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细菌4B6三甲胺脱氢酶的纯化及性质

Purification and properties of the trimethylamine dehydrogenase of bacterium 4B6.

作者信息

Colby J, Zatman L J

出版信息

Biochem J. 1974 Dec;143(3):555-67. doi: 10.1042/bj1430555.

Abstract
  1. The trimethylamine dehydrogenase of bacterium 4B6 was purified to homogeneity as judged by analytical polyacrylamide-gel electrophoresis. The specific activity of the purified enzyme is 30-fold higher than that of crude sonic extracts. 2. The molecular weight of the enzyme is 161000. 3. The kinetic properties of the purified enzyme were studied by using an anaerobic spectrophotometric assay method allowing the determination of trimethylamine dehydrogenase activity at pH8.5, the optimum pH. The apparent K(m) for trimethylamine is 2.0+/-0.3mum and the apparent K(m) for the primary hydrogen acceptor, phenazine methosulphate, is 1.25mm. 4. Of 13 hydrogen acceptors tested, only Brilliant Cresyl Blue and Methylene Blue replace phenazine methosulphate. 5. A number of secondary and tertiary amines with N-methyl and/or N-ethyl groups are oxidized by the purified enzyme; primary amines and quaternary ammonium salts are not oxidized. Of the compounds that are oxidized by the purified enzyme, only trimethylamine and ethyldimethylamine support the growth of bacterium 4B6. 6. Trimethylamine dehydrogenase catalyses the anaerobic oxidative N-demethylation of trimethylamine with the formation of stoicheiometric amounts of dimethylamine and formaldehyde. Ethyldimethylamine is also oxidatively N-demethylated yielding ethylmethylamine and formaldehyde; diethylamine is oxidatively N-de-ethylated. 7. The activity of the purified enzyme is unaffected by chelating agents and carbonyl reagents, but is inhibited by some thiol-binding reagents and by Cu(2+), Co(2+), Ni(2+), Ag(+) and Hg(2+). Trimethylamine dehydrogenase activity is potently inhibited by trimethylsulphonium chloride, by tetramethylammonium chloride and other quaternary ammonium salts, and by monoamine oxidase inhibitors of the substituted hydrazine and the non-hydrazine types. 8. Inhibition by the substituted hydrazines is time-dependent, is prevented by the presence of trimethylamine or trimethylamine analogues and in some cases requires the presence of the hydrogen acceptor phenazine methosulphate. The inhibition was irreversible with the four substituted hydrazines that were tested.
摘要
  1. 通过分析聚丙烯酰胺凝胶电泳判断,细菌4B6的三甲胺脱氢酶已纯化至同质。纯化酶的比活性比粗制超声提取物高30倍。2. 该酶的分子量为161000。3. 使用厌氧分光光度测定法研究纯化酶的动力学性质,该方法可在最适pH值8.5下测定三甲胺脱氢酶活性。三甲胺的表观K(m)为2.0±0.3μm,一级氢受体吩嗪硫酸甲酯的表观K(m)为1.25mm。4. 在测试的13种氢受体中,只有灿烂甲酚蓝和亚甲蓝可替代吩嗪硫酸甲酯。5. 许多带有N-甲基和/或N-乙基的仲胺和叔胺可被纯化酶氧化;伯胺和季铵盐不被氧化。在被纯化酶氧化的化合物中,只有三甲胺和乙二甲基胺支持细菌4B6的生长。6. 三甲胺脱氢酶催化三甲胺的厌氧氧化N-去甲基化反应,生成化学计量的二甲胺和甲醛。乙二甲基胺也被氧化N-去甲基化生成乙甲基胺和甲醛;二乙胺被氧化N-去乙基化。7. 纯化酶的活性不受螯合剂和羰基试剂的影响,但受一些巯基结合试剂以及Cu(2+)、Co(2+)、Ni(2+)、Ag(+)和Hg(2+)的抑制。三甲胺脱氢酶活性受到氯化三甲基锍、氯化四甲基铵和其他季铵盐以及取代肼和非肼类型的单胺氧化酶抑制剂的强烈抑制。8. 取代肼的抑制作用具有时间依赖性,可被三甲胺或三甲胺类似物的存在所阻止,在某些情况下需要氢受体吩嗪硫酸甲酯的存在。所测试的四种取代肼的抑制作用是不可逆的。

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