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细胞因子TRP-185调节RNA聚合酶II与HIV-1 TAR RNA的结合。

The cellular factor TRP-185 regulates RNA polymerase II binding to HIV-1 TAR RNA.

作者信息

Wu-Baer F, Lane W S, Gaynor R B

机构信息

Department of Internal Medicine, University of Texas Southwestern Medical Center, Dallas 75235-8594, USA.

出版信息

EMBO J. 1995 Dec 1;14(23):5995-6009. doi: 10.1002/j.1460-2075.1995.tb00288.x.

Abstract

Activation of HIV-1 gene expression by the transactivator Tat is dependent on an RNA regulatory element located downstream of the transcription initiation site known as TAR. To characterize cellular factors that bind to TAR RNA and are involved in the regulation of HIV-1 transcription, HeLa nuclear extract was fractionated and RNA gel-retardation analysis was performed. This analysis indicated that only two cellular factors, RNA polymerase II and the previously characterized TAR RNA loop binding protein TRP-185, were capable of binding specifically to TAR RNA. To elucidate the function of TRP-185, it was purified from HeLa nuclear extract, amino acid microsequence analysis was performed and a cDNA encoding TRP-185 was isolated. TRP-185 is a novel protein of 1621 amino acids which contains a leucine zipper and potentially a novel RNA binding motif. In gel-retardation assays, the binding of both recombinant TRP-185 and RNA polymerase II was dependent on the presence of an additional group of proteins designated cellular cofactors. Both the TAR RNA loop and bulge sequences were critical for RNA polymerase II binding, while TRP-185 binding was dependent only on TAR RNA loop sequences. Since binding of TRP-185 and RNA polymerase II to TAR RNA was found to be mutually exclusive, our results suggest that TRP-185 may function either alone or in conjunction with Tat to disengage RNA polymerase II which is stalled upon binding to nascently synthesized TAR RNA during transcriptional elongation.

摘要

反式激活因子Tat对HIV-1基因表达的激活作用依赖于位于转录起始位点下游的一个RNA调控元件,即TAR。为了鉴定与TAR RNA结合并参与HIV-1转录调控的细胞因子,对HeLa细胞核提取物进行了分级分离,并进行了RNA凝胶阻滞分析。该分析表明,只有两种细胞因子,即RNA聚合酶II和先前鉴定的TAR RNA环结合蛋白TRP-185,能够特异性结合TAR RNA。为了阐明TRP-185的功能,从HeLa细胞核提取物中对其进行了纯化,进行了氨基酸微序列分析,并分离出了编码TRP-185的cDNA。TRP-185是一种由1621个氨基酸组成的新型蛋白质,它含有一个亮氨酸拉链和一个潜在的新型RNA结合基序。在凝胶阻滞试验中,重组TRP-185和RNA聚合酶II的结合均依赖于另一组称为细胞辅因子的蛋白质的存在。TAR RNA环和凸起序列对RNA聚合酶II的结合至关重要,而TRP-185的结合仅依赖于TAR RNA环序列。由于发现TRP-185和RNA聚合酶II与TAR RNA的结合是相互排斥的,我们的结果表明,TRP-185可能单独发挥作用,或与Tat协同作用,使在转录延伸过程中与新合成的TAR RNA结合而停滞的RNA聚合酶II解离。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8713/394719/b62fd9a4cbf9/emboj00047-0253-a.jpg

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