Sequential inactivation of ζ-crystallin by o-phthalaldehyde

Mohammad D. Bazzi, Nayyar Rabbani, Ali S. Duhaiman
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引用次数: 1

Abstract

o-Phthalaldehyde, a bifunctional cross-linking reagent, is commonly used as a probe for the active site of enzymes. In this study, the interaction of o-phthalaldehyde with camel lens ζ-crystallin was examined by activity and fluorescence measurements. Predictably, the oxidoreductase activity of ζ-crystallin was inhibited irreversibly by o-phthalaldehyde in a time- and concentration-dependent manner, and the presence of NADPH with the enzyme appeared to provide a high degree of protection against o-phthalaldehyde inactivation. Interaction of o-phthalaldehyde with ζ-crystallin resulted in formation of isoindole adduct, which exhibited characteristic fluorescence at 415 nm. However, neither inactivation nor modification of the enzyme showed the expected pseudo-first-order kinetics; both events were highly sequential reaching different levels of saturation at different concentrations of o-phthalaldehyde. The modified enzyme had a maximum stoichiometry of 1 mol isoindole/subunit, and bound NADPH to nearly the same extent as unmodified enzyme. Gel filtration experiments suggested that o-phthalaldehyde-modified ζ-crystallin had higher apparent molecular weight than unmodified enzyme, even though the enzyme remained largely monomeric as revealed by electrophoresis on denaturing gel. These results suggested that modification by o-phthalaldehyde might have been so intrusive as to sequentially modify the tetrameric structure of ζ-crystallin.

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邻苯二醛序贯失活ζ-结晶蛋白
邻苯二醛是一种双功能交联试剂,常被用作酶活性位点的探针。本研究通过活性和荧光测定考察了邻苯二醛与骆驼透镜ζ-晶体蛋白的相互作用。可以预见的是,邻苯二醛会以时间和浓度依赖性的方式不可逆地抑制ζ-结晶蛋白的氧化还原酶活性,NADPH的存在似乎对邻苯二醛失活提供了高度的保护。邻苯二醛与ζ-晶蛋白相互作用形成异吲哚加合物,在415 nm处表现出特征荧光。然而,酶的失活和修饰都没有表现出预期的准一级动力学;这两个事件都是高度连续的,在不同浓度的邻苯二醛下达到不同的饱和水平。修饰酶的最大化学计量量为1 mol异吲哚/亚基,与未修饰酶结合NADPH的程度几乎相同。凝胶过滤实验表明,邻苯二醛修饰的ζ-晶体蛋白比未修饰的酶具有更高的表观分子量,尽管变性凝胶电泳显示酶在很大程度上仍是单体。这些结果表明邻苯二醛的修饰可能是侵入性的,从而顺序地修饰了ζ-结晶蛋白的四聚体结构。
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