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An enzyme system for replication of duplex circular DNA: the replicative form of phage phi X174.

机译:用于复制双链环状DNA的酶系统:噬菌体phi X174的复制形式。

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摘要

Viral single strands (SS) are converted to the duplex from (RF) by a soluble enzyme fraction uninfected Escherichia coli [Schekman et al. (1975) J. Biol. Chem. 250, 5859-5865]. When reactions were supplemented with a soluble enzyme fraction from phi X174-infected cells, replication of phi X174 superhelical RF I DNA was observed. The activity supplied by infected cells was absent in cells treated with chloramphenicol or in cells infected with a phi X174 phage mutant in cistron A (cis A). A host function coded by the rep gene, essential in vivo for RF replication (but not for SS leads to RF), was supplied by enzyme fractions from either infected or uninfected cells. Based on complementation assays, the cisA-dependent and the rep-dependent proteins have each been purified about 1000-fold. The synthetic products of the enzymatic reaction were identified as RF I and RF II in which viral (+) and complementary (-) strands were newly synthesized.
机译:病毒单链(SS)通过未感染的可溶酶部分从大肠杆菌(RF)转化为双链体(Schekman et al。 (1975)生物化学杂志。化学250,5859-5865]。当反应中添加了来自phi X174感染细胞的可溶性酶部分时,观察到phi X174超螺旋RF I DNA的复制。在用氯霉素处理的细胞或在顺反子A(顺式A)中被phi X174噬菌体突变体感染的细胞中,缺少被感染细胞提供的活性。由rep基因编码的宿主功能,在体内是RF复制所必需的(但不是SS导致RF),由感染或未感染细胞的酶部分提供。基于互补分析,已将cisA依赖性蛋白和rep依赖性蛋白各自纯化约1000倍。酶促反应的合成产物被鉴定为RF I和RF II,其中新合成了病毒(+)和互补(-)链。

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