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一种逆转录病毒作为传递单纯疱疹病毒胸苷激酶基因的真核载体的改造。

Adaptation of a retrovirus as a eucaryotic vector transmitting the herpes simplex virus thymidine kinase gene.

作者信息

Tabin C J, Hoffmann J W, Goff S P, Weinberg R A

出版信息

Mol Cell Biol. 1982 Apr;2(4):426-36. doi: 10.1128/mcb.2.4.426-436.1982.

Abstract

We investigated the feasibility of using retroviruses as vectors for transferring DNA sequences into animal cells. The thymidine kinase (tk) gene of herpes simplex virus was chosen as a convenient model. The internal BamHI fragments of a DNA clone of Moloney leukemia virus (MLV) were replaced with a purified BamHI DNA segment containing the tk gene. Chimeric genomes were created carrying the tk insert in both orientations relative to the MLV sequence. Each was transfected into TK- cells along with MLV helper virus, and TK+ colonies were obtained by selection in the presence of hypoxanthine, aminopterin, and thymidine (HAT). Virus collected from TK+-transformed, MLV producer cells passed the TK+ phenotype to TK- cells. Nonproducer cells were isolated, and TK+ transducing virus was subsequently rescued from them. The chimeric virus showed single-hit kinetics in infections. Virion and cellular RNA and cellular DNA from infected cells were all shown to contain sequences which hybridized to both MLV- and tk-specific probes. The sizes of these sequences were consistent with those predicted for the chimeric virus. In all respects studied, the chimeric MLV-tk virus behaved like known replication-defective retroviruses. These experiments suggest great general applicability of retroviruses as eucaryotic vectors.

摘要

我们研究了使用逆转录病毒作为载体将DNA序列导入动物细胞的可行性。单纯疱疹病毒的胸苷激酶(tk)基因被选作一个便利的模型。莫洛尼白血病病毒(MLV)DNA克隆的内部BamHI片段被含有tk基因的纯化BamHI DNA片段所取代。构建了相对于MLV序列以两种方向携带tk插入片段的嵌合基因组。将每个嵌合基因组与MLV辅助病毒一起转染到TK-细胞中,并通过在次黄嘌呤、氨基蝶呤和胸腺嘧啶(HAT)存在下进行选择获得TK+菌落。从TK+转化的MLV生产细胞收集的病毒将TK+表型传递给TK-细胞。分离出非生产细胞,随后从中拯救出TK+转导病毒。嵌合病毒在感染中表现出单次打击动力学。感染细胞的病毒粒子、细胞RNA和细胞DNA均显示含有与MLV特异性探针和tk特异性探针均杂交的序列。这些序列的大小与嵌合病毒预测的大小一致。在所有研究的方面,嵌合MLV-tk病毒的行为与已知的复制缺陷型逆转录病毒相似。这些实验表明逆转录病毒作为真核载体具有广泛的适用性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9c78/369806/ef54ac66a35d/molcellb00116-0100-a.jpg

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