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The regulatory mechanism of 2,4,6-trichlorophenol catabolic operon expression by HadR in Ralstonia pickettii DTP0602

机译:HadR在Pickersi DTP0602中通过HadR调控2,4,6-三氯苯酚代谢操纵子的调控机制

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Ralstonia pickettii DTP0602 utilizes 2,4,6-trichlorophenol (2,4,6-TCP) as its sole source of carbon. The expression of catabolic pathway genes (hadA, hadB and hadC) for 2,4,6-TCP has been reported to be regulated by the LysR-type transcriptional regulator (LTTR) HadR. Generally, coinducers are recognized as being important for the function of LTTRs, and alteration of the LTTR-protection sequence and the degree of DNA bending are characteristic of LTTRs with or without a recognized coinducer. In this study, we describe the mechanism by which HadR regulates the expression of 2,4,6-TCP catabolic genes. The 2,4,6-TCP catabolic pathway genes in DTP0602 consist of two transcriptional units: hadX-hadA-hadB-hadC and monocistronic hadR. Purified HadR binds to the hadX promoter and HadR–DNA complex formation was induced in the presence of 16 types of substituted phenols, including chloro- and nitro-phenols and tribromo-phenol. In contrast with observations of other well-characterized LTTRs, the tested phenols showed no diversity of the bending angle of the HadR binding fragment. The expression of 2,4,6-TCP catabolic pathway genes, which are regulated by HadR, was not influenced by the DNA bending angle of HadR. Moreover, the transcription of hadX, hadA and hadB was induced in the presence of seven types of substituted phenols, whereas the other substituted phenols, which induced formation of the HadR–DNA complex, did not induce the transcription of hadX, hadA or hadB in vivo.
机译:Ralstonia pickettii DTP0602利用2,4,6-三氯苯酚(2,4,6-TCP)作为唯一碳源。据报道,2,4,6-TCP的分解代谢途径基因(hadA,hadB和hadC)的表达受LysR型转录调节子(LTTR)HadR调节。通常,公认的共诱导子对于LTTR的功能很重要,并且在有或没有公认的共诱导子的情况下,LTTR保护序列的改变和DNA弯曲的程度都是LTTR的特征。在这项研究中,我们描述了HadR调节2,4,6-TCP分解代谢基因表达的机制。 DTP0602中的2,4,6-TCP分解代谢途径基因由两个转录单元组成:hadX-hadA-hadB-hadC和单顺反子hadR。纯化的HadR与hadX启动子结合,并在16种取代酚的存在下诱导HadR-DNA复合物的形成,包括氯酚和硝基酚以及三溴酚。与其他表征良好的LTTR的观察结果相反,所测试的酚显示HadR结合片段的弯曲角度没有变化。由HadR调节的2,4,6-TCP分解代谢途径基因的表达不受HadR的DNA弯曲角度的影响。此外,在七种取代酚的存在下诱导了hadX,hadA和hadB的转录,而其他诱导HadR-DNA复合物形成的取代酚却没有诱导hadR-DNA复合体的转录。体内。

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