WO2022206821A1 - Rna delivery system for treating parkinson's disease - Google Patents
Rna delivery system for treating parkinson's disease Download PDFInfo
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- WO2022206821A1 WO2022206821A1 PCT/CN2022/083996 CN2022083996W WO2022206821A1 WO 2022206821 A1 WO2022206821 A1 WO 2022206821A1 CN 2022083996 W CN2022083996 W CN 2022083996W WO 2022206821 A1 WO2022206821 A1 WO 2022206821A1
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- sequence
- rna
- delivery system
- targeting
- treating parkinson
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Definitions
- the present application relates to the field of biomedical technology, in particular to an RNA delivery system for treating Parkinson's disease.
- Parkinson's disease also known as tremor palsy, is a common neurodegenerative disease of the middle-aged and elderly people. The main lesions are in the substantia nigra and striatum. Parkinson's disease is the fourth most common neurodegenerative disease in older adults.
- RNA interference (RNAi) therapy has been considered a promising strategy for the treatment of human diseases since its invention, but many problems have been encountered during clinical practice, and the development of this therapy has lagged far behind expectations.
- RNA cannot exist stably outside the cell for a long time, because RNA will be degraded into fragments by RNases rich in extracellular, so it is necessary to find a method that can make RNA stable outside the cell and can enter specific tissues in a targeted manner. Highlight the effect of RNAi therapy.
- Virus (Biological virus) is a small individual, simple structure, containing only one nucleic acid (DNA or RNA), must be parasitic in living cells and replicated non-cellular organisms. Viral vectors can bring genetic material into cells. The principle is to use the molecular mechanism of viruses to transmit their genomes into other cells for infection. It can occur in a complete living body (in vivo) or cell culture (in vitro), mainly used in Basic research, gene therapy or vaccines. However, there are few related studies on the use of viruses as vectors to deliver RNA, especially siRNA, using a special self-assembly mechanism.
- the Chinese Patent Publication No. CN108624590A discloses a siRNA capable of inhibiting the expression of DDR2 gene; the Chinese Patent Publication No. CN108624591A discloses a siRNA capable of silencing the ARPC4 gene, and the siRNA is modified with ⁇ -phosphorus-selenium;
- the Chinese Patent Publication No. CN108546702A discloses a siRNA targeting long-chain non-coding RNA DDX11-AS1.
- the Chinese Patent Publication No. CN106177990A discloses a siRNA precursor that can be used for various tumor treatments. These patents design specific siRNAs to target certain diseases caused by genetic changes.
- Chinese Patent Publication No. CN108250267A discloses a polypeptide, polypeptide-siRNA induced co-assembly, using polypeptide as a carrier of siRNA.
- the Chinese Patent Publication No. CN108117585A discloses a polypeptide for promoting apoptosis of breast cancer cells through targeted introduction of siRNA, and the polypeptide is also used as the carrier of siRNA.
- the Chinese Patent Publication No. CN108096583A discloses a nanoparticle carrier, which can be loaded with siRNA with breast cancer curative effect while containing chemotherapeutic drugs.
- exosomes can deliver miRNAs to recipient cells, which secrete miRNAs at relatively low concentrations , which can effectively block the expression of target genes.
- Exosomes are biocompatible with the host immune system and possess the innate ability to protect and transport miRNAs across biological barriers in vivo, thus becoming a potential solution to overcome problems associated with siRNA delivery.
- the Chinese Patent Publication No. CN110699382A discloses a method for preparing siRNA-delivering exosomes, and discloses the technology of separating exosomes from plasma and encapsulating siRNA into exosomes by electroporation .
- the embodiments of the present application provide an RNA delivery system for treating Parkinson's and its application, so as to solve the technical defects existing in the prior art.
- One of the inventions of the present application is to provide an RNA delivery system for treating Parkinson's disease.
- the system includes a viral vector carrying an RNA segment capable of treating Parkinson's disease. It is enriched in the host organ tissue and endogenously and spontaneously forms a composite structure containing the RNA fragment capable of treating Parkinson's disease, and the composite structure can deliver the RNA fragment into the target tissue to achieve Parkinson's disease. Treatment. After the RNA fragment is delivered to the target tissue, it can inhibit the expression of the matching gene, thereby inhibiting the development of disease in the target tissue.
- the target tissue is the brain.
- the viral vector is an adenovirus-associated virus.
- adenovirus-associated virus is adenovirus-associated virus type 5, adenovirus-associated virus type 8 or adenovirus-associated virus type 9.
- RNA fragment comprises one, two or more specific RNA sequences with medical significance, and the RNA sequences are siRNA, shRNA or miRNA with medical significance.
- the viral vector comprises a promoter and a targeting tag
- the targeting tag can form the targeting structure of the composite structure in the organ tissue of the host
- the targeting structure is located on the surface of the composite structure
- the The complex structure is capable of finding and binding to the target tissue through the targeting structure, delivering the RNA fragment into the target tissue.
- the viral vector includes any one of the following circuits or a combination of several circuits: promoter-RNA fragment, promoter-targeting tag, promoter-RNA fragment-targeting tag; each of the viral vectors including at least one RNA segment and one targeting tag, the RNA segment and targeting tag are located in the same circuit or are located in different circuits.
- the viral vector also includes a flanking sequence, a compensation sequence and a loop sequence that can make the circuit fold into a correct structure and express, and the flanking sequence includes a 5' flanking sequence and a 3' flanking sequence;
- the viral vector includes any one of the following lines or a combination of several lines: 5'-promoter-5' flanking sequence-RNA fragment-loop sequence-compensating sequence-3' flanking sequence, 5'-promoter-target To tag, 5'-promoter-targeting tag-5'flanking sequence-RNA fragment-loop sequence-compensating sequence-3'flanking sequence.
- the 5' flanking sequence is ggatcctggaggcttgctgaaggctgtatgctgaattc or a sequence whose homology is greater than 80%;
- the loop sequence is gttttggccactgactgac or a sequence whose homology is greater than 80%;
- flanking sequence is accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag or its homology is greater than 80% sequence;
- the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-5 bases are deleted.
- the purpose of deleting bases 1-5 of the reverse complement of the RNA is to make the sequence unexpressed.
- siRNA and miRNA precursors due to deletion of the 9th and 10th bases of the reverse complementary strand of the active strand (such as the reverse complementary strand of siRNA), the active strand of siRNA and miRNA will form a bulge. structure, which facilitates more efficient silencing of gene expression. To sum up, it is an accepted conclusion that the silencing efficiency can be improved by deleting the reverse complementary sequence of the 9th and 10th bases.
- the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 bases are deleted.
- the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 consecutive bases are deleted.
- the compensation sequence is the reverse complement of the RNA fragment, and the 9th and/or 10th bases are deleted.
- adjacent lines are connected by a sequence composed of sequences 1-3 (sequence 1-sequence 2-sequence 3);
- sequence 1 is CAGATC
- sequence 2 is a sequence consisting of 5-80 bases
- sequence 3 is TGGATC.
- adjacent lines are connected by sequence 4 or a sequence with more than 80% homology to sequence 4;
- sequence 4 is CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC.
- organ tissue is liver
- composite structure is exosome
- the targeting tag is selected from targeting peptides or targeting proteins with targeting function.
- the targeting peptides include RVG targeting peptides, GE11 targeting peptides, PTP targeting peptides, TCP-1 targeting peptides, and MSP targeting peptides;
- the targeting proteins include RVG-LAMP2B fusion protein, GE11-LAMP2B fusion protein, PTP-LAMP2B fusion protein, TCP-1-LAMP2B fusion protein, and MSP-LAMP2B fusion protein.
- the targeting tag is preferably an RVG targeting peptide or RVG-LAMP2B fusion protein that can precisely target brain tissue.
- the length of the RNA sequence is 15-25 nucleotides.
- the length of the RNA sequence can be 16, 17, 18, 19, 20, 21, 22, 23, 24, 25 nucleotides.
- the RNA sequence is 18-22 nucleotides in length.
- RNA capable of treating Parkinson's is selected from: siRNA of the LRRK2 gene, or an RNA sequence with a homology of more than 80% to the above sequence, or a nucleic acid molecule encoding the above RNA. It should be noted that the RNA sequences in the "nucleic acid molecules encoding the above RNA sequences" here also include RNA sequences with a homology of more than 80% of each RNA.
- the siRNA of LRRK2 gene includes AUUAACAUGAAAAUAUCACUU, UUAACAAUAUCAUAUAAUCUU, AUCUUUAAAAUUUGUUAACGC, UUGAUUUAAGAAAAUAGUCUC, UUUGAUAACAGUAUUUUUCUG, other sequences that inhibit the expression of LRRK2 gene and sequences with more than 80% homology to the above sequences.
- the RNA fragment includes an RNA sequence ontology and a modified RNA sequence obtained by modifying the RNA sequence ontology with ribose sugar. That is, the RNA fragment can be composed of only at least one RNA sequence ontology, or only at least one modified RNA sequence, and can also be composed of RNA sequence ontology and modified RNA sequence.
- the isolated nucleic acid also includes its variants and derivatives.
- the nucleic acid can be modified by one of ordinary skill in the art using general methods. Modification methods include (but are not limited to): methylation modification, hydrocarbyl modification, glycosylation modification (such as 2-methoxy-glycosyl modification, hydrocarbyl-glycosyl modification, sugar ring modification, etc.), nucleic acid modification, peptide modification Segment modification, lipid modification, halogen modification, nucleic acid modification (such as "TT" modification) and the like.
- the modification is an internucleotide linkage, for example selected from: phosphorothioate, 2'-O methoxyethyl (MOE), 2'-fluoro, phosphine Acid alkyl esters, phosphorodithioates, alkyl phosphorothioates, phosphoramidates, carbamates, carbonates, phosphoric triesters, acetamidates, carboxymethyl esters, and combinations thereof.
- phosphorothioate 2'-O methoxyethyl (MOE), 2'-fluoro
- phosphine Acid alkyl esters phosphorodithioates, alkyl phosphorothioates, phosphoramidates, carbamates, carbonates, phosphoric triesters, acetamidates, carboxymethyl esters, and combinations thereof.
- the modification is a modification of nucleotides, such as selected from: peptide nucleic acid (PNA), locked nucleic acid (LNA), arabinose-nucleic acid (FANA), analogs, derivatives objects and their combinations.
- the modification is a 2' fluoropyrimidine modification.
- 2'Fluoropyrimidine modification is to replace the 2'-OH of pyrimidine nucleotides on RNA with 2'-F.
- 2'-F can make RNA not easily recognized by RNase in vivo, thereby increasing the stability of RNA fragment transmission in vivo. sex.
- the delivery system is a delivery system for use in mammals including humans.
- Another inventive point of the present application is to provide an application of the above-mentioned RNA delivery system for treating Parkinson's in medicine.
- the drug is a drug for the treatment of Parkinson's and its related diseases, and the related diseases here refer to the associated diseases or complications, sequelae, etc. that occur in the formation or development of Parkinson's, or other diseases that are related to Parkinson's. disease.
- the drug includes the above-mentioned viral vector, specifically, the viral vector here refers to a viral vector carrying RNA fragments, or carrying RNA fragments and targeting tags, and can enter the host body, can be enriched in the liver, and self-assemble. A composite structure exosome is formed, which can deliver RNA fragments to the target tissue, so that the RNA fragments are expressed in the target tissue, thereby inhibiting the expression of matching genes, and achieving the purpose of treating diseases.
- the viral vector here refers to a viral vector carrying RNA fragments, or carrying RNA fragments and targeting tags, and can enter the host body, can be enriched in the liver, and self-assemble.
- a composite structure exosome is formed, which can deliver RNA fragments to the target tissue, so that the RNA fragments are expressed in the target tissue, thereby inhibiting the expression of matching genes, and achieving the purpose of treating diseases.
- the dosage forms of the drug can be tablets, capsules, powders, granules, pills, suppositories, ointments, solutions, suspensions, lotions, gels, pastes and the like.
- administration modes of the drug include oral, inhalation, subcutaneous injection, intramuscular injection, and intravenous injection. Intravenous injection is preferred.
- the RNA delivery system for the treatment of Parkinson's uses a virus as a vector, and the virus vector is used as a mature injection, and its safety and reliability have been fully verified, and the drugability is very good.
- the final effective RNA sequence is packaged and delivered by endogenous exosomes, and there is no immune response, so there is no need to verify the safety of the exosomes.
- the delivery system can deliver all kinds of small molecule RNAs, and has strong versatility. And the preparation of viral vectors is much cheaper and more economical than the preparation of exosomes or proteins, polypeptides and other substances.
- RNA delivery system for the treatment of Parkinson's provided in this application can be tightly combined with AGO 2 and enriched into a composite structure (exosome) after self-assembly in vivo, which can not only prevent its premature degradation, but also maintain its circulation in the circulation. It is stable, and facilitates uptake by recipient cells, intracytoplasmic release and lysosomal escape, and requires a low dose.
- RNA delivery system for the treatment of Parkinson's disease provided in this application is applied to medicine, that is, it provides a drug delivery platform, which can greatly improve the therapeutic effect of Parkinson's disease, and can also form a research and development basis for more RNA drugs through this platform. , which greatly promotes the development and use of RNA drugs.
- Fig. 1 is a comparison diagram of the Parkinson's treatment situation of transgenic mice provided by an embodiment of the present application
- FIG. 2 is a comparison diagram of the activation of mouse microglia and the secretion of inflammatory factors according to an embodiment of the present application
- FIG. 3 is a comparison diagram of the number of mouse microglia provided in an example of the present application.
- FIG. 4 is an effect diagram of in vivo enrichment of the siRNA-loaded lentiviral vector provided in an embodiment of the present application.
- FIG. 5 is an effect diagram of in vivo self-assembly of the siRNA-loaded lentiviral vector provided in an embodiment of the present application.
- Fig. 6 is the data result graph that the lentiviral vector loaded with siRNA provided by an embodiment of the present application has the therapeutic effect of Parkinson's disease.
- FIG. 7 is a graph showing the effect of in vivo enrichment of adeno-associated virus type 1, type 4, and type 7 vectors loaded with siRNA provided in an example of the present application.
- FIG. 8 is a diagram showing the effect of in vivo self-assembly of the siRNA-loaded adeno-associated virus type 1, type 4, and type 7 vectors provided in an embodiment of the present application.
- Fig. 9 is a graph showing the data of the Parkinson's treatment effect of adeno-associated virus type 1, 4, and 7 vectors loaded with siRNA provided in an example of the present application.
- Figure 10 is an effect diagram of in vivo enrichment of adenovirus-associated virus type 8 vectors loaded with 6 individual RNA sequences provided by an embodiment of the present application.
- FIG. 11 is an effect diagram of in vivo self-assembly of adeno-associated virus type 8 and type 9 vectors loaded with 6 individual RNA sequences provided in an example of the present application.
- FIG. 12 is a diagram showing the effect of in vivo enrichment of an adeno-associated virus type 9 vector loaded with RNA fragments of any two RNA sequences provided in an example of the present application.
- FIG. 13 is a diagram showing the effect of in vivo self-assembly of adeno-associated virus type 8 and type 9 vectors loaded with RNA fragments of any two RNA sequences provided in an example of the present application.
- FIG. 14 is an electrophoresis result of the Parkinson's treatment effect of an adenovirus vector loaded with RNA fragments of any three RNA sequences provided in an example of the present application.
- FIG. 15 is a graph showing the in vivo enrichment data of the adeno-associated virus type 9 sequences provided in an example of the present application when siRNA and RVG are included.
- Figure 16 is a graph showing the effect of Parkinson's treatment according to the expression data of LRRK2 mRNA when the sequence in the adenovirus-associated virus type 9 provided in an example of the present application includes siRNA and RVG.
- FIG. 17 is a data diagram of in vivo enrichment of adenovirus vectors loaded with RVG-LAMP2B fusion proteins and other fusion proteins provided in an example of the present application.
- Figure 18 is a data comparison diagram of the therapeutic effect of RVG-LAMP2B fusion protein and other fusion proteins on adenovirus vectors for Parkinson's disease provided in an example of the present application, and the data is reflected by the relative level of LRRK2 mRNA.
- Figure 19 is a graph of in vivo enrichment data of the adenoviral vector system provided in an example of the present application when three RNA sequences with more than 80% homology to the siRNA sequence of the LRRK2 gene are included.
- Figure 20 is a data comparison diagram of the therapeutic effect on Parkinson's disease when the adenovirus vector system provided by an embodiment of the present application includes 3 RNA sequences with a homology of more than 80% to the siRNA sequence of the LRRK2 gene. to reflect the relative level.
- Western Blot (Western Blot) is to transfer the protein to the membrane, and then use the antibody for detection.
- the corresponding antibody can be used as the primary antibody for detection, and the expression product of the new gene can be detected by the fusion part of the antibody. .
- Western Blot uses polyacrylamide gel electrophoresis, the detected object is protein, the "probe” is an antibody, and the "color development” is a labeled secondary antibody.
- the protein sample separated by PAGE is transferred to a solid phase carrier (such as nitrocellulose membrane), and the solid phase carrier adsorbs proteins in the form of non-covalent bonds, and can keep the types of polypeptides separated by electrophoresis and their biological activities unchanged.
- the protein or polypeptide on the solid phase carrier is used as an antigen, which reacts with the corresponding antibody, and then reacts with the enzyme or isotope-labeled secondary antibody to detect the specific target gene separated by electrophoresis through substrate color development or autoradiography.
- expressed protein components The steps mainly include: protein extraction, protein quantification, gel preparation and electrophoresis, membrane transfer, immunolabeling and development.
- Immunohistochemistry using antigen-antibody reaction, that is, the principle of specific binding of antigen and antibody, determines the antigen (polypeptide) in tissue cells by developing the color of the chromogenic reagent (fluorescein, enzyme, metal ion, isotope) labeled antibody through chemical reaction. and protein), the localization, qualitative and relative quantitative research, called immunohistochemistry (immunohistochemistry) or immunocytochemistry (immunocytochemistry).
- chromogenic reagent fluorescein, enzyme, metal ion, isotope
- the main steps of immunohistochemistry include: section soaking, overnight drying, xylene dewaxing, gradient alcohol dewaxing (100%, 95%, 90%, 80%, 75%, 70%, 50%, 3min each time) , double-distilled water, dropwise addition of 3% hydrogen peroxide solution to remove catalase, water washing, antigen retrieval, dropwise addition of 5% BSA, blocking for 1 h, dilution of primary antibody, washing with PBS buffer, incubation with secondary antibody, washing with PBS buffer , color developing solution, washing with water, hematoxylin staining, dehydration with gradient ethanol, and sealing with neutral gum.
- the detection of the siRNA level, the protein content and the mRNA content involved in the present invention is to establish the mouse stem cell in vitro model by injecting the RNA delivery system into the mouse.
- the expression levels of mRNA and siRNA in cells and tissues were detected by qRT-PCR. Absolute quantification of siRNA was determined by plotting a standard curve using the standards.
- the internal reference gene is U6snRNA (in tissue) or miR-16 (in serum, exosomes)
- the gene is GAPDH or 18s RNA.
- Western blotting was used to detect protein expression levels in cells and tissues, and ImageJ software was used for protein quantitative analysis.
- This embodiment provides an RNA delivery system for treating Parkinson's, the system comprising a viral vector carrying RNA fragments capable of treating Parkinson's, the viral vector can be enriched in the organ tissue of a host, And endogenously and spontaneously form a composite structure containing the RNA fragment capable of treating Parkinson's disease in the host organ tissue, and the composite structure can send the RNA fragment into the target tissue to achieve Parkinson's treatment.
- lentivirus In addition to adenovirus, other viral vectors also have in vivo enrichment, self-assembly and Parkinson's treatment effects, such as lentivirus.
- CTX stands for cortex
- STR stands for Striatum (Striatum).
- the viral vector is preferably adeno-associated virus, more preferably adeno-associated virus type 5, adenovirus-associated virus type 8 or adenovirus-associated virus type 9.
- adeno-associated virus types 5, 8 and 9 include other viral vectors also have in vivo enrichment, self-assembly and Parkinson's treatment effects, such as adenovirus types 1, 4 and 7, the data of which are shown in Figure 7- 9 shown.
- the viral vector also includes a promoter and a targeting tag.
- the viral vector includes any one of the following circuits or a combination of several circuits: promoter-RNA sequence, promoter-targeting tag, promoter-RNA sequence-targeting tag, and each of the viral vectors includes at least one RNA fragments and a targeting tag, either in the same circuit or in different circuits.
- the viral vector may only include a promoter-RNA sequence-targeting tag, or may include a combination of a promoter-RNA sequence, a promoter-targeting tag, or a promoter-targeting tag, a promoter A combination of RNA-seq-targeting tags.
- the viral vector may also include a flanking sequence, a compensation sequence and a loop sequence that can make the circuit fold into a correct structure and express, and the flanking sequence includes a 5' flanking sequence and a 3' flanking sequence; the viral vector Including any one of the following lines or a combination of several lines: 5'-promoter-5' flanking sequence-RNA fragment-loop sequence-compensating sequence-3' flanking sequence, 5'-promoter-targeting tag, 5' - Promoter - Targeting Tag - 5' Flanking Sequence - RNA Fragment - Loop Sequence - Compensation Sequence - 3' Flanking Sequence.
- the viral vector contains 5'-promoter-targeting tag-5'flanking sequence-RNA fragment-loop sequence-compensating sequence-3'flanking sequence
- its RNA delivery system has in vivo enrichment and Parkinson's treatment
- the effect is shown in Figure 15-16, the targeting tag is RVG, and the RNA fragment is siRNA with therapeutic effect.
- the 5' flanking sequence is preferably ggatcctggaggcttgctgaaggctgtatgctgaattc or a sequence with a homology greater than 80%, including a sequence with 85%, 90%, 92%, 95%, 98%, 99% homology with ggatcctggaggcttgctgaaggctgtatgctgaattc, etc.
- the loop sequence is preferably gttttggccactgactgac or a sequence with more than 80% homology thereto, including sequences with 85%, 90%, 92%, 95%, 98%, 99% homology with gttttggccactgactgac, and the like.
- the 3' flanking sequence is preferably accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag or a sequence with a homology greater than 80%, including a sequence with 85%, 90%, 92%, 95%, 98%, 99% homology with accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag, etc.
- the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-5 bases are deleted.
- the compensation sequence can be the reverse complementary sequence of the RNA sequence by deleting any 1-5 bases therein.
- the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 bases are deleted.
- the compensation sequence can be the reverse complementary sequence of the RNA sequence by deleting any 1-3 bases therein.
- the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 consecutive bases are deleted.
- the compensation sequence may be the reverse complementary sequence of the RNA sequence by deleting any 1-3 consecutively arranged bases.
- the compensation sequence is the reverse complement of the RNA fragment, and the 9th and/or 10th bases are deleted.
- the compensation sequence may be the reverse complementary sequence of the 9th position and/or the 10th position in the deletion of the RNA sequence. Deleting bases 9 and 10 works best.
- flanking sequences are not randomly selected, but are determined based on a large number of theoretical studies and experiments. increase the expression rate of RNA fragments.
- sequence 1 is preferably CAGATC
- sequence 2 can be composed of 5-80 bases
- Sequence of bases such as 10, 15, 20, 25, 30, 35, 40, 45, 50, 55, 60, 65, 70, 75 bases
- sequence of 10-50 bases is preferable, and the sequence of 20-40 bases is more preferable.
- Sequence 3 is preferably TGGATC.
- Sequence 2 is specifically shown in Table 1 below.
- sequence 4 is CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC.
- sequence 4 CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC Sequence 4-1 CAGATCTGGCCGCACTCGTAGAGGTGAGTCGACCAGTGGATC Sequence 4-2 CAGATCTGGCACCCGTCGAGGTAGTGAGTCGACCAGTGGATC Sequence 4-3 CAGATCTGGCCGCACAGGTCGTAGTGAGTCGACCAGTGGATC
- RNA fragments comprise one, two or more specific RNA sequences of medical significance, the RNA sequences can be expressed in the target receptor, and the compensatory sequence cannot be expressed in the target receptor.
- the RNA sequence can be an siRNA sequence, a shRNA sequence or a miRNA sequence, preferably an siRNA sequence.
- the RNA capable of treating Parkinson's disease is selected from: siRNA of LRRK2 gene or nucleic acid molecule encoding the above RNA.
- LRRK2 siRNA sequences were selected, namely UUGGUCAUCUGGAUACAUC, CAUGAUGCUGUUAUUCU, GAUUGGAAAUAAAGGACCA, and the first siRNA was used as an example to verify the effect of the sequences with homology of 80%, 90% and 98%.
- the delivery system of the source sequence, its in vivo enrichment and Parkinson's treatment effect are shown in Figures 19-20.
- the number of required delivery RNA effective sequences is one, two or more.
- the functional structural region of the viral vector can be expressed as: (promoter-siRNA1)-connector sequence-(promoter-siRNA2)-connector sequence- (promoter-targeting tag), or (promoter-targeting tag-siRNA1)-linker-(promoter-targeting tag-siRNA2), or (promoter-siRNA1)-linker-(promoter- Targeting tag-siRNA2) etc.
- the functional structural region of the viral vector can be expressed as: (5'-promoter-5'flanking sequence-siRNA1-loop sequence-compensating sequence-3'flanking sequence)-connector sequence-(5'-promoter - 5' flanking sequence - siRNA2-loop sequence - compensation sequence - 3' flanking sequence) - linking sequence - (5'-promoter-targeting tag), or (5'-promoter-targeting tag-5' flanking sequence-siRNA1-loop sequence-compensation sequence-3' flanking sequence)-linker sequence-(5'-promoter-targeting tag-5'flanking sequence-siRNA2-loop sequence-compensating sequence-3'flanking sequence), or (5'-promoter-5'flanking sequence-siRNA1-loop sequence-compensating sequence-3'flanking sequence)-linking sequence-(5'-promoter-targeting tag-5'flanking sequence-siRNA2-loop sequence-compensating sequence-3'flanking
- the above RNA can also be obtained by ribose modification of the RNA sequence (siRNA, shRNA or miRNA) therein, preferably 2' fluoropyrimidine modification.
- 2'Fluoropyrimidine modification is to replace the 2'-OH of pyrimidine nucleotides on siRNA, shRNA or miRNA with 2'-F.
- 2'-F can make it difficult for RNase in the human body to recognize siRNA, shRNA or miRNA, so it can Increases the stability of RNA transport in vivo.
- the liver will phagocytose exogenous viruses, and up to 99% of the exogenous viruses will enter the liver. Therefore, when viruses are used as vectors, they can be enriched in liver tissue without specific design. After being opened, RNA molecules (siRNA, shRNA, or miRNA) are released, and liver tissue spontaneously wraps the above RNA molecules into exosomes, and these exosomes become RNA delivery mechanisms.
- RNA molecules siRNA, shRNA, or miRNA
- RNA delivery mechanism in order to make the RNA delivery mechanism (exosome) have the ability of "precision guidance”, we design a targeting tag in the viral vector injected into the body, and the targeting tag will also be assembled into exosomes by liver tissue
- the targeting tags can be inserted into the surface of exosomes to become targeting structures that can guide exosomes, which greatly improves the RNA delivery of the present invention.
- the accuracy of the mechanism on the one hand, can greatly reduce the amount of viral vector that needs to be introduced, and on the other hand, greatly improves the efficiency of potential drug delivery.
- the targeting tag is selected from one of the peptides, proteins or antibodies with targeting function.
- the selection of the targeting tag is a process that requires creative work. On the one hand, it is necessary to select the available targeting tags according to the target tissue. It is ensured that the targeting label can stably appear on the surface of exosomes, so as to achieve the targeting function.
- Targeting tags that have been screened include: targeting peptides, targeting proteins, and antibodies.
- targeting peptides include but are not limited to RVG targeting peptide (nucleotide sequence shown in SEQ ID No: 1), GE11 targeting peptide (nucleotide sequence shown in SEQ ID No: 2), PTP targeting peptide Peptide (nucleotide sequence shown in SEQ ID No: 3), TCP-1 targeting peptide (nucleotide sequence shown in SEQ ID No: 4), MSP targeting peptide (nucleotide sequence shown in SEQ ID No: 4) : 5); targeting proteins include but are not limited to RVG-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 6), GE11-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 7) shown), PTP-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 8), TCP-1-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No:
- Figures 17-18 show the in vivo enrichment and Parkinson's treatment effect of RVG-LAMP2B fusion protein on adenovirus vector, and its therapeutic effect is reflected by the level of LRRK2 mRNA.
- the viral vector can also be composed of multiple viruses with different structures, one of which contains a promoter promoters and targeting tags, other viruses contain promoters and RNA segments. Loading the targeting tag and RNA fragment into different viral vectors, and injecting the two viral vectors into the body, the targeting effect is no worse than the targeting effect produced by loading the same targeting tag and RNA fragment into one viral vector .
- the viral vector containing the RNA sequence can be injected first, and then the viral vector containing the targeting tag can be injected after 1-2 hours, so that a better target can be achieved. to the effect.
- the delivery systems described above can all be used in mammals, including humans.
- the RNA delivery system for the treatment of Parkinson's uses a virus as a vector, and the virus vector is used as a mature injection. Its safety and reliability have been fully verified, and its druggability is very good. The final effective RNA sequence is packaged and delivered by endogenous exosomes, and there is no immune response, so there is no need to verify the safety of the exosomes.
- the delivery system can deliver all kinds of small molecule RNAs, and has strong versatility. And the preparation of viral vectors is much cheaper and more economical than the preparation of exosomes or proteins, polypeptides and other substances.
- RNA delivery system for the treatment of Parkinson's disease provided in this example can be tightly combined with AGO 2 and enriched into a complex structure (exosome) after self-assembly in vivo, which can not only prevent its premature degradation, but also maintain its circulation in the circulation. It is stable, and is beneficial to receptor cell uptake, intracytoplasmic release and lysosomal escape, and the required dose is low.
- the medicament includes a viral vector carrying an RNA segment capable of treating Parkinson's, the viral vector being capable of enriching in the organ tissue of a host, and endogenously and spontaneously forming in the organ tissue of the host an RNA segment capable of treating Parkinson's disease
- the composite structure of the RNA fragment for treating Parkinson's disease, the composite structure can deliver the RNA fragment into the target tissue to realize the treatment of Parkinson's disease.
- the RNA fragment comprises one, two or more specific RNA sequences with medical significance, and the RNA sequences are siRNA, shRNA or miRNA with medical significance.
- Adenovirus-associated virus types 8 and 9 are used as viral vectors, which have in vivo enrichment, self-assembly and Parkinson's treatment effects when carrying one or more RNA fragments.
- Figure 10-11 shows that the vectors carry
- Figures 12-13 show data presented for RNA fragments with 6 individual RNA sequences;
- Figures 12-13 show data presented for vectors carrying 4 sets of RNA fragments containing any two RNA sequences;
- Figure 14 shows vectors carrying 3 Groups contain therapeutic data results presented by RNA fragments of any of the 3 RNA sequences.
- the viral vector includes a promoter and a targeting tag
- the targeting tag can form the targeting structure of the composite structure in the organ tissue of the host
- the targeting structure is located on the surface of the composite structure, so The complex structure can seek and bind to the target tissue through the targeting structure, and deliver the RNA fragment into the target tissue.
- the drug can be administered orally, inhaled, subcutaneously injected, intramuscularly injected or intravenously injected into the human body, it can be delivered to the target tissue through the RNA delivery system described in Example 1 to exert a therapeutic effect.
- the drug can be used in combination with other Parkinson's disease drugs to improve the treatment effect, such as anticholinergics (Antan, etc.), antihistamines (diphenhydramine, amantadine, etc.), levodopa Drugs (Dopa, Sining, Xilaimei, etc.), dopamine receptor agonists (Texida, Xie Liangxing, Crepa, bromocriptine, etc.), monoamine oxidase B inhibitors (Sgining, Jin Siping, etc.) ), catecholamine oxygen methyltransferase inhibitors (Entocapone, etc.).
- Parkinson's disease drugs such as anticholinergics (Antan, etc.), antihistamines (diphenhydramine, amantadine, etc.), levodopa Drugs (Dopa, Sining, Xilaimei, etc.), dopamine receptor agonists (Texida, Xie Liangxing, Cre
- the medicine of this embodiment may also include a pharmaceutically acceptable carrier, which includes but is not limited to diluents, buffers, emulsions, encapsulation agents, excipients, fillers, adhesives, sprays, transdermal absorption Agents, wetting agents, disintegrating agents, absorption enhancers, surfactants, colorants, flavoring agents, adjuvants, desiccants, adsorption carriers, etc.
- a pharmaceutically acceptable carrier includes but is not limited to diluents, buffers, emulsions, encapsulation agents, excipients, fillers, adhesives, sprays, transdermal absorption Agents, wetting agents, disintegrating agents, absorption enhancers, surfactants, colorants, flavoring agents, adjuvants, desiccants, adsorption carriers, etc.
- the dosage forms of the medicine provided in this embodiment can be tablets, capsules, powders, granules, pills, suppositories, ointments, solutions, suspensions, lotions, gels, pastes, and the like.
- the medicine provided in this example uses a virus as a carrier, and the virus carrier is used as a mature injection. Its safety and reliability have been fully verified, and the druggability is very good.
- the final effective RNA sequence is packaged and delivered by endogenous exosomes, and there is no immune response, so there is no need to verify the safety of the exosomes.
- the drug can deliver various kinds of small molecule RNAs and has strong versatility. And the preparation of viral vectors is much cheaper and more economical than the preparation of exosomes or proteins, polypeptides and other substances.
- the drug provided by this application can be closely combined with AGO 2 and enriched into a composite structure (exosome) after self-assembly in vivo, which can not only prevent its premature degradation and maintain its stability in circulation, but also benefit the receptor.
- Cellular uptake, intracytoplasmic release and lysosomal escape require low doses.
- this embodiment provides an application of an RNA delivery system for treating Parkinson's disease in a drug, and the drug is a drug for treating Parkinson's disease.
- the application of the RNA delivery system in the treatment of Parkinson's disease is specifically described in conjunction with the following experiments.
- LRRK2R1441G transgenic mice were selected for the experiment when they were 3 months old, and the experiment set up LPS intervention group and LPS non-intervention group.
- the LPS intervention group was treated with AAV-CMV-scrR/AAV-CMV-RVG-siR LRRK2 after 7 days of LPS intervention (AAV-CMV-scrR, AAV-CMV-RVG-siR LRRK2 are abbreviated as CMV-scrR, CMV- RVG-siR LRRK2 ).
- the quantitative display of LRRK2 protein levels shows that the LRRK2 protein levels in mice treated with AAV-CMV-scrR after LPS intervention were significantly higher than those in other groups, while the LRRK2 in mice treated with AAV-CMV-RVG-siR LRRK2 Protein levels were significantly lower.
- anti-iba-1 antibody immunostaining shows activation of microglia in the striatum and substantia nigra pars compacta of R1441G mice, scale bar: 50 ⁇ m.
- Figure 3 after quantifying the number of microglia in the striatum and SNpc in Figure 2, it can be seen that the number of microglia in the striatum and SNpc of mice treated with AAV-CMV-scrR after LPS intervention was significantly higher Compared with the other groups, the number of microglia in the striatum and SNpc of mice treated with AAV-CMV-RVG-siR LRRK2 was significantly lower.
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Abstract
The present application provides an RNA delivery system for treating Parkinson's disease. The system comprises a viral vector. The viral vector carries an RNA fragment capable of treating Parkinson's disease. The viral vector can be enriched in an organ tissue of a host, and endogenously and spontaneously form, in the organ tissue of the host, a composite structure containing the RNA fragment capable of treating Parkinson's disease. The composite structure can deliver the RNA fragment to a target tissue to achieve the treatment of Parkinson's disease. The safety and reliability of the RNA delivery system for treating Parkinson's disease provided by the present application has been fully verified, and the RNA delivery system has remarkable druggability and high universality, and thus has excellent economic benefits and application prospects.
Description
本申请涉及生物医学技术领域,特别涉及一种用于治疗帕金森的RNA递送系统。The present application relates to the field of biomedical technology, in particular to an RNA delivery system for treating Parkinson's disease.
帕金森病(PD)又名震颤麻痹,是一种常见的中老年人神经系统变性疾病,主要病变在黑质和纹状体,震颤、肌强直及运动减少是本病的主要临床特征。帕金森病是老年人中第四位最常见的神经变性疾病。Parkinson's disease (PD), also known as tremor palsy, is a common neurodegenerative disease of the middle-aged and elderly people. The main lesions are in the substantia nigra and striatum. Parkinson's disease is the fourth most common neurodegenerative disease in older adults.
RNA干扰(RNAi)疗法自从被发明以来,一直被认为是治疗人类疾病的一种很有前途的策略,但在临床实践过程中遇到了许多问题,该疗法的发展进度远远落后于预期。RNA interference (RNAi) therapy has been considered a promising strategy for the treatment of human diseases since its invention, but many problems have been encountered during clinical practice, and the development of this therapy has lagged far behind expectations.
一般认为RNA无法在细胞外长期稳定存在,因为RNA会被细胞外富含的RNase降解成碎片,因此必须找到能够使RNA稳定存在于细胞外,并且能够靶向性地进入特定组织的方法,才能将RNAi疗法的效果凸显出来。It is generally believed that RNA cannot exist stably outside the cell for a long time, because RNA will be degraded into fragments by RNases rich in extracellular, so it is necessary to find a method that can make RNA stable outside the cell and can enter specific tissues in a targeted manner. Highlight the effect of RNAi therapy.
目前与siRNA相关的专利很多,主要聚焦在以下几个方面:1、设计具有医学效果的siRNA。2、对siRNA进行化学修饰,提高siRNA在生物体内的稳定性,提高产率。3、提高设计各种人工载体(如脂质纳米粒子、阳离子聚合物和病毒),以提高siRNA在体内传递的效率。其中第3方面的专利很多,其根本原因是研究人员们已经意识到目前缺乏合适的siRNA传递系统,将siRNA安全地、精确地、高效地输送到目标组织,该问题已经成为制约RNAi疗法的核心问题。At present, there are many patents related to siRNA, mainly focusing on the following aspects: 1. Designing siRNA with medical effects. 2. Chemical modification of siRNA to improve the stability of siRNA in vivo and increase the yield. 3. Improve the design of various artificial carriers (such as lipid nanoparticles, cationic polymers and viruses) to improve the efficiency of siRNA delivery in vivo. Among them, there are many patents in the third aspect. The fundamental reason is that researchers have realized that there is currently a lack of suitable siRNA delivery systems to safely, precisely and efficiently deliver siRNA to target tissues. This problem has become the core restricting RNAi therapy. question.
病毒(Biological virus)是一种个体微小,结构简单,只含一种核酸(DNA或RNA),必须在活细胞内寄生并以复制方式增殖的非细胞型生物。病毒载体可将遗传物质带入细胞,原理是利用病毒具有传送其基因组进入其他细胞,进行感染的分子机制,可发生于完整活体(in vivo)或是细胞培养(in vitro)中,主要应用于基础研究、基因疗法或疫苗。但是目前很少有针对将病毒作为载体利用特殊的自组装机制递送RNA,特别是siRNA的相关研究。Virus (Biological virus) is a small individual, simple structure, containing only one nucleic acid (DNA or RNA), must be parasitic in living cells and replicated non-cellular organisms. Viral vectors can bring genetic material into cells. The principle is to use the molecular mechanism of viruses to transmit their genomes into other cells for infection. It can occur in a complete living body (in vivo) or cell culture (in vitro), mainly used in Basic research, gene therapy or vaccines. However, there are few related studies on the use of viruses as vectors to deliver RNA, especially siRNA, using a special self-assembly mechanism.
公开号为CN108624590A的中国专利公开了一种能够抑制DDR2基因表达的siRNA;公开号为CN108624591A的中国专利公开了一种能够沉默ARPC4基因的siRNA,并且对该siRNA进行了α-磷-硒修饰;公开号为CN108546702A的中国专利公开了一种靶向长链非编码RNA DDX11-AS1的siRNA。公开号为CN106177990A的中国专利公开了一种可以用于多种肿瘤治疗的siRNA前体。这些专利均设计了特定的siRNA并且来针对某些由基因变化引起的疾病。The Chinese Patent Publication No. CN108624590A discloses a siRNA capable of inhibiting the expression of DDR2 gene; the Chinese Patent Publication No. CN108624591A discloses a siRNA capable of silencing the ARPC4 gene, and the siRNA is modified with α-phosphorus-selenium; The Chinese Patent Publication No. CN108546702A discloses a siRNA targeting long-chain non-coding RNA DDX11-AS1. The Chinese Patent Publication No. CN106177990A discloses a siRNA precursor that can be used for various tumor treatments. These patents design specific siRNAs to target certain diseases caused by genetic changes.
公开号为CN108250267A的中国专利公开了一种多肽、多肽-siRNA诱导共组装体,使用多肽作为siRNA的载体。公开号为CN108117585A的中国专利公开了一种靶向导入siRNA促进乳腺癌细胞凋亡的多肽,同样使用多肽作为siRNA的载体。公开号为CN108096583A的中国专利公开了一种纳米粒子载体,该载体在包含化疗药物的同时还可以装载具有乳腺癌疗效的siRNA。这些专利均为在siRNA载体方面的发明创造,但是其技术方案具有一个共同特征,那就是载体和siRNA均在体外预先组装,然后再引入宿主体内。事实上,目前绝大部分设计的传递技术均是如此。然而这类传递体系具有共同的问题,那就是这些人工合成的外源性传递体系很容易被宿主的循环系统清除,也有可能引起免疫原性反应,甚至可能对特定的细胞类型和组织有毒。Chinese Patent Publication No. CN108250267A discloses a polypeptide, polypeptide-siRNA induced co-assembly, using polypeptide as a carrier of siRNA. The Chinese Patent Publication No. CN108117585A discloses a polypeptide for promoting apoptosis of breast cancer cells through targeted introduction of siRNA, and the polypeptide is also used as the carrier of siRNA. The Chinese Patent Publication No. CN108096583A discloses a nanoparticle carrier, which can be loaded with siRNA with breast cancer curative effect while containing chemotherapeutic drugs. These patents are all inventions and creations in terms of siRNA vectors, but their technical solutions have a common feature, that is, the vectors and siRNA are pre-assembled in vitro and then introduced into the host. In fact, this is the case with most of the delivery technologies currently designed. However, this type of delivery system has a common problem, that is, these synthetic exogenous delivery systems are easily cleared by the host's circulatory system, may also cause immunogenic responses, and may even be toxic to specific cell types and tissues.
本发明的研究团队发现内源性细胞可以选择性地将miRNAs封装到外泌体(exosome)中,外泌体可以将miRNA传递到受体细胞中,其分泌的miRNA在相对较低的浓度下,即可有力阻断靶基因的表达。外泌体与宿主免疫系统生物相容,并具有在体内保护和运输miRNA跨越生物屏障的先天能力,因此成为克服与siRNA传递相关的问题的潜在解决方案。例如,公开号为CN110699382A的中国专利就公开了一种 递送siRNA的外泌体的制备方法,公开了从血浆中分离外泌体,并将siRNA通过电穿孔的方式封装到外泌体中的技术。The research team of the present invention found that endogenous cells can selectively encapsulate miRNAs into exosomes, and exosomes can deliver miRNAs to recipient cells, which secrete miRNAs at relatively low concentrations , which can effectively block the expression of target genes. Exosomes are biocompatible with the host immune system and possess the innate ability to protect and transport miRNAs across biological barriers in vivo, thus becoming a potential solution to overcome problems associated with siRNA delivery. For example, the Chinese Patent Publication No. CN110699382A discloses a method for preparing siRNA-delivering exosomes, and discloses the technology of separating exosomes from plasma and encapsulating siRNA into exosomes by electroporation .
但是这类在体外分离或制备外泌体的技术,往往需要通过细胞培养获取大量的外泌体,再加上siRNA封装的步骤,这使得大规模应用该产品的临床费用变得非常高,一般患者无法负担;更重要的是,外泌体复杂的生产/纯化过程,使其几乎不可能符合GMP标准。However, such techniques of in vitro isolation or preparation of exosomes often require obtaining a large amount of exosomes through cell culture, coupled with the step of siRNA encapsulation, which makes the clinical cost of large-scale application of this product very high. Patients cannot afford it; more importantly, the complex production/purification process of exosomes makes it almost impossible to comply with GMP standards.
到目前为止,以外泌体为有效成分的药物从未获得CFDA批准,其核心问题就是无法保证外泌体产品的一致性,而这一问题直接导致此类产品无法获得药品生产许可证。如果能解决这一问题,则对推动RNAi疗法治疗帕金森病意义非凡。So far, drugs with exosomes as active ingredients have never been approved by the CFDA. The core problem is that the consistency of exosome products cannot be guaranteed, and this problem directly leads to the inability of such products to obtain drug production licenses. If this problem can be solved, it will be of great significance to promote RNAi therapy for Parkinson's disease.
因此,开发一个安全、精确和高效的siRNA传递系统是对提高RNAi治疗效果,推进RNAi疗法至关重要的一环。Therefore, the development of a safe, precise and efficient siRNA delivery system is a crucial part of improving the effect of RNAi therapy and advancing RNAi therapy.
发明内容SUMMARY OF THE INVENTION
有鉴于此,本申请实施例提供了一种用于治疗帕金森的RNA递送系统及其应用,以解决现有技术中存在的技术缺陷。In view of this, the embodiments of the present application provide an RNA delivery system for treating Parkinson's and its application, so as to solve the technical defects existing in the prior art.
本申请的一个发明点为提供一种用于治疗帕金森的RNA递送系统,该系统包括病毒载体,所述病毒载体携带有能够治疗帕金森的RNA片段,所述病毒载体能够在宿主的器官组织中富集,并在所述宿主器官组织中内源性地自发形成含有能够治疗帕金森的所述RNA片段的复合结构,所述复合结构能够将所述RNA片段送入目标组织,实现帕金森的治疗。RNA片段送入目标组织后,能够抑制与其相匹配的基因的表达,进而抑制目标组织中疾病的发展。目标组织为大脑。One of the inventions of the present application is to provide an RNA delivery system for treating Parkinson's disease. The system includes a viral vector carrying an RNA segment capable of treating Parkinson's disease. It is enriched in the host organ tissue and endogenously and spontaneously forms a composite structure containing the RNA fragment capable of treating Parkinson's disease, and the composite structure can deliver the RNA fragment into the target tissue to achieve Parkinson's disease. Treatment. After the RNA fragment is delivered to the target tissue, it can inhibit the expression of the matching gene, thereby inhibiting the development of disease in the target tissue. The target tissue is the brain.
进一步地,所述病毒载体为腺病毒相关病毒。Further, the viral vector is an adenovirus-associated virus.
进一步地,所述腺病毒相关病毒为腺病毒相关病毒5型、腺病毒相关病毒8型或腺病毒相关病毒9型。Further, the adenovirus-associated virus is adenovirus-associated virus type 5, adenovirus-associated virus type 8 or adenovirus-associated virus type 9.
进一步地,所述RNA片段包含1个、两个或多个具有医疗意义的具体RNA序列,所述RNA序列是具有医学意义的siRNA、shRNA或miRNA。Further, the RNA fragment comprises one, two or more specific RNA sequences with medical significance, and the RNA sequences are siRNA, shRNA or miRNA with medical significance.
进一步地,所述病毒载体包括启动子和靶向标签,所述靶向标签能够在宿主的器官组织中形成所述复合结构的靶向结构,所述靶向结构位于复合结构的表面,所述复合结构能够通过所述靶向结构寻找并结合目标组织,将所述RNA片段递送进入目标组织。Further, the viral vector comprises a promoter and a targeting tag, the targeting tag can form the targeting structure of the composite structure in the organ tissue of the host, the targeting structure is located on the surface of the composite structure, the The complex structure is capable of finding and binding to the target tissue through the targeting structure, delivering the RNA fragment into the target tissue.
进一步地,所述病毒载体中包括以下任意一种线路或几种线路的组合:启动子-RNA片段、启动子-靶向标签、启动子-RNA片段-靶向标签;每一个所述病毒载体中至少包括一个RNA片段和一个靶向标签,所述RNA片段和靶向标签位于相同的线路中或位于不同的线路中。Further, the viral vector includes any one of the following circuits or a combination of several circuits: promoter-RNA fragment, promoter-targeting tag, promoter-RNA fragment-targeting tag; each of the viral vectors including at least one RNA segment and one targeting tag, the RNA segment and targeting tag are located in the same circuit or are located in different circuits.
进一步地,所述病毒载体还包括能够使所述线路折叠成正确结构并表达的侧翼序列、补偿序列和loop序列,所述侧翼序列包括5’侧翼序列和3’侧翼序列;Further, the viral vector also includes a flanking sequence, a compensation sequence and a loop sequence that can make the circuit fold into a correct structure and express, and the flanking sequence includes a 5' flanking sequence and a 3' flanking sequence;
所述病毒载体中包括以下任意一种线路或几种线路的组合:5'-启动子-5'侧翼序列-RNA片段-loop序列-补偿序列-3'侧翼序列、5'-启动子-靶向标签、5'-启动子-靶向标签-5'侧翼序列-RNA片段-loop序列-补偿序列-3'侧翼序列。The viral vector includes any one of the following lines or a combination of several lines: 5'-promoter-5' flanking sequence-RNA fragment-loop sequence-compensating sequence-3' flanking sequence, 5'-promoter-target To tag, 5'-promoter-targeting tag-5'flanking sequence-RNA fragment-loop sequence-compensating sequence-3'flanking sequence.
进一步地,所述5’侧翼序列为ggatcctggaggcttgctgaaggctgtatgctgaattc或与其同源性大于80%的序列;Further, the 5' flanking sequence is ggatcctggaggcttgctgaaggctgtatgctgaattc or a sequence whose homology is greater than 80%;
所述loop序列为gttttggccactgactgac或与其同源性大于80%的序列;The loop sequence is gttttggccactgactgac or a sequence whose homology is greater than 80%;
所述3’侧翼序列为accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag或与其同 源性大于80%的序列;Described 3 ' flanking sequence is accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag or its homology is greater than 80% sequence;
所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-5位碱基。删除RNA反向互补序列的1-5位碱基的目的是使该序列不表达。The compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-5 bases are deleted. The purpose of deleting bases 1-5 of the reverse complement of the RNA is to make the sequence unexpressed.
与shRNA不同,在siRNA和miRNA前体中,由于删除作用链的反向互补链(例如siRNA的反向互补链)的第9,10位碱基,导致siRNA和miRNA的作用链会形成凸起结构,以上结构有利于更有效的沉默基因的表达。综上,通过删除第9,10位碱基的反向互补序列来提高沉默效率是目前已公认的结论。Unlike shRNA, in siRNA and miRNA precursors, due to deletion of the 9th and 10th bases of the reverse complementary strand of the active strand (such as the reverse complementary strand of siRNA), the active strand of siRNA and miRNA will form a bulge. structure, which facilitates more efficient silencing of gene expression. To sum up, it is an accepted conclusion that the silencing efficiency can be improved by deleting the reverse complementary sequence of the 9th and 10th bases.
优选地,所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-3位碱基。Preferably, the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 bases are deleted.
更为优选地,所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-3位连续排列的碱基。More preferably, the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 consecutive bases are deleted.
最为优选地,所述补偿序列为所述RNA片段的反向互补序列,并删除其中的第9位和/或第10位碱基。Most preferably, the compensation sequence is the reverse complement of the RNA fragment, and the 9th and/or 10th bases are deleted.
进一步地,在病毒载体中存在至少两种线路的情况下,相邻的线路之间通过序列1-3组成的序列(序列1-序列2-序列3)相连;Further, when there are at least two lines in the viral vector, adjacent lines are connected by a sequence composed of sequences 1-3 (sequence 1-sequence 2-sequence 3);
其中,序列1为CAGATC,序列2是由5-80个碱基组成的序列,序列3为TGGATC。Wherein, sequence 1 is CAGATC, sequence 2 is a sequence consisting of 5-80 bases, and sequence 3 is TGGATC.
进一步地,在病毒载体中存在至少两种线路的情况下,相邻的线路之间通过序列4或与序列4同源性大于80%的序列相连;Further, when there are at least two lines in the viral vector, adjacent lines are connected by sequence 4 or a sequence with more than 80% homology to sequence 4;
其中,序列4为CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC。Wherein, sequence 4 is CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC.
进一步地,所述器官组织为肝脏,所述复合结构为外泌体。Further, the organ tissue is liver, and the composite structure is exosome.
进一步地,所述靶向标签选自具有靶向功能的靶向肽或靶向蛋白。Further, the targeting tag is selected from targeting peptides or targeting proteins with targeting function.
进一步地,所述靶向肽包括RVG靶向肽、GE11靶向肽、PTP靶向肽、TCP-1靶向肽、MSP靶向肽;Further, the targeting peptides include RVG targeting peptides, GE11 targeting peptides, PTP targeting peptides, TCP-1 targeting peptides, and MSP targeting peptides;
所述靶向蛋白包括RVG-LAMP2B融合蛋白、GE11-LAMP2B融合蛋白、PTP-LAMP2B融合蛋白、TCP-1-LAMP2B融合蛋白、MSP-LAMP2B融合蛋白。The targeting proteins include RVG-LAMP2B fusion protein, GE11-LAMP2B fusion protein, PTP-LAMP2B fusion protein, TCP-1-LAMP2B fusion protein, and MSP-LAMP2B fusion protein.
靶向标签优选为能够精准靶向脑组织的RVG靶向肽或RVG-LAMP2B融合蛋白。The targeting tag is preferably an RVG targeting peptide or RVG-LAMP2B fusion protein that can precisely target brain tissue.
进一步地,所述RNA序列的长度为15-25个核苷酸。比如,所述RNA序列的长度可以为16、17、18、19、20、21、22、23、24、25个核苷酸。优选地,所述RNA序列的长度为18-22个核苷酸。Further, the length of the RNA sequence is 15-25 nucleotides. For example, the length of the RNA sequence can be 16, 17, 18, 19, 20, 21, 22, 23, 24, 25 nucleotides. Preferably, the RNA sequence is 18-22 nucleotides in length.
进一步地,所述能够治疗帕金森的RNA选自:LRRK2基因的siRNA,或与上述序列同源性大于80%的RNA序列,或编码上述RNA的核酸分子。需要说明的是,此处“编码上述RNA序列的核酸分子”中的RNA序列也同时包括每种RNA的同源性大于80%的RNA序列。Further, the RNA capable of treating Parkinson's is selected from: siRNA of the LRRK2 gene, or an RNA sequence with a homology of more than 80% to the above sequence, or a nucleic acid molecule encoding the above RNA. It should be noted that the RNA sequences in the "nucleic acid molecules encoding the above RNA sequences" here also include RNA sequences with a homology of more than 80% of each RNA.
LRRK2基因的siRNA包括AUUAACAUGAAAAUAUCACUU、UUAACAAUAUCAUAUAAUCUU、AUCUUUAAAAUUUGUUAACGC、UUGAUUUAAGAAAAUAGUCUC、UUUGAUAACAGUAUUUUUCUG、其他具有抑制LRRK2基因表达的序列以及与上述序列同源性大于80%的序列。The siRNA of LRRK2 gene includes AUUAACAUGAAAAUAUCACUU, UUAACAAUAUCAUAUAAUCUU, AUCUUUAAAAUUUGUUAACGC, UUGAUUUAAGAAAAUAGUCUC, UUUGAUAACAGUAUUUUUCUG, other sequences that inhibit the expression of LRRK2 gene and sequences with more than 80% homology to the above sequences.
需要说明的是,以上所述的“同源性大于80%的序列”可以为同源性为85%、88%、90%、95%、98%等。可选地,所述RNA片段包括RNA序列本体和对RNA序列本体进行核糖修饰得到的修饰RNA序列。即RNA片段既可以仅由至少一个RNA序列本体组成,也可以仅由至少一个修饰RNA序列组成,还可以由RNA序列本体与修饰RNA序列组成。It should be noted that the above-mentioned "sequences with more than 80% homology" may be 85%, 88%, 90%, 95%, 98%, etc. homology. Optionally, the RNA fragment includes an RNA sequence ontology and a modified RNA sequence obtained by modifying the RNA sequence ontology with ribose sugar. That is, the RNA fragment can be composed of only at least one RNA sequence ontology, or only at least one modified RNA sequence, and can also be composed of RNA sequence ontology and modified RNA sequence.
在本发明中,所述分离的核酸还包括其变体和衍生物。本领域的普通技术人员可以使用通用的方法对 所述核酸进行修饰。修饰方式包括(但不限于):甲基化修饰、烃基修饰、糖基化修饰(如2-甲氧基-糖基修饰、烃基-糖基修饰、糖环修饰等)、核酸化修饰、肽段修饰、脂类修饰、卤素修饰、核酸修饰(如“TT”修饰)等。在本发明的其中一种实施方式中,所述修饰为核苷酸间键合,例如选自:硫代磷酸酯、2'-O甲氧基乙基(MOE)、2'-氟、膦酸烷基酯、二硫代磷酸酯、烷基硫代膦酸酯、氨基磷酸酯、氨基甲酸酯、碳酸酯、磷酸三酯、乙酰胺酯、羧甲基酯及其组合。在本发明的其中一种实施方式中,所述修饰为对核苷酸的修饰,例如选自:肽核酸(PNA)、锁核酸(LNA)、阿拉伯糖-核酸(FANA)、类似物、衍生物及其组合。优选的,所述修饰为2’氟嘧啶修饰。2’氟嘧啶修饰是将RNA上嘧啶核苷酸的2’-OH用2’-F替代,2’-F能够使RNA不易被体内的RNA酶识别,由此增加RNA片段在体内传输的稳定性。In the present invention, the isolated nucleic acid also includes its variants and derivatives. The nucleic acid can be modified by one of ordinary skill in the art using general methods. Modification methods include (but are not limited to): methylation modification, hydrocarbyl modification, glycosylation modification (such as 2-methoxy-glycosyl modification, hydrocarbyl-glycosyl modification, sugar ring modification, etc.), nucleic acid modification, peptide modification Segment modification, lipid modification, halogen modification, nucleic acid modification (such as "TT" modification) and the like. In one of the embodiments of the present invention, the modification is an internucleotide linkage, for example selected from: phosphorothioate, 2'-O methoxyethyl (MOE), 2'-fluoro, phosphine Acid alkyl esters, phosphorodithioates, alkyl phosphorothioates, phosphoramidates, carbamates, carbonates, phosphoric triesters, acetamidates, carboxymethyl esters, and combinations thereof. In one of the embodiments of the present invention, the modification is a modification of nucleotides, such as selected from: peptide nucleic acid (PNA), locked nucleic acid (LNA), arabinose-nucleic acid (FANA), analogs, derivatives objects and their combinations. Preferably, the modification is a 2' fluoropyrimidine modification. 2'Fluoropyrimidine modification is to replace the 2'-OH of pyrimidine nucleotides on RNA with 2'-F. 2'-F can make RNA not easily recognized by RNase in vivo, thereby increasing the stability of RNA fragment transmission in vivo. sex.
进一步地,所述递送系统为用于包括人在内的哺乳动物中的递送系统。Further, the delivery system is a delivery system for use in mammals including humans.
本申请的另一个发明点为提供一种如上所述的用于治疗帕金森的RNA递送系统在药物中的应用。Another inventive point of the present application is to provide an application of the above-mentioned RNA delivery system for treating Parkinson's in medicine.
所述药物为治疗帕金森及其相关疾病的药物,这里的相关疾病指的是帕金森的形成或发展过程中出现的关联疾病或并发症、后遗症等,或与帕金森具有一定相关性的其他疾病。The drug is a drug for the treatment of Parkinson's and its related diseases, and the related diseases here refer to the associated diseases or complications, sequelae, etc. that occur in the formation or development of Parkinson's, or other diseases that are related to Parkinson's. disease.
所述药物包括上述病毒载体,具体而言,此处的病毒载体表示携带有RNA片段、或携带有RNA片段及靶向标签的病毒载体,并且能够进入宿主体内能够在肝脏部位富集,自组装形成复合结构外泌体,该复合结构能够将RNA片段递送至目标组织,使RNA片段在目标组织中表达,进而抑制与其匹配的基因的表达,实现治疗疾病的目的。The drug includes the above-mentioned viral vector, specifically, the viral vector here refers to a viral vector carrying RNA fragments, or carrying RNA fragments and targeting tags, and can enter the host body, can be enriched in the liver, and self-assemble. A composite structure exosome is formed, which can deliver RNA fragments to the target tissue, so that the RNA fragments are expressed in the target tissue, thereby inhibiting the expression of matching genes, and achieving the purpose of treating diseases.
所述药物的剂型可以为片剂、胶囊剂、粉剂、颗粒剂、丸剂、栓剂、软膏剂、溶液剂、混悬剂、洗剂、凝胶剂、糊剂等。The dosage forms of the drug can be tablets, capsules, powders, granules, pills, suppositories, ointments, solutions, suspensions, lotions, gels, pastes and the like.
进一步地,所述药物的给药方式包括口服、吸入、皮下注射、肌肉注射、静脉注射。优选静脉注射。Further, the administration modes of the drug include oral, inhalation, subcutaneous injection, intramuscular injection, and intravenous injection. Intravenous injection is preferred.
本申请的技术效果为:The technical effects of this application are:
本申请提供的用于治疗帕金森的RNA递送系统以病毒作为载体,病毒载体作为成熟的注入物,其安全性和可靠性已被充分验证,成药性非常好。最终发挥效果的RNA序列由内源性外泌体包裹输送,不存在任何免疫反应,无需验证该外泌体的安全性。该递送系统可以递送各类小分子RNA,通用性强。并且病毒载体的制备要比外泌体或是蛋白质、多肽等物质的制备便宜地多,经济性好。本申请提供的用于治疗帕金森的RNA递送系统在体内自组装后能够与AGO
2紧密结合并富集为复合结构(外泌体),不仅能防止其过早降解,维持其在循环中的稳定性,而且有利于受体细胞吸收、胞浆内释放和溶酶体逃逸,所需剂量低。
The RNA delivery system for the treatment of Parkinson's provided in this application uses a virus as a vector, and the virus vector is used as a mature injection, and its safety and reliability have been fully verified, and the drugability is very good. The final effective RNA sequence is packaged and delivered by endogenous exosomes, and there is no immune response, so there is no need to verify the safety of the exosomes. The delivery system can deliver all kinds of small molecule RNAs, and has strong versatility. And the preparation of viral vectors is much cheaper and more economical than the preparation of exosomes or proteins, polypeptides and other substances. The RNA delivery system for the treatment of Parkinson's provided in this application can be tightly combined with AGO 2 and enriched into a composite structure (exosome) after self-assembly in vivo, which can not only prevent its premature degradation, but also maintain its circulation in the circulation. It is stable, and facilitates uptake by recipient cells, intracytoplasmic release and lysosomal escape, and requires a low dose.
本申请提供的用于治疗帕金森的RNA递送系统应用于药物中,即提供了一个药物递送平台,可以大大提高帕金森病的治疗效果,还可以通过该平台形成更多RNA类药物的研发基础,对RNA类药物研发和使用具有极大的推动作用。The RNA delivery system for the treatment of Parkinson's disease provided in this application is applied to medicine, that is, it provides a drug delivery platform, which can greatly improve the therapeutic effect of Parkinson's disease, and can also form a research and development basis for more RNA drugs through this platform. , which greatly promotes the development and use of RNA drugs.
图1是本申请一实施例提供的转基因小鼠帕金森治疗情况对比图;Fig. 1 is a comparison diagram of the Parkinson's treatment situation of transgenic mice provided by an embodiment of the present application;
图2是本申请一实施例提供的小鼠小胶质细胞的激活和炎症因子的分泌情况对比图;2 is a comparison diagram of the activation of mouse microglia and the secretion of inflammatory factors according to an embodiment of the present application;
图3是本申请一实施例提供的小鼠小胶质细胞的数量对比图。FIG. 3 is a comparison diagram of the number of mouse microglia provided in an example of the present application.
图4是本申请一实施例提供的负载有siRNA的慢病毒载体具有体内富集的效果图。FIG. 4 is an effect diagram of in vivo enrichment of the siRNA-loaded lentiviral vector provided in an embodiment of the present application.
图5是本申请一实施例提供的负载有siRNA的慢病毒载体具有体内自组装的效果图。FIG. 5 is an effect diagram of in vivo self-assembly of the siRNA-loaded lentiviral vector provided in an embodiment of the present application.
图6是本申请一实施例提供的负载有siRNA的慢病毒载体具有帕金森治疗效果的数据结果图,数据 图中是以LRRK2mRNA水平进行对比。Fig. 6 is the data result graph that the lentiviral vector loaded with siRNA provided by an embodiment of the present application has the therapeutic effect of Parkinson's disease.
图7是本申请一实施例提供的负载有siRNA的腺病毒相关病毒1型、4型、7型载体具有体内富集的效果图。FIG. 7 is a graph showing the effect of in vivo enrichment of adeno-associated virus type 1, type 4, and type 7 vectors loaded with siRNA provided in an example of the present application.
图8是本申请一实施例提供的负载有siRNA的腺病毒相关病毒1型、4型、7型载体具有体内自组装的效果图。FIG. 8 is a diagram showing the effect of in vivo self-assembly of the siRNA-loaded adeno-associated virus type 1, type 4, and type 7 vectors provided in an embodiment of the present application.
图9是本申请一实施例提供的负载有siRNA的腺病毒相关病毒1型、4型、7型载体具有帕金森治疗效果的数据结果图,数据图中是以LRRK2mRNA水平进行对比。Fig. 9 is a graph showing the data of the Parkinson's treatment effect of adeno-associated virus type 1, 4, and 7 vectors loaded with siRNA provided in an example of the present application.
图10是本申请一实施例提供的负载有6种单独RNA序列的腺病毒相关病毒8型载体具有体内富集的效果图.Figure 10 is an effect diagram of in vivo enrichment of adenovirus-associated virus type 8 vectors loaded with 6 individual RNA sequences provided by an embodiment of the present application.
图11是本申请一实施例提供的负载有6种单独RNA序列的腺病毒相关病毒8型和9型载体具有体内自组装的效果图。FIG. 11 is an effect diagram of in vivo self-assembly of adeno-associated virus type 8 and type 9 vectors loaded with 6 individual RNA sequences provided in an example of the present application.
图12是本申请一实施例提供的负载有任意2种RNA序列的RNA片段的腺病毒相关病毒9型载体具有体内富集的效果图。FIG. 12 is a diagram showing the effect of in vivo enrichment of an adeno-associated virus type 9 vector loaded with RNA fragments of any two RNA sequences provided in an example of the present application.
图13是本申请一实施例提供的负载有任意2种RNA序列的RNA片段的腺病毒相关病毒8型和9型载体具有体内自组装的效果图。13 is a diagram showing the effect of in vivo self-assembly of adeno-associated virus type 8 and type 9 vectors loaded with RNA fragments of any two RNA sequences provided in an example of the present application.
图14是本申请一实施例提供的负载有任意3种RNA序列的RNA片段的腺病毒载体具有帕金森治疗效果的电泳结果图。FIG. 14 is an electrophoresis result of the Parkinson's treatment effect of an adenovirus vector loaded with RNA fragments of any three RNA sequences provided in an example of the present application.
图15是本申请一实施例提供的腺病毒相关病毒9型中的序列包含有siRNA和RVG的情况下,其所具有的体内富集数据图。FIG. 15 is a graph showing the in vivo enrichment data of the adeno-associated virus type 9 sequences provided in an example of the present application when siRNA and RVG are included.
图16是本申请一实施例提供的腺病毒相关病毒9型中的序列包含有siRNA和RVG的情况下,通过LRRK2mRNA的表达数据所体现出的针对帕金森治疗的效果图。Figure 16 is a graph showing the effect of Parkinson's treatment according to the expression data of LRRK2 mRNA when the sequence in the adenovirus-associated virus type 9 provided in an example of the present application includes siRNA and RVG.
图17是本申请一实施例提供的负载有RVG-LAMP2B融合蛋白及其它融合蛋白在腺病毒载体具有体内富集的数据图。FIG. 17 is a data diagram of in vivo enrichment of adenovirus vectors loaded with RVG-LAMP2B fusion proteins and other fusion proteins provided in an example of the present application.
图18是本申请一实施例提供的RVG-LAMP2B融合蛋白及其它融合蛋白在腺病毒载体上针对帕金森治疗效果的数据对比图,数据通过LRRK2mRNA的相对水平来体现。Figure 18 is a data comparison diagram of the therapeutic effect of RVG-LAMP2B fusion protein and other fusion proteins on adenovirus vectors for Parkinson's disease provided in an example of the present application, and the data is reflected by the relative level of LRRK2 mRNA.
图19是本申请一实施例提供的腺病毒载体系统中包括有与LRRK2基因的siRNA序列同源性大于80%的3条RNA序列时,其所具有的体内富集数据图。Figure 19 is a graph of in vivo enrichment data of the adenoviral vector system provided in an example of the present application when three RNA sequences with more than 80% homology to the siRNA sequence of the LRRK2 gene are included.
图20是本申请一实施例提供的腺病毒载体系统中包括有与LRRK2基因的siRNA序列同源性大于80%的3条RNA序列时,其针对帕金森治疗效果的数据对比图,数据通过LRRK2mRNA的相对水平来体现。Figure 20 is a data comparison diagram of the therapeutic effect on Parkinson's disease when the adenovirus vector system provided by an embodiment of the present application includes 3 RNA sequences with a homology of more than 80% to the siRNA sequence of the LRRK2 gene. to reflect the relative level.
下面结合附图对本申请的具体实施方式进行描述。The specific embodiments of the present application will be described below with reference to the accompanying drawings.
在本发明中,除非另有说明,否则本文中使用的科学和技术名词具有本领域技术人员所通常理解的含义。并且,本文中所用的试剂、材料和操作步骤均为相应领域内广泛使用的试剂、材料和常规步骤。In the present invention, unless otherwise specified, scientific and technical terms used herein have the meanings commonly understood by those skilled in the art. In addition, the reagents, materials and operation steps used herein are the reagents, materials and conventional steps widely used in the corresponding fields.
Western免疫印迹(Western Blot)是将蛋白质转移到膜上,然后利用抗体进行检测.对已知表达蛋白,可 用相应抗体作为一抗进行检测,对新基因的表达产物,可通过融合部分的抗体检测。Western blot (Western Blot) is to transfer the protein to the membrane, and then use the antibody for detection. For the known expressed protein, the corresponding antibody can be used as the primary antibody for detection, and the expression product of the new gene can be detected by the fusion part of the antibody. .
Western Blot采用的是聚丙烯酰胺凝胶电泳,被检测物是蛋白质,“探针”是抗体,“显色”用标记的二抗。经过PAGE分离的蛋白质样品,转移到固相载体(例如硝酸纤维素薄膜)上,固相载体以非共价键形式吸附蛋白质,且能保持电泳分离的多肽类型及其生物学活性不变,以固相载体上的蛋白质或多肽作为抗原,与对应的抗体起免疫反应,再与酶或同位素标记的第二抗体起反应,经过底物显色或放射自显影以检测电泳分离的特异性目的基因表达的蛋白成分。其步骤主要包括:提取蛋白、蛋白定量、制胶和电泳、转膜、免疫标记及显影。Western Blot uses polyacrylamide gel electrophoresis, the detected object is protein, the "probe" is an antibody, and the "color development" is a labeled secondary antibody. The protein sample separated by PAGE is transferred to a solid phase carrier (such as nitrocellulose membrane), and the solid phase carrier adsorbs proteins in the form of non-covalent bonds, and can keep the types of polypeptides separated by electrophoresis and their biological activities unchanged. The protein or polypeptide on the solid phase carrier is used as an antigen, which reacts with the corresponding antibody, and then reacts with the enzyme or isotope-labeled secondary antibody to detect the specific target gene separated by electrophoresis through substrate color development or autoradiography. expressed protein components. The steps mainly include: protein extraction, protein quantification, gel preparation and electrophoresis, membrane transfer, immunolabeling and development.
免疫组化,应用抗原抗体反应,即抗原与抗体特异性结合的原理,通过化学反应使标记抗体的显色剂(荧光素、酶、金属离子、同位素)显色来确定组织细胞内抗原(多肽和蛋白质),对其进行定位、定性及相对定量的研究,称为免疫组织化学技术(immunohistochemistry)或免疫细胞化学技术(immunocytochemistry)。Immunohistochemistry, using antigen-antibody reaction, that is, the principle of specific binding of antigen and antibody, determines the antigen (polypeptide) in tissue cells by developing the color of the chromogenic reagent (fluorescein, enzyme, metal ion, isotope) labeled antibody through chemical reaction. and protein), the localization, qualitative and relative quantitative research, called immunohistochemistry (immunohistochemistry) or immunocytochemistry (immunocytochemistry).
免疫组化的主要步骤包括:切片浸泡、过夜晾干、二甲苯脱蜡、梯度酒精脱蜡(100%、95%、90%、80%、75%、70%、50%,每次3min)、双蒸水、滴加3%过氧化氢溶液去除过氧化氢酶、水洗、抗原修复、滴加5%BSA、封闭1h、稀释一抗、PBS缓冲液清洗、孵二抗、PBS缓冲液清洗、显色液显色、水洗、苏木精染色、梯度乙醇脱水、中性树胶封片。The main steps of immunohistochemistry include: section soaking, overnight drying, xylene dewaxing, gradient alcohol dewaxing (100%, 95%, 90%, 80%, 75%, 70%, 50%, 3min each time) , double-distilled water, dropwise addition of 3% hydrogen peroxide solution to remove catalase, water washing, antigen retrieval, dropwise addition of 5% BSA, blocking for 1 h, dilution of primary antibody, washing with PBS buffer, incubation with secondary antibody, washing with PBS buffer , color developing solution, washing with water, hematoxylin staining, dehydration with gradient ethanol, and sealing with neutral gum.
本发明中涉及到的siRNA水平、蛋白含量和mRNA含量的检测,均是通过向小鼠体内注射RNA递送系统,建立了小鼠干细胞体外模型。利用qRT-PCR检测细胞、组织中mRNA和siRNA表达水平。对于siRNA的绝对定量利用标准品绘制标准曲线的方式进行确定。每个siRNA或mRNA相对于内参的表达量可以用2-ΔCT表示,其中ΔCT=C样品-C内参。扩增siRNA时内参基因为U6snRNA(组织中)或miR-16(血清、外泌体中)分子,扩增mRNA时基因为GAPDH或18s RNA。利用Western blotting实验检测细胞、组织中蛋白质的表达水平,用ImageJ软件进行蛋白定量分析。The detection of the siRNA level, the protein content and the mRNA content involved in the present invention is to establish the mouse stem cell in vitro model by injecting the RNA delivery system into the mouse. The expression levels of mRNA and siRNA in cells and tissues were detected by qRT-PCR. Absolute quantification of siRNA was determined by plotting a standard curve using the standards. The expression level of each siRNA or mRNA relative to the internal control can be represented by 2-ΔCT, where ΔCT=C sample-C internal control. When amplifying siRNA, the internal reference gene is U6snRNA (in tissue) or miR-16 (in serum, exosomes), and when amplifying mRNA, the gene is GAPDH or 18s RNA. Western blotting was used to detect protein expression levels in cells and tissues, and ImageJ software was used for protein quantitative analysis.
实施例1Example 1
本实施例提供一种用于治疗帕金森的RNA递送系统,该系统包括病毒载体,所述病毒载体携带有能够治疗帕金森的RNA片段,所述病毒载体能够在宿主的器官组织中富集,并在所述宿主器官组织中内源性地自发形成含有能够治疗帕金森的所述RNA片段的复合结构,所述复合结构能够将所述RNA片段送入目标组织,实现帕金森的治疗。This embodiment provides an RNA delivery system for treating Parkinson's, the system comprising a viral vector carrying RNA fragments capable of treating Parkinson's, the viral vector can be enriched in the organ tissue of a host, And endogenously and spontaneously form a composite structure containing the RNA fragment capable of treating Parkinson's disease in the host organ tissue, and the composite structure can send the RNA fragment into the target tissue to achieve Parkinson's treatment.
除了腺病毒外,其它病毒载体也具有体内富集、自组装和帕金森的治疗效果,如慢病毒,慢病毒的数据如图4-6所示,其中,CTX代表皮层(cortex),STR代表纹状体(Striatum)。In addition to adenovirus, other viral vectors also have in vivo enrichment, self-assembly and Parkinson's treatment effects, such as lentivirus. The data of lentivirus are shown in Figure 4-6, where CTX stands for cortex and STR stands for Striatum (Striatum).
所述病毒载体优选为腺病毒相关病毒,更优选为腺病毒相关病毒5型、腺病毒相关病毒8型或腺病毒相关病毒9型。The viral vector is preferably adeno-associated virus, more preferably adeno-associated virus type 5, adenovirus-associated virus type 8 or adenovirus-associated virus type 9.
除了腺病毒相关病毒5型、8型和9型以外,其它病毒载体也具有体内富集、自组装及帕金森治疗效果,如腺病毒1型、4型和7型,其数据如图7-9所示。In addition to adeno-associated virus types 5, 8 and 9, other viral vectors also have in vivo enrichment, self-assembly and Parkinson's treatment effects, such as adenovirus types 1, 4 and 7, the data of which are shown in Figure 7- 9 shown.
在本实施例中,病毒载体还包括启动子和靶向标签。所述病毒载体包括以下任意一种线路或几种线路的组合:启动子-RNA序列、启动子-靶向标签、启动子-RNA序列-靶向标签,每一个所述病毒载体中至少包括一个RNA片段和一个靶向标签,所述RNA片段和靶向标签位于相同的线路中或位于不同的线路中。换而言之,病毒载体中可以仅包括启动子-RNA序列-靶向标签,也可以包括启动子-RNA序列、启动子-靶向标签的组合,或是启动子-靶向标签、启动子-RNA序列-靶向标签的组合。In this embodiment, the viral vector also includes a promoter and a targeting tag. The viral vector includes any one of the following circuits or a combination of several circuits: promoter-RNA sequence, promoter-targeting tag, promoter-RNA sequence-targeting tag, and each of the viral vectors includes at least one RNA fragments and a targeting tag, either in the same circuit or in different circuits. In other words, the viral vector may only include a promoter-RNA sequence-targeting tag, or may include a combination of a promoter-RNA sequence, a promoter-targeting tag, or a promoter-targeting tag, a promoter A combination of RNA-seq-targeting tags.
进一步地,所述病毒载体还可以包括能够使所述线路折叠成正确结构并表达的侧翼序列、补偿序列和loop序列,所述侧翼序列包括5’侧翼序列和3’侧翼序列;所述病毒载体包括以下任意一种线路或几种线路的组合:5’-启动子-5’侧翼序列-RNA片段-loop序列-补偿序列-3’侧翼序列、5’-启动子-靶向标签、5’-启动子-靶向标签-5’侧翼序列-RNA片段-loop序列-补偿序列-3’侧翼序列。Further, the viral vector may also include a flanking sequence, a compensation sequence and a loop sequence that can make the circuit fold into a correct structure and express, and the flanking sequence includes a 5' flanking sequence and a 3' flanking sequence; the viral vector Including any one of the following lines or a combination of several lines: 5'-promoter-5' flanking sequence-RNA fragment-loop sequence-compensating sequence-3' flanking sequence, 5'-promoter-targeting tag, 5' - Promoter - Targeting Tag - 5' Flanking Sequence - RNA Fragment - Loop Sequence - Compensation Sequence - 3' Flanking Sequence.
病毒载体中包含有5'-启动子--靶向标签-5'侧翼序列-RNA片段-loop序列-补偿序列-3'侧翼序列时,其RNA递送系统所具有的体内富集和帕金森治疗效果如图15-16所示,靶向标签为RVG,RNA片段为具有治疗作用的siRNA。When the viral vector contains 5'-promoter-targeting tag-5'flanking sequence-RNA fragment-loop sequence-compensating sequence-3'flanking sequence, its RNA delivery system has in vivo enrichment and Parkinson's treatment The effect is shown in Figure 15-16, the targeting tag is RVG, and the RNA fragment is siRNA with therapeutic effect.
其中,所述5’侧翼序列优选为ggatcctggaggcttgctgaaggctgtatgctgaattc或与其同源性大于80%的序列,包括与ggatcctggaggcttgctgaaggctgtatgctgaattc同源性为85%、90%、92%、95%、98%、99%的序列等。Wherein, the 5' flanking sequence is preferably ggatcctggaggcttgctgaaggctgtatgctgaattc or a sequence with a homology greater than 80%, including a sequence with 85%, 90%, 92%, 95%, 98%, 99% homology with ggatcctggaggcttgctgaaggctgtatgctgaattc, etc.
所述loop序列优选为gttttggccactgactgac或与其同源性大于80%的序列,包括与gttttggccactgactgac同源性为85%、90%、92%、95%、98%、99%的序列等。The loop sequence is preferably gttttggccactgactgac or a sequence with more than 80% homology thereto, including sequences with 85%, 90%, 92%, 95%, 98%, 99% homology with gttttggccactgactgac, and the like.
所述3’侧翼序列优选为accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag或与其同源性大于80%的序列,包括与accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag同源性为85%、90%、92%、95%、98%、99%的序列等。The 3' flanking sequence is preferably accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag or a sequence with a homology greater than 80%, including a sequence with 85%, 90%, 92%, 95%, 98%, 99% homology with accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag, etc.
所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-5位碱基。在RNA片段中仅包含一个RNA序列时,所述补偿序列可以为该RNA序列的删除其中任意1-5位碱基的反向互补序列。The compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-5 bases are deleted. When the RNA fragment contains only one RNA sequence, the compensation sequence can be the reverse complementary sequence of the RNA sequence by deleting any 1-5 bases therein.
优选地,所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-3位碱基。在RNA片段中仅包含一个RNA序列时,所述补偿序列可以为该RNA序列的删除其中任意1-3位碱基的反向互补序列。Preferably, the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 bases are deleted. When the RNA fragment contains only one RNA sequence, the compensation sequence can be the reverse complementary sequence of the RNA sequence by deleting any 1-3 bases therein.
更为优选地,所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-3位连续排列的碱基。在RNA片段中仅包含一个RNA序列时,所述补偿序列可以为该RNA序列的删除其中任意1-3位连续排列的碱基的反向互补序列。More preferably, the compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-3 consecutive bases are deleted. When the RNA fragment contains only one RNA sequence, the compensation sequence may be the reverse complementary sequence of the RNA sequence by deleting any 1-3 consecutively arranged bases.
最为优选地,所述补偿序列为所述RNA片段的反向互补序列,并删除其中的第9位和/或第10位碱基。在RNA片段中仅包含一个RNA序列时,所述补偿序列可以为该RNA序列的删除其中第9位和/或第10位的反向互补序列。删除第9位和第10位碱基效果最优。Most preferably, the compensation sequence is the reverse complement of the RNA fragment, and the 9th and/or 10th bases are deleted. When the RNA fragment contains only one RNA sequence, the compensation sequence may be the reverse complementary sequence of the 9th position and/or the 10th position in the deletion of the RNA sequence. Deleting bases 9 and 10 works best.
需要说明的是,上述侧翼序列、补偿序列、loop序列均不是随意选择的,而是基于大量的理论研究和试验确定的,在上述特定侧翼序列、补偿序列、loop序列的配合下,能够最大程度的提高RNA片段的表达率。It should be noted that the above-mentioned flanking sequences, compensation sequences and loop sequences are not randomly selected, but are determined based on a large number of theoretical studies and experiments. increase the expression rate of RNA fragments.
在病毒载体携带两个或多个线路的情况下,相邻的线路之间可以通过序列1-序列2-序列3相连;其中,序列1优选为CAGATC,序列2可以为由5-80个碱基组成的序列,比如10个、15个、20个、25个、30个、35个、40个、45个、50个、55个、60个、65个、70个、75个碱基组成的序列均可,优选为10-50个碱基组成的序列,更优选为20-40个碱基组成的序列,序列3优选为TGGATC。In the case that the viral vector carries two or more lines, the adjacent lines can be connected by sequence 1-sequence 2-sequence 3; wherein, sequence 1 is preferably CAGATC, and sequence 2 can be composed of 5-80 bases Sequence of bases, such as 10, 15, 20, 25, 30, 35, 40, 45, 50, 55, 60, 65, 70, 75 bases The sequence of 10-50 bases is preferable, and the sequence of 20-40 bases is more preferable. Sequence 3 is preferably TGGATC.
序列2具体如下表1所示。 Sequence 2 is specifically shown in Table 1 below.
更为优选地,在病毒载体携带两个或多个线路的情况下,相邻的线路之间通过序列4或与序列4同源性大于80%的序列相连;其中,序列4为CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC。More preferably, when the viral vector carries two or more lines, adjacent lines are connected by sequence 4 or a sequence with more than 80% homology to sequence 4; wherein, sequence 4 is CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC.
序列具体如下表4所示。The sequence is specifically shown in Table 4 below.
| 序列4sequence 4 | CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATCCAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC |
| 序列4-1Sequence 4-1 | CAGATCTGGCCGCACTCGTAGAGGTGAGTCGACCAGTGGATCCAGATCTGGCCGCACTCGTAGAGGTGAGTCGACCAGTGGATC |
| 序列4-2Sequence 4-2 | CAGATCTGGCACCCGTCGAGGTAGTGAGTCGACCAGTGGATCCAGATCTGGCACCCGTCGAGGTAGTGAGTCGACCAGTGGATC |
| 序列4-3Sequence 4-3 | CAGATCTGGCCGCACAGGTCGTAGTGAGTCGACCAGTGGATCCAGATCTGGCCGCACAGGTCGTAGTGAGTCGACCAGTGGATC |
以上所述的RNA片段包含1个、两个或多个具有医疗意义的具体RNA序列,所述RNA序列能够在目标受体中被表达,所述补偿序列在目标受体中不能被表达。RNA序列可以为siRNA序列、shRNA序列或miRNA序列,优选为siRNA序列。The above-mentioned RNA fragments comprise one, two or more specific RNA sequences of medical significance, the RNA sequences can be expressed in the target receptor, and the compensatory sequence cannot be expressed in the target receptor. The RNA sequence can be an siRNA sequence, a shRNA sequence or a miRNA sequence, preferably an siRNA sequence.
一个RNA序列的长度为15-25个核苷酸(nt),优选为18-22nt,比如18nt、19nt、20nt、21nt、22nt均可。此序列长度的范围并不是随意选择的,而是经过反复的试验后确定的。大量试验证明,在RNA序列的长度小于18nt,特别是小于15nt的情况下,该RNA序列大多无效,不会发挥作用,而在RNA序列的长度大于22nt,特别是大于25nt的情况下,则不仅线路的成本大大提高,而且效果也并未优于长度为18-22nt的RNA序列,经济效益差。因此,在RNA序列的长度为15-25nt,特别是18-22nt时,能够兼顾成本与作用的发挥,效果最好。The length of an RNA sequence is 15-25 nucleotides (nt), preferably 18-22nt, such as 18nt, 19nt, 20nt, 21nt, and 22nt. This range of sequence lengths was not chosen arbitrarily, but was determined through trial and error. A large number of experiments have proved that when the length of the RNA sequence is less than 18nt, especially less than 15nt, the RNA sequence is mostly invalid and will not play a role. The cost of the line is greatly increased, and the effect is not better than the RNA sequence with a length of 18-22nt, and the economic benefit is poor. Therefore, when the length of the RNA sequence is 15-25nt, especially 18-22nt, the cost and the effect can be taken into consideration, and the effect is the best.
所述能够治疗帕金森的RNA选自:LRRK2基因的siRNA或编码上述RNA的核酸分子。The RNA capable of treating Parkinson's disease is selected from: siRNA of LRRK2 gene or nucleic acid molecule encoding the above RNA.
选取3条LRRK2siRNA序列,分别为UUGGUCAUCUGGAUACAUC,CAUGAUGCUGUUAUUCU,GAUCUGGAAAUAAAGGACCA,并以第一条siRNA为例进行了其同源性为80%,90%和98%的序 列的效果验证,分别负载有siRNA三个同源序列的递送系统,其所具有的体内富集和帕金森治疗效果如图19-20所示。Three LRRK2 siRNA sequences were selected, namely UUGGUCAUCUGGAUACAUC, CAUGAUGCUGUUAUUCU, GAUUGGAAAUAAAGGACCA, and the first siRNA was used as an example to verify the effect of the sequences with homology of 80%, 90% and 98%. The delivery system of the source sequence, its in vivo enrichment and Parkinson's treatment effect are shown in Figures 19-20.
所需递送RNA有效序列的数量为1条、2条或多条。The number of required delivery RNA effective sequences is one, two or more.
以在同一个病毒载体上联合使用“siRNA1”和“siRNA2”为例,该病毒载体的功能结构区可以表示为:(启动子-siRNA1)-连接序列-(启动子-siRNA2)-连接序列-(启动子-靶向标签),或(启动子-靶向标签-siRNA1)-连接序列-(启动子-靶向标签-siRNA2),或(启动子-siRNA1)-连接序列-(启动子-靶向标签-siRNA2)等。Taking the combined use of "siRNA1" and "siRNA2" on the same viral vector as an example, the functional structural region of the viral vector can be expressed as: (promoter-siRNA1)-connector sequence-(promoter-siRNA2)-connector sequence- (promoter-targeting tag), or (promoter-targeting tag-siRNA1)-linker-(promoter-targeting tag-siRNA2), or (promoter-siRNA1)-linker-(promoter- Targeting tag-siRNA2) etc.
更加具体地,该病毒载体的功能结构区可以表示为:(5’-启动子-5’侧翼序列-siRNA1-loop序列-补偿序列-3’侧翼序列)-连接序列-(5’-启动子-5’侧翼序列-siRNA2-loop序列-补偿序列-3’侧翼序列)-连接序列-(5’-启动子-靶向标签),或(5’-启动子-靶向标签-5’侧翼序列-siRNA1-loop序列-补偿序列-3’侧翼序列)-连接序列-(5’-启动子-靶向标签-5’侧翼序列-siRNA2-loop序列-补偿序列-3’侧翼序列),或(5’-启动子-5’侧翼序列-siRNA1-loop序列-补偿序列-3’侧翼序列)-连接序列-(5’-启动子-靶向标签-5’侧翼序列-siRNA2-loop序列-补偿序列-3’侧翼序列)、(5’-启动子-靶向标签-5’侧翼序列-siRNA1-siRNA2-loop序列-补偿序列-3’侧翼序列)等。其他情况均可以此类推,在此不再赘述。以上连接序列可以为“序列1-序列2-序列3”或“序列4”,一个括号表示一个完整的线路(circuit)。More specifically, the functional structural region of the viral vector can be expressed as: (5'-promoter-5'flanking sequence-siRNA1-loop sequence-compensating sequence-3'flanking sequence)-connector sequence-(5'-promoter - 5' flanking sequence - siRNA2-loop sequence - compensation sequence - 3' flanking sequence) - linking sequence - (5'-promoter-targeting tag), or (5'-promoter-targeting tag-5' flanking sequence-siRNA1-loop sequence-compensation sequence-3' flanking sequence)-linker sequence-(5'-promoter-targeting tag-5'flanking sequence-siRNA2-loop sequence-compensating sequence-3'flanking sequence), or (5'-promoter-5'flanking sequence-siRNA1-loop sequence-compensating sequence-3'flanking sequence)-linking sequence-(5'-promoter-targeting tag-5'flanking sequence-siRNA2-loop sequence- Compensation sequence-3'flanking sequence), (5'-promoter-targeting tag-5'flanking sequence-siRNA1-siRNA2-loop sequence-compensating sequence-3'flanking sequence), etc. Other situations can be deduced by analogy, and details are not repeated here. The above connecting sequence can be "sequence 1-sequence 2-sequence 3" or "sequence 4", and a bracket indicates a complete circuit.
优选地,上述RNA还可以通过对其中的RNA序列(siRNA、shRNA或miRNA)进行核糖修饰得到,优选2’氟嘧啶修饰。2’氟嘧啶修饰是将siRNA、shRNA或miRNA上嘧啶核苷酸的2’-OH用2’-F替代,2’-F能够使人体内的RNA酶不易识别siRNA、shRNA或miRNA,如此能够增加RNA在体内传输的稳定性。Preferably, the above RNA can also be obtained by ribose modification of the RNA sequence (siRNA, shRNA or miRNA) therein, preferably 2' fluoropyrimidine modification. 2'Fluoropyrimidine modification is to replace the 2'-OH of pyrimidine nucleotides on siRNA, shRNA or miRNA with 2'-F. 2'-F can make it difficult for RNase in the human body to recognize siRNA, shRNA or miRNA, so it can Increases the stability of RNA transport in vivo.
具体地,肝脏会吞噬外源性的病毒,高达99%的外源性病毒会进入肝脏,因此当以病毒作为载体时并不需要做特异性设计即可在肝脏组织中富集,随后病毒载体被打开,释放出RNA分子(siRNA、shRNA或miRNA),肝脏组织自发地将上述RNA分子包裹进外泌体内部,这些外泌体就变成了RNA输送机构。Specifically, the liver will phagocytose exogenous viruses, and up to 99% of the exogenous viruses will enter the liver. Therefore, when viruses are used as vectors, they can be enriched in liver tissue without specific design. After being opened, RNA molecules (siRNA, shRNA, or miRNA) are released, and liver tissue spontaneously wraps the above RNA molecules into exosomes, and these exosomes become RNA delivery mechanisms.
优选地,为了使该RNA输送机构(外泌体)具有“精确制导”的能力,在注入体内的病毒载体中我们设计了靶向标签,该靶向标签也会被肝脏组织组装到外泌体中,尤其是当选择某些特定的靶向标签时,靶向标签能够被插入外泌体表面,从而成为能够引导外泌体的靶向结构,这就大大提高了本发明所述的RNA输送机构的精准性,一方面可以使所需引入的病毒载体的用量大大减少,另一方面还大大提高了潜在药物递送的效率。Preferably, in order to make the RNA delivery mechanism (exosome) have the ability of "precision guidance", we design a targeting tag in the viral vector injected into the body, and the targeting tag will also be assembled into exosomes by liver tissue In particular, when certain specific targeting tags are selected, the targeting tags can be inserted into the surface of exosomes to become targeting structures that can guide exosomes, which greatly improves the RNA delivery of the present invention. The accuracy of the mechanism, on the one hand, can greatly reduce the amount of viral vector that needs to be introduced, and on the other hand, greatly improves the efficiency of potential drug delivery.
靶向标签选自具有靶向功能的肽、蛋白质或抗体中的一种,靶向标签的选择是需要创造性劳动的过程,一方面需要根据目标组织选取可用的靶向标签,另一方面还需要保证该靶向标签能够在稳定地出现在外泌体的表面,从而达到靶向功能。目前已经筛选出的靶向标签包括:靶向肽、靶向蛋白、抗体。其中,靶向肽包括但不限于RVG靶向肽(核苷酸序列如SEQ ID No:1所示)、GE11靶向肽(核苷酸序列如SEQ ID No:2所示)、PTP靶向肽(核苷酸序列如SEQ ID No:3所示)、TCP-1靶向肽(核苷酸序列如SEQ ID No:4所示)、MSP靶向肽(核苷酸序列如SEQ ID No:5所示);靶向蛋白包括但不限于RVG-LAMP2B融合蛋白(核苷酸序列如SEQ ID No:6所示)、GE11-LAMP2B融合蛋白(核苷酸序列如SEQ ID No:7所示)、PTP-LAMP2B融合蛋白(核苷酸序列如SEQ ID No:8所示)、TCP-1-LAMP2B融合蛋白(核苷酸序列如SEQ ID No:9所示)、MSP-LAMP2B融合蛋白(核苷酸序列如SEQ ID No:10所示)。在本实施例中,靶向标签优选采用能够精准靶向脑组织的RVG靶向肽、RVG-LAMP2B融合蛋白。The targeting tag is selected from one of the peptides, proteins or antibodies with targeting function. The selection of the targeting tag is a process that requires creative work. On the one hand, it is necessary to select the available targeting tags according to the target tissue. It is ensured that the targeting label can stably appear on the surface of exosomes, so as to achieve the targeting function. Targeting tags that have been screened include: targeting peptides, targeting proteins, and antibodies. Wherein, targeting peptides include but are not limited to RVG targeting peptide (nucleotide sequence shown in SEQ ID No: 1), GE11 targeting peptide (nucleotide sequence shown in SEQ ID No: 2), PTP targeting peptide Peptide (nucleotide sequence shown in SEQ ID No: 3), TCP-1 targeting peptide (nucleotide sequence shown in SEQ ID No: 4), MSP targeting peptide (nucleotide sequence shown in SEQ ID No: 4) : 5); targeting proteins include but are not limited to RVG-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 6), GE11-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 7) shown), PTP-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 8), TCP-1-LAMP2B fusion protein (nucleotide sequence shown in SEQ ID No: 9), MSP-LAMP2B fusion protein (The nucleotide sequence is shown in SEQ ID No: 10). In this embodiment, the targeting tag preferably adopts RVG targeting peptide and RVG-LAMP2B fusion protein that can accurately target brain tissue.
RVG-LAMP2B融合蛋白在腺病毒载体上所具有的体内富集和帕金森治疗效果如图17-18所示,其治疗效果通过LRRK2mRNA的水平来体现。Figures 17-18 show the in vivo enrichment and Parkinson's treatment effect of RVG-LAMP2B fusion protein on adenovirus vector, and its therapeutic effect is reflected by the level of LRRK2 mRNA.
此外,为了达到精准递送的目的,我们实验了多种病毒载体搭载的方案,得出另一优化的方案:所述病毒载体还可以由具有不同结构的多种病毒构成,其中一种病毒包含启动子和靶向标签,其他病毒包含启动子和RNA片段。即将靶向标签与RNA片段装载到不同的病毒载体中,将两种病毒载体注入体内,其靶向效果不差于将相同的靶向标签与RNA片段装载在一个病毒载体中产生的靶向效果。In addition, in order to achieve the purpose of precise delivery, we have experimented with a variety of viral vector loading schemes, and came up with another optimized scheme: the viral vector can also be composed of multiple viruses with different structures, one of which contains a promoter promoters and targeting tags, other viruses contain promoters and RNA segments. Loading the targeting tag and RNA fragment into different viral vectors, and injecting the two viral vectors into the body, the targeting effect is no worse than the targeting effect produced by loading the same targeting tag and RNA fragment into one viral vector .
更优选地,两种不同的病毒载体注入宿主体内时,可以先将装有RNA序列的病毒载体注入,在1-2小时后再注入含有靶向标签的病毒载体,如此能够达到更优的靶向效果。More preferably, when two different viral vectors are injected into the host, the viral vector containing the RNA sequence can be injected first, and then the viral vector containing the targeting tag can be injected after 1-2 hours, so that a better target can be achieved. to the effect.
以上所述的递送系统均可用于包括人在内的哺乳动物。The delivery systems described above can all be used in mammals, including humans.
本实施例提供的用于治疗帕金森的RNA递送系统以病毒作为载体,病毒载体作为成熟的注入物,其安全性和可靠性已被充分验证,成药性非常好。最终发挥效果的RNA序列由内源性外泌体包裹输送,不存在任何免疫反应,无需验证该外泌体的安全性。该递送系统可以递送各类小分子RNA,通用性强。并且病毒载体的制备要比外泌体或是蛋白质、多肽等物质的制备便宜地多,经济性好。本实施例提供的用于治疗帕金森的RNA递送系统在体内自组装后能够与AGO
2紧密结合并富集为复合结构(外泌体),不仅能防止其过早降解,维持其在循环中的稳定性,而且有利于受体细胞吸收、胞浆内释放和溶酶体逃逸,所需剂量低。
The RNA delivery system for the treatment of Parkinson's provided in this example uses a virus as a vector, and the virus vector is used as a mature injection. Its safety and reliability have been fully verified, and its druggability is very good. The final effective RNA sequence is packaged and delivered by endogenous exosomes, and there is no immune response, so there is no need to verify the safety of the exosomes. The delivery system can deliver all kinds of small molecule RNAs, and has strong versatility. And the preparation of viral vectors is much cheaper and more economical than the preparation of exosomes or proteins, polypeptides and other substances. The RNA delivery system for the treatment of Parkinson's disease provided in this example can be tightly combined with AGO 2 and enriched into a complex structure (exosome) after self-assembly in vivo, which can not only prevent its premature degradation, but also maintain its circulation in the circulation. It is stable, and is beneficial to receptor cell uptake, intracytoplasmic release and lysosomal escape, and the required dose is low.
实施例2Example 2
在实施例1的基础上,本实施例提供一种药物。该药物包括病毒载体,所述病毒载体携带有能够治疗帕金森的RNA片段,所述病毒载体能够在宿主的器官组织中富集,并在所述宿主器官组织中内源性地自发形成含有能够治疗帕金森的所述RNA片段的复合结构,所述复合结构能够将所述RNA片段送入目标组织,实现帕金森的治疗。On the basis of Embodiment 1, this embodiment provides a medicine. The medicament includes a viral vector carrying an RNA segment capable of treating Parkinson's, the viral vector being capable of enriching in the organ tissue of a host, and endogenously and spontaneously forming in the organ tissue of the host an RNA segment capable of treating Parkinson's disease The composite structure of the RNA fragment for treating Parkinson's disease, the composite structure can deliver the RNA fragment into the target tissue to realize the treatment of Parkinson's disease.
可选地,所述RNA片段包含1个、两个或多个具有医疗意义的具体RNA序列,所述RNA序列是具有医学意义的siRNA、shRNA或miRNA。Optionally, the RNA fragment comprises one, two or more specific RNA sequences with medical significance, and the RNA sequences are siRNA, shRNA or miRNA with medical significance.
以腺病毒相关病毒8型和9型为病毒载体,其在携带有1个或多个RNA片段的情况下,具有体内富集、自组装和帕金森治疗效果,图10-11显示了载体携带有6种单独RNA序列的RNA片段所呈现的数据结果;图12-13显示了载体携带有4组包含有任意2种RNA序列的RNA片段所呈现的数据结果;图14显示了载体携带有3组包含有任意3种RNA序列的RNA片段所呈现的治疗数据结果。Adenovirus-associated virus types 8 and 9 are used as viral vectors, which have in vivo enrichment, self-assembly and Parkinson's treatment effects when carrying one or more RNA fragments. Figure 10-11 shows that the vectors carry Figures 12-13 show data presented for RNA fragments with 6 individual RNA sequences; Figures 12-13 show data presented for vectors carrying 4 sets of RNA fragments containing any two RNA sequences; Figure 14 shows vectors carrying 3 Groups contain therapeutic data results presented by RNA fragments of any of the 3 RNA sequences.
序列具体如下表3所示。The specific sequence is shown in Table 3 below.
可选地,所述病毒载体包括启动子和靶向标签,所述靶向标签能够在宿主的器官组织中形成所述复合结构的靶向结构,所述靶向结构位于复合结构的表面,所述复合结构能够通过所述靶向结构寻找并结合目标组织,将所述RNA片段递送进入目标组织。Optionally, the viral vector includes a promoter and a targeting tag, the targeting tag can form the targeting structure of the composite structure in the organ tissue of the host, and the targeting structure is located on the surface of the composite structure, so The complex structure can seek and bind to the target tissue through the targeting structure, and deliver the RNA fragment into the target tissue.
关于本实施例中上述病毒载体、RNA片段、靶向标签等的解释说明均可以参考实施例1,在此不再赘述。For explanations about the above-mentioned viral vectors, RNA fragments, targeting tags, etc. in this embodiment, reference may be made to Embodiment 1, which will not be repeated here.
该药物可以通过口服、吸入、皮下注射、肌肉注射或静脉注射的方式进入人体后,通过实施例1所述的RNA递送系统递送至目标组织,发挥治疗作用。After the drug can be administered orally, inhaled, subcutaneously injected, intramuscularly injected or intravenously injected into the human body, it can be delivered to the target tissue through the RNA delivery system described in Example 1 to exert a therapeutic effect.
该药物可以与其他治疗帕金森病的药物联合使用,以提高治疗效果,比如抗胆碱能药(安坦等)、抗组织胺药(苯海拉明、金刚烷胺等)、左旋多巴类药(多芭、息宁、西莱美等)、多巴胺受体激动剂(泰舒达、协良行、克瑞帕、溴隐亭等)、单胺氧化酶B抑制剂(司吉宁、金思平等)、儿茶酚胺氧位甲基转移酶抑制剂(恩托卡朋等)。The drug can be used in combination with other Parkinson's disease drugs to improve the treatment effect, such as anticholinergics (Antan, etc.), antihistamines (diphenhydramine, amantadine, etc.), levodopa Drugs (Dopa, Sining, Xilaimei, etc.), dopamine receptor agonists (Texida, Xie Liangxing, Crepa, bromocriptine, etc.), monoamine oxidase B inhibitors (Sgining, Jin Siping, etc.) ), catecholamine oxygen methyltransferase inhibitors (Entocapone, etc.).
本实施例的药物还可以包括药学上可以接受的载体,该载体包括但不限于稀释剂、缓冲剂、乳剂、包囊剂、赋形剂、填充剂、粘合剂、喷雾剂、透皮吸收剂、湿润剂、崩解剂、吸收促进剂、表面活性剂、着色剂、矫味剂、佐剂、干燥剂、吸附载体等。The medicine of this embodiment may also include a pharmaceutically acceptable carrier, which includes but is not limited to diluents, buffers, emulsions, encapsulation agents, excipients, fillers, adhesives, sprays, transdermal absorption Agents, wetting agents, disintegrating agents, absorption enhancers, surfactants, colorants, flavoring agents, adjuvants, desiccants, adsorption carriers, etc.
本实施例提供的药物的剂型可以为片剂、胶囊剂、粉剂、颗粒剂、丸剂、栓剂、软膏剂、溶液剂、混悬剂、洗剂、凝胶剂、糊剂等。The dosage forms of the medicine provided in this embodiment can be tablets, capsules, powders, granules, pills, suppositories, ointments, solutions, suspensions, lotions, gels, pastes, and the like.
本实施例提供的药物以病毒作为载体,病毒载体作为成熟的注入物,其安全性和可靠性已被充分验证,成药性非常好。最终发挥效果的RNA序列由内源性外泌体包裹输送,不存在任何免疫反应,无需验证该外泌体的安全性。该药物可以递送各类小分子RNA,通用性强。并且病毒载体的制备要比外泌体或是蛋白质、多肽等物质的制备便宜地多,经济性好。本申请提供的药物在体内自组装后能够与AGO
2紧密结合并富集为复合结构(外泌体),不仅能防止其过早降解,维持其在循环中的稳定性,而且有利于受体细胞吸收、胞浆内释放和溶酶体逃逸,所需剂量低。
The medicine provided in this example uses a virus as a carrier, and the virus carrier is used as a mature injection. Its safety and reliability have been fully verified, and the druggability is very good. The final effective RNA sequence is packaged and delivered by endogenous exosomes, and there is no immune response, so there is no need to verify the safety of the exosomes. The drug can deliver various kinds of small molecule RNAs and has strong versatility. And the preparation of viral vectors is much cheaper and more economical than the preparation of exosomes or proteins, polypeptides and other substances. The drug provided by this application can be closely combined with AGO 2 and enriched into a composite structure (exosome) after self-assembly in vivo, which can not only prevent its premature degradation and maintain its stability in circulation, but also benefit the receptor. Cellular uptake, intracytoplasmic release and lysosomal escape require low doses.
实施例3Example 3
在实施例1或2的基础上,本实施例提供一种用于治疗帕金森的RNA递送系统在药物中的应用,该药物为治疗帕金森的药物。本实施例结合以下试验对RNA递送系统在帕金森治疗方面的应用进行具体说明。On the basis of Embodiment 1 or 2, this embodiment provides an application of an RNA delivery system for treating Parkinson's disease in a drug, and the drug is a drug for treating Parkinson's disease. In this example, the application of the RNA delivery system in the treatment of Parkinson's disease is specifically described in conjunction with the following experiments.
首先,选择LRRK2R1441G转基因小鼠3月龄时进行试验,试验设置LPS干预组和LPS非干预组。LPS干预组LPS干预7天后进行AAV-CMV-scrR/AAV-CMV-RVG-siR
LRRK2的治疗(图中将AAV-CMV-scrR、AAV-CMV-RVG-siR
LRRK2简写为CMV-scrR、CMV-RVG-siR
LRRK2)。
First, LRRK2R1441G transgenic mice were selected for the experiment when they were 3 months old, and the experiment set up LPS intervention group and LPS non-intervention group. The LPS intervention group was treated with AAV-CMV-scrR/AAV-CMV-RVG-siR LRRK2 after 7 days of LPS intervention (AAV-CMV-scrR, AAV-CMV-RVG-siR LRRK2 are abbreviated as CMV-scrR, CMV- RVG-siR LRRK2 ).
如图1所示,我们选取12周龄的LRRK2
R1441G小鼠,腹腔注射5mg/kg LPS进行炎症诱导,7天后,每2天静脉注射5mg/kg CMV-scrR或CMV-RVG-siR
LRRK2线路(Genetic),共注射2周。治疗后处死小鼠,定量检测LRRK2/S935在纹状体和黑质致密部的表达。参见图1A,Western blot分析纹状体和黑质致密部LRRK2/S935蛋白水平,结果显示α-微管蛋白作为内部加载控制。参见图1B,定量显示LRRK2蛋 白水平可看出,LPS干预后进行AAV-CMV-scrR治疗的小鼠LRRK2蛋白水平明显高于其他组,而接受AAV-CMV-RVG-siR
LRRK2治疗的小鼠LRRK2蛋白水平显著较低。参见图1C-D,这几幅图展示了纹状体(Striatum)和黑质致密部(SNpc)的LRRK2/S935免疫荧光染色(红色)、神经元免疫荧光染色(红色)的结果,比例尺:50μm,结果表明注射AV-CMV-RVG-siR
LRRK2的小鼠挽救了TH神经元的丢失,能够抑制小胶质的激活,说明AV-CMV-RVG-siR
LRRK2在肝脏释放siRNA组装进入外泌体后可以穿过血脑屏障进入脑深部发挥功能。
As shown in Figure 1, we selected 12-week-old LRRK2 R1441G mice, intraperitoneally injected 5 mg/kg LPS for inflammation induction, and 7 days later, intravenously injected 5 mg/kg CMV-scrR or CMV-RVG-siR LRRK2 line ( Genetic) for a total of 2 weeks of injection. Mice were sacrificed after treatment, and the expression of LRRK2/S935 in striatum and substantia nigra pars compacta was quantitatively detected. Referring to Figure 1A, Western blot analysis of LRRK2/S935 protein levels in the striatum and substantia nigra pars compacta revealed α-tubulin as an internal loading control. Referring to Figure 1B, the quantitative display of LRRK2 protein levels shows that the LRRK2 protein levels in mice treated with AAV-CMV-scrR after LPS intervention were significantly higher than those in other groups, while the LRRK2 in mice treated with AAV-CMV-RVG-siR LRRK2 Protein levels were significantly lower. See Figure 1C-D, which show the results of LRRK2/S935 immunofluorescence staining (red) and neuronal immunofluorescence staining (red) of the striatum (Striatum) and substantia nigra pars compacta (SNpc), scale bar: 50 μm, the results showed that mice injected with AV-CMV-RVG-siR LRRK2 rescued the loss of TH neurons and could inhibit the activation of microglia, indicating that AV-CMV-RVG-siR LRRK2 released siRNA in the liver to assemble into exosomes After passing through the blood-brain barrier, it can enter the deep brain to function.
如图2所示,选取12周龄的LRRK2
R1441G小鼠,腹腔注射5mg/kg LPS进行炎症诱导,7天后,每2天静脉注射5mg/kg AAV-CMV-scrR或AAV-CMV-RVG-siR
LRRK2Genetic,共注射2周。终止治疗后,处死小鼠,观察小胶质细胞的激活和炎症因子的分泌情况。(图中将AAV-CMV-scrR、AAV-CMV-RVG-siR
LRRK2简写为CMV-scrR、CMV-RVG-siR
LRRK2)
As shown in Figure 2, 12-week-old LRRK2 R1441G mice were selected and injected intraperitoneally with 5 mg/kg LPS to induce inflammation. After 7 days, 5 mg/kg AAV-CMV-scrR or AAV-CMV-RVG-siR was intravenously injected every 2 days. LRRK2 Genetic, injected for 2 weeks. After the treatment was terminated, the mice were sacrificed to observe the activation of microglia and the secretion of inflammatory factors. (AAV-CMV-scrR, AAV-CMV-RVG-siR LRRK2 are abbreviated as CMV-scrR, CMV-RVG-siR LRRK2 in the figure)
参见图2,抗iba-1抗体免疫染色显示R1441G小鼠纹状体和黑质致密部小胶质细胞激活,比例尺:50μm。参见图3,量化图2中纹状体和SNpc中小胶质细胞的数量后可以看出,LPS干预后进行AAV-CMV-scrR治疗的小鼠纹状体和SNpc中小胶质细胞的数量显著高于其他组,而接受AAV-CMV-RVG-siR
LRRK2治疗的小鼠纹状体和SNpc中小胶质细胞的数量显著较低。
See Figure 2, anti-iba-1 antibody immunostaining shows activation of microglia in the striatum and substantia nigra pars compacta of R1441G mice, scale bar: 50 μm. Referring to Figure 3, after quantifying the number of microglia in the striatum and SNpc in Figure 2, it can be seen that the number of microglia in the striatum and SNpc of mice treated with AAV-CMV-scrR after LPS intervention was significantly higher Compared with the other groups, the number of microglia in the striatum and SNpc of mice treated with AAV-CMV-RVG-siR LRRK2 was significantly lower.
以上试验可以说明,静脉注射AAV-CMV-RVG-siR
LRRK2有助于抑制多巴胺能神经元中的LRRK2,从而减轻帕金森PD小鼠的神经病理发展。
The above experiments can illustrate that intravenous injection of AAV-CMV-RVG-siR LRRK2 helps to inhibit LRRK2 in dopaminergic neurons, thereby reducing the neuropathological development of Parkinson's PD mice.
在本文中,“上”、“下”、“前”、“后”、“左”、“右”等仅用于表示相关部分之间的相对位置关系,而非限定这些相关部分的绝对位置。In this document, "upper", "lower", "front", "rear", "left", "right", etc. are only used to indicate the relative positional relationship between related parts, rather than limit the absolute positions of these related parts .
在本文中,“第一”、“第二”等仅用于彼此的区分,而非表示重要程度及顺序、以及互为存在的前提等。In this document, "first", "second", etc. are only used to distinguish each other, but do not indicate the degree of importance and order, and the premise of mutual existence.
在本文中,“相等”、“相同”等并非严格的数学和/或几何学意义上的限制,还包含本领域技术人员可以理解的且制造或使用等允许的误差。In this paper, "equal", "same" and the like are not limitations in strict mathematical and/or geometric senses, and also include errors that can be understood by those skilled in the art and allowed by manufacturing or use.
除非另有说明,本文中的数值范围不仅包括其两个端点内的整个范围,也包括含于其中的若干子范围。Unless otherwise indicated, numerical ranges herein include not only the entire range between its two endpoints, but also several subranges subsumed therein.
上面结合附图对本申请优选的具体实施方式和实施例作了详细说明,但是本申请并不限于上述实施方式和实施例,在本领域技术人员所具备的知识范围内,还可以在不脱离本申请构思的前提下做出各种变化。The preferred specific embodiments and embodiments of the present application have been described in detail above in conjunction with the accompanying drawings, but the present application is not limited to the above-mentioned embodiments and embodiments. Various changes are made under the premise of the application concept.
Claims (19)
- 一种用于治疗帕金森的RNA递送系统,其特征在于,该系统包括病毒载体,所述病毒载体携带有能够治疗帕金森的RNA片段,所述病毒载体能够在宿主的器官组织中富集,并在所述宿主器官组织中内源性地自发形成含有能够治疗帕金森的所述RNA片段的复合结构,所述复合结构能够将所述RNA片段送入目标组织,实现帕金森的治疗。An RNA delivery system for treating Parkinson's, characterized in that the system comprises a viral vector, the viral vector carries an RNA fragment capable of treating Parkinson's, and the viral vector can be enriched in the organ tissue of a host, And endogenously and spontaneously form a composite structure containing the RNA fragment capable of treating Parkinson's disease in the host organ tissue, and the composite structure can send the RNA fragment into the target tissue to achieve Parkinson's treatment.
- 如权利要求1所述的用于治疗帕金森的RNA递送系统,其特征在于,所述病毒载体为腺病毒相关病毒。The RNA delivery system for treating Parkinson's according to claim 1, wherein the viral vector is an adenovirus-associated virus.
- 如权利要求2所述的用于治疗帕金森的RNA递送系统,其特征在于,所述腺病毒相关病毒为腺病毒相关病毒5型、腺病毒相关病毒8型或腺病毒相关病毒9型。The RNA delivery system for treating Parkinson's according to claim 2, wherein the adeno-associated virus is adeno-associated virus type 5, adenovirus-associated virus type 8 or adenovirus-associated virus type 9.
- 如权利要求1所述的用于治疗帕金森的RNA递送系统,其特征在于,所述RNA片段包含1个、两个或多个具有医疗意义的具体RNA序列,所述RNA序列是具有医学意义的siRNA、shRNA或miRNA。The RNA delivery system for treating Parkinson's according to claim 1, wherein the RNA fragment comprises one, two or more specific RNA sequences with medical significance, and the RNA sequences are medically significant siRNA, shRNA or miRNA.
- 如权利要求1所述的用于治疗帕金森的RNA递送系统,其特征在于,所述病毒载体包括启动子和靶向标签,所述靶向标签能够在宿主的器官组织中形成所述复合结构的靶向结构,所述靶向结构位于复合结构的表面,所述复合结构能够通过所述靶向结构寻找并结合目标组织,将所述RNA片段递送进入目标组织。The RNA delivery system for treating Parkinson's according to claim 1, wherein the viral vector comprises a promoter and a targeting tag, and the targeting tag can form the composite structure in the organ tissue of the host The targeting structure is located on the surface of the composite structure, and the composite structure can find and bind to the target tissue through the targeting structure, and deliver the RNA fragment into the target tissue.
- 如权利要求4所述的用于治疗帕金森的RNA递送系统,其特征在于,所述病毒载体中包括以下任意一种线路或几种线路的组合:启动子-RNA片段、启动子-靶向标签、启动子-RNA片段-靶向标签;每一个所述病毒载体中至少包括一个RNA片段和一个靶向标签,所述RNA片段和靶向标签位于相同的线路 中或位于不同的线路中。The RNA delivery system for treating Parkinson's according to claim 4, wherein the viral vector comprises any one of the following lines or a combination of several lines: promoter-RNA fragment, promoter-targeting Tag, promoter-RNA segment-targeting tag; each of the viral vectors includes at least one RNA segment and one targeting tag, and the RNA segment and targeting tag are located in the same line or in different lines.
- 如权利要求6所述的用于治疗帕金森的RNA递送系统,其特征在于,所述病毒载体还包括能够使所述线路折叠成正确结构并表达的侧翼序列、补偿序列和loop序列,所述侧翼序列包括5’侧翼序列和3’侧翼序列;The RNA delivery system for treating Parkinson's according to claim 6, wherein the viral vector further comprises a flanking sequence, a compensation sequence and a loop sequence that can fold the circuit into a correct structure and express it, the Flanking sequences include 5' flanking sequences and 3' flanking sequences;所述病毒载体中包括以下任意一种线路或几种线路的组合:5'-启动子-5'侧翼序列-RNA片段-loop序列-补偿序列-3'侧翼序列、5'-启动子-靶向标签、5'-启动子-靶向标签-5'侧翼序列-RNA片段-loop序列-补偿序列-3'侧翼序列。The viral vector includes any one of the following lines or a combination of several lines: 5'-promoter-5' flanking sequence-RNA fragment-loop sequence-compensating sequence-3' flanking sequence, 5'-promoter-target To tag, 5'-promoter-targeting tag-5'flanking sequence-RNA fragment-loop sequence-compensating sequence-3'flanking sequence.
- 如权利要求6所述的用于治疗帕金森的RNA递送系统,其特征在于,所述5’侧翼序列为ggatcctggaggcttgctgaaggctgtatgctgaattc或与其同源性大于80%的序列;The RNA delivery system for treating Parkinson's according to claim 6, wherein the 5' flanking sequence is ggatcctggaggcttgctgaaggctgtatgctgaattc or a sequence with a homology greater than 80%;所述loop序列为gttttggccactgactgac或与其同源性大于80%的序列;The loop sequence is gttttggccactgactgac or a sequence whose homology is greater than 80%;所述3’侧翼序列为accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag或与其同源性大于80%的序列;The 3' flanking sequence is accggtcaggacacaaggcctgttactagcactcacatggaacaaatggcccagatctggccgcactcgag or a sequence whose homology is greater than 80%;所述补偿序列为所述RNA片段的反向互补序列,并删除其中任意1-5位碱基。The compensation sequence is the reverse complementary sequence of the RNA fragment, and any 1-5 bases are deleted.
- 如权利要求6所述的用于治疗帕金森的RNA递送系统,其特征在于,在病毒载体中存在至少两种线路的情况下,相邻的线路之间通过序列1-3组成的序列相连;The RNA delivery system for treating Parkinson's as claimed in claim 6, characterized in that, when there are at least two circuits in the viral vector, adjacent circuits are connected by a sequence consisting of sequences 1-3;其中,序列1为CAGATC,序列2是由5-80个碱基组成的序列,序列3为TGGATC。Wherein, sequence 1 is CAGATC, sequence 2 is a sequence consisting of 5-80 bases, and sequence 3 is TGGATC.
- 如权利要求9所述的用于治疗帕金森的RNA递送系统,其特征在于,在病毒载体中存在至少两种线路的情况下,相邻的线路之间通过序列4或与序 列4同源性大于80%的序列相连;The RNA delivery system for treating Parkinson's as claimed in claim 9, characterized in that, when there are at least two lines in the viral vector, adjacent lines pass through sequence 4 or homology with sequence 4 More than 80% of the sequences are connected;其中,序列4为CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC。Wherein, sequence 4 is CAGATCTGGCCGCACTCGAGGTAGTGAGTCGACCAGTGGATC.
- 如权利要求1所述的用于治疗帕金森的RNA递送系统,其特征在于,所述器官组织为肝脏,所述复合结构为外泌体。The RNA delivery system for treating Parkinson's according to claim 1, wherein the organ tissue is liver, and the composite structure is exosome.
- 如权利要求5所述的用于治疗帕金森的RNA递送系统,其特征在于,所述靶向标签选自具有靶向功能的靶向肽或靶向蛋白。The RNA delivery system for treating Parkinson's according to claim 5, wherein the targeting tag is selected from targeting peptides or targeting proteins with targeting function.
- 如权利要求12所述的用于治疗帕金森的RNA递送系统,其特征在于,所述靶向肽包括RVG靶向肽、GE11靶向肽、PTP靶向肽、TCP-1靶向肽、MSP靶向肽;The RNA delivery system for treating Parkinson's according to claim 12, wherein the targeting peptide comprises RVG targeting peptide, GE11 targeting peptide, PTP targeting peptide, TCP-1 targeting peptide, MSP targeting peptide targeting peptide;所述靶向蛋白包括RVG-LAMP2B融合蛋白、GE11-LAMP2B融合蛋白、PTP-LAMP2B融合蛋白、TCP-1-LAMP2B融合蛋白、MSP-LAMP2B融合蛋白。The targeting proteins include RVG-LAMP2B fusion protein, GE11-LAMP2B fusion protein, PTP-LAMP2B fusion protein, TCP-1-LAMP2B fusion protein, and MSP-LAMP2B fusion protein.
- 如权利要求4所述的用于治疗帕金森的RNA递送系统,其特征在于,所述RNA序列的长度为15-25个核苷酸。The RNA delivery system for treating Parkinson's according to claim 4, wherein the length of the RNA sequence is 15-25 nucleotides.
- 如权利要求14所述的用于治疗帕金森的RNA递送系统,其特征在于,所述能够治疗帕金森的RNA选自:LRRK2基因的siRNA,或与上述序列同源性大于80%的RNA序列,或编码上述RNA的核酸分子。The RNA delivery system for treating Parkinson's according to claim 14, wherein the RNA capable of treating Parkinson's is selected from the group consisting of: siRNA of LRRK2 gene, or an RNA sequence with more than 80% homology to the above sequence , or a nucleic acid molecule encoding the above RNA.
- 如权利要求15所述的用于治疗帕金森的RNA递送系统,其特征在于,LRRK2基因的siRNA包括AUUAACAUGAAAAUAUCACUU、UUAACAAUAUCAUAUAAUCUU、AUCUUUAAAAUUUGUUAACGC、UUGAUUUAAGAAAAUAGUCUC、UUUGAUAACAGUAUUUUUCUG、其他具有抑制LRRK2基因表达的序列以及与上述序列同源性大于80%的序列。The RNA delivery system for treating Parkinson's according to claim 15, wherein the siRNA of the LRRK2 gene comprises AUUAACAUGAAAAUAUCACUU, UUAACAAUAUCAUAUAAUCUU, AUCUUUAAAAUUUGUUAACGC, UUGAUUUAAGAAAAUAGUCUC, UUUGAUAACAGUAUUUUUCUG, other sequences that inhibit the expression of the LRRK2 gene, and sequences homologous to the above sequences Sequences with sex greater than 80%.
- 如权利要求1所述的用于治疗帕金森的RNA递送系统,其特征在于,所述递送系统为用于包括人在内的哺乳动物中的递送系统。The RNA delivery system for treating Parkinson's of claim 1, wherein the delivery system is a delivery system for use in mammals including humans.
- 一种权利要求1-17任意一项所述的用于治疗帕金森的RNA递送系统在药物中的应用。A use of the RNA delivery system for treating Parkinson's according to any one of claims 1-17 in medicine.
- 如权利要求18所述的应用,其特征在于,所述药物为治疗帕金森及其相关疾病的药物,所述药物的给药方式包括口服、吸入、皮下注射、肌肉注射、静脉注射。The application according to claim 18, wherein the medicine is a medicine for the treatment of Parkinson's and related diseases, and the administration mode of the medicine comprises oral administration, inhalation, subcutaneous injection, intramuscular injection, and intravenous injection.
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| FU ZHENG; ZHANG XIANG; ZHOU XINYAN; UR-REHMAN UZAIR; YU MENGCHAO; LIANG HONGWEI; GUO HONGYUAN; GUO XU; KONG YAN; SU YUANYUAN; YE Y: "In vivo self-assembled small RNAs as a new generation of RNAi therapeutics", CELL RESEARCH, SPRINGER SINGAPORE, SINGAPORE, vol. 31, no. 6, 29 March 2021 (2021-03-29), Singapore , pages 631 - 648, XP037469825, ISSN: 1001-0602, DOI: 10.1038/s41422-021-00491-z * |
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