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RmpA2是肺炎克雷伯菌CG43中荚膜生物合成的激活因子,在转录水平上调节K2 cps基因的表达。

RmpA2, an activator of capsule biosynthesis in Klebsiella pneumoniae CG43, regulates K2 cps gene expression at the transcriptional level.

作者信息

Lai Yi-Chyi, Peng Hwei-Ling, Chang Hwan-You

机构信息

Department of Life Science, National Tsing Hua University, 101 Kuan-Fu Road, 2nd Section, Hsin Chu, Taiwan, Republic of China.

出版信息

J Bacteriol. 2003 Feb;185(3):788-800. doi: 10.1128/JB.185.3.788-800.2003.

Abstract

The rmpA2 gene, which encodes an activator for capsular polysaccharide (CPS) synthesis, was isolated from a 200-kb virulence plasmid of Klebsiella pneumoniae CG43. Based on the sequence homology with LuxR at the carboxyl-terminal DNA-binding motif, we hypothesized that RmpA2 exerts its effect by activating the expression of cps genes that are responsible for CPS biosynthesis. Two luxAB transcriptional fusions, each containing a putative promoter region of the K. pneumoniae K2 cps genes, were constructed and were found to be activated in the presence of multicopy rmpA2. The activation is likely due to direct binding of RmpA2 to the cps gene promoter through its C-terminal DNA binding motif. Moreover, the loss of colony mucoidy in a K. pneumoniae strain deficient in RcsB, a regulator for cps gene expression, could be recovered by complementing the strain with a multicopy plasmid carrying rmpA2. The CPS production in Lon protease-deficient K. pneumoniae significantly increased, and the effect was accompanied by an increase of RmpA2 stability. The expression of the rmpA2 gene was negatively autoregulated and could be activated when the organism was grown in M9 minimal medium. An IS3 element located upstream of the rmpA2 was required for the full activation of the rmpA2 promoter. In summary, our results suggest that the enhancement of K2 CPS synthesis in K. pneumoniae CG43 by RmpA2 can be attributed to its transcriptional activation of K2 cps genes, and the expression level of rmpA2 is autoregulated and under the control of Lon protease.

摘要

rmpA2基因编码一种荚膜多糖(CPS)合成激活因子,它是从肺炎克雷伯菌CG43的一个200 kb毒力质粒中分离得到的。基于其羧基末端DNA结合基序与LuxR的序列同源性,我们推测RmpA2通过激活负责CPS生物合成的cps基因的表达来发挥作用。构建了两个luxAB转录融合体,每个融合体都包含肺炎克雷伯菌K2 cps基因的一个假定启动子区域,结果发现它们在多拷贝rmpA2存在时被激活。这种激活可能是由于RmpA2通过其C末端DNA结合基序直接与cps基因启动子结合所致。此外,在一个缺乏RcsB(一种cps基因表达调节因子)的肺炎克雷伯菌菌株中,菌落黏液性的丧失可以通过用携带rmpA2的多拷贝质粒对该菌株进行互补来恢复。Lon蛋白酶缺陷型肺炎克雷伯菌中的CPS产量显著增加,并且这种效应伴随着RmpA2稳定性的增加。rmpA2基因的表达受到负向自我调节,当该生物体在M9基本培养基中生长时可被激活。rmpA2启动子的完全激活需要位于rmpA2上游的一个IS3元件。总之,我们的结果表明,RmpA2对肺炎克雷伯菌CG43中K2 CPS合成的增强作用可归因于其对K2 cps基因的转录激活,并且rmpA2的表达水平受到自我调节且受Lon蛋白酶的控制。

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