首页> 外国专利> GENE-THERAPEUTIC DNA-VECTOR BASED ON THE GENE-THERAPEUTIC DNA-VECTOR VTvaf17, CARRYING THE TARGET GENE SELECTED FROM THE GROUP OF GENES COL1A1, COL1A2, BMP2, BMP7, TO INCREASE THE LEVEL OF EXPRESSION OF THESE TARGET GENES, METHOD FOR PRODUCTION AND USE THEREOF, ESCHERICHIA COLI SCS110-AF/VTvaf17-COL1A1 STRAIN OR ESCHERICHIA COLI SCS110-AF/VTvaf17-COL1A2 OR ESCHERICHIA COLI SCS110-AF/VTvaf17-BMP2 OR ESCHERICHIA COLI SCS110-AF/VTvaf17-BMP7, CARRYING A GENE-THERAPEUTIC DNA VECTOR, METHOD FOR PRODUCTION THEREOF, A METHOD FOR INDUSTRIAL PRODUCTION OF A GENE-THERAPEUTIC DNA-VECTOR

GENE-THERAPEUTIC DNA-VECTOR BASED ON THE GENE-THERAPEUTIC DNA-VECTOR VTvaf17, CARRYING THE TARGET GENE SELECTED FROM THE GROUP OF GENES COL1A1, COL1A2, BMP2, BMP7, TO INCREASE THE LEVEL OF EXPRESSION OF THESE TARGET GENES, METHOD FOR PRODUCTION AND USE THEREOF, ESCHERICHIA COLI SCS110-AF/VTvaf17-COL1A1 STRAIN OR ESCHERICHIA COLI SCS110-AF/VTvaf17-COL1A2 OR ESCHERICHIA COLI SCS110-AF/VTvaf17-BMP2 OR ESCHERICHIA COLI SCS110-AF/VTvaf17-BMP7, CARRYING A GENE-THERAPEUTIC DNA VECTOR, METHOD FOR PRODUCTION THEREOF, A METHOD FOR INDUSTRIAL PRODUCTION OF A GENE-THERAPEUTIC DNA-VECTOR

机译：基于基因治疗DNA载体VTvaf17的基因治疗DNA载体，携带选自基因组COL1A1，COL1A2，BMP2，BMP7的靶基因，以增加这些靶基因的表达水平和方法，使用它们，ESCHERICHIA COLI SCS110-AF / VTvaf17-COL1A1菌株或ESCHERICHIA COLI SCS110-AF / VTvaf17-COL1A2或ESCHERICHIA COLI SCS110-AF / VTvaf17-BMP2或ESCHERICHIA COLI SCS110-AF / VTvaf17-BMP7，向量，其生产方法，基因治疗DNA载体的工业生产方法

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FIELD: genetics.;SUBSTANCE: invention relates to genetic engineering. Described is a gene-therapeutic DNA-vector based on a gene-therapeutic DNA-vector VTvaf17, carrying a target gene selected from a group of genes COL1A1, COL1A2, BMP2, BMP7, to increase the level of expression of this target gene in the human body and animals, wherein the gene-therapeutic DNA vector VTvaf17-COL1A1, or VTvaf17-COL1A2, or VTvaf17-BMP2, or VTvaf17-BMP7 has the nucleotide sequence SEQ ID No. 1 or SEQ ID No. 2 or SEQ ID No. 3 or SEQ ID No. 4, respectively. Each of the created genotyping DNA-vectors: VTvaf17-COL1A1, or VTvaf17-COL1A2, or VTvaf17-BMP2, or VTvaf17-BMP7 due to the VTvaf17 vector part limited size, which does not exceed 3,200 base pairs, is capable of efficiently penetrate into cells and to express the target gene cloned therein, selected from the group of COL1A1, COL1A2, BMP2, BMP7 genes. Gene-therapeutic DNA-vector does not contain nucleotide sequences of viral origin and there are no antibiotic resistance genes, providing the possibility of its safe application for genetic therapy of humans and animals. There is also developed a method for obtaining a gene-therapeutic DNA-vector on the basis of gene-therapeutic DNA-vector VTvaf17 carrying the target gene selected from a group of genes: COL1A1, COL1A2, BMP2, BMP7, which consists in that each gene-therapeutic DNA vector: VTvaf17-COL1A1, or VTvaf17-COL1A2, or VTvaf17-BMP2, or VTvaf17-BMP7, are obtained as follows: coding part of the target gene from the group of COL1A1, COL1A2, BMP2, BMP7 genes is cloned into a VTvaf17 DNA-vector and a gene-therapeutic DNA-vector VTvaf17-COL1A1, SEQ ID No. 1 or VTvaf17-COL1A2, SEQ ID No. 2 or VTvaf17-BMP2, SEQ ID No. 3, or VTvaf17-BMP7, SEQ ID No. 4 is obtained, respectively. Method for using the created DNA-vector based on the gene-therapeutic VTvaf17 DNA-vector carrying a target gene selected from a group of genes: COL1A1, COL1A2, BMP2, BMP7, to increase expression level of these target genes consists in introduction of selected gene-therapeutic DNA-vector or several selected gene-therapeutic DNA-vectors into cells, organs and tissues of human or animal, and/or introduction into human and animal organs and tissues of human or animal autologous cells transfected with a selected gene-therapeutic DNA-vector or several selected gene-therapeutic DNA-vectors, or in a combination of said methods. Disclosed is a method of producing Escherichia coli strain SCS110-AF/VTvaf17-COL1A1 or strain Escherichia coli SCS110-AF/VTvaf17-COL1A2, or strain Escherichia coli SCS110-AF/VTvaf17-BMP2, or strain Escherichia coli SCS110-AF/VTvaf17-BMP7 consists in electroporation of competent cells of strain Escherichia coli SCS110-AF with created gene-therapeutic DNA-vector and further selection of stable clones of strain using selective medium. Disclosed is Escherichia coli strain SCS110-AF/VTvaf17-COL1A1, or strain Escherichia coli SCS110-AF/VTvaf17-COL1A2, or strain Escherichia coli SCS110-AFA/Tvaf17-BMP2, or strain Escherichia coli SCS110-AF/VTvaf17-BMP7, carrying a gene-therapeutic DNA-vector for its development with the possibility of culturing the strain without using antibiotics. Method for industrial production of a genotyping DNA-vector consists in scaling a bacterial strain culture to quantities required for growth of bacterial biomass in an industrial fermenter, after which the biomass is used to extract a fraction containing the target DNA product – the gene-therapeutic DNA-vector VTvaf17-COL1A1, or VTvaf17-COL1A2, or VTvaf17-VTvaf17-BMP2, or VTvaf17-BMP7, is multi-step filtered and purified by chromatographic methods.;EFFECT: invention can be used in biotechnology, medicine and agriculture for creation of gene therapy preparations.;14 cl, 14 dwg, 19 ex

机译：技术领域本发明涉及基因工程。描述了基于基因治疗性DNA载体VTvaf17的基因治疗性DNA载体，其携带选自基因组COL1A1，COL1A2，BMP2，BMP7的靶基因，以增加该靶基因在肝癌中的表达水平。其中基因治疗性DNA载体VTvaf17-COL1A1或VTvaf17-COL1A2或VTvaf17-BMP2或VTvaf17-BMP7具有人的核苷酸序列SEQ ID No.1或SEQ ID No.2或SEQ ID No. 3或SEQ ID No.4。每个创建的基因分型DNA载体：VTvaf17-COL1A1或VTvaf17-COL1A2或VTvaf17-BMP2或VTvaf17-BMP7（由于VTvaf17载体部分的大小不超过3200个碱基对）能够有效地渗透细胞并表达克隆到其中的靶基因，所述靶基因选自COL1A1，COL1A2，BMP2，BMP7基因。基因治疗性DNA载体不含病毒来源的核苷酸序列，也没有抗生素抗性基因，为将其安全地用于人类和动物的基因治疗提供了可能性。还开发了一种基于携带有选自以下基因组中的靶标基因的基因治疗性DNA载体VTvaf17的基因治疗性DNA载体的方法，该目标基因选自：COL1A1，COL1A2，BMP2，BMP7。基因治疗性DNA载体：VTvaf17-COL1A1或VTvaf17-COL1A2或VTvaf17-BMP2或VTvaf17-BMP7如下获得：从COL1A1，COL1A2，BMP2，BMP7基因组中克隆目标基因的编码部分插入VTvaf17 DNA载体和基因治疗DNA载体VTvaf17-COL1A1，SEQ ID No.1或VTvaf17-COL1A2，SEQ ID No.2或VTvaf17-BMP2，SEQ ID No.3，或VTvaf17-BMP7，SEQ分别获得ID号4。使用基于携带有选自以下基因组中的靶标基因的基因治疗性VTvaf17 DNA载体的所创建DNA载体的方法，该方法包括：导入选定的基因，以提高这些靶标基因的表达水平。基因治疗性DNA载体或几种选定的基因治疗性DNA载体进入人或动物的细胞，器官和组织，和/或将经选定的基因治疗性转染的人或动物自体细胞引入人和动物的器官和组织DNA载体或几种选择的基因治疗性DNA载体，或上述方法的组合。公开了生产大肠杆菌菌株SCS110-AF / VTvaf17-COL1A1或大肠杆菌SCS110-AF / VTvaf17-COL1A2或大肠杆菌SCS110-AF / VTvaf17-BMP2或大肠杆菌SCS110-AF / VTvaf17的方法BMP7包括用产生的基因治疗性DNA载体对大肠杆菌SCS110-AF感受态细胞进行电穿孔，并使用选择培养基进一步选择稳定的克隆。公开的是大肠杆菌菌株SCS110-AF / VTvaf17-COL1A1，或菌株大肠杆菌SCS110-AF / VTvaf17-COL1A2，或大肠杆菌SCS110-AFA / Tvaf17-BMP2，或大肠杆菌SCS110-AF / VTvaf17-B一种基因治疗性DNA载体，可用于开发，无需使用抗生素即可培养菌株。工业生产基因分型DNA载体的方法包括将细菌菌株培养物按比例缩放至工业发酵罐中细菌生物量生长所需的量，然后使用生物量提取含有目标DNA产物的部分-基因治疗DNA载体VTvaf17-COL1A1或VTvaf17-COL1A2或VTvaf17-VTvaf17-BMP2或VTvaf17-BMP7通过色谱方法进行多步过滤和纯化;效果：发明可用于生物技术，医学和农业领域基因治疗制剂的种类。; 14 cl，14 dwg，19 ex

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公开/公告号RU2707537C1

专利类型
公开/公告日2019-11-27

原文格式PDF
申请/专利权人 CELL AND GENE THERAPY LTD;
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申请/专利号RU20180131708
发明设计人 SAVELIEVA NATALIA (AT);LAZAREV VASILIJ NIKOLAEVICH (RU);SHMARINA GALINA VASILEVNA (RU);
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申请日2018-09-04
分类号C12N15/12;C12N15/53;C12N15/70;A61K48;C12N1/21;C12R1/19;
国家 RU
入库时间 2022-08-21 11:02:49

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