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来自三株SV40转化小鼠细胞系的整合病毒DNA的克隆与特性分析

Cloning and characterization of the integrated viral DNA from three lines of SV40-transformed mouse cells.

作者信息

Clayton C E, Rigby P W

出版信息

Cell. 1981 Aug;25(2):547-59. doi: 10.1016/0092-8674(81)90073-8.

Abstract

Recombinant DNA techniques have been used to isolate the integrated viral DNA, together with flanking cellular sequences, from three independently isolated lines of SV40-transformed BALB/c 3T3 cells. We have determined the structures of these cloned segments and their relationships to one another by restriction enzyme mapping, electron microscopic heteroduplex analysis and transfer hybridization experiments. Our data indicate that the structure of the integrated viral DNA is consistent with the idea that integration involves a tandemly repeated intermediate, that extensive amplification and rearrangement of viral and adjacent cellular sequences occurs after integration and that the majority of viral DNA insertions do not contain an intact early transcription unit. The altered templates presumably encode the truncated and super T antigens found in these cells. Either they are interrupted in the middle of the early region, in which case they generally retain the region in which tsA mutations map, or they contain tandem duplications of the tsA region. Further structural analysis will allow the prediction of the precise structures of these unusual T antigens, and the availability of the corresponding templates opens the way to an analysis of the functions of these proteins.

摘要

重组DNA技术已被用于从三个独立分离的SV40转化的BALB/c 3T3细胞系中分离整合的病毒DNA以及侧翼细胞序列。我们通过限制性内切酶图谱分析、电子显微镜异源双链分析和转移杂交实验确定了这些克隆片段的结构及其相互关系。我们的数据表明,整合病毒DNA的结构与以下观点一致:整合涉及串联重复中间体,整合后病毒和相邻细胞序列会发生广泛扩增和重排,并且大多数病毒DNA插入片段不包含完整的早期转录单位。这些改变的模板大概编码了在这些细胞中发现的截短型和超T抗原。它们要么在早期区域中间被打断,在这种情况下,它们通常保留tsA突变所在的区域,要么包含tsA区域的串联重复。进一步的结构分析将有助于预测这些异常T抗原的精确结构,并且相应模板的可得性为分析这些蛋白质的功能开辟了道路。

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