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首页> 美国卫生研究院文献>Journal of Bacteriology >The Escherichia coli lipB Gene Encodes Lipoyl (Octanoyl)-Acyl Carrier Protein:Protein Transferase
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The Escherichia coli lipB Gene Encodes Lipoyl (Octanoyl)-Acyl Carrier Protein:Protein Transferase

机译:大肠杆菌lipB基因编码脂酰(辛酰基)-酰基载体蛋白:蛋白质转移酶

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In an earlier study (S. W. Jordan and J. E. Cronan, Jr., J. Biol. Chem. 272:17903-17906, 1997) we reported a new enzyme, lipoyl-[acyl carrier protein]-protein N-lipoyltransferase, in Escherichia coli and mitochondria that transfers lipoic acid from lipoyl-acyl carrier protein to the lipoyl domains of pyruvate dehydrogenase. It was also shown that E. coli lipB mutants lack this enzyme activity, a finding consistent with lipB being the gene that encoded the lipoyltransferase. However, it remained possible that lipB encoded a positive regulator required for lipoyltransferase expression or action. We now report genetic and biochemical evidence demonstrating that lipB encodes the lipoyltransferase. A lipB temperature-sensitive mutant was shown to produce a thermolabile lipoyltransferase and a tagged version of the lipB-encoded protein was purified to homogeneity and shown to catalyze the transfer of either lipoic acid or octanoic acid from their acyl carrier protein thioesters to the lipoyl domain of pyruvate dehydrogenase. In the course of these experiments the ATG initiation codon commonly assigned to lipB genes in genomic databases was shown to produce a nonfunctional E. coli LipB protein, whereas initiation at an upstream TTG codon gave a stable and enzymatically active protein. Prior genetic results (T. W. Morris, K. E. Reed, and J. E. Cronan, Jr., J. Bacteriol. 177:1-10, 1995) suggested that lipoate protein ligase (LplA) could also utilize (albeit poorly) acyl carrier protein substrates in addition to its normal substrates lipoic acid plus ATP. We have detected a very slow LplA-catalyzed transfer of lipoic acid and octanoic acid from their acyl carrier protein thioesters to the lipoyl domain of pyruvate dehydrogenase. A nonhydrolyzable lipoyl-AMP analogue was found to competitively inhibit both ACP-dependent and ATP-dependent reactions of LplA, suggesting that the same active site catalyzes two chemically diverse reactions.
机译:在较早的研究中(SW Jordan和JE Cronan,Jr.,J. Biol。Chem。272:17903-17906,1997),我们报道了一种新的酶,大肠杆菌中的脂酰-[酰基载体蛋白]-蛋白N-脂酰转移酶线粒体将硫辛酸从脂酰酰基载体蛋白转移到丙酮酸脱氢酶的脂酰结构域。还显示大肠杆菌lipB突变体缺乏这种酶活性,这一发现与lipB是编码脂酰转移酶的基因一致。但是,lipB仍可能编码脂酰转移酶表达或作用所需的正调节剂。现在,我们报告遗传和生物化学证据,证明lipB编码脂酰转移酶。 lipB温度敏感突变体显示产生不耐热的脂酰转移酶,lipB编码蛋白的标记版本被纯化至均质,并显示出催化硫辛酸或辛酸从其酰基载体蛋白硫酯转移至脂酰结构域的能力。丙酮酸脱氢酶。在这些实验过程中,显示​​了通常分配给基因组数据库中lipB基因的ATG起始密码子可产生无功能的大肠杆菌LipB蛋白,而在上游TTG密码子处的起始密码子可产生稳定且具有酶活性的蛋白。先前的遗传结果(TW Morris,KE Reed和JE Cronan,Jr.,J。Bacteriol。177:1-10,1995)表明,脂酸盐蛋白连接酶(LplA)还可以利用(尽管很差)酰基载体蛋白底物到其正常底物硫辛酸加ATP。我们已经检测到硫辛酸和辛酸从其酰基载体蛋白硫酯到丙酮酸脱氢酶的脂酰结构域的LplA催化转移非常缓慢。发现不可水解的脂酰-AMP类似物竞争性抑制LplA的ACP依赖性和ATP依赖性反应,表明相同的活性位点催化两个化学上不同的反应。

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