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嗜热栖热菌中汞抗性的调控

Regulation of mercury resistance in the crenarchaeote Sulfolobus solfataricus.

作者信息

Schelert James, Drozda Melissa, Dixit Vidula, Dillman Amanda, Blum Paul

机构信息

George Beadle Center for Genetics, University of Nebraska, Lincoln, NE 68588-0666, USA.

出版信息

J Bacteriol. 2006 Oct;188(20):7141-50. doi: 10.1128/JB.00558-06.

Abstract

Mercuric ion, Hg(II), inactivates generalized transcription in the crenarchaeote Sulfolobus solfataricus. Metal challenge simultaneously derepresses transcription of mercuric reductase (merA) by interacting with the archaeal transcription factor aMerR. Northern blot and primer extension analyses identified two additional Hg(II)-inducible S. solfataricus genes, merH and merI (SSO2690), located on either side of merA. Transcription initiating upstream of merH at promoter merHp was metal inducible and extended through merA and merI, producing a merHAI transcript. Northern analysis of a merRA double mutant produced by linear DNA recombination demonstrated merHp promoter activity was dependent on aMerR to overcome Hg(II) transcriptional inhibition. Unexpectedly, in a merA disruption mutant, the merH transcript was transiently induced after an initial period of Hg(II)-mediated transcription inhibition, indicating continued Hg(II) detoxification. Metal challenge experiments using mutants created by markerless exchange verified the identity of the MerR binding site as an inverted repeat (IR) sequence overlapping the transcription factor B binding recognition element of merHp. The interaction of recombinant aMerR with merHp DNA, studied using electrophoretic mobility shift analysis, demonstrated that complex formation was template specific and dependent on the presence of the IR sequence but insensitive to Hg(II) addition and site-specific IR mutations that relieved in vivo merHp repression. Despite containing a motif resembling a distant ArsR homolog, these results indicate aMerR remains continuously DNA bound to protect and coordinate Hg(II)-responsive control over merHAI transcription. The new genetic methods developed in this work will promote experimental studies on S. solfataricus and other Crenarchaeota.

摘要

汞离子Hg(II)可使嗜热栖热菌(Sulfolobus solfataricus)中的通用转录失活。金属刺激通过与古菌转录因子aMerR相互作用,同时解除对汞还原酶(merA)转录的抑制。Northern印迹和引物延伸分析鉴定出另外两个受Hg(II)诱导的嗜热栖热菌基因merH和merI(SSO2690),它们位于merA的两侧。在启动子merHp处,merH上游起始的转录受金属诱导,并延伸通过merA和merI,产生merHAI转录本。通过线性DNA重组产生的merRA双突变体的Northern分析表明,merHp启动子活性依赖于aMerR来克服Hg(II)的转录抑制。出乎意料的是,在merA缺失突变体中,merH转录本在Hg(II)介导的转录抑制初始阶段后被短暂诱导,表明持续进行Hg(II)解毒。使用无标记交换产生的突变体进行的金属刺激实验证实,MerR结合位点的身份是一个反向重复(IR)序列,与merHp的转录因子B结合识别元件重叠。使用电泳迁移率变动分析研究重组aMerR与merHp DNA的相互作用,结果表明复合物的形成具有模板特异性,依赖于IR序列的存在,但对添加Hg(II)和解除体内merHp抑制的位点特异性IR突变不敏感。尽管含有类似于遥远的ArsR同源物的基序,但这些结果表明aMerR一直与DNA结合,以保护并协调对merHAI转录的Hg(II)响应控制。这项工作中开发的新遗传方法将促进对嗜热栖热菌和其他泉古菌的实验研究。

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