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采用毛细管电泳和高压下动力学的综合分析方法,解析调节人对氧磷酶 1(PON1)活性和稳定性的内在和外在辅助因子。

Integrative analytical approach by capillary electrophoresis and kinetics under high pressure optimized for deciphering intrinsic and extrinsic cofactors that modulate activity and stability of human paraoxonase (PON1).

机构信息

Département de Toxicologie, Institut de Recherche Biomédicale des Armées, Antenne La Tronche-CRSSA, BP 87, 38702 La Tronche cedex, France.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2010 May 15;878(17-18):1346-55. doi: 10.1016/j.jchromb.2009.11.027. Epub 2009 Nov 27.

Abstract

Paraoxonase (PON1) is working in vivo in a particular dynamic environment including HDL particles and associated molecules. To decipher the respective and/or concomitant role of the different cofactors involved in this molecular organization, an approach using multiple experimental techniques based on capillary electrophoresis and classical kinetics or kinetics under high pressure was implemented. The effects of calcium and phosphate as protein or plasma cofactor, of human phosphate binding protein (HPBP) as enzyme chaperone, and of a PON1 inhibitor as an active site stabilizer, on the catalytic activities and functional oligomerization of PON1 were scrutinized. PON1 displays two distinct catalytic behaviors, one against esters and lactones, the other against organophosphorus compounds; its functional states and catalytic activities against these substrates are differently modulated by the molecular environment; PON1 exists under several active multimeric forms; the binding of HPBP amends the size of the oligomeric states and exerts a stabilizing effect on the activities of PON1; PON1 functional properties are modulated by HPBP, calcium and phosphate. This integrative approach using several optimized analytical techniques allowed performing comparison of catalytic properties and oligomeric states of functional PON1 in different enzyme preparations. Relevance of these data to understand in vivo physiological PON1 functioning is mandatory.

摘要

对氧磷酶 1(PON1)在包括高密度脂蛋白颗粒和相关分子在内的特定动态环境中发挥作用。为了解析不同辅助因子在这种分子组织中的各自和/或协同作用,采用了基于毛细管电泳和经典动力学或高压下动力学的多种实验技术方法。研究了钙和磷酸盐作为蛋白质或血浆辅助因子、人磷酸盐结合蛋白(HPBP)作为酶伴侣以及 PON1 抑制剂作为活性位点稳定剂对 PON1 的催化活性和功能寡聚化的影响。PON1 显示出两种不同的催化行为,一种针对酯和内酯,另一种针对有机磷化合物;其针对这些底物的功能状态和催化活性受到分子环境的不同调节;PON1 以几种活性多聚体形式存在;HPBP 的结合改变了寡聚体状态的大小,并对 PON1 的活性产生稳定作用;PON1 的功能特性受 HPBP、钙和磷酸盐的调节。这种使用多种优化分析技术的综合方法允许比较不同酶制剂中功能性 PON1 的催化特性和寡聚状态。了解体内生理 PON1 功能的这些数据是必需的。

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