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利用DNA-DNA退火技术检测禽肉瘤病毒感染后鸡胚成纤维细胞中新的病毒特异性DNA序列。

Use of DNA-DNA annealing to detect new virus-specific DNA sequences in chicken embryo fibroblasts after infection by avian sarcoma virus.

作者信息

Varmus H E, Heasley S, Bishop J M

出版信息

J Virol. 1974 Oct;14(4):895-903. doi: 10.1128/JVI.14.4.895-903.1974.

Abstract

Labeled, virus-specific DNA synthesized in vitro by the virion-associated polymerase of avian sarcoma virus (ASV) was used to measure virus-specific sequences in cell DNA in three ways: (i) by determining the effect of cell DNA upon the reassociation rate of double-stranded polymerase products; (ii) by measuring the kinetics of annealing of single-stranded polymerase product (cDNA) to cell DNA; or (iii) by measuring the amount of cDNA which anneals to a large excess of cell DNA. With these three assays and modifications of them, we show that fewer than five copies of ASV-specific DNA sequences are present per diploid cell in uninfected chicken embryos; that a two- to several-fold increase in copy number of viral DNA follows infection by ASV; that infection introduces to the cell viral sequences not present before infection; and that DNAs from uninfected Pekin duck and Japanese quail embryos show no homology with DNA synthesized by the ASV polymerase. Some of these results differ from data in a previous report from this laboratory (H. E. Varmus, R. A. Weiss, R. R. Friis, W. Levinson, and J. M. Bishop, 1972) and, in general, reconcile our observations with those from other laboratories.

摘要

用禽肉瘤病毒(ASV)的病毒体相关聚合酶在体外合成的标记病毒特异性DNA,通过三种方式来测量细胞DNA中的病毒特异性序列:(i)通过确定细胞DNA对双链聚合酶产物重新缔合速率的影响;(ii)通过测量单链聚合酶产物(cDNA)与细胞DNA退火的动力学;或(iii)通过测量与大量过量细胞DNA退火的cDNA的量。通过这三种检测方法及其改进,我们发现未感染的鸡胚中二倍体细胞中ASV特异性DNA序列的拷贝数少于五个;ASV感染后病毒DNA的拷贝数增加了两到几倍;感染将感染前不存在的病毒序列引入细胞;并且未感染的北京鸭和日本鹌鹑胚胎的DNA与ASV聚合酶合成的DNA没有同源性。其中一些结果与本实验室先前报告中的数据(H. E. Varmus、R. A. Weiss、R. R. Friis、W. Levinson和J. M. Bishop,1972)不同,总体而言,使我们的观察结果与其他实验室的观察结果相一致。

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