通过可溶性复制复合物在体外终止腺病毒DNA合成
In vitro termination of adenovirus DNA synthesis by a soluble replication complex.
作者信息
Arens M, Yamashita T
出版信息
J Virol. 1978 Feb;25(2):698-702. doi: 10.1128/JVI.25.2.698-702.1978.
Abstract
The double-stranded DNA from a soluble DNA replication complex that was labeled with deoxyribonucleoside triphosphates and completed in vitro was digested with EcoRI, Sma I, and Hpa I restriction endonucleases. All regions of the adenovirus type 2 genome were labeled in vitro, but restriction fragments derived from the ends of the DNA molecules were relatively more highly labeled than those derived from internal regions. The in vitro endogenous DNA polymerase reaction also exhibited strand-specific labeling near the molecular ends, in that restriciton fragments from the left end were labeled predominantly in the r strand and fragments from the right end were labeled predominantly in the l strand.
摘要
用脱氧核糖核苷三磷酸标记并在体外完成的可溶性DNA复制复合物中的双链DNA,用EcoRI、Sma I和Hpa I限制性内切酶进行消化。2型腺病毒基因组的所有区域在体外均被标记,但源自DNA分子末端的限制性片段比源自内部区域的片段标记程度相对更高。体外内源性DNA聚合酶反应在分子末端附近也表现出链特异性标记,即左端的限制性片段主要在r链上被标记,而右端的片段主要在l链上被标记。
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