Treatment of cancer cells overexpressing somatostatin receptors using ocreotide derivatives chelated to radioisotopes
11541133 · 2023-01-03
Assignee
Inventors
- Izabela Tworowska (Houston, TX, US)
- Nilesh Wagh (Houston, TX, US)
- Ebrahim S. Delpassand (Houston, TX, US)
- Federico Rojas-Quijano (Bedford, TX, US)
- Paul Jurek (Red Oak, TX, US)
- Garry E. Kiefer (Richardson, TX, US)
- Tania A. Stallons (Wylie, TX, US)
- Amal Saidi (Thomon-les-Bains., FR)
- Julien Torgue (Gaithersburg, MD, US)
Cpc classification
A61K51/088
HUMAN NECESSITIES
A61K51/083
HUMAN NECESSITIES
A61K45/06
HUMAN NECESSITIES
A61K47/10
HUMAN NECESSITIES
A61K47/22
HUMAN NECESSITIES
International classification
A61K51/08
HUMAN NECESSITIES
A61K47/22
HUMAN NECESSITIES
A61K47/18
HUMAN NECESSITIES
A61P35/00
HUMAN NECESSITIES
Abstract
A cancer targeting composition, kit, and method for treatment of cancer cells overexpressing somatostatin receptors is disclosed. The composition includes a radioisotope, a chelator, and a targeting moiety. The chelator includes a nitrogen ring structure including a tetraazacyclododecane, a triazacyclononane, and/or a tetraazabicyclo [6.6.2] hexadecane derivative. The targeting moiety includes a somatostatin receptor targeting peptide. The somatostatin receptor targeting peptide includes an octreotide derivative. The targeting moiety is chelated to the radioisotope by the chelator whereby the cancer cells are targeted for elimination.
Claims
1. A cancer targeting composition comprising a molecule of Formula (I) or a pharmaceutically acceptable salt thereof:
M-Ch-L.sup.1-Tm, Formula (I) wherein: M is .sup.212Pb or .sup.203Pb; Ch is a chelator having a structure of Formula (V): ##STR00024## wherein: R.sup.5, R.sup.6, and R.sup.8 are each (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.7 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26 or L.sup.1; R.sup.13 and R.sup.14 are each independently H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, or L.sup.1; R.sup.25 and R.sup.26 are each independently H, D, (C.sub.1-C.sub.6)alkyl, or (C.sub.1-C.sub.6)alkyl-C(═O)—OH; L.sup.1 is R(C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, or (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and Tm has a structure of Formula (VI): ##STR00025## wherein: R.sup.27 is CH.sub.2—OH or C(═O)—OH; and (L.sup.1) is L.sup.1 and connects to Ch to Tm, provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1.
2. The cancer targeting composition of claim 1, having a structure of Formula (VII) or a pharmaceutically acceptable salt thereof: ##STR00026## wherein: M is .sup.212Pb or .sup.203Pb; R.sup.5, R.sup.6, and R.sup.8 are each independently (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.13 and R.sup.14 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.25 and R.sup.26 are each independently H, D, (C.sub.1-C.sub.6)alkyl, or (C.sub.1-C.sub.6)alkyl-C(═O)—OH; L.sup.1 is (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, or (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and R.sup.27 is CH.sub.2—OH or C(═O)—OH.
3. The cancer targeting composition of claim 1, having a structure of Formula (VIII) or a pharmaceutically acceptable salt thereof: ##STR00027## wherein: M is .sup.212Pb or .sup.203Pb; R.sup.5, R.sup.6, and R.sup.8 are each independently (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.7 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.13 is H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.25 and R.sup.26 are each independently H, D, (C.sub.1-C.sub.6)alkyl, or (C.sub.1-C.sub.6)alkyl-C(═O)—OH; L.sup.1 is (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH; and R.sup.27 is CH.sub.2—OH or C(═O)—OH.
4. The cancer targeting composition of claim 1, having a structure of Formula (IX) or a pharmaceutically acceptable salt thereof: ##STR00028## wherein: M is .sup.212Pb or .sup.203Pb; R.sup.5, R.sup.6, and R.sup.8 are each independently (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.13 and R.sup.14 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.25 and R.sup.26 are each independently H, D, (C.sub.1-C.sub.6)alkyl, or (C.sub.1-C.sub.6)alkyl-C(═O)—OH; and R.sup.27 is CH.sub.2—OH or C(═O)—OH.
5. A cancer targeting kit for treatment of cancer cells overexpressing somatostatin receptors, the cancer targeting kit comprising: the cancer targeting composition of claim 1; and at least one of a pharmaceutically acceptable buffer, an antioxidant, and a scavenger.
6. The cancer targeting kit of claim 5, which comprises 25 μg to 50 μg of the cancer targeting composition and 0.4M ammonium acetate buffer.
7. The cancer targeting kit of claim 5, wherein the pharmaceutically acceptable buffer is an ammonium acetate buffer.
8. The cancer targeting kit of claim 5, wherein the antioxidant is ascorbic acid, gentisic acid, ethanol, or a combination thereof.
9. The cancer targeting kit of claim 5, wherein the scavenger is diethylenetriaminopentaacetic; ethylene diamine tetraacetic acid; 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic; or a combination thereof.
10. A pharmaceutical formulation comprising the cancer targeting composition of claim 1 and a pharmaceutically acceptable buffer.
11. A method of treating cancer cells overexpressing somatostatin receptors to a subject in need thereof, the method comprising: administering a therapeutically effective dosage of a cancer targeting composition, the cancer targeting composition comprising a molecule of Formula (I) or a pharmaceutically acceptable salt thereof:
M-Ch-L.sup.1-Tm, Formula (I) wherein: M is .sup.212Pb or .sup.203Pb; Ch is a chelator having a structure of Formula (V): ##STR00029## wherein: R.sup.5, R.sup.6, and R.sup.8 are each (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.7 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26 or L.sup.1; R.sup.13 and R.sup.14 are each independently H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, or L.sup.1; R.sup.25 and R.sup.26 are each independently H, D, or (C.sub.1-C.sub.6)alkyl, or (C.sub.1-C.sub.6)alkyl-C(═O)—OH; L.sup.1 is (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, or (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; Tm has a structure of Formula (VI): ##STR00030## wherein: R.sup.27 is CH.sub.2—OH or C(═O)—OH; and (L.sup.1) is L.sup.1 and connects to Ch to Tm, provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1.
12. The method of claim 11, wherein the cancer comprises cells overexpressing somatostatin receptors.
13. The method of claim 11, wherein the cancer is a cardiac cancer, a lung cancer, a gastrointestinal cancer, genitourinary tract cancer, a liver cancer, a bone cancer, a nervous system cancer, gynecological cancer, a hematologic cancer, or a combination thereof.
14. The method of claim 11, wherein the subject is a mammal.
15. The method of claim 11, wherein the cancer targeting composition is administered in combination with at least one anti-cancer compound, wherein the at least one anti-cancer compound is aldesleukin; alemtuzumab; alitretinoin; allopurinol; altretamine; amifostine; anastrozole; arsenic trioxide; asparaginase; BCG Live; bexarotene; bleomycin; busulfan; calusterone; capecitabine; carboplatin; carmustine; carmustine with polifeprosan 20 implant; celecoxib; chlorambucil; cisplatin; cladribine; cyclophosphamide; cytarabine; cytarabine liposomal; dacarbazine; dactinomycin, actinomycin D; darbepoetin alfa; daunorubicin liposomal; daunorubicin, daunomycin; denileukin diftitox, dexrazoxane; docetaxel; doxorubicin; doxorubicin liposomal; dromostanolone propionate; Elliott's B Solution; epirubicin; epoetin alfa estramustine; etoposide; exemestane; filgrastim; floxuridine; fludarabine; 5-fluorouracil; fulvestrant; gemcitabine; gemtuzumab ozogamicin; imatinib; goserelin; hydroxyurea; ibritumomab tiuxetan; idarubicin; ifosfamide; imatinib mesylate; interferon alfa-2a; interferon alfa-2b; irinotecan; letrozole; leucovorin; levamisole; lomustine; mechlorethamine; megestrol; melphalan; 6-mercaptopurine; mesna; methotrexate; methoxsalen; mitomycin C; mitotane; mitoxantrone; nandrolone phenpropionate; nofetumomab; LOddC; oprelvekin; oxaliplatin; paclitaxel; pamidronate; pegademase; pegaspargase; pegfilgrastim; pentostatin; pipobroman; plicamycin; mithramycin; porfimer sodium; procarbazine; quinacrine; rasburicase; rituximab; sargramostim; streptozocin; surafenib; talbuvidine; talc; tamoxifen; erlotinib; temozolomide; teniposide; testolactone; 6-thioguanine; thiotepa; topotecan; toremifene; tositumomab; trastuzumab; tretinoin; uracil mustard; valrubicin; valtorcitabine; vinblastine; vinorelbine; zoledronate; or a mixture thereof.
16. The method of claim 15, wherein the anti-cancer compound is administered in a therapeutically effective dosage.
17. A method of treating cancer cells overexpressing somatostatin receptors to a subject in need thereof, the method comprising: administering a therapeutically effective dosage of a molecule of Formula (I), or a pharmaceutically acceptable salt thereof, and at least one anti-cancer compound in a pharmaceutically acceptable carrier,
M-Ch-L.sup.1-Tm, Formula (I) wherein: M is .sup.212Pb or .sup.203Pb; Ch is a chelator having a structure of Formula (V): ##STR00031## wherein R.sup.5, R.sup.6, and R.sup.8 are each (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently H, D, F, Cl, or (C.sub.1-C.sub.6)alkyl; R.sup.7 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26 or L.sup.1; R.sup.13 and R.sup.14 are each independently H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, or L.sup.1; R.sup.25 and R.sup.26 are each independently H, D, (C.sub.1-C.sub.6)alkyl, or (C.sub.1-C.sub.6)alkyl-C(═O)—OH; L.sup.1 is (C.sub.1-Q)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, or (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and Tm has a structure of Formula (VI): ##STR00032## wherein: R.sup.27 is CH.sub.2—OH or C(═O)—OH; and (L.sup.1) is L.sup.1 and connects to Ch to Tm, provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1.
18. The method of claim 17, wherein the at least one anti-cancer compound is aldesleukin; alemtuzumab; alitretinoin; allopurinol; altretamine; amifostine; anastrozole; arsenic trioxide; asparaginase; BCG Live; bexarotene; bleomycin; busulfan; calusterone; capecitabine; carboplatin; carmustine; carmustine with polifeprosan 20 implant; celecoxib; chlorambucil; cisplatin; cladribine; cyclophosphamide; cytarabine; cytarabine liposomal; dacarbazine; dactinomycin, actinomycin D; darbepoetin alfa; daunorubicin liposomal; daunorubicin, daunomycin; denileukin diftitox, dexrazoxane; docetaxel; doxorubicin; doxorubicin liposomal; dromostanolone propionate; Elliott's B Solution; epirubicin; epoetin alfa estramustine; etoposide; exemestane; filgrastim; floxuridine; fludarabine; 5-fluorouracil; fulvestrant; gemcitabine; gemtuzumab ozogamicin; imatinib; goserelin; hydroxyurea; ibritumomab tiuxetan; idarubicin; ifosfamide; imatinib mesylate; interferon alfa-2a; interferon alfa-2b; irinotecan; letrozole; leucovorin; levamisole; lomustine; mechlorethamine; megestrol; melphalan; 6-mercaptopurine; mesna; methotrexate; methoxsalen; mitomycin C; mitotane; mitoxantrone; nandrolone phenpropionate; nofetumomab; LOddC; oprelvekin; oxaliplatin; paclitaxel; pamidronate; pegademase; pegaspargase; pegfilgrastim; pentostatin; pipobroman; plicamycin; mithramycin; porfimer sodium; procarbazine; quinacrine; rasburicase; rituximab; sargramostim; streptozocin; surafenib; talbuvidine; talc; tamoxifen; erlotinib; temozolomide; teniposide; testolactone; 6-thioguanine; thiotepa; topotecan; toremifene; tositumomab; trastuzumab; tretinoin; uracil mustard; valrubicin; valtorcitabine; vinblastine; vinorelbine; zoledronate; or a combination or a mixture thereof.
19. The method of claim 18, wherein the at least one anti-cancer compound is administered in a therapeutically effective dosage.
20. The cancer targeting composition of claim 2, having the structure represented by the following Formula: ##STR00033##
21. The cancer targeting composition of claim 3, having the structure represented by the following Formula: ##STR00034##
22. The method of claim 14, wherein the mammal is a dog, a cat, or a horse.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
(1) A more particular description of the disclosure may be had by reference to embodiments illustrated in the appended drawings. It is to be noted, however, that the appended drawings illustrate examples and are, therefore, not to be considered limiting of its scope. The figures are not necessarily to scale and certain features, and certain views of the figures may be shown exaggerated in scale or in schematic in the interest of clarity and conciseness.
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(3) FIGS. 2A1-2A4 and 2B1-2B4 are example chemical structures of chelators of the cancer targeting composition.
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DETAILED DESCRIPTION
(46) The description that follows includes exemplary apparatus, methods, techniques, and/or instruction sequences that embody techniques of the present subject matter. However, it is understood that the described embodiments may be practiced without these specific details.
(47) A cancer targeting composition for treating cancer cells overexpressing somatostatin receptors is disclosed herein. The cancer targeting composition includes a molecule of Formula (I) or a pharmaceutically acceptable salt thereof:
M-Ch-L.sub.1-Tm, Formula (I)
wherein
(48) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(49) Ch is a chelator having a structure selected from the group consisting of:
(50) Formula (II), Formula (III), Formula (IV), and Formula (V), wherein
(51) ##STR00009##
(52) wherein
(53) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(54) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(55) R.sup.7 is independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26, and Li;
(56) R.sup.13 and R.sup.14 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, and L.sup.1;
(57) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH;
(58) L.sup.1 is independently selected from a group consisting of, and (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and
(59) Tm has a structure of Formula (VI),
(60) ##STR00010##
(61) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH; and
(62) provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1. Unless otherwise noted, the use of L.sup.1 in parenthesis indicates that that L.sup.1 is not formally part of, for example, Tm, but is being shown as part of Tm to indicate the relevant points of attachment.
(63) The cancer targeting composition may have one, two, or three of R.sup.5, R.sup.6, and R.sup.8 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26. M may be selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho. M may be independently selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, and .sup.67Cu. M may be selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, and .sup.212Bi; and Ch may have a structure of Formula (V); and R.sup.27 is CH.sub.2—OH. M may also be selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, and .sup.213Bi; and Ch may have a structure of Formula (V), and R.sup.27 is C(═O)—OH. The molecule of Formula (I) is produced by reacting at least one compound with a chelator, wherein the chelator is selected from the group consisting of:
(64) ##STR00011## ##STR00012##
(65) The cancer targeting composition may have a structure represented by Formula (VII) or a pharmaceutically acceptable salt thereof:
(66) ##STR00013##
wherein
(67) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(68) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(69) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(70) R.sup.13 and R.sup.14 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(71) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH;
(72) L.sup.1 is independently selected from a group consisting of, and (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, and (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and
(73) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH.
(74) The cancer targeting composition may have a structure represented by Formula (VIII) or a pharmaceutically acceptable salt thereof:
(75) ##STR00014##
(76) wherein
(77) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(78) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(79) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(80) R.sup.7 is independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(81) R.sup.13 is independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(82) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH;
(83) L.sup.1 is (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH; and
(84) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH.
(85) The cancer targeting composition may have a structure of Formula (IX) or a pharmaceutically acceptable salt thereof:
(86) ##STR00015##
(87) wherein
(88) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(89) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(90) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(91) R.sup.13 and R.sup.14 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(92) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH; and
(93) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH.
(94) The cancer targeting composition may have a structure of Formula (X) or a pharmaceutically acceptable salt thereof:
(95) ##STR00016##
(96) wherein
(97) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy 148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(98) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(99) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(100) R.sup.7 is independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(101) R.sup.13 is independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(102) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, and (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH; and
(103) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH.
(104) The composition may include a molecule of Formula (I) or a pharmaceutically acceptable salt thereof:
M-Ch-L.sub.1-Tm, Formula (I)
wherein
(105) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(106) Ch is a chelator having a structure of Formula (V), wherein
(107) ##STR00017##
(108) wherein
(109) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(110) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(111) R.sup.7 is independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26, and L.sub.1;
(112) R.sup.13 and R.sup.14 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, and L.sup.1;
(113) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH;
(114) L.sup.1 is independently selected from a group consisting of (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and
(115) Tm has a structure of Formula (VI),
(116) ##STR00018##
(117) wherein R.sup.27 is CH.sub.2—OH; and
(118) provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1.
(119) A cancer targeting kit for treatment of cancer cells overexpressing somatostatin receptors is disclosed herein. The cancer targeting kit may include the cancer targeting composition of as disclosed herein, and at least one of a pharmaceutically acceptable buffer, an antioxidant, and a scavenger. The cancer targeting kit may include 25-50 μg of the cancer targeting composition and 0.4M ammonium acetate buffer. The cancer targeting kit may include an ammonium acetate buffer. In an embodiment, the buffer comprises an ammonium acetate buffer. The antioxidant may include ascorbic acid, gentisic acid, ethanol, or combinations thereof. The scavenger may be one selected from the group consisting of: diethylenetriaminopentaacetic; ethylene diamine tetraacetic acid; 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic; and combinations thereof.
(120) A pharmaceutical formulation is disclosed herein. The pharmaceutical formulation may include the cancer targeting composition as disclosed herein and a pharmaceutically acceptable buffer. A cancer targeting composition as disclosed herein for use as a medicine for treating cancerous cells overexpressing somatostatin receptors is disclosed.
(121) A method of administering a cancer targeting composition for treating cancer cells overexpressing somatostatin receptors to a subject in need thereof is disclosed herein. The method may include administering a therapeutically effective dosage of a cancer targeting composition, the cancer targeting composition comprising a molecule of Formula (I) or a pharmaceutically acceptable salt thereof:
(122) wherein M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In, .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(123) Ch is a chelator having a structure selected from the group consisting of:
(124) Formula (II), Formula (III), Formula (IV), and Formula (V), wherein
(125) ##STR00019##
(126) wherein
(127) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(128) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(129) R.sup.7 is independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26, and L.sub.1;
(130) R.sup.13 and R.sup.14 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, and L.sup.1;
(131) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, and (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH;
(132) L.sup.1 is independently selected from a group consisting of, and (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, and (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and
(133) Tm has a structure of Formula (VI),
(134) ##STR00020##
(135) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH; and
(136) provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1.
(137) The cancer may comprise cells overexpressing somatostatin receptors. The cancer may include a cardiac cancer, a lung cancer, a gastrointestinal cancer, genitourinary tract cancer, a liver cancer, a bone cancer, a nervous system cancer, gynecological cancer, a hematologic cancer, or a combination thereof. The subject may be a human, dog, cat, horse, or other mammal. The cancer targeting composition may be administered in combination with at least one anti-cancer compound, wherein the at least one anti-cancer compounds includes Aldesleukin; Alemtuzumab; alitretinoin; allopurinol; altretamine; amifostine; anastrozole; arsenic trioxide; Asparaginase; BCG Live; bexarotene capsules; bexarotene gel; bleomycin; busulfan intravenous; busulfan oral; calusterone; capecitabine; carboplatin; carmustine; carmustine with Polifeprosan 20 Implant; celecoxib; chlorambucil; cisplatin; cladribine; cyclophosphamide; cytarabine; cytarabine liposomal; dacarbazine; dactinomycin, actinomycin D; Darbepoetin alfa; daunorubicin liposomal; daunorubicin, daunomycin; Denileukin diftitox, dexrazoxane; docetaxel; doxorubicin; doxorubicin liposomal; Dromostanolone propionate; Elliott's B Solution; epirubicin; Epoetin alfa estramustine; etoposide phosphate; etoposide (VP-16); exemestane; Filgrastim; floxuridine (intraarterial); fludarabine; fluorouracil (5-FU); fulvestrant; gemcitabine; gemtuzumab ozogamicin; gleevec (imatinib); goserelin acetate; hydroxyurea; Ibritumomab Tiuxetan; idarubicin; ifosfamide; imatinib mesyflate; Interferon alfa-2a; Interferon alfa-2b; irinotecan; letrozole; leucovorin; levamisole; lomustine (CCNU); meclorethamine (nitrogen mustard); megestrol acetate; melphalan (L-PAM); mercaptopurine (6-MP); mesna; methotrexate; methoxsalen; mitomycin C; mitotane; mitoxantrone; nandrolone phenpropionate; Nofetumomab; LOddC; Oprelvekin; oxaliplatin; paclitaxel; pamidronate; pegademase; Pegaspargase; Pegfilgrastim; pentostatin; pipobroman; plicamycin; mithramycin; porfimer sodium; procarbazine; quinacrine; Rasburicase; Rituximab; Sargramostim; streptozocin; surafenib; talbuvidine (LDT); talc; tamoxifen; tarceva (erlotinib); temozolomide; teniposide (VM-26); testolactone; thioguanine (6-TG); thiotepa; topotecan; toremifene; Tositumomab; Trastuzumab; tretinoin (ATRA); Uracil Mustard; valrubicin; valtorcitabine (monoval LDC); vinblastine; vinorelbine; zoledronate; or a mixture thereof. The anti-cancer compound may be administered in a therapeutically effective dosage.
(138) A method of administering a cancer targeting composition for treating cancer cells overexpressing somatostatin receptors to a subject in need thereof is disclosed. The method may include administering a therapeutically effective dosage of a molecule of Formula (I), or a pharmaceutically acceptable salt thereof; and
(139) at least one anti-cancer compound in a pharmaceutically acceptable carrier,
(140) the molecule of Formula (I), wherein
M-Ch-L.sub.1-Tm, Formula (I)
(141) M is a radioisotope selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, .sup.68Ga, .sup.213Bi, .sup.225Ac, .sup.243Am, .sup.211At, .sup.217At, .sup.154Dy, .sup.148Gd, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.86Y, .sup.111In .sup.153Gd, .sup.153Sm, and .sup.166Ho;
(142) Ch is a chelator having a structure selected from the group consisting of:
(143) Formula (II), Formula (III), Formula (IV), and Formula (V), wherein
(144) ##STR00021##
(145) wherein
(146) R.sup.5, R.sup.6, and R.sup.8 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, and (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26;
(147) R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H, D, F, Cl, and (C.sub.1-C.sub.6)alkyl;
(148) R.sup.7 is independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26, and Li;
(149) R.sup.13 and R.sup.14 are each independently selected from the group consisting of H, D, F, Cl, (C.sub.1-C.sub.6)alkyl, and L.sup.1;
(150) R.sup.25 and R.sup.26 are each independently selected from the group consisting of H, D, (C.sub.1-C.sub.6)alkyl, and (C.sub.1-C.sub.6)alkyl-C(═O)—OH;
(151) L.sup.1 is independently selected from a group consisting of, and (C.sub.1-C.sub.6)alkyl-C(═O)—NH—(C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, C(—CO.sub.2H)—(C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—NH, (C.sub.1-C.sub.6)alkyl-C(═O)—(O—CH.sub.2—CH.sub.2).sub.1-20—C(═O)—NH; and
(152) Tm has a structure of Formula (VI),
(153) ##STR00022##
(154) wherein R.sup.27 is independently selected from the group consisting of CH.sub.2—OH and C(═O)—OH; and
(155) provided that only one of R.sup.7, R.sup.13, or R.sup.14 is L.sup.1.
(156) The at least one anti-cancer compound may include Aldesleukin; Alemtuzumab; alitretinoin; allopurinol; altretamine; amifostine; anastrozole; arsenic trioxide; Asparaginase; BCG Live; bexarotene capsules; bexarotene gel; bleomycin; busulfan intravenous; busulfan oral; calusterone; capecitabine; carboplatin; carmustine; carmustine with Polifeprosan 20 Implant; celecoxib; chlorambucil; cisplatin; cladribine; cyclophosphamide; cytarabine; cytarabine liposomal; dacarbazine; dactinomycin, actinomycin D; Darbepoetin alfa; daunorubicin liposomal; daunorubicin, daunomycin; Denileukin diftitox, dexrazoxane; docetaxel; doxorubicin; doxorubicin liposomal; Dromostanolone propionate; Elliott's B Solution; epirubicin; Epoetin alfa estramustine; etoposide phosphate; etoposide (VP-16); exemestane; Filgrastim; floxuridine (intraarterial); fludarabine; fluorouracil (5-FU); fulvestrant; gemcitabine; gemtuzumab ozogamicin; gleevec (imatinib); goserelin acetate; hydroxyurea; Ibritumomab Tiuxetan; idarubicin; ifosfamide; imatinib mesyflate; Interferon alfa-2a; Interferon alfa-2b; irinotecan; letrozole; leucovorin; levamisole; lomustine (CCNU); meclorethamine (nitrogen mustard); megestrol acetate; melphalan (L-PAM); mercaptopurine (6-MP); mesna; methotrexate; methoxsalen; mitomycin C; mitotane; mitoxantrone; nandrolone phenpropionate; Nofetumomab; LOddC; Oprelvekin; oxaliplatin; paclitaxel; pamidronate; pegademase; Pegaspargase; Pegfilgrastim; pentostatin; pipobroman; plicamycin; mithramycin; porfimer sodium; procarbazine; quinacrine; Rasburicase; Rituximab; Sargramostim; streptozocin; surafenib; talbuvidine (LDT); talc; tamoxifen; tarceva (erlotinib); temozolomide; teniposide (VM-26); testolactone; thioguanine (6-TG); thiotepa; topotecan; toremifene; Tositumomab; Trastuzumab; tretinoin (ATRA); Uracil Mustard; valrubicin; valtorcitabine (monoval LDC); vinblastine; vinorelbine; zoledronate; or a combination or a mixture thereof. In an embodiment of the method, the at least one anti-cancer compound is administered in a therapeutically effective dosage.
(157) The Formula (I) or a pharmaceutically acceptable salt thereof may include at least one of R.sup.5, R.sup.6, and R.sup.8 is (C.sub.1-C.sub.6)alkyl-C(═O)—OR.sup.25, wherein R.sup.25 is H or (C.sub.1-C.sub.6)alkyl.
(158) The Formula (I) or a pharmaceutically acceptable salt thereof may include at least one of R.sup.5, R.sup.6, and R.sup.8 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26, wherein R.sup.25 and R.sup.26 are each independently selected from the group consisting of H and (C.sub.1-C.sub.6)alkyl. Preferably, when M is .sup.213Bi, then R.sup.5, R.sup.6, and R.sup.8 are not C.sub.1alkyl-C(═O)—OH. Preferably, when M is .sup.213Bi, then one, two, or three of R.sup.5, R.sup.6, and R.sup.8 is CH.sub.2—C(═O)—NH.sub.2.
(159) The Formula (I) or a pharmaceutically acceptable salt thereof may include at least one of R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H and (C.sub.1-C.sub.6)alkyl. The Formula (I) or a pharmaceutically acceptable salt thereof may include at least one of R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from the group consisting of H and D.
(160) In the Formula (I) or a pharmaceutically acceptable salt thereof, M may be independently selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, and .sup.67Cu; Ch is Formula (V), wherein R.sup.5, R.sup.6, and R.sup.8 are (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from H or D; R.sup.7 is L.sup.1; L.sup.1 is (C.sub.1-C.sub.6)alkyl-C(═O)—NH; R.sup.13 and R.sup.14 are each independently selected from the group consisting of H and D; R.sup.25 and R.sup.26 are each independently selected from the group consisting of H and D; Tm has a structure of Formula (VI); and R.sup.27 is C(═O)—OH.
(161) In the Formula (I) or a pharmaceutically acceptable salt thereof, M may be independently selected from the group consisting of .sup.212Pb, .sup.203Pb, .sup.64Cu, and .sup.67Cu; Ch is Formula (V), wherein R.sup.5, R.sup.6, and R.sup.8 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.9, R.sup.10, R.sup.11, R.sup.12, R.sup.15, R.sup.16, R.sup.17, R.sup.18, R.sup.19, R.sup.20, R.sup.21, R.sup.22, R.sup.23, and R.sup.24 are each independently selected from H or D; R.sup.7 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26; R.sup.13 is independently selected from the group consisting of H and D; R.sup.14 is L.sup.1; L.sup.1 is (C.sub.1-C.sub.6)alkyl-(C.sub.6H.sub.4)—NH—C(═S)—NH; and R.sup.27 is C(═O)—OH.
(162) The term “alkyl”, by itself or as part of another substituent means, unless otherwise stated, a straight, branched (chiral or achiral) or cyclic chain hydrocarbon having the number of carbon atoms designated (e.g. (C.sub.1-C.sub.6) means one to six carbons) and includes straight, branched chain or cyclic groups. Examples include: methyl, ethyl, propyl, isopropyl, butyl, isobutyl, tert-butyl, pentyl, neopentyl, hexyl, cyclohexyl and cyclopropylmethyl, including particularly ethyl, methyl and isopropyl. This terms is used in the context of both a substituent and linker group.
(163) Depending on the context, parentheticals used in a formula can convey in a single line information regarding a branch. For example, (C.sub.1-C.sub.6)alkyl-C(═O)—OH can also be represented as:
(164) ##STR00023##
Unless otherwise noted, (C.sub.6H.sub.4) refers to a benzyl group having with 2 substituents, wherein the two substituents can be meta, ortho, or para substituted.
(165) A cancer targeting kit for treatment of cancer cells overexpressing somatostatin receptors is disclosed herein. The cancer targeting kit for treatment of cancer cells overexpressing somatostatin receptors may include: the cancer targeting composition of Formula (I), (VII), (VIII), (IX), and/or (X) or a pharmaceutically acceptable salt thereof, as defined above; and at least one of a pharmaceutically acceptable buffer, an antioxidant, and a scavenger. The cancer targeting kit includes 25-50 μg of the cancer targeting composition and 0.4M ammonium acetate buffer. In the cancer targeting kit, the buffer comprises an ammonium acetate buffer. In the cancer targeting kit, the antioxidant includes ascorbic acid, gentisic acid, ethanol, or combinations thereof. In the cancer targeting kit, the scavenger is selected from the group consisting of: diethylenetriaminopentaacetic; ethylene diamine tetraacetic acid; 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic; and combinations thereof.
(166) A pharmaceutical formulation is disclosed. The pharmaceutical formulation includes the cancer targeting composition of Formula (I), (VII), (VIII), (IX), and/or (X) or a pharmaceutically acceptable salt thereof, as defined above; and a pharmaceutically acceptable buffer.
(167) A cancer targeting composition for use as a medicine for treating cancerous cells overexpressing somatostatin receptors is disclosed herein. The cancer targeting composition of for use as a medicine for treating cancerous cells overexpressing somatostatin receptors includes a composition having Formula (I), (VII), (VIII), (IX), and/or (X) or a pharmaceutically acceptable salt thereof, as defined above.
(168) A method of a cancer targeting composition for treating cancer cells overexpressing somatostatin receptors to a subject in need thereof is disclosed herein. The method includes administering a dosage of a cancer targeting composition, the cancer targeting composition comprising a molecule of Formula (I), (VII), (VIII), (IX), and/or (X) or a pharmaceutically acceptable salt thereof, as defined above. The cancer may include cells overexpressing somatostatin receptors. The cancer may include a cardiac cancer, a lung cancer, a gastrointestinal cancer, genitourinary tract cancer, a liver cancer, a bone cancer, a nervous system cancer, gynecological cancer, a hematologic cancer, or a combination thereof. The subject may be a human, dog, cat, horse, or other mammal.
(169) The compounds of the present invention may take the form of salts when appropriately substituted with groups or atoms capable of forming salts. Such groups and atoms are well known to those of ordinary skill in the art of organic chemistry. The term “salts” embraces addition salts of free acids or free bases which are compounds of the invention. The term “pharmaceutically-acceptable salt” refers to salts which possess toxicity profiles within a range that affords utility in pharmaceutical applications. Pharmaceutically unacceptable salts may nonetheless possess properties such as high crystallinity, which have utility in the practice of the present invention, such as for example utility in process of synthesis, purification or formulation of compounds of the invention.
(170) Suitable pharmaceutically-acceptable acid addition salts may be prepared from an inorganic acid or from an organic acid. Examples of inorganic acids include hydrochloric, hydrobromic, hydriodic, nitric, carbonic, sulfuric, and phosphoric acids. Appropriate organic acids may be selected from aliphatic, cycloaliphatic, aromatic, araliphatic, heterocyclic, carboxylic and sulfonic classes of organic acids, examples of which include formic, acetic, propionic, succinic, glycolic, gluconic, lactic, malic, tartaric, citric, ascorbic, glucuronic, maleic, fumaric, pyruvic, aspartic, glutamic, benzoic, anthranilic, 4-hydroxybenzoic, phenylacetic, mandelic, embonic (pamoic), methanesulfonic, ethanesulfonic, benzenesulfonic, pantothenic, trifluoromethanesulfonic, 2-hydroxyethanesulfonic, p-toluenesulfonic, sulfanilic, cyclohexylaminosulfonic, stearic, alginic, β-hydroxybutyric, salicylic, galactaric and galacturonic acid. Examples of pharmaceutically unacceptable acid addition salts include, for example, perchlorates and tetrafluoroborates.
(171) Suitable pharmaceutically acceptable base addition salts of compounds of the invention include, for example, metallic salts including alkali metal, alkaline earth metal and transition metal salts such as, for example, calcium, magnesium, potassium, sodium and zinc salts. Pharmaceutically acceptable base addition salts also include organic salts made from basic amines such as, for example, N,N-dibenzylethylenediamine, chloroprocaine, choline, diethanolamine, ethylenediamine, meglumine (N-methylglucamine) and procaine. Examples of pharmaceutically unacceptable base addition salts include lithium salts and cyanate salts.
(172) The present disclosure describes compositions, kits and methods of treatment (e.g., imaging, diagnosis, therapy, radiotherapy, etc.) of neuroendocrine tumors (NETs) overexpressing somatostatin receptors (SSTR). This treatment involves the use of a cancer targeting composition comprising a radioisotope (e.g., an α-emitter, a β-emitter, a γ-emitter, a positron emitter, and/or other radioactive emitters), chelated by a chelator [CA] or “Ch” to a targeting moiety comprising a somatostatin receptor targeting peptide (e.g., octreotate, octreotide, and/or other derivatives, including “Tm”). The chelator may have a nitrogen ring structure, such as a tetraazacyclododecane derivative, a triazacyclononane derivative, and/or a tetraazabicyclo [6.6.2] hexadecane derivative (e.g., DOTAM, TCMC, DOTA, etc.). See, Tm of Formula (I).
(173) In particular, DOTAM and TCMC may be used to chelate a radioisotope (e.g., lead (Pb) or copper (Cu)) to a targeting moiety (e.g., octreotate, octreotide derivative) in a manner that provides stable coordination of radioisotope and its products of radioactive decay. Experiments herein indicate that molecules having a target moiety and a chelator (e.g., DOTAM, TCMC) are capable of selectively delivering a radioisotope to cancer cells while limiting cytotoxic effects on healthy tissues.
(174) Radiolabeled conjugates are derivatives of chelator coordinating the radioisotope and cancer specific targeting ligands that recognize receptors or transporters on cancer cells. This approach may be used for selective delivery of the radioisotope to the cancer cells with limited effect on healthy cells and tissues. The compositions herein seek to provide conjugates of the chelator modified with a peptide targeting SSTR in the cancer cells. The compositions may be administered by injection of a solution of a radioactive complex of this composition. The conjugates described herein seek to offer a platform for generating stable complexes with α, β.sup.+, β.sup.−, and/or γ-emitting radionuclides for cancer treatment. The techniques herein seek to treat a disease state in the patient by administering a pharmaceutically-acceptable injectable solution into the patient.
(175) While the methods and compositions described herein relate to certain cancer treatment, such may also be applicable to cardiovascular disease, infection, diabetes, cancer, and/or other conditions. For cases involving cancer, the cancer may be, for example, a solid tumor derived, for example, either primarily or as a metastatic form, from cancers such as of the liver, prostate, pancreas, head and neck, breast, brain, colon, adenoid, oral, skin, lung, testes, ovaries, cervix, endometrium, bladder, stomach, epithelium, etc.
(176) In another aspect, a method of treating an individual suffering from a cellular proliferative disorder, particularly cancer, is provided, comprising administering to said individual an effective amount of at least one compound according to Formula I, or a pharmaceutically acceptable salt thereof, either alone, or in combination with a pharmaceutically acceptable carrier.
(177) In yet another aspect, a method of inducing apoptosis of cancer cells, such as tumor cells, in an individual afflicted with cancer is provided, comprising administering to said individual an effective amount of at least one compound according to Formula I, or a pharmaceutically acceptable salt thereof, either alone, or in combination with a pharmaceutically acceptable carrier.
(178) The compounds of Formula I may be administered by any route, including oral, rectal, sublingual, and parenteral administration. Parenteral administration includes, for example, intravenous, intramuscular, intraarterial, intraperitoneal, intranasal, intravaginal, intravesical (e.g., to the bladder), intradermal, transdermal, topical or subcutaneous administration. Also contemplated within the scope of the invention is the instillation of a drug in the body of the patient in a controlled formulation, with systemic or local release of the drug to occur at a later time. For example, the drug may be localized in a depot for controlled release to the circulation, or for release to a local site of tumor growth.
(179) One or more compounds useful in the practice of the present disclosure may be administered simultaneously, by the same or different routes, or at different times during treatment. The compounds may be administered before, along with, or after other medications, including other antiproliferative compounds.
(180) The treatment may be carried out for as long a period as necessary, either in a single, uninterrupted session, or in discrete sessions. The treating physician will know how to increase, decrease, or interrupt treatment based on patient response. The treatment may be carried out for from about four to about sixteen weeks. The treatment schedule may be repeated as required.
(181) Targeted Cancer Treatment
(182) 1. DOTATATE
(183) Cancer treatment may involve the use of compositions that target and trigger cell death (apoptosis) of the cancer cells in the patient. Some forms of targeted treatment of cancer cells may use compositions having molecules which bind to specific antigens of the cancer cells. For example, targeting moieties, such as small molecular weight proteins or monoclonal antibodies, may be used to recognize and bind to the cancer cells using specific cellular antigens which may be located on a surface of the cancer cells. The peptides can be tagged with cytotoxic agents or isotopes/metals to label them and/or to induce the apoptosis. The binding of the peptides may enable specific recognition of cancer antigen-presenting cells which may be used for imaging and/or treatment. For example, targeting agents such as peptides, antibodies and antibody fragments and the like, may be coupled with various cell cytotoxic agents, such as chemotherapeutic agents and/or other promoters of the apoptosis.
(184) Cancer targeting compositions, such as DOTATATE, may be used in treatment of cancer overexpressing specific somatostatin receptors, including neuroendocrine tumors (NETs). DOTATATE as used herein refers to a DOTA chelator conjugated with a targeting moiety, such as octreotate. DOTA as used herein refers to an organic compound having the formula (CH.sub.2CH.sub.2NCH.sub.2CO.sub.2H).sub.4 and is a 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic acid. DOTA may refer to a tetracarboxylic acid and its various conjugate bases. DOTA includes a tetraaza ring of nitrogen atoms with terminal groups ready for conjugation of ligands. DOTA may be used as a chelator (chelating agent) for bonding metal ions and radioisotopes. Targeting moiety as used herein refers to, for example, a peptide, a protein, an antibody, a nucleoside, a nucleotide, an alcohol, a heterocyclic compound, and/or other ligand that bonds to an antigen on a target cell, such as the cancer cell. The targeting moiety may enter and induce apoptosis of the target cancer cell.
(185) DOTATATE includes a chelator, DOTA, and coordinated metals or radioisotopes. The radioisotope may be coordinated by the cancer targeting composition (e.g., contained, complexed) and may be delivered selectively to the cancer cells. This coordination may be used to minimize side effects of the free radioisotope and/or its radioactive decay products. For example, radiolabeled SSTR-ligands, such as .sup.90Y-DOTATOC or .sup.177Lu-DOTATATE, may be used in the treatment of NETs. Due to its potential for enhanced safety, DOTATATE has been used in numerous clinical trials. See, e.g., Bushnell et. al., 90Y-Edotreotide for Metastatic Carcinoid Refractory to Octreotide, J. Clin. Oncol., 28:1652-1659 (2010); and Kwekkeboom D J, Bakker W H, Kam B L, et al., Treatment of Patients With Gastro-Entero-Pancreatic (GEP) Tumours With The Novel Radiolabelled Somatostatin Analogue [.sup.177Lu-DOTA0,Tyr3] Octreotate, European Journal of Nuclear Medicine and Molecular Imaging, 2003; 30(3):417-422, the entire contents of which are hereby incorporated by reference herein. Experiments indicate positive effects, such as an increased median progression-free survival (mPFS) and increased disease control rates (DCR, proportion of patients with stable disease, partial or complete response).
(186) As described further herein, DOTATATE may chelate both the diagnostic, as well as the precursor radioisotope, and the spent atom after radioactive decay, as well as any atoms in between. For example, DOTATATE may initially chelate the radioisotope, and then retain chelation of the decay product(s) of the radioisotope. This may prevent free (non-chelated) radioisotopes from entering the blood by dissociating from the carrier (DOTATATE). The chelator may also chelate the spent radioisotope after its decay in vivo. This may potentially prevent radioactive and/or toxic free decay atoms from dissociating from the chelator and entering the blood.
(187) 2. DOTAMTATE and TCMCTATE
(188) Other chelators may be used for stable coordination of isotopes, such as DOTAM, TCMC-monoacid, and TCMC (defined further herein). Such chelating agents can coordinate both diagnostic and therapeutic radioisotopes and may be used for treatment of cancer cells. The DOTAM and TCMC are similar to DOTA, with different terminal groups which give them increased coordination stability and increased radiochemical stability properties, for example, when used with certain radioisotopes and targeting moieties. The targeted radiotherapy may use chelators, such as DOTAM and TCMC, in combination with compositions, such as octreotate peptide, that are designed to hold (e.g., prevent, slow dissociation, etc.) of the radioisotope. These compositions seek to selectively deliver the radioisotope to target cancer cells and prevent dissociation of the radioisotope from the chelator.
(189) In particular, cancer treating compositions may include the DOTAM, TCMC, and TCMC-monoacid chelators used in combination with radioisotopes and octreotate peptide targeting moieties to further enhance treatment properties. The radioisotopes, such as .sup.212Pb, .sup.203Pb, .sup.64Cu, and/or other radionuclide α-emitters, have high linear energy transfer (LET) emission and short path lengths that irradiates a short distance, such as within about 1-2 cell diameters, and/or that may not require oxygenation or reproduction to irreversibly damage (e.g., kill) a tumor cell.
(190) As shown herein, these components form stable complexes with isotopes that seek to prevent dissociation of the lead radioisotope from the conjugate under mildly acidic conditions, such as in vivo. Examples herein use .sup.212Pb, .sup.203Pb, or .sup.64Cu as the radioisotope bound to the DOTAM, TCMC, and TCMC-monoacid for the targeted imaging and therapy of cancer. Other radioisotopes may include, for example, iron, cobalt, zinc, and other metals with a density of over about 3.5 g/cm.sup.3.
(191) The DOTAM, TCMC, and TCMC-monoacid based cancer treating compositions may also form stable complexes with other radioisotopes, and therefore selectively deliver the radioisotopes to the cancer cells and prevent their dissociation that could induce cytotoxic effect in normal cells. Due to their properties, such compositions may be used for treatment of NET tumors with specific cancer treatment wherein the isotopes are selectively delivered to the SSTR expressing cancer cells by targeting moieties, such as octreotate, octreotide, or other somatostatin analogs. The octreotate based compounds may be used, for example, for diagnosis of patients with SSTR-positive NETs using γ-emitting isotopes, and/or in treatment of NET patients using β-emitting isotopes (e.g., .sup.177Lu and .sup.90Y). See, e.g., Kwekkeboom, D. J. et. al., Radiolabeled Somatostatin analogue 177Lu-DOTA-tyr3 Octreotate in Patients with Endocrine Gastoentoeropancreatic Tumors, J Clin Oncol 23:2754-2762, (2005); van Essen, M. Krenning E P, et. al, Peptide Receptor Radionuclide Therapy With .sup.177Lu-Octreotate in Patients With Foregut Carcinoid Tumors of Bronchial, Gastric and Thymic Origin, European Jnl. of Nuclear Medicine and Molecular Imaging (2007), the entire contents of which are hereby incorporated by reference herein. In the composition comprising a molecule of Formula (I) or a pharmaceutically acceptable salt thereof, at least one of R.sup.5, R.sup.6, and R.sup.8 is (C.sub.1-C.sub.6)alkyl-C(═O)—N(—R.sup.25)—R.sup.26, which can provide increased coordination stability and increased radiochemical stability properties, for example, when used with certain radioisotopes and targeting moieties.
(192) The radioisotopes may be used, for example, to provide a source of alpha irradiation via indirect emission. The radioisotopes (e.g., .sup.212Pb, .sup.203Pb, .sup.64Cu, etc.) may be combined with chelators (e.g. DOTAM, TCMC, etc.) and targeting moieties (e.g., octreotate), into a cancer targeting composition for rapid uptake of the composition into the cancer cells. The DOTAM and TCMC chelators may be used to avoid dissociation of the radioisotope from the conjugate under mildly acidic conditions, such as within the patient's body.
(193) The targeted cancer treatment may involve the use of radioisotopes bound to the chelators which are bound to the targeting moiety which recognizes and binds to cell surface receptors expressed on (or which are up-regulated on) specific cancer cells. This may cause binding of the radioisotope-chelators to the specific cancer cells, and thus targeted radiation of the specific cancer cell when the radioisotope undergoes radioactive decay.
(194) Treatment (e.g., imaging and/or apoptosis) of cancer cells may involve use of emitters (such as e.g., α (alpha), β (beta), γ (gamma), and/or positron emitting radioisotopes) as the radioisotope(s). The α-emitting radioisotopes may be delivered to targeted cancer cells, e.g., NET via SSTR targeting moieties, such as octreotate or other octreotide derivatives. These α-emitting radioisotopes may be of particular interest because they have a high LET compared to other radioisotopes such as .sup.177Lu, .sup.90Y, and/or other β-emitters, and may deposit their high energy within about a 70 to about a 100 μm long pathway tracking within about 1 to about 2 cancer cell clusters. This high LET radiation may not depend on active cell proliferation or oxygenation, and/or the resulting Deoxyribonucleic acid (DNA) damage caused by α-particles may be more difficult to repair than that caused by β-emitting radioisotopes, due to α-emitting radioisotopes higher LET.
(195) The α-emitting radioisotopes may have an LET that is powerful, and is also generally limited to within the internal region of the cancer cell. The emissions from the α-emitting radioisotopes may also have the ability to cause irreversible damage, such as oxygenation or reproduction, to the cancer cell that does not require waiting for the life cycle of the cancer cell. Further still, α-emitting radioisotopes can cause death and apoptosis of the cancer cells that developed resistance to β-emitter therapy.
(196) The α-emitting radioisotopes may be, for example, produced during decay of lead based radioisotopes, such as .sup.212Pb radioisotopes. The .sup.212Pb is a β-emitting radioisotope with a half-life of about 10.6 hours with a radioactive emission profile having decay products which are α-emitters having the properties of α-emitting radioisotopes. Since .sup.212Pb decays to .sup.212Bi (which is an α-emitting radioisotope having a half-life of about 60 minutes), which decays whether by α-emission to .sup.208Tl (with a half-life of about 3 min), which decays by β-emission to .sup.208Pb (which is stable), or by β-emission to .sup.212Po (with a half-life of about 0.3 μs), which decays by α-emission to 208Pb.
(197) The use of a radioisotope with a relatively long half-life, such as .sup.212Pb having a half-life of about 10.6 hours, may allow for centralized production of radiolabeled compositions at the radiopharmacy and shipment to the clinic where it is administered to the patient. The α-emitter decay of .sup.212Bi may be maximized to occur within the cancer cells, thereby providing maximum alpha radiation damage once inside the cancer cells and their apoptosis and killing of the cancer cell. After α-emission by the .sup.212Bi, the ultimate result is the stable .sup.208Pb.
(198) As indicated by the experimental data provided herein, a combination of certain radioisotopes chelated using DOTAM or TCMC conjugated to octreotide derivative somatostatin receptor targeting moieties provides treatment properties, such as increased radiochemical stability, enhanced binding and increased uptake by cancer cells, and/or high LET emission within cancer cells that results in their apoptosis and/or targeted biodistribution. For example, radiolabeled-octreotate, octreotide conjugates may consist of a SSTR-targeting peptide modified with the chelator (e.g., TCMC, DOTAM) radiolabeled with the β-emitting or α-emitting radioisotope.
(199) Composition
(200)
(201) The radioisotope (or radioactive atom or ion) 102 may be an atom or an ion, such as an α-emitter, a β-emitter, a γ-emitter, a positron emitter, and/or other radioactive emitter, capable of undergoing radioactive decay within the patient. The radioisotope 102 may be, for example, a radioactive emitter, such as .sup.212Pb, .sup.203Pb, .sup.64Cu, .sup.67Cu, .sup.212Bi, and/or other radioactive emitter. Examples of non-limiting radioactive emitters that may be used as the radioisotope include .sup.68Ga, .sup.177Lu, .sup.213Bi, and .sup.90Y. Other example radioisotopes that may be used may include .sup.225Ac, .sup.231Am, .sup.243Am, .sup.211At, .sup.217At, .sup.247Bk, .sup.248Cf, .sup.250Cf, .sup.251Cf, 240Cm, .sup.243Cm, .sup.245Cm, .sup.154Dy, .sup.252Es, .sup.253Es, .sup.255Es, .sup.252Fm, .sup.253Fm, .sup.221Fr, .sup.148Gd, .sup.174Hf, .sup.258Md, .sup.144Nd, .sup.237Np, .sup.186Os, .sup.190Pt, .sup.236Pu, .sup.238Pu, .sup.213Pa, .sup.231Pa, .sup.223Ra, .sup.224Ra, .sup.219Rn, .sup.146Sm, .sup.147Sm, .sup.149Tb, .sup.227Th, .sup.229Th, .sup.230U and/or .sup.236U. Other possible radionuclides may include .sup.45Ti, .sup.59Fe, .sup.60Cu, .sup.61Cu, .sup.62Cu, .sup.67Ga, .sup.89Sr, .sup.86Y, .sup.94mTc, .sup.99mTc, .sup.111In, .sup.149Pm, .sup.153Gd, .sup.153Sm, .sup.166Ho, .sup.186Re, .sup.188Re, or .sup.211At.
(202) The chelator [CA] 104 is a chemical (e.g., organic chemical) capable of binding to the radioisotope 102 and to the targeting moiety 108. The chelator 104 includes a ring structure 110 and multiple terminal groups 112. The chelator 104 may include, for example, a tetraaza ring 110, such as DOTA (1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic acid), DOTAM (1,4,7,10-Tetrakis(carbamoylmethyl)-1,4,7,10-tetraazacyclododecane), TCMC (2-(4-isothiocyanotobenzyl)-1, 4, 7, 10-tetraaza-1, 4, 7, 10-tetra-(2-carbamonyl methyl)-cyclododecane), and/or other chelating agents. When bound with the targeting moiety 108, the chelator 104 may form a compound, such as DOTAMTATE, DOTATATE, TCMCTATE, and/or other chelating compound.
(203) Example chemical structures of chelators 204a-h usable as the chelator 104 are provided in FIGS. 2A1-2B4. FIGS. 2A1-2A4 show example chelators usable with .sup.212Pb, .sup.203Pb, and .sup.212Bi. FIGS. 2B1-2B4 show example chelators usable with .sup.64Cu and .sup.67Cu.
(204) Referring back to
(205) The targeting moiety 108 is a chemical which binds to the cancer cells, such as a somatostatin receptor (SSTR) targeting peptide (somatostatin analog), in the patient. The targeting moiety 108 may be, for example, a peptide, such as octreotate (H-D-Phe-Cys-Phe-D-Trp-Lys-Thr-Cys-Thr-OH, C.sub.49H.sub.64N.sub.10O.sub.11S.sub.2), octreotide (H.sub.2N-D-Phe-Cys-Phe-D-Trp-Lys-Thr-Cys-Thr-ol, C.sub.49H.sub.66N.sub.10O.sub.10S.sub.2), other octreotate/octreotide derivatives, and/or other cancer targeting chemicals.
(206) The targeting moiety 108 may be linked to the chelating agent 104 by a covalent bond 114. The covalent bond may be coupled to an amide group as schematically shown by the solid bond 114, or to another portion of the tetraaza ring structure 110, such as a Carbon, as schematically shown by the dashed bond 114′.
(207) A linker [L]x 116 may also optionally be provided to bind the chelator 104 to the targeting moiety 108. The linker 116 may be, for example, an organic compound, such as an amino acid, alkane, alkyne, etc. Linkers may be selected from the group of amino acids, peptides, amino alcohols, polyethylene glycols, alkanes, alkenes, alkynes, azide aromatic compounds, carbohydrates, carboxylic acids, esters, phospho-organic compounds, and sulfonates. The linker 116 may be defined to provide a spacer between the chelator 104 and targeting moiety 108, for example, to avoid ionic interactions.
(208)
(209) In this version, the terminal groups 112′ and the targeting moiety 108 are both depicted as being an oxygen atom and an R.sup.2 bonded to each nitrogen atom of the ring structure 110′. As indicated in the Legend of
(210) The functional group 304a of
(211) Referring back to
(212) As shown in
(213) While
(214)
(215) In these versions, the targeting moieties 508a,b comprise TOC and TATE, respectively. DOTATOC (or Edotreotide, SMT487, DOTA0-Phe1-Tyr3 octreotide or DOTA-Tyr3-octreotide) has the chemical formula C.sub.65H.sub.92N.sub.14O.sub.18S.sub.2. DOTATATE (or DOTA-TATE or DOTA-octreotate or DOTA-(Tyr.sup.3)-octreotate) is an amide of the acid DOTA which acts as a chelator, and which has the chemical formula C.sub.65H.sub.90N.sub.14O.sub.19S.sub.2. TCMCTATE (described further herein) is a chelator having the chemical formula S-2-(4-isothiocyantobenzl)-1, 4, 7, 10-tetraaza-1, 4, 7, 10=tetra (2-carbamoylmethl) cyclododecane.
(216) DOTAMTOC, DOTAMTATE, and TCMCTATE may be synthesized as described further therein.
(217)
(218) In the DOTATATE cancer targeting composition 600a of
(219) In the DOTAMTATE version of
(220) In the TCMCTATE version of
(221) While
EXAMPLES
(222) Peptide Synthesis:
(223) The examples herein may involve peptide synthesis. Cyclic peptide may be synthesized, for example, via solid-phase peptide synthesis using a fluorenylmethyloxycarbonyl (FMOC) strategy. After cleavage from the solid support, disulfide bond formation can be accomplished with peroxide in tetrahydrofuran (THF) and 5 mM ammonium acetate buffer (NH.sub.4OAc). The final product may be purified by a preparative, such as liquid chromatography-mass spectrometry (LC-MS or HPLC-MS). Examples of synthesis that may be used are described in Schottelius et al, H. J. Wester Tetrahedron Letters vol. 44, pp. 2393-2396 (2003), the entire contents of which is hereby incorporated by reference herein.
(224) The 1,4,7,10-tetraazacyclododecane-1,4,7(2-carbamolymethyl)-10(mono-N-hydroxysuccinimide ester [DOTAM-monocarboxylic acid] may be synthesized by the following: 1. 1,4,7,10-Tetraazacyclododecane-1,4,7-tris (t-butoxycarbonyl) is dissolved in acetonitrile. Potassium carbonate is added. Benzyl bromoacetate is added neat. The solution is stirred at room temperature. After four days, the solids are removed by filtration. The solvent is removed by rotary evaporation at 40° C. The residue is dissolved in dichloromethane and washed with water. The organic layer is dried over sodium sulfate. The drying agent is removed by filtration. The solvent is removed from the filtrate by rotary evaporation. The resulting solid is dried under high vacuum to yield the product. 2. The isolated product from step 1 is dissolved in neat trifluoroacetic acid (TFA). The solution is stirred for 1 day. The TFA is removed by rotary evaporation. The resulting oil is dissolved in water and washed with chloroform. The aqueous layer is basified with sodium hydroxide to pH=1. The product is extracted with chloroform. The organic layer is dried with sodium sulfate. The solution is filtered. The solvent is removed by rotary evaporation. The residue is dried under high vacuum to yield the product as an oil. 3. The isolated product from step 2 is dissolved in ethanol and diisopropylethylamine is added. 2-Bromoacetamide in ethanol is then added and the solution is stirred for ≥4 hours. The solvent is removed by rotary evaporation at 35° C. The oil residue is dissolved in chloroform and any solids that form are filtered and discarded. The solvent is removed from the filtrate by rotary evaporation. The residue is dried under high vacuum for ≥2 hours. The residue is taken in acetone. A solid precipitates. The solids are filtered and washed with cold acetone. The solids are dried under high vacuum to yield the product. 4. The isolated product from step 3 is hydrogenated in water in the presence of 10% Pd (palladium) on activated carbon under 30 psi (207 kPa) of hydrogen pressure. The solution is filtered and the solvent is removed by rotary evaporation. The residue is taken in ethanol and stirred vigorously. The product precipitates. It is filtered and dried under high vacuum.
(225) TCMCTATE may be synthesized by the following: TATE is synthesized by solid phase peptide synthesis (SPPS) and cleaved from the resin without removing the protecting groups of its side chains. TATE is then dissolved in acetonitrile along with diisoproplyethylamine (2× molar excess). A solution of TCMC (Macrocyclics product B-1005) is added and the reaction mixture is stirred at room temperature. Reaction progress is monitored by liquid chromatography-mass spectroscopy (LC/MS). Upon completion the solution is concentrated in vacuo. The protecting groups of the side chains are removed with a cocktail of trifluoroacetic acid and radical scavengers, and then the product is precipitated with diethyl ether. The linear peptide is cyclized in solution and the crude is purified by preparative reversed phase liquid chromatography (RP/LC).
(226) DOTAMTATE may be synthesized by the following: TATE is synthesized by SPPS and DOTAM-monocarboxylic acid (Macrocyclics product B-170) is attached to the peptide while it is still in the resin. The peptide conjugate is cleaved from the resin with a cocktail of trifluoroacetic acid (TFA) and radical scavengers, and the product is precipitated with diethyl ether. The linear peptide is cyclized in solution and the crude is purified by preparative reversed phase liquid chromatography (RP/LC).
(227) DOTAMTOC may be synthesized by the following: TOC is synthesized by SPPS and DOTAM-monocarboxylic acid (Macrocyclics product B-170) is attached to the peptide while it is still in the resin. The peptide conjugate is cleaved from the resin with a cocktail of trifluoroacetic acid (TFA) and radical scavengers, and the product is precipitated with diethyl ether. The linear peptide is cyclized in solution and the crude is purified by preparative reversed phase liquid chromatography (RP/LC).
(228) TCMCTOC may be synthesized by the following: TOC is synthesized by solid phase peptide synthesis (SPPS) and cleaved from the resin without removing the protecting groups of its side chains. TOC is then dissolved in acetonitrile along with diisoproplyethylamine (2× molar excess). A solution of TCMC (Macrocyclics product B-1005) is added and the reaction mixture is stirred at room temperature. Reaction progress is monitored by liquid chromatography-mass spectroscopy (LC/MS). Upon completion the solution is concentrated in vacuo. The protecting groups of the side chains are removed with a cocktail of trifluoroacetic acid and radical scavengers, and then the product is precipitated with diethyl ether. The linear peptide is cyclized in solution and the crude is purified by preparative reversed phase liquid chromatography (RP/LC).
(229) Experiment 1—Radioisotope Binding to Chelator
(230)
(231) In particular,
(232) These graphs also demonstrate post-labeling to determine the radiochemical yield and radiochemical stability of the agent. The .sup.203Pb-DOTAMTATE is synthesized with a radiochemical yield greater than or equal to 99.9%. The peak in all three chromatographs 700a-c indicates a high radiochemical stability for .sup.203Pb-DOTAMTATE. In particular, since there are no secondary peaks indicating free .sup.203Pb, the chromatographs indicate a radiochemical yield of ≥98% for up to at least 24 h post-labeling. As demonstrated by these graphs, the .sup.203Pb DOTAMTATE remains radiochemically and chemically stable over time for the duration of the tests.
(233)
(234) The experiments in
(235) Experiment 2—Radioisotope Uptake
(236)
(237) The TCMCTATE and DOTAMTATE chelators indicate stable chelation of both .sup.203Pb and .sup.64Cu isotopes. The graph 900 shows that the SSTR-selectivity of both .sup.203Pb-labeled and .sup.64Cu-labeled TCMCTATE and DOTAMTATE conjugates with specificity toward AR42J cancer cell lines (which express the SSTR). The .sup.64Cu-conjugates show a similar rate of uptake and accumulation in AR42J cell lines as the .sup.203Pb-conjugates and a similar selectivity toward SSTR in AR42J cell line. The in vitro accumulation of .sup.203Pb-DOTAMTATE and .sup.203Pb-TCMCTATE in the AR42J cancer cell line are, respectively, 21.4±2.26% ID/mg and 33.41±0.49% ID/mg. Similar trends in accumulation of both are observed for their .sup.64Cu-labeled analogs, including the accumulation of .sup.64Cu-DOTAMTATE is 33.41±0.49% ID/mg, and the accumulation for .sup.64Cu-TCMCTATE is 41.59±1.79% ID/mg. This indicates that radiolabeled DOTAMTATE and TCMCTATE selectively accumulate in SSTR expressing cancer cells.
(238)
(239)
(240)
(241) .sup.203Pb-TCMCTATE is prepared by labeling of the TCMCTATE (10 μg) with either 37 MBq (1 mCi), 152 MBq (4.1 mCi) or 233 MBq (6.3 mCi) of the .sup.203Pb radioisotope. The .sup.203Pb-DOTAMTATE is prepared by labeling of DOTAMTATE (5 Gg) with either 5.1 MBq (0.14 mCi), 21.4 MBq (0.58 mCi) or 26.6 MBq (0.72 mCi) of the .sup.203Pb isotope. The .sup.203Pb-TCMC without a targeting moiety serves as a negative control in these studies.
(242) The increased accumulation of .sup.203Pb-TCMCTATE and .sup.203Pb-DOTAMTATE in AR42J cells measured in CPM/mg of cells correlates with increasing amounts of octreotate conjugates added to the tested cells (0.018 μg, 0029 μg and 0.12 μg for TCMCTATE and 0.108 μg and 0.453 μg for DOTAMTATE). The bars represent values of the CPM per mg of cells (background corrected). The lines represent values of the CPM/mg of cells per mg of peptide conjugates used in the studies. As may be seen from the similar slopes of lines, both .sup.203Pb-DOTAMTATE and .sup.203Pb-TCMCTATE behave in similar manners with increasing concentration.
(243)
(244) In More Detail
(245) Biodistribution Study in Athymic Mice Bearing AR42J Xenografts
(246) Methods:
(247) Female athymic nude mice (˜20 g) are injected subcutaneously with 2×10.sup.6 AR42J cells in 50% RPMI media and 50% Matrigel. Tumors are grown until an approximate tumor volume of 300 mm.sup.3 is reached. Doses of .sup.212Pb-DOTAMTATE are prepared (5 μCi) in phosphate buffered saline (PBS) and 200 μl is administered to the mice via intravenous injection. The animals are sacrificed at predetermined timepoints of 1 hour, 4 hours and 24 hours post drug injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to 12×55 mm polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected.
(248) Results and Conclusions:
(249) Tumor uptake exceeded 20% one hour after drug administration and remained constant through 4 and 24 hours. Other non-target organs showed the highest accumulation of drug at 1-hour post-injection but decreased significantly by 24 hours post administration. The pancreas and kidneys are the two organs with the highest non-target uptake but these organs also showed significantly less accumulation by 24 hours post-injection. This observation is not of concern based on the toxicology and efficacy data we have accumulated thus far. In addition, these organs have also shown high drug uptake in other nonclinical rodent studies involving alpha emitters which have not translated into adverse effects in human studies (Kratochwil et al., 2014; Norenberg et al., 2006).
(250) Experiment 3—Biodistribution
(251)
(252)
(253) Both the .sup.203Pb-DOTAMTATE and .sup.203Pb-TCMCTATE show limited or no uptake in bone marrow, liver, or other organs, thereby indicating radiochemical stability of these particular cancer targeting compositions. The kidneys have increased accumulation of agents, while the retention of the cancer targeting compositions in other organs is lower than 2% ID/g (% of initial dose per gram of organ). Both compositions have similar pharmacokinetic properties and high radiochemical stability indicated by limited/no uptake of agents by bone marrow, liver and lung. In particular, the kidneys have higher retention of .sup.203Pb-labeled TCMCTATE and .sup.203Pb-DOTAMTATE at 23.53±1.54% ID/g and 9.79±2.9% ID/g, respectively. The high kidney retention of radiolabeled DOTATATE analogs reduces by co-administration of positively charged amino-acids during peptide receptor radionuclide therapy (PRRT). This indicates that the radioisotope remains tightly bound to the chelator-targeting moiety within the body, and that the cancer targeting composition does not bind to non-targeted cells.
(254) In comparison,
(255) As may be seen by comparing
(256)
(257)
(258) Similarly,
(259) As may be seen from
(260)
(261) In More Detail
(262) .sup.203Pb-DOTAMTATE Biodistribution in Athymic Nude Mice
(263) .sup.203Pb-DOTAMTATE is examined by our group in both animal and human models and the use of .sup.203Pb-DOTAMTATE as a surrogate for .sup.212Pb-DOTAMTATE is the subject of a recent eIND (130,960).
(264) Methods:
(265) Female athymic nude mice (˜20 g) are injected with a single dose of .sup.203Pb-DOTAMTATE. Specifically, 10 μCi of .sup.203Pb-DOTAMTATE is diluted in PBS and 100 μl is administered to the mice via intravenous injection. The animals are sacrificed at predetermined time points of 4 hr, 24 hours and 48 hours post drug injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected.
(266) Results and Conclusion:
(267) Referring to
(268)
(269) In More Detail
(270) Biodistribution of .sup.212Pb-DOTAMTATE in Male and Female Non-Tumor Bearing Mice
(271) As a basis for selecting female mice for numerous studies and particularly in the GLP toxicity study, an extensive literature search is conducted to support that there is little difference between male and female mice. Furthermore, what little difference is observed shows higher sensitivity in female mice suggesting they would be the worst-case scenario between the two sexes (Lipnick et al., 1995) and as a result are more commonly used in safety evaluation (OECD, 2000).
(272) Several clinical studies of .sup.68Ga-DOTATATE PET/CT showed no differences in radiotracer distribution and its organ retention between male and female patients. However, the recent retrospective evaluation of data of 161 patients enrolled the clinical studies of .sup.68Ga-DOTATATE PET/CT showed age and sex-related variations in the radiotracer accumulation in some organs (Watts, Singh, Shukla, Sharma, & Mittal, 2014). Female patients (n=31) demonstrated (p<0.05) higher standardized uptake value (SUV) in pituitary, thyroid, parotids, spleen and kidneys as compared to males (n=34).
(273) The renal radioactivity in female rats injected with 111In-DTPA-octreotide showed a different localization pattern. Female rats showed higher uptake in the outer medulla compared with the cortex (Melis et al., 2007).
(274) The kidney retention of radiotherapeutic agent can result in nephrotoxicity and kidney failure. The selection of female mice for toxicity studies allows a determination of the effect of .sup.212Pb-DOTAMTATE on the kidney function especially in case of anticipated of higher retention of agent in female.
(275) To better illustrate how this particular radiotherapeutic agent, .sup.212Pb-DOTAMTATE, is similar between male and female mice, a biodistribution is conducted at two predetermined time points in CD-1 non-tumor bearing mice.
(276) Methods:
(277) Male and female CD-1 mice (˜20 g) are injected with a single dose of .sup.212Pb-DOTAMTATE. Specifically, 5 μCi of .sup.212Pb-DOTAMTATE is diluted in PBS and 100 μl is administered to the mice via intravenous injection. The animals are sacrificed at predetermined time points of 4 hours and 24 hours post drug injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected.
(278) Results and Conclusions:
(279) Referring to
(280) Experiment 4—Efficacy
(281)
(282)
(283)
(284)
(285) Based on the results of in vitro uptake in AR42J cells, competition studies with DOTATATE and the similar biodistribution profile of DOTATATE, DOTAMTATE, and TCMCTATE, including similar renal clearance, DOTAMTATE and TCMCTATE may be considered for further investigation in the exploratory clinical studies of cancer targeting compositions.
(286) While the experiments provided herein use certain radioisotopes, the present disclosure is intended to apply to compositions including a variety of other radioisotopes. For example, the LET of α-emitting radioisotopes is such that they irradiate an area approximately of the size of a cancer cell or small cluster of cancer cells. This indicates that little to no excess radiation may be emitted beyond the targeted cancer cells(s). In comparison, other radioactive emissions can travel for long distances within a body, damaging non-targeted cells.
(287) Additionally, because the data herein indicates the ability of the chelator, such as DOTAM, to coordinate the lead radioisotopes, the substitution of radioisotopes may be considered insignificant. As discussed herein, DOTAM and TCMC show limited to no dissociation of lead radioisotopes compared to other chelators, such as DOTA. This further indicates that stability of the radioisotope coordination by these chelators may be extrapolated to binding of the chelator to the radioisotope.
(288)
(289) The kit may also contain an optional scavenger (e.g., diethylenetriamino-pentaacetic (DTPA), Ethylene Diamine Tetraacetic Acid (EDTA), DOTA, etc.) 1126 and/or antioxidant 1128 (e.g., ascorbic acid, gentisic acid, ethanol, vitamin C, etc.). Various additives may optionally be provided as needed for various applications. As also indicated by the diagram, the composition may be mixed alone or in combination with the other components and administered to the patient.
(290) The method may also involve optional mixing and/or heating. The temperature and duration of the heating may change based on the components of the kit. For example, when the chelator is DOTAM, the mixture may be heated to room temperature for 15 minutes. In another example, when the chelator is DOTA, the mixture may be heated to 85° C. for 15 minutes.
(291) The kits may be used, for example, for preparing a radiopharmaceutical preparation. The kit may include a sealed vial or bag, or any other kind of appropriate container, containing a predetermined quantity of the composition. The components of the kit may be in any appropriate form, such as in liquid, frozen, dry form, and/or lyophilized form.
(292)
(293) The method also involves 2232—administering the cancer targeting composition to a patient having the cancer cells, 2234—binding the targeting moiety to the cancer cells, 2236—uptaking the cancer targeting composition within the cancer cells, 2238—decaying the radioisotope by emitting a beta particle, and 2242—eliminating the cancer targeting composition from the patient. The decaying 2238 may involve decaying .sup.212Pb to .sup.212Bi by emitting the beta particle and decaying the .sup.212Bi to .sup.208Ti by emitting an alpha particle, decaying occurs within the cancer cells, and/or 2240—killing the cancer cells with the alpha particle.
(294) In More Detail
(295) Efficacy Study in Ar42J Xenograft Bearing Athymic Nude Mice Treated with .sup.212Pb-DOTAMTATE
(296) Methods:
(297) Two million (2×10.sup.6) AR42J cells are implanted subcutaneously into the right flank of each mouse and tumors grew until an approximate tumor volume of 300 mm.sup.3 is reached. Animals are then injected with 100 μl of 5 μCi or 10 μCi of .sup.212Pb-DOTAMTATE, cold DOTAMTATE or PBS. Animals are monitored daily and calipered three times per week to monitor tumor volume. Mice are sacrificed when tumor volumes reached 2000 mm.sup.3 or other predetermined termination criteria are met (weight loss over 15% for two consecutive days, serious bleeding, necrosis or ulceration of the tumor, scruffiness or lack of grooming over 5 days, lethargy over 3 days, weakness/balance issues over 5 days, hunchback appearance, diarrhea or hypothermia).
(298) After three weeks, two-thirds of the remaining animals from the .sup.212Pb-DOTAMTATE 10 μCi or .sup.212Pb-DOTAMTATE 5 μCi groups receive a second round of injections with 10 μCi or 5 μCi of .sup.212Pb-DOTAMTATE respectively. Monitoring and tumor volume data is collected for these mice as described above. Animals are maintained until a tumor volume of 2000 mm.sup.3 or termination criteria mentioned above are met.
(299) Three weeks later, one-half of the animals remaining in the 2×10 μCi .sup.212Pb-DOTAMTATE receive a third injection of 10 μCi of .sup.212Pb-DOTAMTATE. Monitoring and tumor volume data is collected for these mice as described above. Animals are maintained until a tumor volume of 2000 mm.sup.3 or termination criteria mentioned above we met. Study is completed at 29 weeks post first injection.
(300) Results and Conclusions:
(301) Animals that are injected with cold-DOTAMTATE had a median survival of 3.4 weeks post injection. Animals that are treated with PBS only had a similar median survival at 3.5 weeks post injection. Mice that receive 1 injection of 5 μCi .sup.212Pb-DOTAMTATE have a median survival of 6.3 weeks while mice who receive 1 injection of 10 μCi .sup.212Pb-DOTAMTATE have a median survival of 8.5 weeks showing that a higher dose has a more efficacious effect. Animals who receive 2 injections of 5 μCi .sup.212Pb-DOTAMTATE have a median survival of 7.1 weeks. The median survival time is similar between animals that receive 1×10 μCi vs 2×5 μCi of drug. Mice who receive 2 injections of 10 μCi .sup.212Pb-DOTAMTATE had a median survival of 10.9 weeks with 20% of the mice tumor free at the end of the study. Mice who receive 3×10 μCi injections had a median survival of 11.6 weeks with 33% of the animals in this group being tumor free at the conclusion of the study (6 months). This suggests a dose dependent efficacious effect with repeat injections at levels where a single injection may have been toxic (see study NET0016). Kaplan-Meier survival curves summarizes the survival for each of the injection groups.
(302) .sup.212Pb-DOTAMTATE Binding Efficiency to SSTR Expressing Cells
(303) Methods:
(304) Peptide binding to somatostatin receptors 2 (SSTR2) and K.sub.d is evaluated in SSTR2 expressing AR42J cells by growing 250,000 cells into the wells of a 24-well plate for 48 hrs. Concentrations from 0.5 nM to 64 nM of .sup.212Pb-DOTAMTATE are incubated in the AR42J containing wells for 10 minutes at 37° C. Four replicates are performed for each concentration. Cells are then washed with PBS and cells from each well are counted for presence of radioactivity. Binding curves are then created and K.sub.d calculated.
(305) Results and Conclusions:
(306) Referring to
(307) Cytotoxic Effect of .sup.212Pb-DOTAMTATE on SSTR Expressing Cells
(308) Methods:
(309) Thirty-thousand (3×10.sup.4) AR42J cells are grown in the wells of a 96 well plate for 2 days. Cells are then incubated for 4 hours with increasing doses of .sup.212Pb-DOTAMTATE ranging from 0 nCi/ml to 800 nCi/ml. Eight wells per group are treated. Cells are washed with PBS to remove drug and then fresh media is introduced. Cells are allowed to incubate for 6 days at 37° C. Cells are then rinsed and incubated with fluorescein diacetate for 30 minutes and read with a fluorimeter at 485/535 nm. Percentage of viable cells is calculated based on untreated cells as a control.
(310) Results and Conclusions:
(311) With reference to
(312) Correlation Between AR42J Tumor Volume and Drug Uptake
(313) Methods:
(314) AR42J tumor volumes in athymic nude mice from the study presented NET001 are calculated by measuring ½×length×width.sup.2 with digital calipers on the day of drug administration. As shown in
(315) Results and Conclusions:
(316) Referring to
(317) Receptor Saturation does not Occur with Decreased Specific Activity in Athymic Nude Mice
(318) Methods:
(319) Female athymic nude mice (˜20 g) are injected subcutaneously with 2×10.sup.6 AR42J cells in 50% RPMI media and 50% Matrigel. Tumors are grown until an approximate tumor volume of 300 mm.sup.3 is reached. Doses of .sup.212Pb-DOTAMTATE are prepared (10 μCi) at three different specific activities in PBS. 200 μl is administered to the mice via intravenous injection. The animals are sacrificed at 24 hours post drug injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected.
(320) Results and Conclusions:
(321) Referring to
(322) Efficacy Study in Ar42J Xenograft Bearing Athymic Nude Mice Treated with .sup.212Pb-DOTAMTATE at Treatment Cycles of Two Weeks and Three Weeks
(323) Methods:
(324) Two million (2×10.sup.6) AR42J cells are implanted subcutaneously into the right flank of each mouse and tumors grew until an approximate tumor volume of 200-300 mm.sup.3 is reached. Animals are then injected with 100 μl of 10 μCi .sup.212Pb-DOTAMTATE or saline. Animals are monitored daily and calipered three times per week to monitor tumor volume. Mice are sacrificed when tumor volumes reached 3000 mm.sup.3 or other predetermined termination criteria are met (weight loss over 15% for two consecutive days or 20% weight loss from initial weight, serious bleeding, necrosis or ulceration of the tumor, scruffiness or lack of grooming over 5 days, lethargy over 3 days, weakness/balance issues over 5 days, hunchback appearance, diarrhea or hypothermia).
(325) After two or three weeks, the animals receive a second dose of 10 μCi .sup.212Pb-DOTAMTATE. Monitoring and tumor volume data is collected for these mice as described above. Animals are maintained until a tumor volume of 3000 mm.sup.3 or termination criteria mentioned above are met.
(326) Two or three weeks later, the animals receive 10 μCi of .sup.212Pb-DOTAMTATE. Monitoring and tumor volume data is collected for these mice as described above. Animals are maintained until a tumor volume of 3000 mm3 or termination criteria mentioned above we met. The study is ongoing.
(327) Results and Conclusions:
(328) Referring to
(329) Animal Blood Pharmacokinetics of IV Injected .sup.212Pb-DOTAMTATE in CD-1 Mice
(330) Methods:
(331) CD-1 mice are injected with 10 μCi of .sup.212Pb-DOTAMTATE as part of a biodistribution study. Blood is collected at 15 minutes; 1 hour and 4 hours post injection. Body weights determined by taking the average of 10 CD-1 mice at 7 weeks old, the age of the mice in this study and using this weight, blood volume is estimated using the equation by Lee and Blaufox (1985). % ID in blood mice is then calculated for 5 mice per group.
(332) Results and Conclusions:
(333) Referring to
(334) TABLE-US-00001 TABLE 1 Average % ID of .sup.212Pb-DOTAMTATE in blood of CD-1 mice Hours Average SD n .25 6.7 1.3 5 1 1.8 0.4 5 4 0.1 0.1 5
Biodistribution of .sup.212Pb-DOTAMTATE in Female Non-Tumor Bearing Mice
(335) Distribution of the .sup.212Pb-DOTAMTATE is assessed in a biodistribution study with CD-1 non-tumor bearing mice at multiple timepoints between 15 minutes and 48 hours.
(336) Methods:
(337) Female CD-1 mice (˜20 g) are injected with a single dose of .sup.212Pb-DOTAMTATE. Specifically, 10 μCi of .sup.212Pb-DOTAMTATE is diluted in PBS and 100 μl is administered to the mice via intravenous injection. The animals are sacrificed at predetermined time points of 15 minutes, 1 hour, 4 hours and 24 hours and 48 hours post drug injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected.
(338) Results and Conclusions:
(339) Referring to
(340) Biodistribution of .sup.203Pb-DOTAMTATE and .sup.212Pb-DOTAMTATE in CD-1 Non-Tumor Bearing Mice
(341) Methods:
(342) Female CD-1 mice (˜20 g) are injected with a single dose of .sup.203Pb-DOTAMTATE or .sup.212Pb-DOTAMTATE. Specifically, 10 μCi of .sup.203Pb-DOTAMTATE or .sup.212Pb-DOTAMTATE is diluted in saline and 100 μl is administered to the mice via intravenous injection. The animals are sacrificed at predetermined time points of 4 hr and 24 hours post drug injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to 12×55 mm polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected, wherein “% ID” means percent injection dosage.
(343) Results and Conclusion:
(344) Referring to
(345) Based on these data and others, an exploratory eIND (Exploratory Investigational New Drug) is conducted to assess the dosimetry and biodistribution of .sup.203Pb-DOTAMTATE in patients with somatostatin expressing neuroendocrine cancers as a surrogate for .sup.212Pb-DOTAMTATE. The distribution and excretion characteristics of .sup.203Pb-DOTAMTATE is very similar to PK (pharmacokinetics) properties of commercially available octreotate drugs with the kidneys being the dose limiting organ.
(346) .sup.212Pb-DOTAMTATE Cumulative Excretion
(347) Methods:
(348) Female, CD-1 mice are injected intravenously with 10 μCi of .sup.212Pb-DOTAMTATE. Animals are then placed into individual metabolic cages to facilitate excretion collection. At predetermined intervals of 1 hour, 2 hours, 3 hours, 4 hours, 5 hours, 6 hours and 24 hours' post injection animals are removed from metabolic cage and placed in to a new metabolic cage. Cage funnels are then rinsed with PBS and 1 ml from each mouse is counted in an auto gamma counter. Feces are collected and analyzed in a separate auto gamma counter tube.
(349) Results and Conclusions:
(350) Referring to
(351) Biodistribution of .sup.212Pb-DOTAMTATE with Kidney Protection Agents
(352) It is not anticipated that .sup.212Pb-DOTAMTATE will interact with major molecular pharmacokinetic determinants such as enzymes, drug transporters, or orphan nuclear receptors. However, renal toxicity has been a reported concern with high dose radionuclide therapy. Co-infusion of the drug with positively charged amino acids is shown to reduce kidney dose of radiolabeled octreotide by 25% (Hammond et al., 1993). As a result, a kidney protection study is conducted with .sup.212Pb-DOTAMTATE and various agents to determine if the exposure to the kidneys could be minimized during treatment.
(353) Methods:
(354) Female CD-1 mice (˜20 g) are injected with a single dose of .sup.212Pb-DOTAMTATE. Specifically, 5 μCi of .sup.212Pb-DOTAMTATE is diluted in PBS (control), 2.5% Lysine-Arginine mixture, Aminomedix (600 mg/kg Lys-Arg, 15 mg/kg amifostine is diluted in half in PBS) or 4.2% Clinisol and is administered to the mice via intravenous injection. The animals are sacrificed at predetermined timepoints of 1 hour and 4 hours post injection. Tissues are collected from each animal and evaluated for amount of radioactive material in each organ by auto gamma counter. Specifically, organs are harvested, weighed and transferred to polypropylene tubes. The tubes are placed in a calibrated Wizard2 γ-counter (PerkinElmer, Shelton, Conn.) and counted for three minutes (204-274 keV). A standard consisting of one-twentieth of the injection volume is counted with each time point. The background is automatically subtracted from the counts. The standard is also used for decay correction. % ID/g is calculated for each organ collected.
(355) Results and Conclusions:
(356) Referring to
(357) Non-GLP Dose Range Finding Study in Athymic Nude Mice
(358) Methods:
(359) Female athymic nude mice (˜20 g) are injected with a single dose of 10 μCi, 20 μCi, 40 μCi or 60 μCi of .sup.212Pb-DOTAMTATE or control PBS intravenously. Five animals are assigned per treatment group. Animals are weighed three times per week and monitored daily for signs of termination criteria (15% weight loss over 2 days, lack of grooming over 5 days, lethargy/weakness over 3 days, reduced motility, hunched back, diarrhea, hypothermia). The study is concluded after 4 weeks.
(360) Results and Conclusions:
(361) Referring to
(362) Intravenous Injection (IV) and Intraperitoneal Injection (IP) Toxicity Study of Free .sup.212Pb in Mice
(363) The purpose of this study is to evaluate and assess the in vivo acute and chronic toxicity of free .sup.212Pb when administered via intravenous injection or intraperitoneal injection to Balb/c mice. Animals are sacrificed on Day 7 (acute) and Day 90 (chronic) to assess the acute and delayed occurrence of test article-induced effects, including the impact of the radionuclide given under a “worst-case” scenario of total radiolabeling chelation sequestration failure. Both intravenous injection and intraperitoneal injection administration routes are studied despite the fact that the former is not a planned use of the radionuclide, to exaggerate any potential toxicity and to identify target organs.
(364) Results:
(365) Administration of the test article by single IV or IP injection at dose levels of above or equal to 2.5 μCi is associated with acute (by Day 7) marked decreases in hematology parameters indicative of bone marrow toxicity. Furthermore, there is renal damage indicative of radiation-induced nephrotoxicity and possibly some hepatic injury at the highest doses. The findings in this study indicate that 2.5 μCi is the NOAEL for free .sup.212Pb in mice for both the IV and IP routes of administration, with mortality occurring at IV doses of 20 μCi and at IP doses of 15 μCi.
(366) There is no mortality at 2.5, 5, 7.5, and 10 μCi by either IV or IP route. However, mortality occurs at 15 μCi IP on Days 11, 40, and 90 (three often animals), and at 20 μCi IV on Day 16 (two of five animals). Mortality also occurs at 10 μCi on Day 69 (one of five animals), at μCi on Days 8, 11, and an unrecorded date (three of four animals), and at 50 μCi on Day 9 (three of five animals) for the IP route. Body weight loss is observed at Day 7 following IV administration at doses of 20 and 30 μCi; the change is significant when comparing IV dosing at 2.5 vs. 30 μCi (P<0.01) or at 7.5 vs. 30 μCi (P<0.05). While no further loss had occurred by Day 90, the significance of weight loss at 30 μCi persisted at the later time point (P<0.01 vs. untreated control). At both time points, body weights correlates inversely with IV dose level. While some weight loss is also observed at Day 7 following IP administration at 10 μCi and higher, the effects are not significant. Recovery in body weight is seen by Day 90, although attenuation of weight gain becomes significant at 15 μCi, IP (P<0.05 vs. untreated control).
(367) Dose-related decreases in hematology parameters occurred in both IV and IP groups. At Day 7, there is a dose-related decrease in the mean values for White Blood Cells and platelet numbers following both IV and IP administration starting at the lowest dose level (2.5 μCi). There is partial recovery at 90 days in all groups. In general, clinical chemistry levels remained within normal ranges, with the exception of the liver parameters ALT (Alanine Amino Transferase) and AST (Aspartate Amino Transferase), which appears to be somewhat increased at 90 days in the high-dose group. Renal parameters are within normal limits.
(368) Target organs for this study are bone marrow, kidneys, and liver. The histopathologic findings in this study indicate that both IV and IP administration of the test article at 5 μCi or above is associated with expected decreases in the erythroid, myeloid, and megakaryocytic series in the bone marrow and is associated with corresponding changes in the hematology parameters. There is also nephritic change at both 7 and 90 days, consistent with radiation-induced nephropathy (Cohen & Robbins, 2003), which, over time, may lead to irreversible renal failure and anemia due to erythropoietin insufficiency. The kidney, while having a substantial capacity for repair, is a radiosensitive organ, and irreversible nephrotoxicity may occur with radiation treatment. Hepatic changes, considered to be possibly treatment-related, are evident at both 7 and 90 days and are associated with increases in ALT and AST at 90 days, 50 μCi IP.
(369) Conclusion:
(370) Administration of .sup.212Pb by single IV or IP injection at dose levels of above or equal to 2.5 μCi is associated with marked decreases in hematology parameters indicative of bone marrow toxicity. Furthermore, there is renal damage indicative of radiation-induced nephrotoxicity and possibly some hepatic injury at the highest doses. The findings in this study indicate that 2.5 μCi is the NOAEL for both the IV and IP routes of administration, with mortality occurring starting at IV doses of 20 μCi and at IP doses of 15, 30, 40, and 50 μCi.
(371) There is no mortality at 2.5, 5, 7.5, and 10 μCi by either IV or IP route. However, mortality occurs at 15 μCi IP on Days 11, 40, and 90 (three often animals), and at 20 μCi IV on Day 16 (two of five animals). Mortality also occurs at 30 μCi on Day 69 (one of five animals), at μCi on Days 8, 11, and an unrecorded date (three of four animals), and at 50 μCi on Day 9 (three of five animals) for the IP route. Among the mice utilized for the hematology blood draws, all mice in the IV-injected groups survive the 90-day study period. In the IP-injected groups, mortality occurs at 30 μCi on Day 69 (one of five animals), at 40 μCi on Days 10 and 16 (two of five animals) and at 50 μCi on days 7, 10, and 16 (three, one, and one of five animals, respectively). Body weight loss is observed at Day 7 following IV administration at doses of 20 and 30 μCi; the change is significant when comparing IV dosing at 2.5 vs. 30 μCi (P<0.01) or at 7.5 vs. 30 μCi (P<0.05). While no further loss had occurred by Day 90, the significance of weight loss at 30 μCi persists at the later time point (P<0.01 vs. untreated control). At both time points, body weights correlates inversely with IV dose level. While some weight loss is also observed at Day 7 following IP administration at 10 μCi and higher, these effects are not significant. Recovery in body weight is seen by Day 90, although attenuation of weight gain became significant at 15 μCi, IP (P<0.05 vs. untreated control).
(372) Marked dose-related decreases in hematology parameters occurred in both IV and IP groups. At Day 7, a dose-related decrease in the mean values for WBCs and platelet numbers is observed following either IV or IP administration, even at the lowest dose level (2.5 μCi). There is partial recovery at 90 days in all groups, although high variability in values is seen within groups (among animals). In general, clinical chemistry levels remain within normal ranges, with the exception of the liver parameters, ALT and AST, which appear to be increased at 90 days in the high-dose group. Renal parameters are within normal limits. Target organs for this study are bone marrow, kidneys, and possibly liver. Histopathologic findings in this study indicate that both IV and IP administration of the .sup.212Pb at 5 μCi or above is associated with expected decreases in the erythroid, myeloid, and megakaryocytic series in the bone marrow and is associated with corresponding changes in the hematology parameters. There is also nephritic change at both 7 and 90 days consistent with radiation-induced nephropathy (Cohen & Robbins, 2003), which, over time, may lead to irreversible renal failure and anemia due to erythropoietin insufficiency. The kidney, while having a substantial capacity for repair, is a radiosensitive organ, and irreversible nephrotoxicity may occur with radiation treatment. Hepatic changes, considered to be possibly treatment-related, are evident at both 7 and 90 days and are associated with increases in ALT and AST at 90 days 50 μCi IP. Particularly careful examination is conducted on the bladder, lungs, intestines, and lymphoid system, and no treatment-related findings are detected in these other organs. There are no changes considered to be due to (elemental) lead toxicity.
(373) Repeat-Dose Toxicity
(374) Methods:
(375) Female, tumor free CD-1 mice are injected with one dose of 40 μCi .sup.212Pb-DOTAMTATE, 2 doses of 20 μCi .sup.212Pb-DOTAMTATE or three doses of 15 μCi .sup.212Pb-DOTAMTATE. Animals are given three weeks between doses for these who received multiple treatments. Animals are weighed three times per week and monitored daily for signs of termination criteria (15% weight loss over 2 days or 20% loss from initial weight, lack of grooming over 5 days, lethargy/weakness over 3 days, reduced motility, hunched back, diarrhea, hypothermia). Blood for hematological analysis is collected weekly.
(376) Results and Conclusion:
(377) Signs of acute toxicity are examined in a non-GLP repeat dose study to compare single administration vs fractionation (described below). This study is designed based on observations made in athymic nude mice. While a 40 μCi dose in an athymic nude mouse is severely toxic resulting in 100% of the animal reaching termination criteria in 8 days, and 40 μCi administered as two separate 20 μCi injections three weeks apart result in the same toxicity profile, however three 15 μCi injections three weeks apart do not show significant or irreversible signs of toxicity. This observation is correlated with the GLP findings that hematological toxicity in the surviving animals from the higher dose groups is recoverable within a month. As renal and hepatic toxicity is cumulative a single dose treatment vs multiple doses leading to the same cumulative dose should be similar (Barendsen, 1964). Fractionated administration of radioactivity three weeks apart compared to a single injection had very similar toxicity profile. Based on these results, a new study is done to compare these 3 dosing regimens in tumor free CD-1 mice.
(378) The fractionated dose vs single dose of .sup.212Pb-DOTAMTATE toxicity study is performed in tumor-free CD-1 mice (
(379) Biodistribution Study of .sup.212Pb-DOTATOC in CD-1 Mice
(380) Method:
(381) .sup.212Pb-DOTATOC is prepared based on activity needed at time of injection. 4.1 ng of peptide per 10 μCi of .sup.212Pb into a tube is added. The mixture is incubated for 10 minutes at 50° C. with shaking. ITLC (Instant thin layer chromatography) is used to verify that chelation is >95%. 100 μl of .sup.212Pb-DOTATOC is intravenously injected into the tail of each mouse. An auto gamma counter is used to determine the counts of each organ and control tube.
(382) Results:
(383) A biodistribution is conducted with 10 μCi of .sup.212Pb-DOTATOC at 30 minutes and 4 hours in female, CD-1 non-tumor bearing mice. The data (
(384) Combination Therapy Efficacy Study in Ar42J Xenograft Bearing Athymic Nude Mice Treated with Adrucil® and .sup.212Pb-DOTAMTATE at Treatment Cycles of Two Weeks and Three Weeks
(385) Methods:
(386) Athymic nude mice are given AR42J tumors and allowed to grow until tumors reach about 300 mm.sup.3. Mice in treatment groups are injected with 100 μl of 15 mg/kg ADRUCIL® once weekly for a total of nine injections. 10 μCi of .sup.212Pb-DOTAMTATE is given at either 2 week or 3 week intervals for a total of 3 treatments. The .sup.212Pb-DOTAMTATE is given within 24 hours after an ADRUCIL® treatment. 10 μCi per 4.1 ng peptide is used, and the cumulative injection dose is 30 μCi. The animals are monitored daily, and calipered and weighed 3 times per week. The animals are sacrificed when termination criteria are met.
(387) Results:
(388) 1.sup.st injections
(389) TABLE-US-00002 .sup.212Pb-DOTAMTATE ITLC - Free Lead 2.5% Actual injected dose 10.4 μCi
(390) 2.sup.nd injections—2 week group
(391) TABLE-US-00003 .sup.212Pb-DOTAMTATE ITLC - Free Lead 1% Actual injected dose 10.6 μCi
(392) 2.sup.nd injections—3 week group
(393) TABLE-US-00004 .sup.212Pb-DOTAMTATE ITLC - Free Lead 2% Actual injected dose 10.9 μCi
(394) 3.sup.rd injections—2 week group
(395) TABLE-US-00005 .sup.212Pb-DOTAMTATE ITLC - Free Lead 2.4% Actual injected dose 9.2 μCi
(396) 3.sup.rd injections—3 week group
(397) TABLE-US-00006 .sup.212Pb-DOTAMTATE ITLC- Free Lead 1.5% Actual injected dose 10.4 μCi
(398) Referring to
(399) Interestingly, the better efficacy is observed by decreasing the time between injections of .sup.212Pb-DOTAMTATE. The treatment group that received 3×10 μCi of .sup.212Pb-DOTAMTATE at 2-week intervals had a median survival rate of 11.9 weeks with 46% of the animals still remaining at 21 weeks post cell injection. The highest efficacy is observed when mice are treated with radiosensitizer ADRUCIL® and .sup.212Pb-DOTAMTATE at 2-week intervals. 85% of the animals are alive at 21 weeks post cell injection with all tumors under the limit of quantification of 200 mm.sup.3.
(400) Dosimetry and Bio-Distribution of .sup.203Pb-DOTAMTATE in Patients with Somatostatin Expressing Neuroendocrine Tumors
(401) Method:
(402) Total of 6 patients are enrolled in the first-in-human open-label, single-dose, dosimetry and bio-distribution of .sup.203Pb-DOTAMTATE.
(403) All patients (1 female and 5 male) receive an average dose of 4.94 (4.66-5.26) mCi of .sup.203Pb-DOTAM-TATE and undergo 1 hour, 4 hour, 24 hour and 48 hour post injection SPECT-CT scans. Ethnicity of all 6 patients is Caucasian.
(404) Pharmacokinetic data from .sup.203Pb-DOTAMTATE imaging are used to calculate the absorbed dose from .sup.203Pb-DOTAMTATE imaging. The data is then extrapolated to calculate the expected tissue absorbed doses following the administration of .sup.212Pb-DOTAMTATE for future Targeted Alpha particle Therapy (TAT).
(405) According to the measured data obtained from the dosimetry of .sup.203Pb-DOTAM-TATE the kidneys and liver receives the highest absorbed doses, averaging 19 and 17 mGy/MBq, respectively, for .sup.212Pb when a Relative Biological Effectiveness (RBE) of 3 is used for the α-particle emissions of .sup.212Bi and .sup.212Po. Experience from external beam radiotherapy suggests that 18-23 Gy to the whole kidney volume gives a 5% risk of kidney injury in 5 years. The liver can tolerate 27-30 Gy (twice daily fractions, 1.5 Gy per fraction). Although the spleen receives the highest absorbed dose it is not a dose-limiting organ since it is not a vital organ. The dose to bone marrow, lungs, heart wall, osteogenic cells and spleen at this administered activity would be 1.6, 2.5, 3.7, 0.5 and 31 Gy, respectively. Except for spleen, for which toxicity limit is not well established, these doses are all below toxicity limits for these organs.
(406) Comparison of .sup.68Ga-DOTATATE PET/CT and .sup.203Pb-DOTAMTATE SPECT/CT Scans
(407) Reports of these two imaging modalities are independently read by two nuclear medicine physicians blinded to the results of the other study for 6 enrolled patients. Total number of 177 lesions in 6 patients are detected by .sup.68Ga-DOTATATE scan while 109 lesions are detectable by .sup.203Pb-DOTAMTATE. There is a very close correlation (with correlation coefficient of 0.89) between lesions detected by these two modalities. Total discovered lesions per organ is comparable in visceral (42 versus 38) and nodal (12 versus 13) but not for skeletal lesions (123 versus 58). It seems that .sup.68Ga PET/CT scan is more sensitive to detect bone lesions in axial skeleton (vertebrae, bony thorax, bony pelvis) area (total of 95) as compared to .sup.203Pb-DOTAMTATE (total of 34).
(408) Results:
(409) There is no statistically significant difference observed between the .sup.68Ga DOTATATE PET/CT and .sup.203Pb-DOTAMTATE SPECT/CT, thereby indicating that .sup.68Ga DOTATATE can be used in lieu of .sup.203Pb-SPECT/CT to evaluate the eligibility of patients undergoing Targeted Alpha Therapy (TAT) with .sup.212Pb-DOTAMTATE.
(410) Based on the dosimetry analysis the maximum theoretical absorbed dose estimate to kidneys is 23 Gy which corresponds to cumulative dose of 32.7 mCi of .sup.212Pb-DOTAM-TATE (10.9 mCi per therapy cycle for a total of 3 cycles).
(411) The methods herein may be performed in any order and repeated as desired.
(412) While the embodiments are described with reference to various implementations and exploitations, it will be understood that these embodiments are illustrative and that the scope of the inventive subject matter is not limited to them. Many variations, modifications, additions and improvements are possible. For example, various combinations of part or all of the techniques described herein may be performed.
(413) Plural instances may be provided for components, operations or structures described herein as a single instance. In general, structures and functionality presented as separate components in the exemplary configurations may be implemented as a combined structure or component. Similarly, structures and functionality presented as a single component may be implemented as separate components. These and other variations, modifications, additions, and improvements may fall within the scope of the inventive subject matter.
(414) Insofar as the description above and the accompanying drawings disclose any additional subject matter that is not within the scope of the claim(s) herein, the inventions are not dedicated to the public and the right to file one or more applications to claim such additional invention is reserved. Although a very narrow claim may be presented herein, it should be recognized the scope of this invention is much broader than presented by the claim(s). Broader claims may be submitted in an application that claims the benefit of priority from this application.