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迈向肝脏导向的基因治疗:逆转录病毒介导的基因导入人肝细胞。

Towards liver-directed gene therapy: retrovirus-mediated gene transfer into human hepatocytes.

作者信息

Grossman M, Raper S E, Wilson J M

机构信息

Department of Internal Medicine, University of Michigan Medical School, Ann Arbor 48109.

出版信息

Somat Cell Mol Genet. 1991 Nov;17(6):601-7. doi: 10.1007/BF01233625.

Abstract

Liver-directed gene therapy is being considered in the treatment of inherited metabolic diseases. One approach we are considering is the transplantation of autologous hepatocytes that have been genetically modified with recombinant retroviruses ex vivo. We describe, in this report, techniques for isolating human hepatocytes and efficiently transducing recombinant genes into primary cultures. Hepatocytes were isolated from tissue of four different donors, plated in primary culture, and exposed to recombinant retroviruses expressing either the LacZ reporter gene or the cDNA for rabbit LDL receptor. The efficiency of gene transfer under optimal conditions, as determined by Southern blot analysis, varied from a maximum of one proviral copy per cell to a minimum of 0.1 proviral copy per cell. Cytochemical assays were used to detect expression of the recombinant derived proteins, E. coli beta-galactosidase and rabbit LDL receptor. Hepatocytes transduced with the LDL receptor gene expressed levels of receptor protein that exceeded the normal endogenous levels. The ability to isolate and genetically modify human hepatocytes, as described in this report, is an important step towards the development of liver-directed gene therapies in humans.

摘要

肝脏靶向基因治疗正被考虑用于遗传性代谢疾病的治疗。我们正在考虑的一种方法是移植经重组逆转录病毒体外基因改造的自体肝细胞。在本报告中,我们描述了分离人肝细胞并将重组基因有效转导至原代培养细胞的技术。从四个不同供体的组织中分离出肝细胞,接种于原代培养,并用表达LacZ报告基因或兔低密度脂蛋白(LDL)受体cDNA的重组逆转录病毒处理。通过Southern印迹分析确定,在最佳条件下基因转移效率有所不同,最高可达每个细胞一个前病毒拷贝,最低为每个细胞0.1个前病毒拷贝。采用细胞化学分析检测重组衍生蛋白、大肠杆菌β-半乳糖苷酶和兔LDL受体的表达。用LDL受体基因转导的肝细胞所表达的受体蛋白水平超过了正常内源性水平。如本报告所述,分离并对人肝细胞进行基因改造的能力是朝着人类肝脏靶向基因治疗发展迈出的重要一步。

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