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赤藓红B及相关化合物对乙酰胆碱酯酶的光灭活作用。

Photoinactivation of acetylcholinesterase by erythrosin B and related compounds.

作者信息

Tomlinson G, Cummings M D, Hryshko L

出版信息

Biochem Cell Biol. 1986 Jun;64(6):515-22. doi: 10.1139/o86-072.

DOI:10.1139/o86-072
PMID:3017385
Abstract

Acetylcholinesterase was rapidly inactivated when exposed to light in the presence of xanthene dyes. Photosensitizing efficiency paralleled the dye triplet state quantum yields, increasing in the order fluorescein less than eosin B less than eosin Y less than erythrosin B less than rose bengal. The observed first-order rate constants of photoinactivation increased hyperbolically with dye concentration. Evidence for the formation of a dye-enzyme complex prior to inactivation was obtained from spectrophotometric and protein fluorescence quenching methods. The latter technique allowed estimates of the dye-enzyme dissociation constants for rose bengal (20 microM) and erythrosin B (30 microM). After photoinactivation, a portion of the dye became covalently bound to the enzyme. The photoinactivation reaction occurs in both aerobic (air saturated) and anaerobic (argon saturated) solution, with the rates of photoinactivation being about three to five times greater under the latter conditions. The aerobic reaction exhibits a large deuterium isotope enhancement effect and is largely (but not completely) quenched by 10(-2) M azide. The anaerobic reaction is unaffected by azide and exhibits only a small deuterium isotope effect. These results indicate that the photoinactivation reaction proceeds mainly by a type II (singlet oxygen mediated) pathway under aerobic conditions and by a type I (radical) pathway under anaerobic conditions. The enzyme was protected from inactivation by edrophonium, a competitive inhibitor, but not by d-tubocurarine, a peripheral-site ligand, indicating that destruction of a crucial residue at or near the catalytic site is an important component of the inactivation process. Extensive destruction of tryptophan undoubtedly occurs, at least under aerobic conditions.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在呫吨染料存在的情况下,乙酰胆碱酯酶暴露于光时会迅速失活。光敏效率与染料三线态量子产率平行,按荧光素<曙红B<曙红Y<赤藓红B<孟加拉玫瑰红的顺序增加。观察到的光失活一级速率常数随染料浓度呈双曲线增加。通过分光光度法和蛋白质荧光猝灭法获得了失活前染料 - 酶复合物形成的证据。后一种技术可以估算孟加拉玫瑰红(20 μM)和赤藓红B(30 μM)的染料 - 酶解离常数。光失活后,一部分染料与酶共价结合。光失活反应在需氧(空气饱和)和厌氧(氩气饱和)溶液中均会发生,在后一种条件下光失活速率大约高3至5倍。需氧反应表现出较大的氘同位素增强效应,并且在很大程度上(但不是完全)被10⁻² M叠氮化物猝灭。厌氧反应不受叠氮化物影响,仅表现出较小的氘同位素效应。这些结果表明,在需氧条件下光失活反应主要通过II型(单线态氧介导)途径进行,而在厌氧条件下通过I型(自由基)途径进行。酶受到竞争性抑制剂依酚氯铵的保护而不被失活,但不受外周位点配体d - 筒箭毒碱的保护,这表明催化位点或其附近关键残基的破坏是失活过程的一个重要组成部分。色氨酸无疑会被大量破坏,至少在需氧条件下是这样。(摘要截断于250字)

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