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从感染的HeLa细胞核中分离出的2型腺病毒转录复合物的特性分析。

Characterization of adenovirus type 2 transcriptional complexes isolated from infected HeLa cell nuclei.

作者信息

Wilhelm J, Brison O, Kedinger C, Chambon P

出版信息

J Virol. 1976 Jul;19(1):61-81. doi: 10.1128/JVI.19.1.61-81.1976.

Abstract

HeLa cell nuclei, isolated 17 h after infection with human adenovirus type 2 (Ad2), were treated with 200 mM ammonium sulfate. The extract (S200 fraction) contained 50 to 70% of the nonintegrated Ad2 DNA, which was in the form of nucleoprotein complexes. These complexes contained native, intact Ad2 DNA (with the exception of replicative intermediates) and could be partially purified and resolved by velocity gradient centrifugation. Using high-salt (200 mM ammonium sulfate) incubation conditions, more than 95% of the nuclear RNA polymerase activity belonged to class B. About 45% of the class B enzyme molecules bound to DNA in the nuclei (those "engaged" in RNA synthesis) were released from the nuclei in the form of Ad2 transcriptional complexes by treatment with 200 mM ammonium sulfate. At least 90% of the RNA synthesized in high salt in the nuclei or in the S200 fraction was Ad2 specific, and essentially all of this RNA was complementary to the l strand of Ad2 DNA. These findings are compatible with what is known about Ad2-specific RNA synthesis in vivo. The analysis of the RNA synthesized from partially purified transcriptional complexes supports the contention that its transcription is almost entirely asymmetric, and that the asymmetry observed in vivo is not a consequence of the rapid degradation of h-strand transcripts. The RNA synthesized in vitro in the absence of detectable RNase activity sedimented with a maximum size of 35 to 40S. Less than 5% of the nuclear or the S200 fraction RNA polymerase activity was class C when assayed under non-reinitiating conditions. Although much of the RNA synthesized by the class C enzyme was Ad2 specific, 5.5S virus-associated RNA was not the predominant product. The isolation of Ad2 DNA transcriptional complexes provides an attractive system for further characterizing the Ad2 DNA template used for transcription and for studying the regulation of the expression of the Ad2 genome during the productive infection cycle.

摘要

用人腺病毒2型(Ad2)感染17小时后分离得到的HeLa细胞核,用200 mM硫酸铵处理。提取物(S200组分)含有50%至70%的非整合型Ad2 DNA,其呈核蛋白复合物形式。这些复合物含有天然、完整的Ad2 DNA(复制中间体除外),可通过速度梯度离心进行部分纯化和分离。在高盐(200 mM硫酸铵)孵育条件下,超过95%的核RNA聚合酶活性属于B类。约45%结合于细胞核中DNA(即那些“参与”RNA合成的)的B类酶分子,经200 mM硫酸铵处理后以Ad2转录复合物形式从细胞核中释放出来。在细胞核或S200组分中高盐条件下合成的RNA至少90%是Ad2特异性的,并且基本上所有这些RNA都与Ad2 DNA的l链互补。这些发现与体内已知的Ad2特异性RNA合成情况相符。对部分纯化的转录复合物合成的RNA的分析支持了这样的观点,即其转录几乎完全是不对称的,并且体内观察到的不对称性不是h链转录本快速降解的结果。在无可检测核糖核酸酶活性的体外合成的RNA沉降时最大大小为35至40S。在非重新起始条件下测定时,核或S200组分RNA聚合酶活性中不到5%属于C类。尽管C类酶合成的许多RNA是Ad2特异性的,但5.5S病毒相关RNA不是主要产物。Ad2 DNA转录复合物的分离为进一步表征用于转录的Ad2 DNA模板以及研究生产性感染周期中Ad2基因组表达的调控提供了一个有吸引力的系统。

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