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慢病毒衍生基因转移载体介导的转基因在豚鼠耳蜗中的表达

Transgene expression in the guinea pig cochlea mediated by a lentivirus-derived gene transfer vector.

作者信息

Han J J, Mhatre A N, Wareing M, Pettis R, Gao W Q, Zufferey R N, Trono D, Lalwani A K

机构信息

Department of Otolaryngology--Head and Neck Surgery, University of California San Francisco, 94143, USA.

出版信息

Hum Gene Ther. 1999 Jul 20;10(11):1867-73. doi: 10.1089/10430349950017545.

Abstract

The utility of lentivirus as a gene delivery vector in the cochlea was evaluated in vitro and in vivo. Lentivirus transduction was assessed through expression analysis of a reporter gene, green fluorescent protein (GFP), integrated within the viral genome. In vitro characterization of lentivirus-GFP was assessed by infection of explants from cochleas of neonatal rat. The lentiviral vector transduced both spiral ganglion neurons (SGNs) and glial cells. In vivo characterization of lentivirus-GFP was assessed by directly infusing the vector into the guinea pig cochlea via an osmotic minipump. Sections of lentivirus-infused cochlea revealed a highly restricted fluorescence pattern limited to the periphery of the perilymphatic space. Transduction of SGNs and glial cells by lentivirus in vitro but not in vivo suggests limited dissemination of the viral vector from the perilymphatic space. The cellular and tissue architecture of the lentivirus-infused cochlea was intact and free of inflammation. Restricted transduction of cell types confined to the periphery of the perilymphatic space by the lentivirus is ideal for stable production of gene products secreted into the perilymph.

摘要

在体外和体内评估了慢病毒作为耳蜗基因传递载体的效用。通过对整合在病毒基因组中的报告基因绿色荧光蛋白(GFP)进行表达分析来评估慢病毒转导。通过感染新生大鼠耳蜗的外植体来评估慢病毒-GFP的体外特性。慢病毒载体转导了螺旋神经节神经元(SGN)和神经胶质细胞。通过将载体经渗透微型泵直接注入豚鼠耳蜗来评估慢病毒-GFP的体内特性。注入慢病毒的耳蜗切片显示荧光模式高度局限于外淋巴间隙的周边。慢病毒在体外而非体内转导SGN和神经胶质细胞,这表明病毒载体从外淋巴间隙的扩散有限。注入慢病毒的耳蜗的细胞和组织结构完整且无炎症。慢病毒对外淋巴间隙周边局限的细胞类型进行有限转导,这对于稳定产生分泌到外淋巴中的基因产物而言是理想的。

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