首页> 美国卫生研究院文献>Journal of Bacteriology >Resolution of Holliday junctions in Escherichia coli: identification of the ruvC gene product as a 19-kilodalton protein.
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Resolution of Holliday junctions in Escherichia coli: identification of the ruvC gene product as a 19-kilodalton protein.

机译:大肠杆菌中霍利迪连接的解析:ruvC基因产物鉴定为19-千达通蛋白。

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摘要

The ruvC gene of Escherichia coli specifies a nuclease that resolves Holliday junction intermediates in genetic recombination (B. Connolly, C.A. Parsons, F.E. Benson, H.J. Dunderdale, G.J. Sharples, R.G. Lloyd, and S.C. West, Proc. Natl. Acad, Sci. USA 88:6063-6067, 1991). The gene was located between aspS and the ruvAB operon by DNA sequencing and deletion analysis of ruvC plasmids and was shown to encode a protein of 18,747 Da. Analysis of the DNA flanking ruvC indicated that the gene is transcribed independently of the LexA-regulated ruvAB operon and is not under direct SOS control. ruvC lies downstream of an open reading frame, orf-33, for a protein which migrates during sodium dodecyl sulfate-polyacrylamide gel electrophoresis as a 33-kDa polypeptide. These two genes probably form an operon. However, expression of ruvC was found to be very poor relative to that of orf-33. A double ribosomal frameshift between these genes is proposed as a possible reason for the low level of RuvC. Two further open reading frames of unknown function were identified, one on either side of the orf-33-ruvC operon.
机译:大肠杆菌的ruvC基因指定了一种核酸酶,可解决基因重组中的霍利迪连接中间物(B. Connolly,CA Parsons,FE Benson,HJ Dunderdale,GJ Sharples,RG Lloyd和SC West,Proc。Natl。Acad,Sci。USA) 88:6063-6067,1991)。通过ruvC质粒的DNA测序和缺失分析,该基因位于aspS和ruvAB操纵子之间,并显示编码18,747 Da的蛋白质。对ruvC侧翼DNA的分析表明,该基因的转录独立于LexA调控的ruvAB操纵子,不受SOS的直接控制。 ruvC位于开放阅读框orf-33的下游,该蛋白在十二烷基硫酸钠-聚丙烯酰胺凝胶电泳期间作为33-kDa多肽迁移。这两个基因可能形成操纵子。然而,相对于orf-33,发现ruvC的表达非常差。这些基因之间的双核糖体移码被认为是RuvC水平低的可能原因。确定了另外两个功能未知的开放阅读框,一个位于orf-33-ruvC操纵子的两侧。

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