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在A1A0-ATP合酶操纵子中具有突变替代的抗三丁基锡嗜热自养甲烷杆菌突变体。

Tributyltin-resistant Methanothermobacter thermautotrophicus mutant with mutational substitutions in the A1A0-ATP synthase operon.

作者信息

Nováková Zuzana, Bobálová Janette, Vidová Monika, Hapala Ivan, Smigán Peter

机构信息

Institute of Animal Biochemistry and Genetics, Slovak Academy of Sciences, Ivanka pri Dunaji, Slovak Republic.

出版信息

FEMS Microbiol Lett. 2009 Sep;298(2):255-9. doi: 10.1111/j.1574-6968.2009.01725.x. Epub 2009 Jul 13.

Abstract

A spontaneous mutant of Methanothermobacter thermautotrophicus resistant to tributyltin chloride (TBT) was isolated. TBT, the inhibitor of the A(0) domain of A(1)A(0)-ATP synthase, inhibits methanogenesis in the wild-type cells; however, the TBT-resistant mutant exhibited methanogenesis even in the presence of 800 microM TBT. ATP synthesis driven by methanogenic electron transport was markedly diminished in the mutant strain. While TBT profoundly inhibited ATP synthesis driven by methanogenic electron transport in the wild type, only a slight inhibition was observed in the mutant strain. These results suggested a modification in the ATP-synthesizing system of the mutant strain. The sequence of the complete A(1)A(0)-ATP synthase operon (Mth952-Mth961) in the wild-type and mutant strains was determined and compared. Three mutations leading to amino acid substitutions in two A(1)A(0)-ATP synthase subunits were identified - Val(338)Ala in subunit A and Leu(252)Ile and Ser(293)Ala in subunit B. Moreover, this study revealed the differential expression of several proteins that may contribute to TBT resistance. The results imply that change of TBT sensitivities of TBT-resistant mutant is due to mutational substitutions in the A(1)A(0)-ATP synthase operon.

摘要

分离出了嗜热自养甲烷杆菌对三丁基氯化锡(TBT)具有抗性的自发突变体。TBT是A₁A₀ - ATP合酶A₀结构域的抑制剂,可抑制野生型细胞中的甲烷生成;然而,耐TBT的突变体即使在存在800微摩尔TBT的情况下仍能进行甲烷生成。在突变菌株中,由产甲烷电子传递驱动的ATP合成显著减少。虽然TBT在野生型中能显著抑制由产甲烷电子传递驱动的ATP合成,但在突变菌株中仅观察到轻微抑制。这些结果表明突变菌株的ATP合成系统发生了改变。测定并比较了野生型和突变菌株中完整的A₁A₀ - ATP合酶操纵子(Mth952 - Mth961)的序列。在两个A₁A₀ - ATP合酶亚基中鉴定出三个导致氨基酸替换的突变——亚基A中的Val(338)Ala以及亚基B中的Leu(252)Ile和Ser(293)Ala。此外,本研究揭示了几种可能有助于TBT抗性的蛋白质的差异表达。结果表明,耐TBT突变体对TBT敏感性的变化是由于A₁A₀ - ATP合酶操纵子中的突变替换所致。

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