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[色氨酸在微球菌属n的组氨酸脱羧酶酶活性中的作用]

[Role of tryptophan in the enzymatic activity of histidine decarboxylase from Micrococcus sp. n].

作者信息

Gonchar N A, Grebenshchikova O G, Komarova N V

出版信息

Biokhimiia. 1981 Nov;46(11):1970-80.

PMID:7317525
Abstract

The effect of N-bromosuccinimide (BSI) on micrococcal histidine decarboxylase in 0.07 M phosphate buffer, pH 5.6 was studied. Data from spectral and amino acid analyses suggest that at 20-fold molar excess of BSI three of 12 tryptophane residues undergo selective modification, resulting in 80-85% loss of the enzyme activity. Using fluorescent method and polyacrylamide gel electrophoresis, it was shown that modification of these reactive tryptophane residues does not cause structural changes of the enzyme. Presumably tryptophane residue responsible for enzymatic activity are either located in the enzyme active site of close to it. At 40-50-fold molar excess of BSI 6 to 9 tryptophane and 2 to 3 cysteine residues are subjected to modification; the other 3 tryptophane residues are unaffected by BSI. These are probably located deep inside the histidine decarboxylase molecule. The maximum of the protein fluorescent spectrum during modification of the 40-50-fold molar excess of BSI is shifted towards higher wavelength values, thus suggesting conformational changes of the enzyme. It can be therefore assumed that the enzyme molecule contains at least 2 groups of structurally and catalytically essential tryptophane residues which significantly differ in reactivity. Some diazonium salts were shown to inhibit micrococcal histidine decarboxylase. The kinetics of the inhibiting effect of these compounds were investigated.

摘要

研究了N-溴代琥珀酰亚胺(BSI)在pH 5.6的0.07 M磷酸盐缓冲液中对微球菌组氨酸脱羧酶的影响。光谱和氨基酸分析数据表明,当BSI的摩尔过量为20倍时,12个色氨酸残基中的3个发生选择性修饰,导致酶活性丧失80-85%。使用荧光法和聚丙烯酰胺凝胶电泳表明,这些活性色氨酸残基的修饰不会引起酶的结构变化。推测负责酶活性的色氨酸残基要么位于酶活性位点,要么靠近该位点。当BSI的摩尔过量为40-50倍时,6至9个色氨酸和2至3个半胱氨酸残基会发生修饰;另外3个色氨酸残基不受BSI影响。这些残基可能位于组氨酸脱羧酶分子的深处。在BSI摩尔过量为40-50倍的修饰过程中,蛋白质荧光光谱的最大值向更高波长值移动,从而表明酶的构象发生了变化。因此可以假设,酶分子至少包含2组在结构和催化上必不可少的色氨酸残基,它们在反应性上有显著差异。一些重氮盐被证明可抑制微球菌组氨酸脱羧酶。研究了这些化合物抑制作用的动力学。

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