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醛还原酶 YqhD 的转录激活及其在大肠杆菌 K-12 中乙二醛代谢中的作用。

Transcriptional activation of the aldehyde reductase YqhD by YqhC and its implication in glyoxal metabolism of Escherichia coli K-12.

机构信息

Department of Biological Sciences, Korea Advanced Institute of Science and Technology, Yuseong-gu, Daejeon, Republic of Korea.

出版信息

J Bacteriol. 2010 Aug;192(16):4205-14. doi: 10.1128/JB.01127-09. Epub 2010 Jun 11.

Abstract

The reactive alpha-oxoaldehydes such as glyoxal (GO) and methylglyoxal (MG) are generated in vivo from sugars through oxidative stress. GO and MG are believed to be removed from cells by glutathione-dependent glyoxalases and other aldehyde reductases. We isolated a number of GO-resistant (GO(r)) mutants from Escherichia coli strain MG1655 on LB plates containing 10 mM GO. By tagging the mutations with the transposon TnphoA-132 and determining their cotransductional linkages, we were able to identify a locus to which most of the GO(r) mutations were mapped. DNA sequencing of the locus revealed that it contains the yqhC gene, which is predicted to encode an AraC-type transcriptional regulator of unknown function. The GO(r) mutations we identified result in missense changes in yqhC and were concentrated in the predicted regulatory domain of the protein, thereby constitutively activating the product of the adjacent gene yqhD. The transcriptional activation of yqhD by wild-type YqhC and its mutant forms was established by an assay with a beta-galactosidase reporter fusion, as well as with real-time quantitative reverse transcription-PCR. We demonstrated that YqhC binds to the promoter region of yqhD and that this binding is abolished by a mutation in the potential target site, which is similar to the consensus sequence of its homolog SoxS. YqhD facilitates the removal of GO through its NADPH-dependent enzymatic reduction activity by converting it to ethadiol via glycolaldehyde, as detected by nuclear magnetic resonance, as well as by spectroscopic measurements. Therefore, we propose that YqhC is a transcriptional activator of YqhD, which acts as an aldehyde reductase with specificity for certain aldehydes, including GO.

摘要

体内通过氧化应激从糖生成反应性α-氧代醛,如乙二醛(GO)和甲基乙二醛(MG)。据信,细胞通过谷胱甘肽依赖的醛糖还原酶和其他醛还原酶从细胞中去除 GO 和 MG。我们从大肠杆菌 MG1655 菌株在含有 10 mM GO 的 LB 平板上分离了许多 GO 抗性(GO(r))突变体。通过将突变标记与转座子 TnphoA-132 并确定它们的共转导联系,我们能够确定大多数 GO(r)突变体映射的基因座。该基因座的 DNA 测序表明它包含 yqhC 基因,该基因预测编码未知功能的 AraC 型转录调节因子。我们鉴定的 GO(r)突变导致 yqhC 中的错义变化,并且集中在蛋白质的预测调节结构域中,从而使相邻基因 yqhD 的产物持续激活。野生型 YqhC 及其突变形式对 yqhD 的转录激活作用通过β-半乳糖苷酶报告融合物测定以及实时定量逆转录-PCR 建立。我们证明 YqhC 与 yqhD 的启动子区域结合,并且该结合通过潜在靶位点的突变而被消除,该潜在靶位点类似于其同源物 SoxS 的共有序列。YqhD 通过其 NADPH 依赖性酶还原活性促进 GO 的去除,通过核磁共振以及光谱测量检测到它将其转化为乙二醛。因此,我们提出 YqhC 是 YqhD 的转录激活剂,其作为具有对某些醛,包括 GO 的特异性的醛还原酶起作用。

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