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来自牛心线粒体的乙酰辅酶A合成酶的分子量和硫醇残基

The molecular weight and thiol residues of acetyl-coenzyme A synthetase from ox heart mitochondria.

作者信息

Londensborough J C, Yuan S L, Webster L T

出版信息

Biochem J. 1973 May;133(1):23-36. doi: 10.1042/bj1330023.

DOI:10.1042/bj1330023
PMID:4737256
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1177667/
Abstract
  1. A constant molecular weight of 57000 was obtained by gel filtration of highly purified acetyl-CoA synthetase over a 1000-fold range of enzyme concentrations. The amino acid analysis is reported. 2. With native enzyme at 20 degrees C the relatively rapid reaction of four thiol residues with p-hydroxymercuribenzoate caused an immediate inhibition reversible by either CoA or mercaptoethanol. Other substrates did not protect against this rapid inhibition. 3. The much slower reaction of the remaining four thiol residues was independent of the concentration of the mercurial, first-order with respect to enzyme, and had a large energy of activation (+136kJ/mol), suggesting that a conformation change in the protein was rate-limiting. This slow phase of the reaction was accompanied by an irreversible inactivation of the enzyme. 4. The effects of substrates on this irreversible inactivation at pH7.0 in 5 mm-MgCl(2) indicated strong binding of ATP and pyrophosphate by the enzyme (concentrations for half-maximal effects, K((1/2)), were <30mum and <10mum respectively) and weaker binding of acetyl-CoA (K((1/2)) about 1 mm), AMP (K((1/2)) about 2mm) and acetate. In the presence of acetate, MgCl(2) and p-hydroxymercuribenzoate, titration of the enzyme with ATP revealed at least two ATP binding sites/mol. 5. The experiments suggest that reaction of the thiol residues with mercurial causes loss of enzymic activity by altering the structure of the enzyme, rather than that the thiol residues play a direct role in the catalysis.
摘要
  1. 通过在1000倍酶浓度范围内对高度纯化的乙酰辅酶A合成酶进行凝胶过滤,得到了57000的恒定分子量。报告了氨基酸分析结果。2. 在20℃下,天然酶的四个巯基残基与对羟基汞苯甲酸发生相对快速的反应,导致立即抑制,CoA或巯基乙醇可使其逆转。其他底物不能防止这种快速抑制。3. 其余四个巯基残基的反应要慢得多,与汞化合物的浓度无关,对酶呈一级反应,且具有较大的活化能(+136kJ/mol),这表明蛋白质的构象变化是限速步骤。反应的这个缓慢阶段伴随着酶的不可逆失活。4. 在pH7.0、5mm-MgCl₂ 中,底物对这种不可逆失活的影响表明,酶与ATP和焦磷酸有很强的结合(半最大效应浓度K((1/2))分别<30μm和<10μm),与乙酰辅酶A的结合较弱(K((1/2))约为1mm),与AMP(K((1/2))约为2mm)和乙酸的结合更弱。在乙酸、MgCl₂ 和对羟基汞苯甲酸存在的情况下,用ATP滴定酶显示每摩尔至少有两个ATP结合位点。5. 实验表明,巯基残基与汞化合物的反应通过改变酶的结构导致酶活性丧失,而不是巯基残基在催化中起直接作用。

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本文引用的文献

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7
The gel-filtration behaviour of proteins related to their molecular weights over a wide range.蛋白质的凝胶过滤行为与其在很宽范围内的分子量相关。
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