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J Bacteriol. 1997 Mar;179(5):1755-63. doi: 10.1128/jb.179.5.1755-1763.1997.
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本文引用的文献

1
Transcription factor recognition surface on the RNA polymerase alpha subunit is involved in contact with the DNA enhancer element.RNA聚合酶α亚基上的转录因子识别表面参与与DNA增强子元件的接触。
EMBO J. 1996 Aug 15;15(16):4358-67.
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Phosphorylation-dependent binding of BvgA to the upstream region of the cyaA gene of Bordetella pertussis.百日咳博德特氏菌BvgA与cyaA基因上游区域的磷酸化依赖性结合
Mol Microbiol. 1996 May;20(3):489-96. doi: 10.1046/j.1365-2958.1996.5231057.x.
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Phosphorylated BvgA is sufficient for transcriptional activation of virulence-regulated genes in Bordetella pertussis.磷酸化的BvgA足以激活百日咳博德特氏菌中毒力调节基因的转录。
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Lrp, a major regulatory protein in Escherichia coli, bends DNA and can organize the assembly of a higher-order nucleoprotein structure.Lrp是大肠杆菌中的一种主要调节蛋白,它能使DNA弯曲,并能组织高阶核蛋白结构的组装。
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Involvement of the RNA polymerase alpha subunit C-terminal region in co-operative interaction and transcriptional activation with OxyR protein.RNA聚合酶α亚基C末端区域参与与OxyR蛋白的协同相互作用和转录激活。
Mol Microbiol. 1993 Mar;7(6):859-64. doi: 10.1111/j.1365-2958.1993.tb01176.x.
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Protein-protein communication within the transcription apparatus.转录装置内的蛋白质-蛋白质通讯。
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Transcriptional regulation by cAMP and its receptor protein.环磷酸腺苷(cAMP)及其受体蛋白的转录调控
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Autophosphorylation and phosphotransfer in the Bordetella pertussis BvgAS signal transduction cascade.百日咳博德特氏菌BvgAS信号转导级联中的自磷酸化和磷酸转移
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A third recognition element in bacterial promoters: DNA binding by the alpha subunit of RNA polymerase.细菌启动子中的第三种识别元件:RNA聚合酶α亚基与DNA的结合。
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DNA recognition by beta-sheets in the Arc repressor-operator crystal structure.Arc阻遏蛋白-操纵基因晶体结构中β折叠对DNA的识别
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百日咳博德特氏菌BvgA转录激活因子在fha启动子处与DNA的结合性质及与RNA聚合酶的相互作用

Nature of DNA binding and RNA polymerase interaction of the Bordetella pertussis BvgA transcriptional activator at the fha promoter.

作者信息

Boucher P E, Murakami K, Ishihama A, Stibitz S

机构信息

Division of Bacterial Products, Center for Biologics Evaluation and Research, Food and Drug Administration, Bethesda, Maryland 20892, USA.

出版信息

J Bacteriol. 1997 Mar;179(5):1755-63. doi: 10.1128/jb.179.5.1755-1763.1997.

DOI:10.1128/jb.179.5.1755-1763.1997
PMID:9045838
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC178891/
Abstract

The expression of virulence factor genes in Bordetella pertussis is mediated by the BvgA-BvgS two-component signal transduction system. The response regulator, BvgA, acts directly as a transcriptional activator at the loci encoding pertussis toxin (ptx) and filamentous hemagglutinin (fha). Previous studies have demonstrated that these two loci are differentially regulated by BvgA. As an initial step in gaining insight into the mechanism underlying this differential regulation, we initiated DNA binding and in vitro transcription analyses to examine the activities of BvgA and RNA polymerase (RNAP) purified from both B. pertussis and Escherichia coli at the fha promoter. We discovered that unphosphorylated BvgA binds to a single region (-100 to -70, relative to the start of transcription), whereas phosphorylated BvgA binds both this region and another, farther downstream, that extends to the -35 nucleotide. In the absence of BvgA, RNAP binds a region farther upstream than expected (-104 to -35). However, occupation of both sites by BvgA phosphate repositions RNAP to the site used in vivo. The binding of BvgA phosphate to the downstream site correlates with in vitro transcriptional activity at the fha promoter. As the DNA binding and transcription activities of the E. coli-derived RNAP are similar to those observed for the B. pertussis enzyme, we employed several mutant E. coli proteins in in vitro transcription analyses. We observed that polymerases carrying either a deletion of the C-terminal domain of the alpha subunit or substitution of alanine at either of two critical residues within this domain were severely impaired in the ability to mediate BvgA-activated transcription at fha.

摘要

百日咳博德特氏菌毒力因子基因的表达由BvgA - BvgS双组分信号转导系统介导。应答调节因子BvgA直接作为编码百日咳毒素(ptx)和丝状血凝素(fha)基因座的转录激活因子。先前的研究表明,这两个基因座受BvgA的差异调节。作为深入了解这种差异调节机制的第一步,我们启动了DNA结合和体外转录分析,以检测从百日咳博德特氏菌和大肠杆菌中纯化的BvgA和RNA聚合酶(RNAP)在fha启动子处的活性。我们发现未磷酸化的BvgA结合到单个区域(相对于转录起始点为-100至-70),而磷酸化的BvgA则结合该区域以及另一个更下游的区域,该区域延伸至-35核苷酸。在没有BvgA的情况下,RNAP结合到比预期更远的上游区域(-104至-35)。然而,BvgA磷酸化占据这两个位点会使RNAP重新定位到体内使用的位点。BvgA磷酸化与fha启动子处的体外转录活性相关。由于大肠杆菌来源的RNAP的DNA结合和转录活性与百日咳博德特氏菌酶观察到的活性相似,我们在体外转录分析中使用了几种突变的大肠杆菌蛋白。我们观察到,携带α亚基C末端结构域缺失或该结构域内两个关键残基之一被丙氨酸取代的聚合酶,在介导fha处BvgA激活的转录能力上严重受损。