首页> 外文期刊>Journal of bacteriology >Alkylation of acetohydroxyacid synthase I from Escherichia coli K-12 by 3-bromopyruvate: evidence for a single active site catalyzing acetolactate and acetohydroxybutyrate synthesis.
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Alkylation of acetohydroxyacid synthase I from Escherichia coli K-12 by 3-bromopyruvate: evidence for a single active site catalyzing acetolactate and acetohydroxybutyrate synthesis.

机译:通过3-溴吡合金来自大肠杆菌Coli K-12的乙酰羟基酸合酶I的烷基化:用于催化丙酸乙酸酯和乙酰羟基丁酯合成的单一活性位点的证据。

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Acetohydroxyacid synthase I (AHAS I) purified from Escherichia coli K-12 was irreversibly inactivated by incubation with 3-bromopyruvate. Inactivation was specific, insofar as bromoacetate and iodoacetate were much less effective than bromopyruvate. Inactivation was accompanied by incorporation of radioactivity from 3-bromo[2-14C]pyruvate into acid-insoluble material. More than 95% of the incorporated radioactivity coelectrophoresed with the 60-kilodalton IlvB subunit of the enzyme through a sodium dodecyl sulfate-polyacrylamide gel; less than 5% coelectrophoresed with the 11.2-kilodalton IlvN subunit. The stoichiometry of incorporation at nearly complete inactivation was 1 mol of 14C per mol of IlvB polypeptide. These data indicate that bromopyruvate inactivates AHAS I by alkylating an amino acid at or near a single active site located in the IlvB subunit of the enzyme. We confirmed that this alkylation inactivated both AHAS reactions normally catalyzed by AHAS I. These results provide the first direct evidence that AHAS I catalyzes both acetohydroxybutyrate and acetolactate synthesis from the same active site.
机译:通过与3-溴硼酸盐孵育来纯化的丙基羟基酸合酶I(AHAs I)纯化的纯化从大肠杆菌K-12中不可逆转地灭活。灭活是特异性的,只要溴乙酸酯和碘乙酸盐比溴硼酸盐的效果要小得多。灭活伴随着从3-溴[2-14℃]丙酮酸液中的放射性掺入酸不溶性物质中。超过95%的掺入式放射性通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶与酶的60千杆耳顿ILVB亚基相同;小于5%的光电电池与11.2千千尔顿伊尔夫特亚基相同。在几乎完全的灭活时掺入的化学计量是每摩尔ILVB多肽的1摩尔14℃。这些数据表明,溴吡喃化物通过在位于酶的ILVB亚基的单个活性位点处或附近烷基化氨基酸而灭活AHAsi。我们证实,这种烷基化灭活了AHAs I通常催化的AHAS反应。这些结果提供了AHAs I催化来自同一活性位点的乙酰羟基丁酸酯和乙酰酸酯合成的第一种直接证据。

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