Vaccine RNA-peptide against SARS-CoV-2 with endogenous exosomes as carrier
11246922 · 2022-02-15
Assignee
Inventors
Cpc classification
A61K39/215
HUMAN NECESSITIES
C12N2770/20034
CHEMISTRY; METALLURGY
International classification
Abstract
A vaccine RNA-peptide against SARS-CoV-2, which has a messenger ribonucleic acid (mRNA) having an open reading frame encoding a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein. The peptide of the severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein is fused to a synthetic poly ADP-ribose polymerase peptide. The vaccine RNA-peptide against SARS-CoV-2 has endogenous exosomes as carrier.
Claims
1. A composition against SARS-CoV-2, comprising a micro ribonucleic acid (miRNA) fused to a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein having an amino acid sequence of SEQ ID NO: 2 wherein endogenous exosomes act as carrier.
2. The composition against SARS-CoV-2 according to claim 1, wherein the miRNA comprises a poly-A sequence.
3. The composition against SARS-CoV-2 according to claim 1, wherein the poly-A sequence is about 10 adenosine nucleotides.
4. The composition against SARS-CoV-2 according to claim 1, wherein the miRNA comprises the nucleic acid sequence of SEQ ID NO: 1.
5. The composition against SARS-CoV-2 according to claim 1, wherein the peptide of the SARS-CoV-2 surface protein of SEQ ID: 2 is fused to a synthetic poly ADP-ribose polymerase peptide.
6. A method for stimulating an immune response against SARS-CoV-2 in a subject comprising administering to said subject an effective amount of the composition of claim 1.
7. A composition against SARS-CoV-2, comprising a micro ribonucleic acid (miRNA) fused to a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein having the amino acid sequence of SEQ ID NO: 2 fused to a synthetic poly ADP-ribose polymerase peptide.
8. The composition against SARS-CoV-2 according to claim 7, wherein the miRNA comprises a poly-A sequence.
9. The composition against SARS-CoV-2 according to claim 7, wherein the poly-A sequence is about 10 adenosine nucleosides.
10. The composition against SARS-CoV-2 according to claim 7, wherein the miRNA comprises the nucleic acid sequence of SEQ ID NO: 1.
11. The composition against SARS-CoV-2 according to claim 7, wherein the synthetic poly ADP-ribose polymerase peptide comprises the amino acid sequence of SEQ ID NO: 3.
12. The composition against SARS-CoV-2 according to claim 7, wherein the micro ribonucleic acid (miRNA) is fused to a peptide that comprises the amino acid sequence of SEQ ID NO: 4.
13. A method for stimulating an immune response against SARS-CoV-2 in a subject in need thereof comprising administering to said subject an effective amount of the composition of claim 7.
14. A composition against SARS-CoV-2 comprising a micro ribonucleic acid (miRNA) having a nucleic acid sequence of SEQ ID NO: 1 fused to a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein fused to a synthetic poly ADP-ribose polymerase peptide that comprises the amino acid sequence of SEQ ID NO: 4, wherein endogenous exosomes act as carrier.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
(1) With the above and other related objects in view, the invention consists in the details of construction and combination of parts as will be more fully understood from the following description, when read in conjunction with the accompanying drawings in which:
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DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT
(94) Present invention is a vaccine RNA-peptide against SARS-CoV-2 with therapeutic action using endogenous exosomes as carrier adjuvant.
(95) In one embodiment, the vaccine RNA-peptide against SARS-CoV-2 comprises a micro ribonucleic acid (mRNA) fused to a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein wherein endogenous exosomes act as carrier.
(96) The vaccine RNA-peptide against SARS-CoV-2 comprising the micro ribonucleic acid (miRNA) fused to the peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein is here also referred as “RNA-peptide-A” vaccine.
(97) The peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein is also here referred as peptide SARS-CoV-2 (peptide A), which has SEQ ID No: 2.
(98) The mRNA comprises a poly-A sequence. In a preferred embodiment, the poly-A sequence is about 10 adenosine nucleotides.
(99) In a preferred embodiment, the miRNA comprises the nucleic acid sequence of SEQ ID NO: 1.
(100) TABLE-US-00002 SEQ ID NO: 1 AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG
(101) Poly-A sequence about 10 adenosine nucleotides is related with a better affinity of the mRNA to endogenous exosomes acting as carrier according to the present invention.
(102) The peptide of the SARS-CoV-2 surface protein is chemically modified.
(103) The term “chemically modified” refers to a modification to the polyprotein of Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) sequence, wherein a fragment of the sequence is modified to CVN-DTF-AGSTFISDEV-D (SEQ ID NO: 2).
(104) The CVN-DTF-AGSTFISDEV-D (SEQ ID NO: 2) is selected as peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein (peptide SARS-CoV-2) target.
(105) In a preferred embodiment, the peptide of the SARS-CoV-2 surface protein, also referred as peptide SARS-CoV-2, and peptide A, comprises the amino acid sequence of SEQ ID NO: 2.
(106) TABLE-US-00003 SEQ ID NO: 2 CVNDTFAGSTFISDEVD Size = 17 aa, MW = 1819.91 daltons
(107) In another preferred embodiment, the peptide of the SARS-CoV-2 surface protein is fused to a synthetic poly ADP-ribose polymerase peptide also here referred as PARP1 peptide (peptide B).
(108) Example 1, shows a preferred realization of the synthesis process of the peptide A, peptide B, and peptide AB according to the present invention.
(109) In another embodiment, present invention is referred to a vaccine RNA-peptide against SARS-CoV-2 comprising a micro ribonucleic acid (miRNA) fused to a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein fused to a synthetic poly ADP-ribose polymerase peptide.
(110) The mRNA comprises a poly-A sequence, wherein the poly-A sequence is about 10 adenosine nucleosides.
(111) In a preferred embodiment, the mRNA comprises the nucleic acid sequence of SEQ ID NO: 1.
(112) In a preferred embodiment, the peptide of the SARS-CoV-2 surface protein comprises the amino acid sequence of SEQ ID NO: 2.
(113) The vaccine RNA-peptide against SARS-CoV-2 comprising the micro ribonucleic acid (miRNA) fused to the peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein fused to the synthetic poly ADP-ribose polymerase peptide is also here referred as “RNA-peptide-AB” vaccine.
(114) MHC class I molecules bind the synthetic poly ADP-ribose polymerase peptide, also referred as, peptide-B (SEQ ID NO: 3) GVDEVAKKKSK (Size=11 aa) generated by hydrolysis of RNA-peptide after apoptosis induction for caspase 3 or caspase 7 in infected cell with SARS-CoV-2. The sequence of origin was from RNA-peptide-AB:
(115) TABLE-US-00004 SEQ ID NO: 1 and SEQ ID NO: 4 5′AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG-Cys-Val- Asn-Asp-Thr-Phe-Ala-Gly-Ser-Thr-Phe-Ile-Ser-Asp- Glu-Val-Asp-Gly-Val-Asp Glu-Val-Ala-Lys-Lys-Lys- Ser-Lys (Size = 34 nt, Size = 28 aa)
(116) In a preferred embodiment, the open reading frame encodes a peptide comprising the amino acid sequence of SEQ ID NO: 4.
(117) TABLE-US-00005 SEQ ID NO: 4 CVNDTFAGSTFISDEVDGVDEVAKKKSK
(118) In a preferred embodiment, the vaccine RNA-peptide against SARS-CoV-2 comprises endogenous exosomes as carrier.
(119) In one embodiment, a method for treating of SARS-CoV-2 in a subject in need thereof comprises administering an effective amount of the RNA-peptide-AB vaccine.
(120) In a preferred embodiment, an effective amount of the composition of the vaccine RNA-peptide comprising micro ribonucleic acid (miRNA) fused to a peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-COV2) surface protein fused to a synthetic poly ADP-ribose polymerase peptide is between about 135 μg/μL and 299 μg/μL.
(121) In one embodiment, a method for treating SARS-CoV-2 in a subject in need thereof comprises administering to the subject an effective amount of a vaccine RNA-peptide against SARS-CoV-2 comprising a micro ribonucleic acid (miRNA) comprising an open reading frame encoding the peptide of the Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein fused to a synthetic poly ADP-ribose polymerase peptide, wherein endogenous exosomes are the carrier. In a preferred embodiment, the miRNA comprises the nucleic acid sequence of SEQ ID NO: 1 and the open reading frame encodes the peptide comprising the amino acid sequence of SEQ ID NO: 4.
(122) The results and efficacy of the vaccine RNA-peptide-A and RNA-peptide-AB of the present invention are showed in Example 9 tables 52 to 59.
(123) In one embodiment, a method for preventing/treating SARS-CoV-2 in a subject comprises administering to the subject a single dose of the RNA-peptide-A/RNA-peptide-AB vaccine of the present invention.
(124) In one embodiment, a method for preventing/treating SARS-CoV-2 in a subject comprises administering to the subject a second dose of the RNA-peptide-A/RNA-peptide-AB vaccine of the present invention.
(125) In one embodiment, a method for preventing/treating SARS-CoV-2 in a subject comprises administering to the subject a third dose of the RNA-peptide-A/RNA-peptide-AB vaccine of the present invention.
(126) As seen in
(127) Given the role that the MHC class I antigen presentation pathway plays in the detection of virally infected cells by CTLs, cell infected by SARS-CoV-2 in MHC class I expose the peptide-B, size 11 aa, and active the elimination of infected cells.
(128) In addition, MHC class II proteins usually accommodate peptides of 13-25 amino acids in length in their open binding groove.
(129) Present invention is also related with a method of stimulating an immune response against SARS-CoV-2 in a subject administering the RNA-peptide-A vaccine. The results and efficacy of the RNA-peptide-A vaccine of the present invention are showed in Example 9 tables 52 to 59.
(130) MHC class II molecules bind the peptide of the SARS-CoV-2 surface protein, also referred as peptide-A (SEQ ID NO: 2), generated by hydrolysis of RNA-peptide after apoptosis induction for caspase 3 or caspase 7 in infected cell with SARS-CoV-2.
(131) TABLE-US-00006 SEQ ID NO: 1 and SEQ ID NO: 2 5′AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG- Cys-Val-Asn-Thr-Phe-Ala-Gly-Ser-Phe-Ser- Glu-Val-Asp (Size = 17 aa)
(132) Given the role that the MHC Class II molecules normally found only on professional antigen-presenting cells such as dendritic cells, mononuclear phagocytes, some endothelial cells, thymic epithelial cells, and B cells. These cells are important in initiating immune responses. Cell infected by SARS-CoV-2 in MHC class II expose the RNA-peptide-A, size 17 aa, and active the pathways action of immune system.
(133) Another object of the present invention is the algorithm by which vaccine RNA-peptide of the present invention was achieved.
(134) The algorithms of present invention are a tool that allows predicting the stability of hybrid oligonucleotide and protein molecules in their most simplified expression of cDNA/RNA and peptide. This hybrid molecule has a high affinity for exosomes, allowing its extracellular transport from cell to cell. These chimeras in cDNA-peptide or RNA-peptide have a specific biological action with antiviral efficacy due to their chemical structure, since they participate in the viral pathway's replication. On the other hand, they present specific antigenic structures that can involve immune responses.
(135) The target peptide and the oligonucleotide are molecules selected according to the three following parameters: 1. Fusion Stability (FS); where FS>80%
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)] 2. Exosome Affinity (EA); where EA>95%
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size Poly
A+RNA primer)]
EA=(ro) 3. Biological Action (BA); where 0.5<BA<2.0
BA=EA/FS
BA=(ro/cruz) 3.1. Optimal Biological Action (OBA); where 0.8<OBA<1.3
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(136) 1) How to Design the Target RNA
(137) The polyadenylation of RNA primer gives it larger molecular stability and a longer half-life due to the action of oligonuclease enzymes. It has been selected as target RNA that may implication in the metabolic pathways of SARS-CoV-2 virogenesis.
(138) Avian infectious bronchitis virus (IBV) is an enveloped virus with a positive-stranded RNA genome. IBV is a member of the genus Gammacoronavirus, family Coronaviridae and is an important viral pathogen in the poultry industry. It causes a highly contagious disease in chickens, mainly affecting the respiratory and reproductive tract.
(139) After research in literature (Table 1) the avian infectious bronchitis virus was selected as target in RNA primers as immune representative model of SARS-CoV-2.
(140) TABLE-US-00007 TABLE 1 Cell miRNA Species type/tissue Infection Findings MiR-34c Human CD4+ T-cells HIV T-cell activation, facilitates virus replication [17] Human HeLa Flaviviruses Inhibits virus replication, Wnt/Notch/ IFN- mediated [18] Chicken Trachea Influenza A Upregulated upon virus H5N3 infection [19] Human A549 Influenza A Enhances virus virus replication [20] MiR-34b Chicken Spleen ALV Promotes virus replication by targeting MDA5 [37] Human Throat swab Influenza B Upregulated upon virus Influenza B virus infection [21] Chicken Spleen Marek's Upregulated in virus- disease resistant line [22] Human Huh7.5 HCV HCV Facilitates virus replication [23] Chicken Trachea Influenza A Upregulated upon virus H5N3 infection [19] MiR- Chicken Cecum Salmonella Upregulated upon 1788 S. Typhimurium infection [24] MiR- Chicken DF- 1 & NDV Enhances virus 203a embryo replication and embryonic death [25] Pig LFBK-avβ6 FMDV Inhibits FMDV replication [26] Human HEPG2 HBV Upregulated upon infection, induces inflammation [27] Human HEPG2 HCV Downregulated .fwdarw. EMT & carcinogenesis [28] Human Nasal RSV Upregulated in RSV- mucosa positive infants [29] MiR- Human HEPG2 HBV Downregulated upon 200a infection .fwdarw. cell division & invasion [30] Chicken Intestine Marek's Upregulated in virus- disease susceptible line [22] MiR- Human CNE1AKATA EBV Induces EBV lytic 200b reactivation [38] Chicken Intestine Marek's Upregulated in virus- disease susceptible line [29] MiR-429 Human EBV-293 EBV Induces EBV lytic reactivation [31] Human Nasal RSV Downregulated in mucosa RSV-positive infants [29] Chicken Intestine Marek's Upregulated in virus- disease susceptible line [22] MiR-1b Chicken Trachea & Influenza A Upregulated upon lung virus H5N3 infection [19] MiR- Chicken Cecum Salmonella Upregulated upon S. 133c enterica infection [32] MiR- Monkey Vero DENV Suppresses viral 133a replication [33] MiR-1a Chicken Kidney IBV Upregulated upon viral infection [38] Chicken Trachea & Influenza A Upregulated upon lung virus H5N3 infection [19] MiR- Dog Lung Influenza A May inhibit innate 133b virus immunity, increasing pathogenicity [34] MiR-206 Chicken Lung Influenza A Downregulated upon virus infection [35] Pig Lung Influenza A Upregulated upon virus H1N2 infection [36] Chicken Trachea & Influenza A Upregulated in lung; lung virus downregulated in trachea (upon H5N3 infection) [19] MiR-499 Chicken Spleen Marek's Upregulated in virus- disease resistant line [22] Chicken Trachea Influenza A Upregulated upon virus] H5N3 infection [19]
(141) Identification of RNA Target
(142) Potential target genes of DE miRNAs were identified using the TargetScan 7.1 and miRBD web platforms. Only targets identified by both programs were considered significant.
(143) A novel insight into the complex interaction between IBV and the chicken host, and specifically the factors that could modulate the human immune response to IBV infection is studied. The results contribute with ribonucleic acid (RNA) involved in IBV infection and pathogenesis.
(144) Based on published data on COVID-19, a preventive vaccine is designed in Silico aimed to protect against COVID-19 infection and transmission. One aim of this is to better understand potential dormant repositories of outbreaks and potential spread of those repositories, together with potential geogenic terrain factors. As mRNA target, are used primers from Kemp V. “miRNA repertoire and host immune factor regulation upon avian coronavirus infection in eggs”: primers Biolegio, Nijmegen, The Netherlands.
(145) The analysis identified a miRNA-peptide with theoretical fusion value stability FS=84.81 cruz, EA=99.15 ro and BA=1.17 to treat COVID-19.
(146) The miRNA selected comprises the nucleic acid sequence as seen in Table 2.
(147) TABLE-US-00008 TABLE 2 SEQ ID NO. Sequence SEQ ID AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG NO: 1
(148) 2) How to Select the Target Protein (Peptide)
(149) Search the epitope that starts with C and finishes with DEV (aa)
(150) Sequence: QQX03240.1
(151) Length: 7101aa
(152) QQX03240.1 ORFlab polyprotein [Severe acute respiratory syndrome coronavirus 2]
(153) TABLE-US-00009 SEQ ID NO: 5 MESLVPGFNEKTHVQLSLPVLQVRDVLVRGFGDSVEEVLSEARQHLKDG TCGLVEVEKGVLPQLEQPYVFIKRSDARTAPHGHVMVELVAELEGIQYG RSGETLGVLVPHVGEIPVAYRKVLLRKNGNKGAGGHSYGADLKSFDLGD ELGTDPYEDFQENWNTKHSSGVTRELMRELNGGAYTRYVDNNFCGPDGY PLECIKDLLARAGKASCTLSEQLDFIDTKRGVYCCREHEHEIAWYTERS EKSYELQTPFEIKLAKKFDIFNGECPNFVFPLNSIIKTIQPRVEKKKLD GFMGRIRSVYPVASPNECNQMCLSTLMKCDHCGETSWQTGDFVKATCEF CGTENLTKEGATTCGYLPQNAVVKIYCPACHNSEVGPEHSLAEYHNESG LKTILRKGGRTIAFGGCVFSYVGCHNKCAYWVPRASANIGCNHTGVVGE GSEGLNDNLLEILQKEKVNINIVGDFKLNEEIAIILASFSASTSAFVET VKGLDYKAFKQIVESCGNFKVTKGKAKKGAWNIGEQKSILSPLYAFASE AARVVRSIFSRTLETAQNSVRVLQKAAITILDGISQYSLRLIDAMMFTS DLATNNLVVMAYITGGVVQLTSQWLTNIFGTVYEKLKPVLDWLEEKFKE GVEFLRDGWEIVKFISTCACEIVGGQIVTCAKEIKESVQTFFKLVNKFL ALCADSIIIGGAKLKALNLGETFVTHSKGLYRKCVKSREETGLLMPLKA PKEIIFLEGETLPTEVLTEEVVLKTGDLQPLEQPTSEAVEAPLVGTPVC INGLMLLEIKDTEKYCALAPNMMVTNNTFTLKGGAPTKVTFGDDTVIEV QGYKSVNITFELDERIDKVLNEKCSAYTVELGTEVNEFACVVADAVIKT LQPVSELLTPLGIDLDEWSMATYYLFDESGEFKLASHMYCSFYPPDEDE EEGDCEEEEFEPSTQYEYGTEDDYQGKPLEFGATSAALQPENPHLEEEQ EEDWLDDDSQQTVGQQDGSEDNQTTTIQTIVEVQPQLEMELTPVVQTIE VNSFSGYLKLTDNVYIKNADIVEEAKKVKPTVVVNAANVYLKHGGGVAG ALNKATNNAMQVESDDYIATNGPLKVGGSCVLSGHNLAKHCLHVVGPNV NKGEDIQLLKSAYENFNQHEVLLAPLLSAGIFGADPIHSLRVCVDTVRT NVYLAVFDKNLYDKLVSSFLEMKSEKQVEQKIAEIPKEEVKPFITESKP SVEQRKQDDKKIKACVEEVTTTLEETKFLTENLLLYIDINGNLHPDSAT LVSDIDITFLKKDAPYIVGDVVQEGVLTAVVIPTKKAGGTTEMLAKALR KVPTDNYMYPGQGLNGYTVEEAKTVLKKCKSAFYILPSIISNEKQEILG TVSWNLREMLAHAEETRKLMPVCVETKAIVSTIQRKYKGIKIQEGVVDY GARFYFYTSKTTVASLINTLNDLNETLVTMPLGYVTHGLNLEEAARYMR SLKVPATVSVSSPDAVTAYNGYLTSSSKTPEEHFIETISLAGSYKDWSY SGQSTQLGIEFLKRGDKSVYYTSNPTTFHLDGEVITFDNLKTLLSLREV RTIKVFTTVDNINLHTQVVDMSMTYGQQFGPTYLDGADVTKIKPHNSHE GKTFYVLPNDDTLRVEAFEYYHTTDPSFLGRYMSALNHTKKWKYPQVNG LTSIKWADNNCYLATALLTLQQIELKFNPPALQDAYYRARAGEAANFCA LILAYCNKTVGELGDVRETMSYLFQHANLDSCKRVLNVVCKTCGQQQTT LKGVEAVMYMGTLSYEQFKKGVQIPCTCGKQATKYLVQQESPFVMMSAP PAQYELKHGTFTCASEYTGNYQCGHYKHITSKETLYCIDGALLTKSSEY KGPITDVFYKENSYTTTIKPVTYKLDGVVCTEIDPKLDNYYKKDNSYFT EQPIDLVPNQPYPNASFDNFKFVCDNIKFADDLNQLTGYKKPASRELKV TFFPDLNGDVVAIDYKHYTPSFKKGAKLLHKPIVWHVNNATNKATYKPN TWCIRCLWSTKPVETSNSFDVLKSEDAQGMDNLACEDLKPVSEEVVENP TIQKDVLECNVKTTEVVGDIILKPANNSLKITEEVGHTDLMAAYVDNSS LTIKKPNELSRVLGLKTLATHGLAAVNSVPWDTIANYAKPFLNKVVSTT TNIVTRCLNRVCTNYMPYFFTLLLQLCTFTRSTNSRIKASMPTTIAKNT VKSVGKFCLEASFNYLKSPNFSKLINIIIWFLLLSVCLGSLIYSTAALG VLMSNLGMPSYCTGYREGYLNSTNVTIATYCTGSIPCSVCLSGLDSLDT YPSLETIQITISSFKWDLTAFGLVAEWFLAYILFTRFFYVLGLAAIMQL FFSYFAVHFISNSWLMWLIINLVQMAPISAMVRMYIFFASFYYVWKSYV HVVDGCNSSTCMMCYKRNRATRVECTTIVNGVRRSFYVYANGGKGFCKL HNWNCVNCDTFCAGSTFISDEVARDLSLQFKRPINPTDQSSYIVDSVTV KNGSIHLYFDKAGQKTYERHSLSHFVNLDNLRANNTKGSLPINVIVFDG KSKCEESSAKSASVYYSQLMCQPILLLDQALVSDVGDSAEVAVKMFDAY VNTFSSTFNVPMEKLKTLVATAEAELAKNVSLDNVLSTFISAARQGFVD SDVETKDVVECLKLSHQSDIEVTGDSCNNYMLTYNKVENMTPRDLGACI DCSARHINAQVAKSHNIALIWNVKDFMSLSEQLRKQIRSAAKKNNLPFK LTCATTRQVVNVVTTKIALKGGKIVNNWLKQLIKVTLVFLFVAAIFYLI IPVHVMSKHTDFSSEIIGYKAIDGGVTRDIASTDTCFANKHADFDTWFS QRGGSYTNDKACPLIAAVITREVGFVVPGLPGTILRTTNGDFLHFLPRV FSAVGNICYTPSKLIEYTDFATSACVLAAECTIFKDASGKPVPYCYDTN VLEGSVAYESLRPDTRYVLMDGSIIQFPNTYLEGSVRVVWFDSEYCRHG TCERSEAGVCVSTSGRWVLNNDYYRSLPGVFCGVDAVNLLTNMFTPLIQ PIGALDISASIVAGGIVAIVVTCLAYYFMRFRRAFGEYSHVVAFNTLLF LMSFTVLCLTPVYSFLPGVYSVIYLYLTFYLTNDVSFLAHIQWMVMFTP LVPFWITIAYIICISTKHFYWFFSNYLKRRVVFNGVSFSTFEEAALCTF LLNKEMYLKLRSDVLLPLTQYNRYLALYNKYKYFSGAMDTTSYREAACC HLAKALNDFSNSGSDVLYQPPQTSITSAVLQSGFRKMAFPSGKVEGCMV QVTCGTTTLNGLWLDDVVYCPRHVICTSEDMLNPNYEDLLIRKSNHNFL VQAGNVQLRVIGHSMQNCVLKFKVDTANPKTPKYKFVRIQPGQTFSVLA CYNGSPSGVYQCAMRPNFTIKGSFLNGSCGSVGFNIDYDCVSFCYMHHM ELPTGVHAGTDLEGNFYGPFVDRQTAQAAGTDTTITVNVLAWLYAAVIN GDRWFLNRFTITLNDFNLVAMKYNYEPLTQDHVDILGPLSAQTGIAVLD MCASLKELLQNGMNGRTILGSALLEDEFTPFDVVRQCSGVTFQSAVKRT IKGTHHWLLLTILTSLLVLVQSTQWSLFFFLYENAFLPFAMGIIAMSAF AMMFVKHKHAFLCLFLLPSLATVAYFNMVYMPASWVMRIMTWLDMVDTS LSGFKLKDCVMYASAVVLLILMTARTVYDDGARRVWTLMNVLTLVYKVY YGNALDQAISMWALIISVTSNYSGVVTTVMFLARGIVFMCVEYCPIFFI TGNTLQCIMLVYCFLGYFCTCYFGLFCLLNRYFRLTLGVYDYLVSTQEF RYMNSQGLLPPKNSIDAFKLNIKLLGVGGKPCIKVATVQSKMSDVKCTS VVLLSVLQQLRVESSSKLWAQCVQLHNDILLAKDTTEAFEKMVSLLSVL LSMQGAVDINKLCEEMLDNRATLQAIASEFSSLPSYAAFATAQEAYEQA VANGDSEVVLKKLKKSLNVAKSEFDRDAAMQRKLEKMADQAMTQMYKQA RSEDKRAKVTSAMQIMLFTMLRKLDNDALNNIINNARDGCVPLNIIPLT TAAKLMVVIPDYNTYKNTCDGTTFTYASALWEIQQVVDADSKIVQLSEI SMDNSPNLAWPLIVTALRANSAVKLQNNELSPVALRQMSCAAGTTQTAC TDDNALAYYNTTKGGRFVLALLSDLQDLKWARFPKSDGTGTIYTELEPP CRFVTDTPKGPKVKYLYFIKGLNNLNRGMVLGSLAATVRLQAGNATEVP ANSTVLSFCAFAVDAAKAYKDYLASGGQPITNCVKMLCTHTGTGQAITV TPEANMDQESFGGASCCLYCRCHIDHPNPKGFCDLKGKYVQIPTTCAND PVGFTLKNTVCTVCGMWKGYGCSCDQLREPMLQSADAQSFLNRVCGVSA ARLTPCGTGTSTDVVYRAFDIYNDKVAGFAKFLKTNCCRFQEKDEDDNL IDSYFVVKRHTFSNYQHEETIYNLLKDCPAVAKHDFFKFRIDGDMVPHI SRQRLTKYTMADLVYALRHFDEGNCDTLKEILVTYNCCDDDYFNKKDWY DFVENPDILRVYANLGERVRQALLKTVQFCDAMRNAGIVGVLTLDNQDL NGNWYDFGDFIQTTPGSGVPVVDSYYSLLMPILTLTRALTAESHVDTDL TKPYIKWDLLKYDFTEERLKLFDRYFKYWDQTYHPNCVNCLDDRCILHC ANFNVLFSTVFPLTSFGPLVRKIFVDGVPFVVSTGYHFRELGVVHNQDV NLHSSRLSFKELLVYAADPAMHAASGNULDKRTTCFSVAALTNNVAFQT VKPGNFNKDFYDFAVSKGFFKEGSSVELKHFFFAQDGNAAISDYDYYRY NLPTMCDIRQLLFVVEVVDKYFDCYDGGCINANQVIVNNLDKSAGFPFN KWGKARLYYDSMSYEDQDALFAYTKRNVIPTITQMNLKYAISAKNRART VAGVSICSTMTNRQFHQKLLKSIAATRGATVVIGTSKFYGGWHNMLKTV YSDVENPHLMGWDYPKCDRAMPNMLRIMASLVLARKHTTCCSLSHRFYR LANECAQVLSEMVMCGGSLYVKPGGTSSGDATTAYANSVFNICQAVTAN VNALLSTDGNKIADKYVRNLQHRLYECLYRNRDVDTDFVNEFYAYLRKH FSMMILSDDAVVCFNSTYASQGLVASIKNFKSVLYYQNNVFMSEAKCWT ETDLTKGPHEFCSQHTMLVKQGDDYVYLPYPDPSRILGAGCFVDDIVKT DGTLMIERFVSLAIDAYPLTKHPNQEYADVFHLYLQYIRKLHDELTGHM LDMYSVMLTNDNTSRYWEPEFYEAMYTPHTVLQAVGACVLCNSQTSLRC GACIRRPFLCCKCCYDHVISTSHKLVLSVNPYVCNAPGCDVTDVTQLYL GGMSYYCKSHKPPISFPLCANGQVFGLYKNTCVGSDNVTDFNAIATCDW TNAGDYILANTCTERLKLFAAETLKATEETFKLSYGIATVREVLSDREL HLSWEVGKPRPPLNRNYVFTGYRVTKNSKVQIGEYTFEKGDYGDAVVYR GTTTYKLNVGDYFVLTSHTVMPLSAPTLVPQEHYVRITGLYPTLNISDE FSSNVANYQKVGMQKYSTLQGPPGTGKSHFAIGLALYYPSARIVYTACS HAAVDALCEKALKYLPIDKCSRIIPARARVECFDKFKVNSTLEQYVFCT VNALPETTADIVVFDEISMATNYDLSVVNARLRAKHYVYIGDPAQLPAP RTLLTKGTLEPEYFNSVCRLMKTIGPDMFLGTCRRCPAEIVDTVSALVY DNKLKAHKDKSAQCFKMFYKGVIMHDVSSAINRPQIGVVREFLTRNPAW RKAVFISPYNSQNAVASKILGLPTQTVDSSQGSEYDYVIFTQTTETAHS CNVNRFNVAITRAKVGILCIMSDRDLYDKLQFTSLEIPRRNVATLQAEN VTGLFKDCSKVITGLHPTQAPTHLSVDTKFKTEGLCVDIPGIPKDMTYR RLISMMGFKMNYQVNGYPNMFITREEAIRHVRAWIGFDVEGCHATREAV GTNLPLQLGFSTGVNLVAVPTGYVDTPDNTDFSRVSAKPPPGDQFKHLI PLMYKGLPWNVVRIKIVQMLSDTLKNLSDRVVFVLWAHGFELTSMKYFV KIGPERTCCLCDRRATCFSTASDTYACWHHSIGFDYVYNPFMIDVQQWG FTGNLQSNHDLYCQVHGNAHVASCDAIMTRCLAVHECFVKRVDWTIEYP IIGDELKINAACRKVQHMVVKAALLADKFPVLHDIGNPKAIKCVPQADV EWKFYDAQPCSDKAYKIEELFYSYATHSDKFTDGVCLFWNCNVDRYPAN SIVCRFDTRVLSNLNLPGCDGGSLYVNKHAFHTPAFDKSAFVNLKQLPF FYYSDSPCESHGKQVVSDIDYVPLKSATCITRCNLGGAVCRHHANEYRL YLDAYNMMISAGFSLWVYKQFDTYNLWNTFTRLQSLENVAFNVVNKGHF DGQQGEVPVSIINNTVYTKVDGVDVELFENKTTLPVNVAFELWAKRNIK PVPEVKILNNLGVDIAANTVIWDYKRDAPAHISTIGVCSMTDIAKKPTE TICAPLTVFFDGRVDGQVDLFRNARNGVLITEGSVKGLQPSVGPKQASL NGVTLIGEAVKTQFNYYKKVDGVVQQLPETYFTQSRNLQEFKPRSQMEI DFLELAMDEFIERYKLEGYAFEHIVYGDFSHSQLGGLHLLIGLAKRFKE SPFELEDFIPMDSTVKNYFITDAQTGSSKCVCSVIDLLLDDFVEIIKSQ DLSVVSKVVKVTIDYTEISFMLWCKDGHVETFYPKLQSSQAWQPGVAMP NLYKMQRMLLEKCDLQNYGDSATLPKGIMMNVAKYTQLCQYLNTLTLAV PYNMRVIHFGAGSDKGVAPGTAVLRQWLPTGTLLVDSDLNDFVSDADST LIGDCATVHTANKWDLIISDMYDPKTKNVTKENDSKEGFFTYICGFIQQ KLALGGSVAIKITEHSWNADLYKLMGHFAWWTAFVTNVNASSSEAFLIG CNYLGKPCEQIDGYVMHANYIFWRNTNPIQLSSYSLFDMSKFPLKLRGT AVMSLKEGQINDMILSLLSKGRLIIRENNRVVISSDVLVNN
(154) The fragment of sequence, marked in bold, was modified to CVN-DTF-AGSTFISDEV-D (SEQ ID NO: 2).
(155) Sequence CVN-DTF-AGSTFISDEV-D (SEQ ID NO: 2) was selected as peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein (peptide SARS-CoV-2) target, peptide A.
(156) Poly [ADP-Ribose] Polymerase-1 Partial [Synthetic Construct]-Human PARP1
(157) Human PARP1 Sequence: 1014 aa
(158) TABLE-US-00010 SEQ ID NO: 6 MAESSDKLYRVEYAKSGRASCKKCSESIPKDSLRMAIMVQSPMFDGKVP HWYHFSCFWKVGHSIRHPDVEVDGFSELRWDDQQKVKKTAEAGGVTGKG QDGIGSKAEKTLGDFAAEYAKSNRSTCKGCMEKIEKGQVRLFKKMVDPE KPQLGMIDRWYHPGCFVKNREELGFRPEYSASQLKGFSLLATEDKEALK KQLPGVKSEGKRKGDEVDGVDEVAKKKSKKEKDKDSKLEKALKAQNDLI WNIKDELKKVCSTNDLKELLIFNKQQVPSGESAILDRVADGMVFGALLP CEECSGQLVFKSDAYYCTGDVTAWTKCMVKTQTPNRKEWVTPKEFREIS YLKKLKVKKQDRIFPPETSASVAATPPPSTASAPAAVNSSASADKPLSN MKILTLGKLSRNKDEVKAMIEKLGGKLTGTANKASLCISTKKEVEKMNK KMEEVKEANIRVVSEDFLQDVSASTKSLQELFLAHILSPWGAEVKAEPV EVVAPRGKSGAALSKKSKGQVKEEGINKSEKRMKLTLKGGAAVDPDSGL EHSAHVLEKGGKVFSATLGLVDIVKGTNSYYKLQLLEDDKENRYWIFRS WGRVGTVIGSNKLEQMPSKEDAIEHFMKLYEEKTGNAWHSKNFTKYPKK FYPLEIDYGQDEEAVKKLTVNPGTKSKLPKPVQDLIKMIFDVESMKKAM VEYEIDLQKMPLGKLSKRQIQAAYSILSEVQQAVSQGSSDSQILDLSNR FYTLIPHDFGMKKPPLLNNADSVQAKVEMLDNLLDIEVAYSLLRGGSDD SSKDPIDVNYEKLKTDIKVVDRDSEEAEIIRKYVKNTHATTHNAYDLEV IDIFKIEREGECQRYKPFKQLHNRRLLWHGSRTTNFAGILSQGLRIAPP EAPVTGYMFGKGIYFADMVSKSANYCHTSQGDPIGLILLGEVALGNMYE LKHASHISKLPKGKHSVKGLGKTTPDPSANISLDGVDVPLGTGISSGVN DTSLLYNEYIVYDIAQVNLKYLLKLKFNFKTSLW
(159) The sequence DEVDGVDEVAKKKSKK (SEQ ID NO: 3) was selected as human PARP1 peptide target, also referred as peptide B.
(160) Peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 Surface Protein (Peptide SARS-Cov-2) and Peptide Human PARP1 Fusion
(161) The peptide SARS-CoV-2 and peptide Human PARP1 are fused with DEVD site junction.
(162) Peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 surface protein (Peptide SARS-CoV-2) and Peptide Human PARP1 are fused obtaining Peptide AB with SEQ ID NO: 4.
(163) TABLE-US-00011 TABLE 3 SEQ ID NO. Sequence SEQ ID NO: 2 CVN-DTF-AGSTFISDEVD SEQ ID NO: 3 DEVDGVDEVAKKKSK SEQ ID NO: 4 CVNDTFAGSTFISDEVDGVDEVAKKKSK
(164) Peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein (Peptide SARS-CoV-2)/Peptide Human PARP1 (SEQ ID No: 4) is used as target using ProtParam.
C.sub.125H.sub.200N.sub.32O46 Formula:
(165) Total number of atoms: 403
(166) Atomic Composition: Carbon C 125 Hydrogen H 200 Nitrogen N 32 Oxygen O 46 Sulfur S 0
(167) Number of amino acids: 27
(168) Molecular weight: 2887.15
(169) Theoretical pI: 4.53
(170) Amino Acid Composition: Ala (A) 2 7.4% Arg (R) 0 0.0% Asn (N) 1 3.7% Asp (D) 4 14.8% Cys (C) 0 0.0% Gin (Q) 0 0.0% Glu (E) 2 7.4% Gly (G) 2 7.4% His (H) 0 0.0% Ile (I) 1 3.7% Leu (L) 0 0.0% Lys (K) 4 14.8% Met (M) 0 0.0% Phe (F) 2 7.4% Pro (P) 0 0.0% Ser (S) 3 11.1% Thr (T) 2 7.4% Trp (W) 0 0.0% Tyr (Y) 0 0.0% Val (V) 4 14.8% Pyl (O) 0 0.0% Sec (U) 0 0.0% (B) 0 0.0% (Z) 0 0.0% (X) 0 0.0%
(171) Total number of negatively charged residues (Asp+Glu): 6
(172) Total number of positively charged residues (Arg+Lys): 4
(173) Extinction Coefficients:
(174) As there are no Trp; Tyr or Cys in the region considered, protein should not be visible by UV spectrophotometry.
(175) Estimated Half-Life:
(176) The N-terminal of the sequence considered is V (Val).
(177) The estimated half-life is: 100 hours (mammalian reticulocytes, in vitro). >20 hours (yeast, in vivo). >10 hours (Escherichia coli, in vivo).
Instability Index:
The instability index (II) is computed to be 2.07
This classifies the protein as stable.
Aliphatic index: 64.81.
Grand average of hydropathicity (GRAVY): −0.526
(178) IFNepitope Prediction—peptide-AB
(179) SEQ ID No: 4 CVNDTFAGSTFISDEVDGVDEVAKKKSK is positive using the method SVM with score 3.1106915.
(180) IFNepitope Score is a webserver that allows users to identify IFN-gamma inducing MHC class II binding peptides in a peptide/antigen. This server permits the user to predict and design IFN-gamma inducing regions in their protein of interest. This prediction method has been trained on 10433 experimentally validated IFN-gamma inducing and non-inducing MHC class II binders/peptides. The prediction server has three major tools, and the algorithm of the prediction is based on three models (motif based, SVM based and hybrid approach). User can select the method of prediction for all the three module.
(181) According to the Algorithms of the Present Invention
(182) Vaccine RNA-peptide-AB according to the present invention, here referred as “Melody”
(183) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7701/2887.15=2.6673
c=27/24=1.125
d=[(2*(8+6)+3*(6+4))/(4.53{circumflex over ( )}2)]=2.8264
FS=10*2.6673*1.125*2.8264(cruz)
FS=84.81 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=84.81*[(2887.15/7701)+(27/34)]=84.81*[(0.374905)+(0.794117)]=84.81*1.169=99.14
EA=99.15ro
Biological Action (BA)
BA=EA/FS
BA=99.14/84.81
BA=1.17ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(184) Meloyd
(185) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6951/2887.15=2.4076
c=27/21=1.28571
d=[(2*(5+4)+3*(2+10))/(4.53{circumflex over ( )}2)]=[(2*9+3*12)/(20.5209)]=[(18+36))/(20.5209)]=2.6315
FS=10*2.4076*1.28571*2.6315(cruz)
FS=81.46 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/MW mRNA)+(Size peptide/Size primer)]
EA=(ro)
EA=81.46*[(2887.15/6951)+(27/31)]=81.46*[(0.415357)+(0.87096)]=81.45*1.2863=104.77ro
EA=104.77ro
Biological Action (BA)
BA=EA/FS
BA=104.77/81.45
BA=1.29ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(186) Moledy
(187) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6775/2887.15=2.3466
c=27/21=1.28571
d=[(2*(6+4)+3*(5+6))/(4.53{circumflex over ( )}2)]=2.5827
FS=10*2.3466*1.28571*2.5827(cruz)
FS=77.92 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=77.92*[(2887.15/6775)+(27/31)]=77.92*[(0.4261)+(0.87096)]=77.92*1.29706=101.07ro
EA=101.07ro
Biological Action (BA)
BA=EA/FS
BA=101.07/77.92
BA=1.30ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(188) Myledo
(189) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6701/2887.15=2.3210
c=27/21=1.2857
d=[(2*(1+10)+3*(4+6))/(4.53{circumflex over ( )}2)]=2.534
FS=10*2.321*1.2857*2.534(cruz)
FS=75.62 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=75.62*[(2887.15/6701)+(27/31)]=98.44ro
EA=98.44ro
Biological Action (BA)
BA=EA/FS
BA=98.44/75.62
BA=1.30ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(190) Lodyme
(191) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7082/2887.15=2.4529
c=27/22=1.2273
d=[(2*(6+6)+3*(5+5))/(4.53{circumflex over ( )}2)]=2.6315
FS=10*2.453*1.2273*2.6315(cruz)
FS=79.22 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=79.22*[(2887.15/7082)+(27/32)]=99.14ro
EA=99.14ro
Biological Action (BA)
BA=EA/FS
BA=99.14/79.22
BA=1.25ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(192) Ledymo
(193) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7059/2887.15=2.4450
c=27/22=1.2273
d=[(2*(5+7)+3*(5+5))/(4.53{circumflex over ( )}2)]=2.6315
FS=10*2.445*1.227*2.631(cruz)
FS=78.96 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=78.96*[(2887.15/7059)+(27/32)]=98.92ro
EA=98.92ro
Biological Action (BA)
BA=EA/FS
BA=98.92/78.96
BA=1.25ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(194) Modyle
(195) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7453/2887.15=2.5814
c=27/23=1.1739
d=[(2*(7+7)+3*(6+7))/(4.53{circumflex over ( )}2)]=2.6802
FS=10*2.5814*1.1739*2.6802(cruz)
FS=81.22 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=81.22*[(2887.15/7453)+(27/33)]=97.92ro
EA=97.92ro
Biological Action (BA)
BA=EA/FS
BA=97.92/81.22
BA=1.21ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(196) Medylo
(197) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6358/2887.15=2.2022
c=27/20=1.350
d=[(2*(8+4)+3*(7+1))/(4.53{circumflex over ( )}2)]=2.3391
FS=10*2.2022*1.35*2.3391(cruz)
FS=69.54 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=69.54*[(2887.15/6358)+(27/30)]=94.16ro
EA=94.16ro
Biological Action (BA)
BA=EA/FS
BA=94.16/69.54
BA=1.35ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(198) Dylome
(199) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7159/2887.15=2.4796
c=27/22=1.2273
d=[(2*(6+3)+3*(6+7))/(4.53{circumflex over ( )}2)]=2.7777
FS=10*2.4796*1.2273*2.7777(cruz)
FS=84.53 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=84.53*[(2887.15/7159)+(27/32)]=105.41ro
EA=105.41ro
Biological Action (BA)
BA=EA/FS
BA=105.41/84.53
BA=1.25ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(200) Lomedy
(201) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6377/2887.15=2.2088
c=27/20=1.350
d=[(2*(2+7)+3*(6+5))/(4.53{circumflex over ( )}2)]=2.4853
FS=10*2.2088*1.35*2.4853(cruz)
FS=74.11 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=74.11*[(2887.15/6377)+(27/30)]=133.59ro
EA=133.59ro
Biological Action (BA)
BA=EA/FS
BA=133.59/74.11
BA=1.80ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(202) Lemody
(203) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=5767/2887.15=1.9975
c=27/18=1.50
d=[(2*(2+7)+3*(4+5))/(4.53{circumflex over ( )}2)]=2.1929
FS=10*1.9975*1.5*2.1929(cruz)
FS=65.70 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=65.70*[(2887.15/5767)+(27/28)]=131.45ro
EA=131.45ro
Biological Action (BA)
BA=EA/FS
BA=131.45/65.7
BA=2.00ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(204) Modyle
(205) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7013/2887.15=2.4290
c=27/22=1.2273
d=[(2*(3+9)+3*(5+5))/(4.53{circumflex over ( )}2)]=2.6315
FS=10*2.429*1.2273*2.6315(cruz)
FS=78.45 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=78.45*[(2887.15/7013)+(27/32)]=98.48ro
EA=98.48ro
Biological Action (BA)
BA=EA/FS
BA=98.48/78.45
BA=1.26ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(206) Medylo
(207) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6213/2887.15=2.1519
c=27/22=1.4211
d=[(2*(3+4)+3*(4+8))/(4.53{circumflex over ( )}2)]=2.4365
FS=10*2.1519*1.4211*2.4365(cruz)
FS=74.51 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=74.51*[(2887.15/6213)+(27/32)]=104.0ro
EA=104.0ro
Biological Action (BA)
BA=EA/FS
BA=104.0/74.51
BA=1.4ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(208) Dyolem
(209) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=6214/2887.15=2.1523
c=27/19=1.4211
d=[(2*(3+5)+3*(3+8))/(4.53{circumflex over ( )}2)]=2.4365
FS=10*2.1523*1.4211*2.4365(cruz)
FS=73.03 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=73.03*[(2887.15/6214)+(27/29)]=137.71
EA=137.71ro
Biological Action (BA)
BA=EA/FS
BA=137.71/73.03
BA=1.89ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(210) Ylomed
(211) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7444/2887.15=2.5783
c=27/23=1.1739
d=[(2*(5+6)+3*(5+7))/(4.53{circumflex over ( )}2)]=2.8264
FS=10*2.5783*1.1739*2.8264(cruz)
FS=85.55 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=85.55*[(2887.15/7444)+(27/33)]=103.17ro
EA=103.17ro
Biological Action (BA)
BA=EA/FS
BA=103.17/85.55
BA=1.21ro/cruz
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(212) Lomedy
(213) Fusion Stability (FS)
FS=a*b*c*d(cruz)
a=Size poly A/Size poly Cys
b=MW mRNA/MW peptide
c=Size peptide/Size mRNA
d=[mRNA(2*(A+U)+3*(C+G))/(PI peptide{circumflex over ( )}2)]
a=10/1=10
b=7278/2887.15=2.5208
c=27/23=1.1739
d=[(2*(3+8)+3*(8+4))/(4.53{circumflex over ( )}2)]=2.8264
FS=10*2.5208*1.1739*2.8264(cruz)
FS=83.64 cruz
Exosome Affinity (EA)
EA=FS*[(MW peptide/mMW RNA)+(Size peptide/Size primer)]
EA=(ro)
EA=83.64*[(2887.15/7278)+(27/33)]=101.61ro
EA=101.61ro
Biological Action (BA)
BA=EA/FS
BA=101.61/83.64
Optimal Biological Action (OBA)
OBA=(ro/cruz)
value for antiviral efficacy to RNA-peptide with exosome as carrier are 0.8<OBA<1.3
(214) According to the algorithms of the present invention, the following table (table 4) shows Fusion Stability, Affinity and Biological Action of the sixteen vaccines candidates.
(215) TABLE-US-00012 TABLE 4 Code FS EA BA Melody 84.81 99.15 1.17 Meloyd 81.46 104.78 1.29 Moledy 77.92 101.07 1.30 Myledo 75.62 98.44 1.30 Lodyme 79.22 99.14 1.25 Ledymo 78.96 98.92 1.25 Modyle 81.22 97.92 1.21 Medylo 69.54 94.16 1.35 Dylome 84.53 105.41 1.25 Lomedy 74.11 133.59 1.80 Lemody 65.70 131.45 2.00 Modyle 78.45 98.48 1.26 Medylo 74.51 104.00 1.40 Dyolem 73.03 137.71 1.89 Ylomed 85.55 103.17 1.21 Lomedy 83.64 101.61 1.21
(216) Results by Stages of the Invention:
(217) Vaccine RNA-peptide against SARS-CoV-2: Exosomes as carrier according to the algorithms of the present invention.
(218) A) Design and Selection of Candidate Isoforms from the Application of the Algorithms of the Present Invention.
(219) The following table (Table 5) shows more significant values of Fusion Stability, Exosome Affinity and Biological Action of the four vaccines candidates:
(220) TABLE-US-00013 TABLE 5 FS EA BA Melody 84.81 99.15 1.17 (RNA-peptide-AB) Lodyme 79.22 99.14 1.25 Ledymo 78.96 98.92 1.25 Modyle 78.45 98.48 1.26
(221) B) Validation of IFNepitope Score for the Four Vaccines Candidates
(222) The following table (Table 6) shows the RNA-peptide-AB vaccine object of the present invention (referred as Melody) as best candidate vaccine according to its highest value of IFNepitope Score=3.21
(223) TABLE-US-00014 TABLE 6 IFNepitope Code FS EA BA score Melody 84.81 99.15 1.17 3.21 Lodyme 79.22 99.14 1.25 3.09 Ledymo 78.96 98.92 1.25 3.09 Modyle 78.45 98.48 1.26 3.02
(224) According to IFNepitope Score from Tox21 program, four candidates were studied (Table 3) and selected melody as the best vaccine candidate. These studies were In silico using “in vitro assays” that evaluate key biological pathways and molecular mechanisms linked to human disease.
(225) Vaccine Candidate (RNA-Peptide-A/RNA-Peptide-AB): Compositions of the Present Invention.
(226) RNA vaccine of the present invention comprises a ribonucleic acid polynucleotide fused to at least one peptide. In a preferred embodiment, the peptide, referred as peptide A, is a surface protein peptide from Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2).
(227) In a preferred embodiment, a ribonucleic acid polynucleotide fragment comprises the following sequence:
(228) TABLE-US-00015 SEQ ID NO: 1 AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG
(229) In another preferred embodiment, a peptide of the Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) surface protein, peptide SARS-CoV-2 (peptide A), comprises the following sequence:
(230) TABLE-US-00016 SEQ ID NO: 2 CVNDTFAGSTFISDEVD
(Number of amino acids: 17 aa; MW=1819.91 daltons, Theoretical pI: 3.37)
(231) In another preferred embodiment, poly ADP-ribose polymerase peptide (peptide B) comprises the following sequence:
(232) TABLE-US-00017 SEQ ID NO: 3 GVDEVAKKKSK
(Number of amino acids: 11 aa; MW=1188.39 daltons, Theoretical pI: 9.53).
(233) In a preferred embodiment, RNA vaccine of the present invention is RNA-peptide-A vaccine comprising SEQ ID NO: 1 fused to SEQ ID NO: 2.
(234) TABLE-US-00018 SEQ ID NO: 1 and SEQ ID NO: 2 AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG- Cys- Val- Asn -Asp- Thr- Phe- Ala- Gly- Ser -Thr- Phe -Ile- Ser -Asp- Glu- Val -Asp
(235) In a preferred embodiment, peptide of a Severe Acute Respiratory Syndrome Coronavirus 2 surface protein (Peptide A) and Peptide Human PARP1 (Peptide B) are fused obtaining Peptide-AB with SEQ ID NO: 4.
(236) TABLE-US-00019 SEQ ID NO: 4 CVNDTFAGSTFISDEVDGVDEVAKKKSK
(237) In preferred embodiment, RNA vaccine of the present invention is RNA-peptide-AB vaccine comprising SEQ ID NO: 1 fused to SEQ ID NO: 4.
(238) TABLE-US-00020 SEQ ID NO: 1 and SEQ ID NO: 4 AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG- Cys- Val -Asn -Asp- Thr- Phe- Ala- Gly- Ser -Thr Phe- Ile -Ser -Asp- Glu -Val- Asp- Gly Asp Glu -Val- Ala- Lys- Lys- Lys- Ser- Lys
EXAMPLES
Example 1
(239) Synthesis and Validation of Peptides Targets
(240) TABLE-US-00021 SEQ ID NO: 4 CVNDTFAGSTFISDEVDGVDEVAKKKSK (Size 28 = aa) SEQ ID NO: 2 CVNDTFAGSTFISDEVD (Size 17 = aa) SEQ ID NO: 3 GVDEVAKKKSK (Size 11 = aa)
(241) Synthesis of Peptides
(242) According to the present invention peptides were synthesized on ChemMatrix Rink Amide resin, using standard Fmoc synthesis protocol with DIC/Cl-HOBt coupling, on an APEX 396 automatic synthesizer. The resin was swollen in DMF for 30 min, treated with 20 volume (v) % Piperidine-DMF for 8 minutes to remove the Fmoc protecting group, at 50° C., and washed with DMF for three times. For the coupling reaction, the resin was added with Fmoc-protected amino acid, Cl-HOBt, DIC and NMP. The mixture was vortexed for 20 minutes at 50° C. Afterwards, the resin was washed with DMF once. The cycle of deprotection and coupling steps was repeated until the last amino acid residue was assembled. After the final Fmoc protecting group was removed, the resin was treated with 20 v % acetic Anhydride-NMP for 20 minutes. The resin was then washed with DMF, DCM and dried with air. The peptides were cleaved using a TFA cocktail (95 v % TFA, 2.5 v % water and 2.5 v % TIS) for three hours. Crude peptides were precipitated by adding ice-chilled anhydrous ethyl ether, washed with anhydrous ethyl ether for three times, and dried in vacuum. After the synthesis, we use the conventional prep-HPLC for peptide purification. Peptide synthesis is robust and fool proof; however, there are a few things that can really mess up the reproducibility of these protocols. Probably chief amongst them is the quality of DMF.
(243) Solid Supports
(244) The first step in solid-phase peptide synthesis was choose cysteine as amino acid with functional group C-terminus to be a carboxylic acid use 2-chlorotrityl resin in order to load Cysteine amino acid onto the resin.
(245) Loading 2-Chlorotrityl Chloride
(246) The purpose of this step was to covalently link the cysteine amino acid onto the resin.
(247) Prep time: 30 min
(248) Reaction time: 8-24 h
(249) The process comprises the following steps:
(250) 1) Weigh out appropriate amount of resin. Generally, we use 300 mg for a 0.1 mmol scale. Transfer the resin into a PolyPrep chromatography column (BioRad).
(251) 2) Swell resin for at least 30 min at room temperature in dry CH.sub.2Cl.sub.2.
(252) 3) Weigh out an appropriate amount of the cysteine amino acid and dissolve it in 8 mL CH.sub.2Cl.sub.2 w/0.3 ml 2,4,6-collidine. When making a macrocyclic peptide cysteine amino acid is preferably Boc-Orn(Fmoc)-OH. Use 100 mg of Boc-Orn(Fmoc)-OH.
(253) 4) Using a flow of nitrogen gas, push out all CH.sub.2Cl.sub.2 from the column that contains the swelled resin and add the amino acid/CH.sub.2Cl.sub.2/collidine mixture.
(254) 5) Rock for at least 8 hours.
(255) 6) Move on to Capping 2-chlorotrityl resin.
(256) Capping 2-Chlorotrityl Chloride Resin
(257) The purpose of this step is to covalently link a small nucleophile (methanol) to the unreacted carbocations on the 2-chlorotrityl chloride resin.
(258) Prep time: 10 mins
(259) Reaction time: 60 mins
(260) The process comprises the following steps:
(261) 1) Wash the loaded resin 3× with CH.sub.2Cl.sub.2. The loaded resin was washed 3× with CH.sub.2Cl.sub.2.
(262) 2) capping solution. The capping solution is CH.sub.2Cl.sub.2:MeOH:DIPEA (17:2:1). It was made fresh each time by adding 1 mL MeOH and 0.5 mL diisopropylethylamine (DIPEA, or DIEA) to 9 mL of CH.sub.2Cl.sub.2.
(263) 3) capping solution is dumped on to the loaded resin and rock for 1 hour at room temperature. It is not recommended to extend the reaction time, as exchange of the loaded amino acid with MeOH is a possibility.
(264) 4) After 1 hour, push out the capping solution with nitrogen and wash the resin 2× with CH.sub.2Cl.sub.2 and 1× with DMF.
(265) 5) The loaded resin goes through repeated Fmoc-deprotections and amino acid couplings to build the rest of your peptide. These deprotections and couplings can be done manually (hand coupling) or on an automatic synthesizer.
(266) Capping Rink Amide Resin
(267) The purpose of this step is to cap unreacted amines on rink amide so that the amino acids are not attached to the resin.
(268) Prep time: 5 min
(269) Reaction time: 30 minutes (mins)
(270) 1) capping solution is prepared by combining acetic anhydride and pyridine in a 3:2 ratio of acetic anhydride:pyridine. Crudely by using a Pasteur pipette to combine 3 “squirts” of acetic anhydride with 2 “squirts” of pyridine in a scintillation vial.
(271) 2) Dump the capping solution on the resin and rock for 30 mins at room temperature.
(272) 3) After the resin is done capping push out the capping solution with nitrogen and wash the resin 4× with DMF.
(273) 4) loaded resin goes through repeated Fmoc-deprotections and amino acid couplings to build the rest of the peptide. These deprotections and couplings are done on APEX 396 automatic synthesizer.
(274) Checking Resin Loading
(275) The purpose of this step is to determine the mmol of amino acid that are on resin. The procedure is the same regardless of the resin are using.
(276) Prep time: 20 mins
(277) Reaction time: 5 mins
(278) 1) Take a small portion (1-2 mg) of resin and transfer it to a new polyprep column. Dry the resin by blowing nitrogen through it.
(279) 2) While the resin drying, it is added 3 mL of 20% piperidine in DMF in a 3-mL quartz cuvette. Blank the UV/Vis with the 20% piperidine at 290 nm.
(280) 3) Add approximately 1 mg of dried resin to 3 mL 20% piperidine in DMF in the quartz cuvette.
(281) 4) Allow the resin to sit in the 20% piperidine for at least 5 min.
(282) 5) Take a UV/Vis reading at 290 nm against the 20% piperidine blank.
(283) 6) Use Ryan's Excel mass spec calculator to determine the loading percentage. This will dictate the mmol of each amino acid should be used when synthesizing the peptide. Good loading percentages fall between 50-70%.
(284) Solid-Phase Peptide Synthesis
(285) The purpose of this step is to sequentially add amino acids to the resin to build a peptide chain. The first step is deprotecting Fmoc from the amino on the resin to expose an amine. The second step is coupling an activated amino acid to the exposed amine. These steps are done the same on 2-chlorotrityl chloride and rink amide resin.
(286) Alloc Deprotection
(287) Alloc protected groups are removed during peptide synthesis
(288) TABLE-US-00022 SEQ ID NO: 4 C-V-N-D-T-F-A-G-S-T-F-I-S-D-E-V-D-G-V-D-E-V-A-K- K-K-S-K
(289) Prep time: 5 min
(290) Reaction time: 40 min
(291) 1) Wash the resin in a polyprep column 3× with CH.sub.2Cl.sub.2.
(292) 2) Based on loading, weigh out 0.1 equiv. of tetrakis(triphenylphosphine) palladium and dissolve in CH.sub.2Cl.sub.2 (6 mL).
(293) 3) Add 20 equiv. of phenylsilane (density 0.878 g/cm3) to the resulting solution.
(294) 4) Transfer the solution to resin in a poly-prep column.
(295) 5) Put it on the rocker for 20 minutes.
(296) 6) Repeat steps 1-5.
(297) 7) Wash the resin in a poly-prep column 3× with CH.sub.2Cl.sub.2.
(298) 8) Check alloc deprotection by cleaving small portion of resin with 20% HFIP in CH.sub.2Cl.sub.2 (15 min).
(299) 9) Rotovap the cleaved solution and re-dissolve in MeCN.
(300) 10) Using the ESI-MS, search for the alloc deprotected mass.
(301) Dde Deprotection
(302) The purpose of this step is to remove Dde protecting groups during peptide synthesis.
(303) Prep time: 5 min
(304) Reaction time: 30 min
(305) 1) Wash the resin in a poly-prep column 3× with DMF.
(306) 2) Add 5 mL of 2% hydrazine in DMF.
(307) 3) Put it on the rocker for 15 min.
(308) 4) Repeat steps 1-3.
(309) 5) Wash the resin in a poly-prep column 3× with DMF.
(310) 6) Check Dde deprotection by cleaving small portion of resin with 20% HFIP in CH.sub.2Cl.sub.2 (15 min).
(311) 7) Rotovap the cleaved solution and re-dissolve in MeCN.
(312) 8) Using the ESI-MS, search for Dde deprotected mass.
(313) Automated Synthesis-APEX 396 Automatic Synthesizer
(314) The peptides are synthesized on ChemMatrix Rink Amide resin, using standard Fmoc synthesis protocol with DIC/Cl-HOBt coupling, on an APEX 396 automatic synthesizer.
(315) To use the APEX 396 automatic synthesizer, firstly it is weigh out 4 equivalents of each amino acid to couple along with 4 equivalents of coupling agent (HCTU or HATU/HOAt) and add the amino acid and coupling agent to amino acid vials.
(316) Prep time: 1-3 h
(317) Reaction time: variable, typically less than 24 h
(318) 1) Transfer the resin to the appropriate reaction vessel and attach it to the synthesizer.
(319) 2) Check the solvent levels and waste levels on the instrument. If the waste is more than halfway full attach a new waste container.
(320) 3) Program the sequence into the APEX 396 automatic synthesizer.
(321) 4) When the peptide finishes synthesizing, the reaction vessel is removed from the synthesizer and the resin is transfered to the poly-prep column.
(322) Cleavage Form Solid Support
(323) Cleavage of side chain protected linear peptide from 2-chlorotrityl chloride resin. The purpose of the step is to cleave the peptide from 2-chlorotrityl resin to expose a free carboxy terminus and maintain the protecting groups on the amino acid side chains
(324) Prep time: 10 min
(325) Reaction time: 1.5 h
(326) 1) Prepare the cleavage solution. The cleavage solution is 20% hexafluoroisopropanol (HFIP) in CH.sub.2Cl.sub.2. This fresh is prepared by adding 3.5 mL HFIP to 11.5 mL CH.sub.2Cl.sub.2 in a small graduated cylinder. Alternatively, 1 squirt of HFIP into 4 squirts of CH.sub.2Cl.sub.2 with a Pasteur pipette.
(327) 2) Add about half of the cleavage solution to the resin in the polyprep column. If the resin is washed with CH.sub.2Cl.sub.2 before add the cleavage solution, it will turn red. Rock for 1 h at room temperature, and then drain into a clean round bottom flask.
(328) 3) Add the other half of the cleavage solution to the resin and rock for an additional 30 min. After the 30 min is complete drain into the same round bottom flask.
(329) 4) Use the rotovap to evaporate the HFIP and CH.sub.2Cl.sub.2.
(330) 5) Make a linear peptide proceeds to Global Deprotection of Acid Labile Protecting Groups.
(331) Cleavage of Linear Peptide from Rink Amide Resin
(332) Prep time: 1 h
(333) Reaction time: 1.5 h
(334) 1) Wash the completed peptide on resin 3× with CH.sub.2Cl.sub.2, and transfer it into a poly prep column.
(335) 2) Dry resin under a stream on N.sub.2 gas for ca-X 1 h.
(336) 3) Add 10 mL of an 18:1:1 TFA:H.sub.2O:TIPS (prepared by adding 9 mL TFA and 0.5 mL of both H.sub.2O and TIPS) to the resin. Let rock for 1-1.5 hours.
(337) 4) Collect solution in a 250 mL round bottom flask.
(338) 5) Remove TFA with the use of a rotovap.
(339) Purification of Peptides
(340) Reverse-Phase HPLC Purification
(341) 1) Dissolve the deprotected peptide in the round bottom flask in a small amount of MeCN (2 mL) and transfer to a 15-mL conical tube. Wash the round bottom flask with ca. 3 mL H.sub.2O to collect the residual peptide in the round bottom flask and transfer to the 15-mL conical. The volume transferred to the 15-mL conical should not exceed 10 mL.
(342) 2) To remove particulates, centrifuge 15-mL conical at 10,000 rpm for 5 min.
(343) 3) Pass through a 0.2-μm syringe filter into a new 15-mL falcon tube. Inject the peptide on to the preparative RP-HPLC column. Before inject, it is advisable to obtain analytical HPLC trace to gauge what percentage of MeCN your peptide will come out. General operation of the semi-preparative RP-HPLCs
(344) Procedure:
(345) 1) Make sure that the solvent bottles are full.
(346) 2) Turn on lamp and flow (10 mL/min) on HPLC. The absorbance should be set to 214 nm.
(347) 30 Wash column at 95% MeCN over 5 min.
(348) 4) Go to 20% MeCN over 5 min at 10 mL/min.
(349) 5) Inject peptide and allow the peptide to load onto the column for 10 min.
(350) 6) Go to 30% MeCN over 20 min at 15 mL/min.
(351) 7) Go to 50% MeCN over 60 min at 15 mL/min. Peptide is likely to come out when going from 30% to 50%.
(352) 8) Collect fractions. Typically count 20 sec for each fraction.
(353) 9) After the peptide comes out, wash the column with 95% MeCN for at least 15 min. Then return the MeCN percentage to 50%.
(354) 10) The column is stored at 50% MeCN.
(355) 11) Turn off flow and UV lamp.
(356) The following table (Table 7) shows the compounds synthesized:
(357) TABLE-US-00023 TABLE 7 CUSTOM PEPTIDES CERTIFICATE OF ANALYSIS Cat. No. Name Sequence Weight Purity Formula M.W. 360662873 #1 primer primer 1.0 mg HPLC C328H403 10912.7 847361 #2 Peptide AB Peptide AB 1.0 mg 98.25% N140 2990.25 O224P33 C128H205 847362 #3 Peptide A Peptide A 1.0 mg 98.76% N33047S 1819.89 C77H114N 847363 #4 Peptide B Peptide B 1.0 mg 98.62% 18O31S 1188.37 C51H93N1 36305 #5 primer primer 1.4 mg HPLC 5O17 14680.75 C492H648 -Peptide AB Peptide AB N180 O282P34S1
(358) The following table (Table 8) shows the ITEM Sequence, Quantity and Purity of each compound synthesized
(359) TABLE-US-00024 TABLE 8 SEQUENCE AND ITEM # MODIFICATION QUANTITY PURITY 1. primer primer 1 mg HPLC 2. Peptide AB Peptide AB 1 mg >98% 3. Peptide A Peptide A 1 mg >98% 4. Peptide B Peptide B 1 mg >98% 5. primer-peptide AB primer-peptide AB 1 mg HPLC
(360) Checking Fractions, and Lyophilizing
(361) 1. To assess the purity of the fractions check them on the analytical HPLC. If there are impurities, an additional preparative HPLC was necessary.
(362) 2. Combine the pure fractions and take a “combined HPLC” and a “combined mass spec”.
(363) 3. Evaporate the MeCN/H2O using a rotovap.
(364) 4. Re-dissolve the peptide film on the side of the flask in H2O and transfer to a clean polypropylene 15-mL conical.
(365) 5. Freeze your peptide in dry ice and then transfer the peptide to a lyophilization vessel. Detach the lid of the 15-mL conical, and use a kimwipe and rubber band to cover the top of the 15-mL conical.
(366) 6. Attach the lyophilization vessel to the lyophilizer. 12-48 hours later you will have a dry powder of your peptide as a TFA salt.
(367) Oligonucleotide (RNA) and RNA-Peptide Conjugation
Example 2
(368) Oligonucleotide (RNA) Synthesis
(369) TABLE-US-00025 The miRNA SEQ ID NO: 1 5'AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG3'
was synthesized according to Phosphoramidite Method.
(370) The RNA with azide group are synthesized by the oligo vendors following the Phosphoramidite method, a solid-phase synthesis like peptide synthesis, including detritylation of the support-bound 3′-nucleoside, activation and coupling, capping, oxidation and detritylation.
(371) The phosphoramidite method is followed according to the next four steps:
(372) 1. Detritylation,
(373) 2. Coupling,
(374) 3. Capping
(375) 4. Oxidation
(376) Step 1 (Detritylation)
(377) The cycle is initiated by removal of the 5′-DMT (4,4′-dimethoxytrityl) protecting group of the solid-support-linked nucleoside adenine (A), contains the terminal 3′ base of the oligonucleotide RNA. The 5′-DMT prevents polymerization of the nucleoside (A) during functionalization of the solid support resin. The detritylation mechanism. The 5′-DMT protecting group is removed by TCA (trichloroacetic acid) in the solvent. The products include the 3′ terminal (A) nucleoside with a free 5′-OH and a DMT carbocation. The nucleoside A proceeds to step 2 in the synthesis while the DMT carbocation absorbs at 495 nm and thereby produces an orange color (used to monitor coupling efficiency).
(378) Step 2 (Coupling)
(379) Once the DMT has been removed, the free 5′-OH of the solid-support-linked A nucleoside is able to react with the next nucleoside A, which is added as a phosphoramidite monomer. (made nine times this step in order to develop the polyadenine arm of ten nucleosides AAAAAAAAAA)
(380) The coupling mechanism. The diisopropylamino group of the incoming phosphoramidite monomer in the solvent acetonitrile is ‘activated’ (protonated) by the acidic catalyst ETT [5-(ethylthio)-1H-tetrazole]. The mixing is carried out in the fluid lines of the synthesis instrument as the reagents are delivered to the solid support. The activated phosphoramidite is delivered in a many-fold excess over the solid-support-linked nucleoside to drive the reaction to as close to completion as possible. The products include a dinucleoside with a phosphite triester linkage and a free diisopropylamino group.
(381) Step 3 (Oxidation)
(382) The phosphite triester formed during the coupling reaction is unnatural and unstable; therefore, it must be converted to a more stable phosphorus species prior to the start of the next cycle. Oxidation converts the phosphite triester to the stable phosphate triester.
(383) The oxidation mechanism. Oxidation of the phosphite triester is achieved with iodine in the presence of water and pyridine. The product is the phosphate triester, which is essentially a standard DNA backbone with a β-cyanoethyl protecting group on the free oxygen.
(384) Step 4 (Capping)
(385) Since 100% coupling efficiency is impossible, there are always some solid-support-linked nucleosides with unreacted 5′-OH. If not blocked, these hydroxyl groups will react during the next cycle, and hence, lead to a missing base. The accumulation of these deletion mutations through successive cycles would create a complex mixture of ‘shortmers’ that are difficult to purify and therefore could render the oligonucleotide useless in the subsequent application. Capping is required to prevent shortmer accumulation.
(386) Acetic anhydride and N-methylimidazole react to form an intermediate in the solvent tetrahydrofuran, which contains a small quantity of pyridine. The mixing is carried out in the fluid lines of the synthesis instrument as the reagents are delivered to the solid support. The product is the solid-support-linked nucleoside with an acetylated 5′-OH (pyridine maintains a basic pH thereby preventing detritylation of the phosphoramidite monomer by the free acetate/acetic acid).
(387) Successive Cycles
(388) The second cycle begins by starting with step 1, detritylation, followed by each of the remaining three steps. The number of cycles repeated equals the desired number of bases. We synthesized oligonucleotide RNA from 2 to 34 bases.
(389) Cleavage
(390) The proprietary solid support/linker is stable to all phosphoramidite reagents but is cleavable from the oligonucleotide at the end of synthesis. Cleavage is necessary so that the free 3′-OH may take part in biochemical reactions, such as extension by DNA Polymerase during PCR when the oligonucleotide serves as a primer.
(391) Deprotection
(392) After cleavage, the solution of oligonucleotide in concentrated aqueous ammonia is heated to remove protecting groups from the bases and phosphates.
(393) Bases
(394) While thymine does not require a protecting group, adenine, cytosine, and guanine do since they contain exocyclic primary amino groups. The protecting groups must be removed so that proper hydrogen bonds between the oligonucleotide and the target nucleic acid may form.
(395) The oligonucleotide in concentrated aqueous ammonia is heated. The protecting groups include: N(6)-benzoyl A, N(4)-benzoyl C, and N(2)-isobutyryl G. The product of the reaction is fully-deprotected A, C, and G bases.
(396) In addition to the standard protecting groups, the labile dimethylformamidyl G and the ‘ultramild’ protecting groups can be used for modified oligonucleotides that are sensitive to ammonia.
(397) Labile and Ultramild Protecting Groups.
(398) The dimethylformamidyl protecting group is typically removed in concentrated aqueous ammonia via heating but in significantly less time than is the isbutyryl group. The ultramild protecting groups include: N(6)-phenoxyacetyl A, N(2)-acetyl C, and N(2)-isopropylphenoxyacetyl G. They are typically removed at room temperature in a concentrated aqueous ammonia/methylamine solution.
(399) Phosphodiester Formation
(400) The β-cyanoethyl group on the free oxygen of the phosphate must be removed to convert it from a phosphate triester to a phosphate diester (phosphodiester).
(401) The mechanism of phosphodiester formation via deprotection.
(402) The cyanoethyl groups are removed in concentrated aqueous ammonia via β-elimination. The reaction is quick because the hydrogen atoms on the carbon adjacent to the electron-withdrawing cyano group are highly acidic. The products are the oligonucleotide with a native phosphodiester backbone and acrylonitrile.
(403) Yield of 5′AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG 3′ (SEQ ID NO: 1)
(404) The RNA oligos were pre-made with azide group and the peptides were pre-made with the diarylcyclooctyne moiety (DBCO). Mix DBCO-NHS ester labeled peptide with 2-4 times molar excess of azide-modified Oligos. The peptides and oligos were incubated at room temperature for 30 min or 2 hours on ice. Validation of conjugation and purification by HPLC.
Example 3
(405) Method to Prepare RNA-Peptide-AB Conjugate
(406) RNA-peptide-AB
(407) TABLE-US-00026 SEQ ID NO: 1 with SEQ ID NO: 4 AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG- Cys- Val -Asn -Asp- Thr- Phe- Ala- Gly- Ser -Thr- Phe- Ile -Ser -Asp- Glu -Val- Asp- Gly -Val- Asp Glu -Val- Ala- Lys- Lys- Lys- Ser- Lys
(408) Conjugation is based on alkyne-azide cycloaddition. This Cu-free click reaction starts from the dibenzocyclooctyne (DBCO) moiety-activated peptide
(409) TABLE-US-00027 SEQ ID NO: 4 (CVNDTFAGSTFISDEVDGVDEVAKKKSK)
and subsequently linked covalently with an azide-modified RNA
(410) TABLE-US-00028 SEQ ID NO: 1 (AAAAAAAAAACUCCUAGAACUAGCAUUACAGAUG).
The reaction is performed under physiological conditions and has no adverse effects on peptide target. This can also be used as the click chemistry fluorescence labeling and the click chemistry in peptide-based antiviral SARS-CoV-2 vaccine design.
(411) 1. Conjugation of DBCO to the peptide. The DBCO-PEGS-NHS was used to react with the NH.sub.2 groups on the peptide. The inclusion of a PEGS linker improves the water solubility of the hydrophobic DBCO, introduces a spacer and flexibility between the cysteine from peptide molecule and the RNA molecule. This will alleviate the steric effect of the peptide on the enzymatic reactions.
(412) 2. Prepare the azido-peptide or azido-oligonucleotide. The laboratory provides click chemistry modified peptide synthesis: C-terminal peptide/oligo-azide.
(413) 3. Covalent attachment of the peptide/RNA to the peptide. The reaction between DBCO and azide is slow compared to CuAAC reaction. The reaction time of 16-18 h in PBS at 4° C. is ideal to increase the final product yield. The DBCO-peptide in the intermediate reaction is stable.
(414) Copper-Free Click Chemistry RNA-Peptide Conjugation
(415) Typically, there are three biological functional groups on the peptide for the further conjugation: amino (—NH2), carboxyl (—COOH), and thiol (—SH). The most effective way is to utilize the free thiol groups from cysteine. The reaction of maleimides with thiols is widely used for bioconjugation and labeling of biomolecules.
(416) Cysteine (—SH) was used as the first amino acid of peptide:
(417) TABLE-US-00029 SEQ ID NO: 4 CVNDTFAGSTFISDEVDGVDEVAKKKSK
(418) The click chemistry is another efficient method to conjugate the peptide with other biomolecules as DNA. Also, the peptide can be modified with azide groups (—N.sub.3). One example of the peptide vaccine conjugation is the RNA-peptide against SARS-CoV-2 codified as a biomolecules fusion according to the present invention.
(419) A Simple Protocol: Conjugation of the Vaccine of the Present Invention
(420) Pre-conjugation considerations
(421) 1) Remove all additives from peptide solutions using dialysis or desalting.
(422) 2) Remove BSA and gelatin from peptide solutions.
(423) 3) Concentrate the peptide after dialysis or purification.
(424) Activation of Peptide with DBCO-NHS Ester
(425) 1) Mix peptide with 20-30 fold molar excess over peptide of DBCO-NHS ester dissolved in DMSO.
(426) 2) Incubates at room temperature for 30 min or 2 hours on ice.
(427) Quenching Activation Reaction
(428) 1) Add Tis-HCl (50-100 mM, pH 8) to the reaction.
(429) 2) Incubate at RT for 5 min or 15 minutes on ice.
(430) Equilibration and Removal of Non-Reactive DBCO-NHS Ester by Zeba Column
(431) Copper-Free Click Reaction
(432) 1) Mix DBCO-NHS ester labeled peptide with 2-4 times molar excess of azide-modified RNA.
(433) 2) Incubated overnight (around 10-12 hours) at 4° C. or 3-4 hours at room temperature.
(434) Validation of conjugation and purification by HPLC
Example 4
(435) In Vitro Assays of Cell Viability
(436) In order to test the toxicity level of RNA-peptide are carried out studies of this target in five cell cultures monitoring dead cell number. Lethal Concentration (LC) at 50% and 100% (LC.sub.50 and LC.sub.100) are calculated in each study.
(437) 1) Bronchial Epithelium obtained from Autopsy of non-cancerous individual cells (BEAS-2Bs). It was originally used as an in vitro non-tumorigenic lung epithelial model in a large variety of studies in association with lung carcinogenesis and more recently with lung virologic diseases.
(438) 2) Human Umbilical Vein Endothelial Cells (HUVECs) are cells derived from the endothelium of veins from the umbilical cord. They are used as a laboratory model system for the study of the function and pathology of endothelial cells.
(439) 3) Human Microvascular Endothelial Cell line (HMEC-1) specifically bind lymphocytes in cell adhesion assays. Thus HMEC-1 is the first immortalized that retains the morphologic, phenotypic, and functional characteristics of normal human microvascular endothelial cells. HMEC-1 possess characteristics of endothelial cells, like HUVECs.
(440) 4) Human Embryonic Kidney 293 cells, (HEK 293), are a specific cell line originally derived from human embryonic kidney cells grown in tissue culture taken from a female fetus.
(441) 5) Human Malignant Melanoma cell lines, (WM-266) used in this study were derived from biopsy of malignant primary or metastatic melanoma.
(442) Study the Toxicological Action of Control Assay:
(443) A) Phorbol myristate acetate (PMA; phorbol ester) activates protein kinase C, which then activates a wide range of signaling pathways, including ERK via effects on the upstream kinase Raf. ERK then activates a wide range of downstream targets, including S6 ribosomal protein. PMA, through its activation of PKC, can activate T-cells and stimulate low-level production of IL-2.
(444) B) Hydrogen peroxide solution (H.sub.2O.sub.2), Oxygen free radicals generated by H.sub.2O.sub.2 are involved in the multistage carcinogenic process; mechanisms include carcinogen activation, oxidative DNA damage, and tumor promotion. In this study, we have evaluated another potential mechanism of H.sub.2O.sub.2 in carcinogenesis modulation of DNA repair activities.
(445) C) Phosphate-buffered saline (PBS) is a buffer solution commonly used in biological. PBS has many uses because it is isotonic and non-toxic to most cells.
(446) D) Exosomes are a type of extracellular vesicle that contain constituents (protein, DNA, and RNA) of the cells that secrete them.
(447) The following table (Table 9) shows the Name, Code, Sigma-Aldrich No, and function pathology of five cell lines such as: BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266.
(448) TABLE-US-00030 TABLE 9 TOXICOLOGICAL ANALYSIS CELL Sigma- Study of the function and Name Code Aldrich No pathology Human Bronchial BEAS- 95102433 with lung cells Epithelium cells 2B Human Umbilical HUVEC C-12203 with endothelial cells vein Endothelial Cells Human Microvascular HMEC- S100-05A with endothelial cells Endothelial Cells 1 Human embryonic HEK293 EJH014 with embryonic kidney kidney 293 cells cells Human Metastatic WM- 91061232 with Melanoma cell line Melanoma cell line 266
(449) The following table (Table 10) shows the Name, Code, provider Cat. No and function of the proliferation controls such as: PMA, H.sub.2O.sub.2, CuSO.sub.4; and assay control such as PBS and exosome and as targets: RNA, peptide-AB, peptide-A, peptide-B and RNA-peptide-AB.
(450) TABLE-US-00031 TABLE 10 TOXICOLOGICAL ANALYSIS Name Code Cat. No Function Proliferation control Phorbol 12- PMA P8139 activates a wide range of myristate 13- downstream targets acetate Hydrogen H.sub.2O.sub.2 H1009 involved in the multistage peroxide carcinogenic process solution Copper(II) CuSO.sub.4 451657 increase in DNA damage sulfate Assay control Phosphate- PBS P5493 buffer solution buffered saline Exosome HEK293 300192exo vesicle carrier of protein, Exosomes DNA and RNA Target RNA RNA LCR- RNA candidate vaccine 008rna peptide-AB peptide-AB LCR- peptide-AB candidate 008pab vaccine peptide-A peptide-A LCR-008pa peptide-A candidate vaccine peptide-B peptide-B LCR-008pb Peptide-B candidate vaccine RNA-peptide- RNA- RNA- RNA-peptide-AB candidate AB peptide-AB peptide-AB vaccine
(451) PMA Toxicological Test: % DEAD CELLS (Flow Cytometry)
(452) In order to test the toxicity level of PMA we made our studies in the five-cell cultures. We monitored dead cell number using flow cytometry according to the manufacturer's recommendations. LC50 and LC100 are calculated, and LC50 values are used as a general indicator of a target's acute toxicity.
(453) 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs)
(454) 2) Human umbilical vein endothelial cells (HUVECs)
(455) 3) Human microvascular endothelial cell line (HMEC-1)
(456) 4) Human embryonic kidney 293 cells, (HEK 293)
(457) 5) Human malignant melanoma cell lines, (WM-266)
(458) Flow Cytometry of Cell Surface Receptor Staining (FACS)
(459) The five-cell cultures are the following:
(460) 1. BEAS-2B
(461) 2. HUVEC
(462) 3. HMEC-1
(463) 4. HEK 293
(464) 5. WM-266
(465) Protocol FACS
(466) After confluency stage of the five cell lines, wash each cell (single cell suspension) and adjust cell number to a concentration of 1-5×10.sup.6 cells/ml in ice cold FACS Buffer (PBS, 0.5-1% BSA or 5-10% FBS, 0.1% NaN.sub.3 sodium azide).
(467) The five-cell cultures are usually stained in polystyrene round-bottom 12×75 mm BD polystyrene tube (cat #Z376787). It is convenient to check the viability of the cells, which should be around 95% but not less than 90%. (Important for HUVEC and HMEC-1 cell lines) Add 100 μL of each cell lines suspension to each tube. Add 0.1-10 μg/ml of the primary labeled antibody. Dilutions, if necessary, should be made in FACS buffer. Incubate for at least 30 min at room temperature or 4° C. in the dark. Wash the cells 3 times by centrifugation at 1500 rpm for 5 minutes and resuspend them in 200 μL to 1 ml of ice cold FACS buffer*. Keep the cells in the dark on ice or at 4° C. in a fridge until your scheduled time for analysis. Resuspend cells in this solution and incubate for at least 20-30 minutes at room temperature or 4° C. in the dark. Wash the cells 3 times by centrifugation at 1500 rpm for 5 minutes and resuspend them in 200 μL to 1 ml of ice cold FACS buffer. Keep the cells in the dark on ice or at 4° C. in a fridge until the scheduled time for analysis. the cells were Analyzed on the flow cytometer within 24 hours.
(468) The following table shows a) the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of PMA (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of PMA LC.sub.50 (μg/μL). c) Shows the values of PMA LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(469) TABLE-US-00032 TABLE 11 PMA Toxicological test: % DEAD CELLS (Flow Cytometry) a) Concentration WM- μg/μL BEAS-2B HUVEC HMEC-1 HEK293 266 5 2 2 3 4 1 10 7 6 8 7 9 20 14 13 11 14 12 40 42 33 29 42 38 80 63 65 72 85 53 160 86 82 91 98 76 320 95 100 100 100 98 640 100 100 100 100 100 b) c) PMA LC.sub.50 PMA LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 297 BEAS-2B 466 HUVEC 272 HUVEC 433 HMEC-1 291 HMEC-1 461 HEK293 275 HEK293 462 WM-266 310 WM-266 464
(470) H.sub.2O.sub.2 Toxicological Test: % DEAD CELLS (Flow Cytometry)
(471) In order to test the toxicity level of H.sub.2O.sub.2 studies were made in the five cell culture. Dead cell number was monitored using flow cytometry. LC.sub.50 and LC.sub.100, were LC.sub.50 values were calculated as general indicator of a target's acute toxicity. 1) Bronchial Epithelium obtained from Autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human Microvascular Endothelial Cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(472) In the following table (table 12) is showed a) the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of H.sub.2O.sub.2 (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL is showed in the following table. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of H.sub.2O.sub.2 LC.sub.50 (μg/μL). c) Shows the values of H.sub.2O.sub.2 LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(473) TABLE-US-00033 TABLE 12 H.sub.2O.sub.2 Toxicological test: % DEAD CELLS (Flow Cytometry) a) Concentration WM- μg/μL BEAS-2B HUVEC HMEC-1 HEK293 266 5 4 6 9 5 3 10 9 16 24 36 27 20 41 38 44 59 42 40 72 91 77 84 66 80 96 100 92 96 82 160 100 100 100 100 98 320 100 100 100 100 100 640 100 100 100 100 100 b) c) H.sub.2O.sub.2 LC.sub.50 H.sub.2O.sub.2 LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 214 BEAS-2B 446 HUVEC 167 HUVEC 444 HMEC-1 131 HMEC-1 461 HEK293 111 HEK293 441 WM-266 195 WM-266 451
(474) CuSO.sub.4 Toxicological Test: % DEAD CELLS (Flow Cytometry)
(475) In order to test the toxicity level of CuSO.sub.4 studies were made in the five cell culture. Dead cell number was monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated and LC.sub.50 value is calculated as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial Cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(476) In the following table (table 13) a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of CuSO.sub.4 (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of CuSO.sub.4 LC.sub.50 (μg/μL). c) Shows the values of CuSO.sub.4 LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(477) TABLE-US-00034 TABLE 13 CuSO.sub.4 Toxicological test: % DEAD CELLS (Flow Cytometry) a) Concentration HMEC- μg/μL BEAS-2B HUVEC 1 HEK293 WM-266 5 10 9 13 15 8 10 25 28 36 44 17 20 64 69 60 55 63 40 86 83 77 79 81 80 100 100 100 100 100 160 100 100 100 100 100 320 100 100 100 100 100 640 100 100 100 100 100 b) c) P CuSO.sub.4 LC.sub.50 CuSO.sub.4 LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 74 BEAS-2B 439 HUVEC 70 HUVEC 434 HMEC-1 30 HMEC-1 438 HEK293 — HEK293 459 WM-266 125 WM-266 440
(478) PBS Toxicological Test: % DEAD CELLS (Flow Cytometry)
(479) In order to test the toxicity level of PBS studies are made in the five cell culture. Dead cell number is monitored using flow cytometry. LC.sub.50 and LC.sub.100, are calculated and LC.sub.50 values are general indicator of a target's acute toxicity. 1. Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2. Human umbilical vein endothelial cells (HUVECs) 3. Human microvascular endothelial Cell line (HMEC-1) 4. Human embryonic kidney 293 cells, (HEK 293) 5. Human malignant melanoma cell lines, (WM-266)
(480) In the following table (Table 14), a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of PBS (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of PBS LC.sub.50 (μg/μL). c) Shows the values of PBS LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(481) TABLE-US-00035 TABLE 14 PBS Toxicological test: % DEAD CELLS (Flow Cytometry) a) Concentration HMEC- μg/μL BEAS-2B HUVEC 1 HEK293 WM-266 5 1 2 1 3 1 10 2 3 3 9 2 20 3 6 5 14 4 40 5 8 7 25 9 80 12 15 15 33 17 160 22 21 25 49 38 320 44 48 45 79 46 640 56 66 77 86 62 b) c) Cell lines PBS LC.sub.50 (μg/μL) Cell lines PBS LC.sub.100 (μg/μL) BEAS-2B 490 BEAS-2B 616 HUVEC 468 HUVEC 612 HMEC-1 451 HMEC-1 580 HEK293 356 HEK293 539 WM-266 456 WM-266 587
(482) Exosome Toxicological Test: % DEAD CELLS (Flow Cytometry)
(483) In order to test the toxicity level of exosome studies are made in the five cell cultures. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1. Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2. Human umbilical vein endothelial cells (HUVECs) 3. Human microvascular endothelial Cell line (HMEC-1) 4. Human embryonic kidney 293 cells, (HEK 293) 5. Human malignant melanoma cell lines, (WM-266)
(484) In the following table (Table 15) a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of exosome (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of exosome LC.sub.50 (μg/μL). c) Shows the values of exosome LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(485) TABLE-US-00036 TABLE 15 a) Exosome Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 1 1 1 1 1 10 1 1 1 1 1 20 1 1 1 1 1 40 3 4 3 3 3 80 8 9 8 8 8 160 21 16 23 20 21 320 74 56 56 89 65 640 100 100 100 100 100 b) c) Exosome LC.sub.50 Exosome LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 423 BEAS-2B 516 HUVEC 434 HUVEC 528 HMEC-1 434 HMEC-1 530 HEK293 420 HEK293 510 WM-266 430 WM-266 524
(486) RNA Toxicological Test: % DEAD CELLS (Flow Cytometry)
(487) In order to test the toxicity level of RNA studies are made in the five cell culture. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated, and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(488) In the following table (Table 16) a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of RNA (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of RNA LC.sub.50 (μg/μL). c) Shows the values of RNA LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(489) TABLE-US-00037 TABLE 16 a) RNA Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 13 15 16 19 11 10 26 35 42 51 39 20 38 49 61 64 61 40 63 69 76 79 80 80 85 82 89 95 98 160 94 98 100 100 100 320 100 100 100 100 100 640 100 100 100 100 100 b) c) RNA LC.sub.50 RNA LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 129 BEAS-2B 459 HUVEC 67 HUVEC 452 HMEC-1 131 HMEC-1 461 HEK293 — HEK293 456 WM-266 36 WM-266 444
(490) Peptide-AB Toxicological Test: % DEAD CELLS (Flow Cytometry)
(491) In order to test the toxicity level of Peptide AB studies are made in the five cell cultures. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated, and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(492) In the following table (Table 17), a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of Peptide-AB (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of Peptide-AB LC.sub.50 (μg/μL). c) Shows the values of Peptide-AB LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(493) TABLE-US-00038 TABLE 17 a) Peptide-AB Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 8 7 6 13 4 10 12 11 12 28 9 20 54 52 75 88 46 40 72 76 92 96 85 80 86 91 100 100 96 160 100 100 100 100 100 320 100 100 100 100 100 640 100 100 100 100 100 b) c) Peptide-AB, LC.sub.50 Peptide-AB, LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 167 BEAS-2B 444 HUVEC 179 HUVEC 456 HMEC-1 149 HMEC-1 450 HEK293 6 HEK293 7 WM-266 36 WM-266 444 b) c)
(494) Peptide-A Toxicological Test: % DEAD CELLS (Flow Cytometry)
(495) In order to test the toxicity level of Peptide A studies are made in the five cell cultures. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated, and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(496) In the following table (Table 18), a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of Peptide-A (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of Peptide-A LC.sub.50 (μg/μL). c) Shows the values of Peptide-A LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(497) TABLE-US-00039 TABLE 18 a) Peptide-A Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 5 6 7 11 3 10 16 19 21 33 12 20 66 51 61 75 39 40 83 74 85 92 74 80 92 95 100 100 100 160 100 100 100 100 100 320 100 100 100 100 100 640 100 100 100 100 100 b) c) Peptide-A, LC.sub.50 Peptide-A, LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 158 BEAS-2B 447 HUVEC 156 HUVEC 445 HMEC- 1 122 HMEC- 1 452 HEK293 16 HEK293 450 WM-266 214 WM-266 445
(498) Peptide-B Toxicological Test: % DEAD CELLS (Flow Cytometry)
(499) In order to test the toxicity level of Peptide B studies are made in the five cell cultures. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated, and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(500) In the following table a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of Peptide-B (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of Peptide-B LC.sub.50 (μg/μL). c) Shows the values of Peptide-B LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry
(501) TABLE-US-00040 TABLE 19 a) Peptide-B Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 7 7 8 9 6 10 21 23 31 27 14 20 49 49 45 41 44 40 67 68 77 71 74 80 86 93 94 86 93 160 97 100 100 95 100 320 100 100 100 100 100 640 100 100 100 100 100 b) c) Peptide-B, LC.sub.50 Peptide-B, LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 161 BEAS-2B 462 HUVEC 145 HUVEC 446 HMEC-1 114 HMEC-1 444 HEK293 135 HEK293 450 WM-266 179 WM-266 445
(502) RNA-peptide-AB Toxicological Test: % DEAD CELLS (Flow Cytometry)
(503) In order to test the toxicity level of RNA-peptide-AB, studies are made in the five cell cultures. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated, and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(504) In the following table (table 20), a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of vaccine RNA-peptide-AB (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of vaccine LC.sub.50 (μg/μL). c) Shows the values of vaccine LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(505) TABLE-US-00041 TABLE 20 a) RNA-peptide-AB (melody) Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 3 4 3 3 2 10 11 7 7 6 5 20 18 12 14 11 14 40 45 35 36 39 33 80 78 79 81 92 65 160 92 96 93 100 91 320 100 100 100 100 100 640 100 100 100 100 100 b) c) vaccine LC.sub.50 vaccine LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 263 BEAS-2B 455 HUVEC 280 HUVEC 458 HMEC-1 286 HMEC-1 463 HEK293 135 HEK293 450 WM-266 299 WM-266 456
(506) According to the previous studies, in a preferred embodiment, an effective amount of the composition of the RNA-peptide-AB according to the present invention is between about 135 μg/μL and 299 μg/μL.
Example 5
(507) Efficacy Studies of the Composition of the Present Invention
(508) 1) RNA Toxicological Test: % DEAD CELLS (Flow Cytometry)
(509) In order to test the toxicity level of RNA after vaccine incubation 16 hours, we made our studies in the five cell cultures. We monitored dead cell number using flow cytometry. LC.sub.50 and LC.sub.100 are calculated and LC.sub.50 values are used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(510) In the following Table (Table 21), a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of RNA (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL after vaccine incubation 16 hours. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of vaccine LC.sub.50 (μg/μL). c) Shows the values of vaccine LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(511) TABLE-US-00042 TABLE 21 a) RNA Toxicological test: % DEAD CELL (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 8 7 5 6 6 10 12 14 18 16 9 20 21 29 24 33 20 40 39 42 38 44 46 80 66 63 68 61 60 160 85 83 77 72 74 320 98 92 89 86 94 640 100 100 100 100 100 b) c) RNALC.sub.50 RNA LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 249 BEAS-2B 472 HUVEC 243 HUVEC 482 HMEC-1 259 HMEC-1 490 HEK293 251 HEK293 499
(512) RNA Toxicological Test: % DEAD CELLS (Flow Cytometry)
(513) In order to test the toxicity level of RNA after incubation of the composition of the present invention, two times of 16 hours each incubation, studies are in the five-cell cultures. Dead cells number are monitored using flow cytometry. LC.sub.50 and LC.sub.100 are calculated and LC.sub.50 values are used as an indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(514) In the following Table: a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of RNA (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL after vaccine incubation 16 hours two times. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of vaccine LC.sub.50 (μg/μL). c) Shows the values of vaccine LC.sub.100 (μg/μL). The number of dead cells was monitored using the flow cytometry.
(515) TABLE-US-00043 TABLE 22 a) Composition+ Composition + RNA Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 4 3 5 4 2 10 9 7 11 9 7 20 16 18 14 25 15 40 31 35 33 44 30 80 49 48 45 66 43 160 68 63 59 80 57 320 89 84 87 92 83 640 100 100 100 100 100 b) c) RNA LC.sub.50 RNA LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 299 BEAS-2B 482 HUVEC 311 HUVEC 489 HMEC-1 306 HMEC-1 498 HEK293 270 HEK293 474 WM-266 330 WM-266 495
(516) RNA Toxicological Test: % DEAD CELLS (Flow Cytometry)
(517) In order to test the toxicity level of RNA after vaccine incubation three times of 16 hours each incubation, we made our studies in the five-cell cultures. We monitored dead cell number using flow cytometry. We calculated LC.sub.50 and LC.sub.100, were LC.sub.50 values are frequently used as a general indicator of a target's acute toxicity. 1) Bronchial epithelium obtained from autopsy of non-cancerous individual cells (BEAS-2Bs) 2) Human umbilical vein endothelial cells (HUVECs) 3) Human microvascular endothelial cell line (HMEC-1) 4) Human embryonic kidney 293 cells, (HEK 293) 5) Human malignant melanoma cell lines, (WM-266)
(518) In the following table (Table 23), a) Shows the percentage of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to serial concentration of RNA (5 μg/μL, 10 μg/μL, 20 μg/μL, 40 μg/μL, 80 μg/μL, 160 μg/μL, 320 μg/μL and 640 μg/μL after vaccine incubation 16 hours three times. It was made using in serial dilution ½ starting from 640 μg/μL). b) Shows the values of vaccine LC.sub.50 (μg/μL). c) Shows the values of vaccine LC.sub.100 (μg/μL). The number of dead cells was monitored.
(519) TABLE-US-00044 TABLE 23 a) vaccine + vaccine + vaccine + RNA Toxicological test: % DEAD CELLS (Flow Cytometry) Concentration μg/μL BEAS-2B HUVEC HMEC-1 HEK293 WM-266 5 4 4 4 5 2 10 8 6 10 7 6 20 14 15 13 24 16 40 32 33 32 43 29 80 48 45 48 65 42 160 68 62 60 79 58 320 88 83 86 91 82 640 100 100 100 100 100 b) c) RNA LC.sub.50 RNA LC.sub.100 Cell lines (μg/μL) Cell lines (μg/μL) BEAS-2B 303 BEAS-2B 481 HUVEC 319 HUVEC 497 HMEC-1 308 HMEC-1 491 HEK293 164 HEK293 258 WM-266 329 WM-266 490
(520) The following table shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of PMA and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(521) TABLE-US-00045 TABLE 24 PMA RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 297 263 HUVEC 272 280 HMEC-1 291 286 HEK293 275 135 WM-266 310 299
(522) The following table (Table 25) shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of H.sub.2O.sub.2 and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(523) TABLE-US-00046 TABLE 25 H.sub.2O.sub.2 RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 214 263 HUVEC 167 280 HMEC-1 131 286 HEK293 111 135 WM-266 195 299
(524) The following table (Table 26) Shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of CuSO.sub.4 and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(525) TABLE-US-00047 TABLE 26 CuSO.sub.4 RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 74 263 HUVEC 70 280 HMEC-1 30 286 WM-266 125 299 HEK293 — 135
(526) The following table (table 27) shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of PBS and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(527) TABLE-US-00048 TABLE 27 PBS RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 490 263 HUVEC 468 280 HMEC-1 451 286 HEK293 356 299 WM-266 456 135
(528) The following Table (Table 28), shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of Exosome and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(529) TABLE-US-00049 TABLE 28 Exosome RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 423 263 HUVEC 434 280 HMEC-1 434 286 WM-266 430 299 HEK293 420 135
(530) The following Table (Table 29), shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of RNA and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry. (The LC.sub.50 of RNA in HEK290 cell lines was not detected)
(531) TABLE-US-00050 TABLE 29 RNA RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 129 263 HUVEC 67 280 HMEC-1 131 286 WM-266 36 299 HEK293 — 135
(532) The following Table (Table 30), shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of peptide-AB and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry. (The LC.sub.50 of peptide-AB in WM-266 and HEK293 cell lines were not detected)
(533) TABLE-US-00051 TABLE 30 peptide-AB RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 167 263 HUVEC 179 280 HMEC-1 149 286 WM-266 — 299 HEK293 — 135
(534) The following Table (Table 31), shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of peptide-A and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry. (The LC.sub.50 of peptide-A in HEK293 cell lines was not detected)
(535) TABLE-US-00052 TABLE 31 peptide-A RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 158 263 HUVEC 156 280 HMEC-1 122 286 WM-266 214 299 HEK293 — 135
(536) The following Table (Table 32), shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of peptide-B and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(537) TABLE-US-00053 TABLE 32 peptide-B RNA-peptide-AB Cell lines LC.sub.50 μg/μL BEAS-2B 161 263 HUVEC 145 280 HMEC-1 114 286 HEK293 135 299 WM-266 179 135
(538) The following Table (Table 33) shows the statistical values of probability (p). Where, we compared the LC.sub.50 from vaccine candidate RNA-peptide-AB (vaccine) with target such as: PMA, H.sub.2O.sub.2, CuSO.sub.4, PBS, Exosome, RNA, peptide-AB, peptide-A and peptide-B. It is used the Student's t-test with n=6 in order to calculate p value. Our conclusion was focused to understand the statistical difference in toxicity action between vaccine and each target.
(539) TABLE-US-00054 TABLE 33 TOXICOLOGICAL ANALYSIS (Student's t-test) student T Toxicological Code (n = 6) analysis Control Proliferation LC.sub.50 PMA RNA-peptide-AB p = 0,2416 Not statistical difference H.sub.2O.sub.2 RNA-peptide-AB p = 0,0193 Statistical difference CuSO.sub.4 RNA-peptide-AB *p = 0,0014 Significative (*) Statistical difference Control assay PBS RNA-peptide-AB p = 0,0110 Statistical difference Exosome RNA-peptide-AB p = 0,0031 Statistical difference Targets assay RNA RNA-peptide-AB p = 0,0072 Statistical difference peptide-AB RNA-peptide-AB p = 0,0131 Statistical difference peptide-A RNA-peptide-AB p = 0,0057 Statistical difference peptide-B RNA-peptide-AB p = 0,0545 Statistical difference
(540) Results
(541) The studies of cell proliferation action of this invention were carried out at concentrations lethal of 50% (LC.sub.50) in cell lines such as: BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266. The result obtained shows that the vaccine RNA-peptide against SARS-CoV-2 of the present invention does not present a statistical difference in toxicity values with PMA (positive inductor of cell proliferation). Meanwhile, the vaccine of the present invention presents a statistical difference with the negative controls of proliferation such as: H.sub.2O.sub.2 and CuSO.sub.4. Being a statistically significant difference with sulfate of copper (II).
(542) In addition, the vaccine RNA-peptide against SARS-CoV-2 of the present invention shows in the five cell lines (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) a statistical difference between the toxicity values LC.sub.50 with the controls assay such as: PBS and Exosomes.
(543) Finally, the vaccine RNA-peptide against SARS-CoV-2 of the present invention shows in the five cell lines (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) a statistical difference between the toxicity values at LC.sub.50 with the test targets: RNA, peptide-AB, peptide-A, and peptide-B.
Conclusion
(544) The vaccine RNA-peptide against SARS-CoV-2 of the present invention has no equivalent mechanisms of toxicity comparing with the toxicity mechanisms different from the inducers of oxidation and DNA damage such as H.sub.2O.sub.2 and CuSO.sub.4. The vaccine candidate does not present a significant difference between the toxicity values at LC.sub.50 with the assay controls and targets statistically. These targets that are the substrate in its chemical construction (fusion between RNA and peptide-AB).
Example 6
(545) The following Table (Table 34), shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of PMA and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(546) TABLE-US-00055 TABLE 34 PMA RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 466 455 HUVEC 433 458 HMEC-1 461 463 HEK293 464 456 WM-266 462 450
(547) The following Table (Table 35), shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of H.sub.2O.sub.2 and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(548) TABLE-US-00056 TABLE 35 H.sub.2O.sub.2 RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 446 455 HUVEC 444 458 HMEC-1 461 463 HEK293 451 456 WM-266 441 450
(549) The following Table (Table 36) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of CuSO.sub.4 and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(550) TABLE-US-00057 TABLE 36 CuSO.sub.4 RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 439 455 HUVEC 434 458 HMEC-1 438 463 HEK293 440 456 WM-266 459 450
(551) The following Table (Table 37) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of PBS and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(552) TABLE-US-00058 TABLE 37 PBS RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 616 455 HUVEC 612 458 HMEC-1 580 463 HEK293 539 456 WM-266 587 450
(553) The following Table (Table 38) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of exosome and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(554) TABLE-US-00059 TABLE 38 Exosome RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 466 455 HUVEC 433 458 HMEC-1 461 463 WM-266 464 456 HEK293 462 450
(555) The following Table (Table 39) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of RNA and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry.
(556) TABLE-US-00060 TABLE 39 RNA RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 459 455 HUVEC 452 458 HMEC-1 461 463 HEK293 456 456 WM-266 444 450
(557) The following Table (Table 40) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of peptide-AB and RNA-peptide-AB. The number of dead cells was monitored using the flow cytometry. (The LC.sub.100 of peptide-AB in HEK293 cell lines was not detected)
(558) TABLE-US-00061 TABLE 40 peptide-AB RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 444 455 HUVEC 456 458 HMEC-1 450 463 WM-266 444 450 HEK293 — 456
(559) The following Table (Table 41) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of peptide-A and RNA-peptide-A. The number of dead cells was monitored using the flow cytometry.
(560) TABLE-US-00062 TABLE 41 peptide-A RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 447 455 HUVEC 445 458 HMEC-1 452 463 HEK293 450 456 WM-266 445 450
(561) The following Table (Table 42), shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of peptide-B and RNA-peptide-A. The number of dead cells was monitored using the flow cytometry.
(562) TABLE-US-00063 TABLE 42 peptide-B RNA-peptide-AB Cell lines LC.sub.100 μg/μL BEAS-2B 462 455 HUVEC 446 458 HMEC-1 444 463 HEK293 450 456 WM-266 445 450
(563) The following Table (Table 42) shows the statistical values of probability (p). Where, we compared the LC.sub.100 from vaccine candidate RNA-peptide-AB (vaccine) with target such as: PMA, H.sub.2O.sub.2, CuSO.sub.4, PBS, exosome, RNA, peptide-AB, peptide-A and peptide-B. We are using the Student's t-test with n=6 to calculate p value. Our conclusion was focused to understand the statistical difference in toxicity action between vaccine and each target.
(564) TABLE-US-00064 TABLE 43 TOXICOLOGICAL ANALYSIS (student Test) student T Toxicological Code (n = 6) analysis Control Proliferation LC.sub.100 PMA RNA-peptide-AB p = 0,9333 Not statistical difference H.sub.2O.sub.2 RNA-peptide-AB p = 0,0146 Statistical difference CuSO.sub.4 RNA-peptide-AB p = 0,0810 Not statistical difference Control assay PBS RNA-peptide-AB *p = 0,0008 Significative (*) Statistical difference Exosome RNA-peptide-AB p = 0,9332 Not statistical difference Targets assay RNA RNA-peptide-AB p = 0,3350 Not statistical difference peptide-AB RNA-peptide-AB p = 0,0594 Not statistical difference peptide-A RNA-peptide-AB p = 0,0041 Statistical difference peptide-B RNA-peptide-AB p = 0,1730 Not statistical difference
(565) Results
(566) The studies of cell proliferation action of this invention were carried out at concentrations lethal of 100% (LC.sub.100) in cell lines such as: BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266. Results obtained are that: The vaccine does not present a statistical difference in toxicity values with PMA and CuSO.sub.4. Meanwhile, the vaccine RNA-peptide against SARS-CoV-2 of the present invention has a statistical difference with the H.sub.2O.sub.2.
(567) In addition the RNA-peptide against SARS-CoV-2 of the present invention shows in the five cell lines (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) a significative statistical difference in the toxicity values LC.sub.100 with the control assay PBS and not presents significant difference in the toxicity values with the exosomes.
(568) Finally, the vaccine RNA-peptide against SARS-CoV-2 of the present invention shows in the five cell lines (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) a not statistical difference between the toxicity values at LC.sub.100 with the test targets: RNA, peptide-AB, and peptide-B. The vaccine RNA-peptide against SARS-CoV-2 of the present invention has statistical difference in the toxicity values with the peptide-A.
Conclusion
(569) This invention at LC.sub.100, comprises equivalents mechanisms of toxicity comparing with the inductor of cell proliferation (PMA) and CuSO.sub.4, as well as do not has equivalents mechanisms of toxicity comparing with H.sub.2O.sub.2. The present invention does not have a significant difference between the toxicity values at LC.sub.100 with the assay controls and targets.
Example 7
(570) The following table (Table 44) shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the RNA action after one incubation of 16 hours with RNA-peptide-AB (vaccine). The number of dead cells was monitored using the flow cytometry. (The LC.sub.50 of RNA in HEK293 cell lines was not detected)
(571) TABLE-US-00065 TABLE 44 RNA vaccine (1 dose) + RNA Cell lines LC.sub.100 μg/μL BEAS-2B 129 249 HUVEC 67 243 HMEC-1 131 259 WM-266 36 272 HEK293 — 251
(572) The following table (Table 45) shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the RNA action after two incubations of 16 hours with RNA-peptide-AB (vaccine). The number of dead cells was monitored using the flow cytometry. (The LC.sub.50 of RNA in HEK293 cell lines was not detected)
(573) TABLE-US-00066 TABLE 45 RNA vaccine(2 doses) + RNA Cell lines LC.sub.50 (μg/μL) BEAS-2B 129 299 HUVEC 67 311 HMEC-1 131 306 WM-266 36 330 HEK293 — 270
(574) The following table (Table 46) shows the comparison of lethal concentration 50% (LC.sub.50 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to RNA action after three incubations of 16 hours with RNA-peptide-AB (vaccine). The number of dead cells was monitored using the flow cytometry. (The LC.sub.50 of RNA in HEK293 cell lines was not detected)
(575) TABLE-US-00067 TABLE 46 RNA vaccine (3 doses) + RNA Cell lines LC.sub.50 (μg/μL) BEAS-2B 129 303 HUVEC 67 319 HMEC-1 131 308 WM-266 36 329 HEK293 — 164
(576) The following table (Table 47) shows the statistical values of probability (p). The Student's t-test with n=6 is used to calculate p value. According to RNA action after one, two and three serial incubations of 16 hours with RNA-peptide-AB (vaccine). The conclusion was focused to understand the statistical difference in LC.sub.50 to estimate the vaccine efficacy as vaccine in “In vitro” test in cell lines such as: BEAS-2B, HUVEC, HMEC-1 and WM-266.
(577) TABLE-US-00068 TABLE 47 EFFICACY ANALYSIS Efficacy of Control Proliferation LC.sub.50 student T Efficacy Code (n = 6) analysis RNA vaccine incubation 16 hours (1 time) + RNA One dose p = 0,0086 Statistical difference RNA vaccine incubation 16 hours (2 times) + RNA Two doses p = 0,0050 Statistical difference RNA vaccine incubation 16 hours (3 times) + RNA Three doses p = 0,0045 Statistical difference
(578) Results
(579) The studies of efficacy of the vaccine RNA-peptide against SARS-CoV-2 of the present invention were monitored by flux cytometry (cell viability) at concentrations lethal of 50% (LC.sub.50) in cell lines such as: BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266. Results obtained are that: The five-cell lines after vaccine incubation of 16 hours before treatment with RNA induced metabolic adaptation and keep this behavior in new adapting cellular pathways as “temporal memory”. The present invention shows statistical difference in the toxicity values between the five cell lines incubated with vaccine vaccine (one, two and three times of incubation or doses) RNA and placebo groups of cells (without vaccine incubation).
Conclusion
(580) The vaccine RNA-peptide against SARS-CoV-2 of the present invention shows not equivalents mechanisms of toxicity at LC.sub.50 comparing the cell lines (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) incubated with the vaccine and the same cell lines with placebo assay. Three doses of the vaccine RNA-peptide against SARS-CoV-2 of the present invention can induce temporal memory in adapting pathway against RNA infection.
Example 8
(581) The following table (Table 48) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of RNA and RNA after one incubation of 16 hours with RNA-peptide-AB (vaccine).
(582) TABLE-US-00069 TABLE 48 RNA vaccine (1 dose) + RNA Cell lines LC.sub.100 (μg/μL) BEAS-2B 459 472 HUVEC 452 482 HMEC-1 461 490 HEK293 456 499 WM-266 444 482
(583) The following table (Table 49) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of RNA and RNA after two incubations of 16 hours with RNA-peptide-AB.
(584) TABLE-US-00070 TABLE 49 RNA vaccine (2 doses) + RNA Cell lines LC.sub.100 (μg/μL) BEAS-2B 459 482 HUVEC 452 489 HMEC-1 461 498 HEK293 456 474 WM-266 444 495
(585) The following table (Table 50) shows the comparison of lethal concentration 100% (LC.sub.100 μg/μL) of dead cells (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) according to the action of RNA and RNA after three incubations of 16 hours with RNA-peptide-AB (vaccine).
(586) TABLE-US-00071 TABLE 50 RNA vaccine (3 doses) + RNA Cell lines LC.sub.100 (μg/μL) BEAS-2B 459 481 HUVEC 452 497 HMEC-1 461 491 HEK293 456 258 WM-266 444 490
(587) The following table (Table 51) shows the statistical values of probability (p). We are using the Student's t-test with n=6 to calculate p value. According to RNA action after one, two and three serial incubations of 16 hours with RNA-peptide-AB (vaccine). Our conclusion was focused to understand the statistical difference in LC.sub.100 in order to estimate the vaccine efficacy as vaccine in “In vitro” test in cell lines such as: cells (BEAS-2B, HUVEC, HMEC-1 and WM-266).
(588) TABLE-US-00072 TABLE 51 EFFICACY ANALYSIS Efficacy of Control Proliferation LC.sub.100 student T Efficacy Code (n = 6) analysis RNA vaccine incubation 16 hours (1 time) + RNA One dose p = 0,0038 Statistical difference RNA vaccine incubation 16 hours (2 times) + RNA Two doses p = 0,0052 Statistical difference RNA vaccine incubation 16 hours (3 times) + RNA Three doses p = 0,8232 Not statistical difference
(589) Results
(590) The studies of the efficacy of the vaccine RNA-peptide against SARS-CoV-2 of the present invention were monitored by flux cytometry (cell viability) at concentrations lethal of 100% (LC.sub.100) in cell lines such as: BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266. Result obtained are that: The five cell lines after vaccine RNA-peptide against SARS-CoV-2 incubation of 16 hours before treatment with RNA induced metabolic adaptation and keep this behavior in new adapting cellular pathways as “temporal memory”. The present invention shows statistical difference in the toxicity values between the five cell lines incubated with vaccine RNA-peptide against SARS-CoV-2 one or two doses and the placebo groups of cells (without vaccine incubation). With three doses of vaccine the five cell lines and placebo not shows statistical difference in the toxicity values.
Conclusion
(591) The vaccine RNA-peptide against SARS-CoV-2 of the present invention at LC.sub.100, comprises equivalents mechanisms of toxicity comparing the cell lines (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266) incubated with the vaccine and placebo assay. Two doses of the vaccine RNA-peptide against SARS-CoV-2 induces temporal memory in adapting pathway against RNA infection.
Example 9
(592) Studies of the efficacy of the vaccine RNA-peptide against SARS-CoV-2 were made in five cell cultures, in vitro assay, where dead cell number was monitored using flow cytometry in percentages of: BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266 cells.
(593) The efficacy of the vaccine RNA-peptide against SARS-CoV-2 was tested by incubating vaccine RpA (RNA-peptide A) and vaccine RpAB (RNA-peptide AB). Both incubations were pending 16 hours with vaccine LC.sub.50 (μg/μL), which was determined in a toxicological assay in the 5 cell cultures previously described.
(594) The incubation of the vaccine RNA-peptide against SARS-CoV-2, also referred as vaccine, was made 1, 2 and 3 times of 16 hours of incubation in the five cell cultures. “Placebo” is used as control in each cell culture without incubation to determinate the percentage of dead cells by comparing incubated cells and placebo dead cells.
(595) In one embodiment, RNA-peptide-A vaccine, as preventive vaccine, comprises an efficacy of about 78.95%.
(596) 1. Studies of Efficacy with a Single Incubation Dose of LC.sub.50 of RNA-Peptide A. (Preventive Vaccine with a Single Dose)
(597) The Table 52 shows the efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with a single dose of LC.sub.50 incubation of the vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(598) TABLE-US-00073 TABLE 52 Dead cell % (2) Dead cell % (1) Placebo: (0 (1 incubation with incubation with vaccine + incubation vaccine + incubation Efficacy: with viral mRNA) with viral mRNA) [100 − (Dead Both incubation Both incubation cell % (1)/ Cell lines were with LC50 were with LC50 Dead cell % confluence (μg/μL) (μg/μL)) (2)] % BEAS-2B 44 249 82.3 HUVEC 58 243 76.13 HMEC-1 49 259 81.08 HEK293 56 251 77.69 WM-266 61 272 77.57 Media value 78.95
(599) 2. Studies of Vaccine Efficacy with a Single Incubation Dose of LC.sub.50 of RNA-Peptide AB.
(600) The Table 53 shows the efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with a single dose of LC.sub.50 incubation of therapeutic vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266). We are showing the vaccine therapeutic efficacy value for each cell culture and the media value.
(601) TABLE-US-00074 TABLE 53 (1 incubation with Vaccine + Placebo: (0 incubation incubation with with viral Vaccine + Vaccine mRNA) incubation with Efficacy: Both viral mRNA) [100 − (Dead incubation Both incubation cell % (1)/ were with were with LC.sub.50 Dead cell % Cell lines confluence LC.sub.50 (μg/μL) (μg/μL) (2)] % BEAS-2B 22 255 91.37 HUVEC 19 266 92.86 HMEC-1 15 288 94.79 HEK293 16 275 94.18 WM-266 12 293 95.90 Media value 93.82
(602) 3. Studies of Efficacy with Two Incubation Doses of LC.sub.50 of RNA-Peptide A. (Preventive Vaccine with Two Doses)
(603) The Table 54 shows the efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with two doses of LC.sub.50 incubation of preventive vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(604) TABLE-US-00075 TABLE 54 Dead cell % Dead cell % (2) (1) (2 incubation Placebo: (0 with vaccine + incubation with incubation vaccine + vaccine with viral mRNA) incubation with Efficacy: Both viral mRNA) [100 − (Dead incubation Both incubation cell % (1)/ were with were with LC.sub.50 Dead cell % Cell lines confluence LC.sub.50 (μg/μL) (μg/μL)) (2)] % BEAS-2B 27 317 91.48 HUVEC 25 340 92.65 HMEC-1 29 344 91.57 HEK293 22 298 92.62 WM-266 17 301 94.35 Media value 92.53
(605) 4. Studies of Efficacy with 2 Incubation Doses of LC.sub.50 of RNA-Peptide AB. (Therapeutic Vaccine with Two Doses).
(606) The Table 55 shows the efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with two doses of LC.sub.50 incubation of vaccine therapeutic vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(607) TABLE-US-00076 TABLE 55 (2 incubation with vaccine + Placebo: (0 incubation incubation with with viral vaccine + vaccine mRNA) incubation with Efficacy: Both viral mRNA) [100 − (Dead incubation Both incubation cell % (1)/ were with were with LC.sub.50 Dead cell % Cell lines confluence LC.sub.50 (μg/μL) (μg/μL) (2)] % BEAS-2B 24 266 90.98 HUVEC 27 273 90.10 HMEC-1 31 282 89.00 HEK293 22 259 91.51 WM-266 29 254 88.58 Media value 90.03
(608) 5. Studies of Vaccine Efficacy with Three Incubation Doses of LC.sub.50 of RNA-Peptide A. (Preventive Vaccine with Three Doses)
(609) The Table 56 shows the vaccine efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with three doses of LC.sub.50 incubation of preventive vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(610) TABLE-US-00077 TABLE 56 Dead cell % Dead cell % (2) (1) (3 incubation Placebo: (0 with Vaccine + incubation with incubation Vaccine + Vaccine with viral mRNA) incubation with Efficacy: Both viral mRNA) [100 − (Dead incubation Both incubation cell % (1)/ were with were with LC.sub.50 Dead cell % Cell lines confluence LC.sub.50 (μg/μL) (μg/μL)) (2)] % BEAS-2B 60 317 81.07 HUVEC 87 354 75.42 HMEC-1 56 342 83.63 HEK293 49 298 83.56 WM-266 65 319 79.62 Media value 80.66
(611) 6) Studies of Vaccine Efficacy with Three Incubation Doses of LC.sub.50 of RNA-Peptide AB. (Therapeutic Vaccine with Three Doses)
(612) The Table 57 shows the vaccine efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with three doses of LC.sub.50 incubation of preventive vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(613) TABLE-US-00078 TABLE 57 (3 incubation with Vaccine + Placebo: (0 incubation incubation with with viral Vaccine + Vaccine mRNA) incubation with Efficacy: Both viral mRNA) [100 − (Dead incubation Both incubation cell % (1)/ were with were with LC.sub.50 Dead cell % Cell lines confluence LC.sub.50 (μg/μL) (μg/μL) (2)] % BEAS-2B 15 238 93.70 HUVEC 11 245 95.51 HMEC-1 17 263 93.54 HEK293 24 278 91.37 WM-266 19 299 93.65 Media value 93.55
(614) 7. Preventive Efficacy
(615) The Table 58 shows the Efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with one, two and three doses of LC.sub.50 incubation of vaccine therapeutic vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(616) The Statistical Values of Probability (p).
(617) Student's t-test with n=6 to calculate p value was used. According to mRNA avian coronavirus action after one, two and three doses incubations of 16 hours with mRNA-peptide-A (vaccine preventive). The conclusion was focused to understand the statistical difference in LC.sub.50 in order to estimate the vaccine preventive efficacy as vaccine in “In vitro” test in cell lines such as: cells (BEAS-2B, HUVEC, HMEC-1 and WM-266). In the present study, the preventive efficacy values obtained in the five cell lines differ statistically between the value of two doses when compared with a single or three doses, p=5.321. These results suggested that the application of two doses is more effective.
(618) TABLE-US-00079 TABLE 58 Vaccine Efficacy: Vaccine Efficacy: Vaccine Efficacy: [100 − (Dead [100 − (Dead cell % [100 − (Dead cell % (1)/Dead (1)/Dead cell % cell % (1)/ Cell lines cell % (2)] (2)] Dead cell % (2)] confluence 1 dose 2 doses 3 doses BEAS-2B 82.3 91.48 81.07 HUVEC 76.13 92.65 75.42 HMEC-1 81.08 91.57 83.63 HEK293 77.69 92.62 83.56 WM-266 77.57 94.35 79.62 Media value 78.95 92.53 80.66
(619) 8. Therapeutic Efficacy
(620) The Table 59 shows the Efficacy studies to face mRNA avian coronavirus (16 hours of incubation with LC.sub.50 mRNA) with one, two and three doses of LC.sub.50 incubation of vaccine therapeutic vaccine pending 16 hours in cell cultures (BEAS-2B, HUVEC, HMEC-1, HEK293 and WM-266).
(621) The Statistical Values of Probability (p).
(622) Student's t-test with n=6 to calculate p value was used. According to mRNA avian coronavirus action after one, two and three doses incubations of 16 hours with mRNA-peptide-A (vaccine therapeutic). The conclusion was focused to understand the statistical difference in LC.sub.50 in order to estimate the vaccine therapeutic efficacy as vaccine in “In vitro” test in cell lines such as: cells (BEAS-2B, HUVEC, HMEC-1 and WM-266). In the present study, the therapeutic efficacy values obtained in the five cell lines do not differ statistically significantly between the three doses applied, p**=0.004. As a result, the application of single doses is recommended.
(623) TABLE-US-00080 TABLE 59 Vaccine Efficacy: Vaccine Efficacy: Vaccine Efficacy: [100 − (Dead [100 − (Dead [100 − (Dead cell % (1)/ cell % (1)/ cell % (1)/ Cell lines Dead cell % (2)] Dead cell % (2)] Dead cell % (2)] confluence 1 dose 2 doses 3 doses BEAS-2B 91.37 90.98 93.70 HUVEC 92.86 90.10 95.51 HMEC-1 94.79 89.00 93.54 HEK293 94.18 91.51 91.37 WM-266 95.90 88.58 93.65 Media value 93.82 90.03 93.55
(624) The foregoing description conveys the best understanding of the objectives and advantages of the present invention. Different embodiments may be made of the inventive concept of this invention. It is to be understood that all matter disclosed herein is to be interpreted merely as illustrative, and not in a limiting sense.
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