol C6 linker at Bio-Synthesis Inc., with BNA bases in capitals, and fully phosphorothioated backbones (Lewisville, Texas).

    RNA Isolation and Gene Expression Analysis Cell Lines

    [0468] RNA from cells was isolated and analysed according to standard protocols (Biorad). qPCR primers that were used are indicated in Table A2.

    TABLE-US-00003 Primers used in qPCR (human cells) are shown below: Gene Primer Sequence (5′-3′) HSP27 Forward GCAGTCCAACGAGATCACCA [SEQ ID NO: 4] Reverse TAAGGCTTTACTTGGCGGCA [SEQ ID NO: 5] ApoB Forward AGGGTCCGGGAATCTGATGA [SEQ ID NO: 6] Reverse TGGGCACGTTGTCTTTCAGAG [SEQ ID NO: 7] HBMS Forward CACCCACACACAGCCTACTT [SEQ ID NO: 8] Reverse GTACCCACGCGAATCACTCT [SEQ ID NO: 9] GUSB Forward GAAAATACGTGGTTGGAGAGCT [SEQ ID NO: 10] Reverse CCGAGTGAAGATCCCCTTTTTA [SEQ ID NO: 11]

    Cell Viability Assay

    [0469] After treatment the cells were incubated for 72 hr at 37° C. before the cell viability was determined by a MTS-assay, performed according to the manufacturer’s instruction (CellTiter 96® AQueous One Solution Cell Proliferation Assay, Promega). Briefly, the MTS solution was diluted 20× in DMEM without phenol red (PAN-Biotech GmbH) supplemented with 10% FBS. The cells were washed once with 200 .Math.L/PBS well, after which 100 .Math.L diluted MTS solution was added/well. The plate was incubated for approximately 20-30 minutes at 37° C. Subsequently, the OD at 492 nm was measured on a Thermo Scientific Multiskan FC plate reader (Thermo Scientific). For quantification the background signal of ‘medium only’ wells was subtracted from all other wells, before the cell viability percentage of treated/untreated cells was calculated, by dividing the background corrected signal of treated wells over the background corrected signal of the untreated wells (x 100).

    FACS Analysis

    [0470] Cells were seeded in DMEM (PAN-Biotech GmbH) supplemented with 10% fetal bovine serum (PAN-Biotech GmbH) and 1% penicillin/streptomycin (PAN-Biotech GmbH), in T75 flasks at appropriate density for each cell-line and incubated for 72-96 hrs (5% CO.sub.2, 37° C.), until a confluency of 90% was reached. Next, the cells were trypsinized (TryplE Express, Gibco Thermo Scientific) to single cells, transferred to a 15 mL falcon tube, and centrifuged (1,400 rpm, 3 min). The supernatant was discarded while leaving the cell pellet submerged. 500.000 Cells were transferred to round bottom FACS tubes and the washed with 3 mL cold DPBS (Mg.sup.2+ and Ca.sup.2+ free, 2% FBS). The cells were centrifuged at 1800 rpm, 3 min 4° C. and resuspended in 200 .Math.L cold DPBS (Mg.sup.2+ and Ca.sup.2+ free, 2% FBS) or 200 .Math.L antibody solution; containing 5 .Math.L antibody in 195 .Math.L cold DPBS (Mg.sup.2+ and Ca.sup.2+ free, 2% FBS). PE anti-human CD71 (#334106, Biolegend) was used to stain the transferrin receptor, PE Mouse IgG2a, κ Isotype Ctrl FC (#400212, Biolegend) was used as its matched isotype control. PE anti-human ASGPR1 (#130-122-963, Miltenyi) was used to stain the ASGPR1 receptor and PE Mouse IgG1, Isotype Ctrl (#130-113-762, Miltenyi) was used as its matched isotype control. Samples were incubated for 30 min. at 4° C. Afterwards, the cells were washed 2x with cold DPBS (Mg.sup.2+ and Ca.sup.2+ free, 2% FBS) and fixated for 20 min at room temperature using a 2% PFA solution in DPBS (Mg.sup.2+ and Ca.sup.2+ free, 2% FBS). Cells were washed 1x with cold DPBS, and resuspended in 1000 .Math.L cold DPBS for FACS analysis. Samples were analyzed with a Sysmex Cube 8 flow cytometry system (Sysmex) and FCS Express 7 Research edition software. Results of the FACS analyses are summarized in Table A3.

    TABLE-US-00004 Cell membrane receptor expression levels of ASPGR1 and CD71 of HepG2 and Huh7 cells Cell line ASPGR1 expression level (MFI) CD71 expression level (MFI) HepG2 8.8 74.7 Huh7 1.6 109

    RNA Isolation and Gene Expression Analysis From Primary Mouse and Human Hepatocytes

    [0471] RNA from cells was isolated using TRI Reagent® Solution (Thermo Scientific) according to the manufacturer’s instruction. Conversion into cDNA was performed using iScript™ cDNA Synthesis Kit (BioRad) using standard protocols. ApoB expression levels and levels of specific hepatocyte housekeeping genes were determined using quantitative real-time PCR assays (qRT-PCR) using iTaq™ Universal SYBR® Green Supermix (BioRad) and the Light Cycler 480 (Roche Diagnostics, Rotkreuz, Switzerland) with specific DNA primers, listed in Table A4 (murine) and Table A2 (human). Analysis was done by the ΔCt method to determine ApoB expression relative to 2 hepatocyte-specific housekeeping control mRNAs. Each analysis reaction was performed in triplicate.

    TABLE-US-00005 Primers used in qPCR analysis of mouse primary hepatocytes ApoB#02 Forward GCTAACACTAAGAACCAGAAGATC [SEQ ID NO: 13] Reverse TGTCCGTCTAAGGATCCTGC [SEQ ID NO: 14] Mm PPIA Forward GCGGCAGGTCCATCTACG [SEQ ID NO: 15] Reverse GCCATCCAGCCATTCAGTC [SEQ ID NO: 16] Mm SDHA Forward GAGGAAGCACACCCTCTCAT [SEQ ID NO: 17] Reverse GGAGCGGATAGCAGGAGGTA [SEQ ID NO: 18]

    Mouse Primary Hepatocyte Treatment

    [0472] Cryopreserved primary mouse hepatocytes (PRIMACYT Cell Culture Technology GmbH, Germany) were thawed in hepatocyte thawing media (HTM, PRIMACYT Cell Culture Technology GmbH, Germany) and washed 1x with hepatocyte wash media (HWM, PRIMACYT Cell Culture Technology GmbH, Germany). Cells were re-suspended in hepatocyte plating media (HPM Cryo, PRIMACYT Cell Culture Technology GmbH, Germany) at a density of approx. 0.275 × 10.sup.6 cells/ml. Cells were seeded onto collagen-I coated plates at a density of 88.000 cells/well or 26.400 cells/well for the 48 or 96-well plates (Greiner BioOne). Cells were pre-cultured for 4-6 hrs at 37° C. allowing for cell attachment to cell culture plates before the start of treatment. Plating medium was replaced by 315 .Math.l or 108 .Math.l assay media (MHM, PRIMACYT Cell Culture Technology GmbH, Germany), after which conjugates were added from a 10x concentrated stock solution in PBS. Plates were incubated for 72 hr at 37° C. being harvested for gene expression and cell viability analysis.

    Human Primary Hepatocyte Treatment

    [0473] Cryopreserved primary human hepatocytes (Cytes Biotechnologies S.L., Spain) were thawed in hepatocyte thawing media (Cytes Biotechnologies S.L., Spain). Cells were re-suspended in hepatocyte plating media (Cytes Biotechnologies S.L., Spain). Cells were seeded onto collagen-I coated plates at a density of 215.600 cells/well or 66.600 cells/well for the 48 or 96-well plates (Greiner BioOne). Cells were pre-cultured for 4-6 hrs at 37° C. allowing for cell attachment to cell culture plates before the start of treatment. Plating medium was replaced by 315 .Math.l or 108 .Math.l maintenance media (Cytes Biotechnologies S.L., Spain), after which conjugates were added from a 10x concentrated stock solution in PBS. Plates were incubated for 72 hr at 37° C. being harvested for gene expression and cell viability analysis.