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细小病毒H-1的复制过程。III. 影响H-1 RF DNA合成的因素。

Replication process of the parvovirus H-1. III. Factors affecting H-1 RF DNA synthesis.

作者信息

Rhode S L

出版信息

J Virol. 1974 Oct;14(4):791-801. doi: 10.1128/JVI.14.4.791-801.1974.

Abstract

Replication of the single-stranded DNA parvovirus H-1 involves the synthesis of a double-stranded DNA replicative form (RF). In this study, the metabolism of RF DNA was examined in parasynchronous hamster embryo cells. The initiation of RF DNA replication was found to occur late in S phase, as was the synthesis of the DNA upon which subsequent viral hemagglutinin synthesis is dependent. Evidence is presented which indicates that initiation of RF replication requires proteins synthesized in late S phase, but that concomittant protein synthesis is not required for the continuation of RF replication. The data also suggest a requirement for viral protein(s) for progeny strand synthesis. Incorporation of 5-bromo-2'-deoxyuridine (BUdR) into viral DNA resulted in an "all-or-none" inhibition of viral hemagglutinin and viral antigen synthesis. BUdR inactivation of viral protein function was used to explore the time of synthesis of viral DNA serving as template for viral RNA synthesis and the effect of viral protein on RF replication and progeny strand synthesis. Results of this study suggest that parental RF DNA is synthesized shortly after infection, and that viral mRNA is transcribed from only a few copies of the viral genome in each cell. They also support the conclusion that viral protein is inhibitory to RF DNA replication. Density labeling of RF DNA with BUdR, allowing separation of viral strand DNA (V) from viral complementary strand (C), provided additional data in support of the above findings.

摘要

单链DNA细小病毒H-1的复制涉及双链DNA复制型(RF)的合成。在本研究中,我们检测了同步化仓鼠胚胎细胞中RF DNA的代谢情况。发现RF DNA复制的起始发生在S期晚期,随后病毒血凝素合成所依赖的DNA合成也是如此。有证据表明,RF复制的起始需要在S期晚期合成的蛋白质,但RF复制的持续进行并不需要同时进行蛋白质合成。数据还表明子代链合成需要病毒蛋白。将5-溴-2'-脱氧尿苷(BUdR)掺入病毒DNA会导致病毒血凝素和病毒抗原合成的“全或无”抑制。利用BUdR对病毒蛋白功能的失活作用,来探究作为病毒RNA合成模板的病毒DNA的合成时间,以及病毒蛋白对RF复制和子代链合成的影响。本研究结果表明,亲代RF DNA在感染后不久即被合成,并且每个细胞中只有少数几份病毒基因组转录出病毒mRNA。这些结果还支持了病毒蛋白对RF DNA复制具有抑制作用这一结论。用BUdR对RF DNA进行密度标记,从而能够将病毒链DNA(V)与病毒互补链(C)分离,这为上述发现提供了更多支持数据。

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