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霍乱弧菌染色体II复制调控位点的转录失活

Transcriptional inactivation of a regulatory site for replication of Vibrio cholerae chromosome II.

作者信息

Venkova-Canova Tatiana, Srivastava Preeti, Chattoraj Dhruba K

机构信息

Laboratory of Biochemistry, Center for Cancer Research, National Cancer Institute, National Institutes of Health, Bethesda, MD 20892-4260, USA.

出版信息

Proc Natl Acad Sci U S A. 2006 Aug 8;103(32):12051-6. doi: 10.1073/pnas.0605120103. Epub 2006 Jul 27.

Abstract

The bacterium Vibrio cholerae has two chromosomes. The origin of replication of chromosome I is similar to that of Escherichia coli. The origin-containing region of chromosome II (oriCII) resembles replicons of plasmids such as P1, except for the presence of an additional gene, rctA [Egan, E. S. & Waldor, M. K. (2003) Cell 114, 521-530]. The oriCII region that includes the initiator gene, rctB, can function as a plasmid in E. coli. Here we show that RctB suffices for the oriCII-based plasmid replication, and rctA in cis or trans reduces the plasmid copy number, thereby serving as a negative regulator. The inhibitory activity could be overcome by increasing the concentration of RctB, suggesting that rctA titrates the initiator. Purified RctB bound to a DNA fragment carrying rctA, confirming that the two can interact. Although rctA apparently works as a titrating site, it is nonetheless transcribed. We find that the transcription attenuates the inhibitory activity of the gene, presumably by interfering with RctB binding. RctB, in turn, repressed the rctA promoter and, thereby, could control its own titration by modulating the transcription of rctA. This control circuit appears to be a putative novel mechanism for homeostasis of initiator availability.

摘要

霍乱弧菌有两条染色体。染色体I的复制起点与大肠杆菌的相似。染色体II的含起点区域(oriCII)类似于质粒(如P1)的复制子,但存在一个额外的基因rctA [伊根,E.S. & 沃尔多,M.K.(2003年)《细胞》114卷,521 - 530页]。包含起始基因rctB的oriCII区域在大肠杆菌中可作为质粒发挥作用。在此我们表明,RctB足以实现基于oriCII的质粒复制,顺式或反式的rctA会降低质粒拷贝数,从而作为负调控因子。通过增加RctB的浓度可克服这种抑制活性,这表明rctA对起始因子进行了滴定。纯化的RctB与携带rctA的DNA片段结合,证实二者能够相互作用。尽管rctA显然起到滴定位点的作用,但它仍会被转录。我们发现转录会减弱该基因的抑制活性,推测是通过干扰RctB的结合来实现的。反过来,RctB抑制rctA启动子,从而可通过调节rctA的转录来控制自身的滴定。这种控制回路似乎是起始因子可用性稳态的一种假定新机制。

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