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色氨酸酶反应的可逆性:由吲哚、丙酮酸和氨合成色氨酸。

Reversibility of the tryptophanase reaction: synthesis of tryptophan from indole, pyruvate, and ammonia.

作者信息

Watanabe T, Snell E E

出版信息

Proc Natl Acad Sci U S A. 1972 May;69(5):1086-90. doi: 10.1073/pnas.69.5.1086.

Abstract

Degradation of tryptophan to indole, pyruvate, and ammonia by tryptophanase (EC 4....) from Escherichia coli, previously thought to be an irreversible reaction, is readily reversible at high concentrations of pyruvate and ammonia. Tryptophan and certain of its analogues, e.g., 5-hydroxytryptophan, can be synthesized by this reaction from pyruvate, ammonia, and indole or an appropriate derivative at maximum velocities approaching those of the degradative reactions. Concentrations of ammonia required for the synthetic reactions produce specific changes in the spectrum of tryptophanase that differ from those produced by K(+) and indicate that ammonia interacts with bound pyridoxal 5'-phosphate to form an imine. Kinetic results indicate that pyruvate is the second substrate bound, hence indole must be the third. These results favor a modified mechanism for the multitude of tryptophanase-catalyzed reactions in which alpha-aminoacrylate, which functions as a common enzyme-bound intermediate in both synthetic and degradative reactions, is not released into the medium during the latter reactions, but is degraded to pyruvate and ammonia by sequential reversible steps via enzyme-bound intermediates.

摘要

先前认为由大肠杆菌色氨酸酶(EC 4....)将色氨酸降解为吲哚、丙酮酸和氨是不可逆反应,但在高浓度丙酮酸和氨的情况下,该反应很容易逆转。色氨酸及其某些类似物,例如5-羟色氨酸,可以通过此反应由丙酮酸、氨和吲哚或适当的衍生物以接近降解反应的最大速度合成。合成反应所需的氨浓度会使色氨酸酶的光谱产生特定变化,这些变化与钾离子产生的变化不同,表明氨与结合的磷酸吡哆醛5'-磷酸相互作用形成亚胺。动力学结果表明丙酮酸是第二个结合的底物,因此吲哚必定是第三个。这些结果支持了一种经修改的机制,用于解释色氨酸酶催化的众多反应,其中α-氨基丙烯酸酯作为合成和降解反应中共同的酶结合中间体,在后一种反应过程中不会释放到介质中,而是通过与酶结合的中间体经连续可逆步骤降解为丙酮酸和氨。

相似文献

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Enzyme synthesis of L-tryptophan.L-色氨酸的酶促合成
Folia Microbiol (Praha). 1990;35(3):200-4. doi: 10.1007/BF02820485.
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Catalytic studies on tryptophanase from Bacillus alvei.对蜂房芽孢杆菌色氨酸酶的催化研究。
J Bacteriol. 1973 Apr;114(1):341-50. doi: 10.1128/jb.114.1.341-350.1973.

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