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用于通过酶解羧酶的质谱测量的膜入口。

Membrane inlet for mass spectrometric measurement of catalysis by enzymatic decarboxylases.

机构信息

Department of Chemistry, University of Florida, Gainesville, FL 32610, USA.

出版信息

Anal Biochem. 2011 Nov 1;418(1):73-7. doi: 10.1016/j.ab.2011.06.031. Epub 2011 Jun 30.

Abstract

Membrane inlet mass spectrometry (MIMS) uses diffusion across a permeable membrane to detect in solution uncharged molecules of small molecular weight. We point out here the application of MIMS to determine catalytic properties of decarboxylases using as an example catalysis by oxalate decarboxylase (OxDC) from Bacillus subtilis. The decarboxylase activity generates carbon dioxide and formate from the nonoxidative reaction but is accompanied by a concomitant oxidase activity that consumes oxalate and oxygen and generates CO(2) and hydrogen peroxide. The application of MIMS in measuring catalysis by OxDC involves the real-time and continuous detection of oxygen and product CO(2) from the ion currents of their respective mass peaks. Steady-state catalytic constants for the decarboxylase activity obtained by measuring product CO(2) using MIMS are comparable to those acquired by the traditional endpoint assay based on the coupled reaction with formate dehydrogenase, and measuring consumption of O(2) using MIMS also estimates the oxidase activity. The use of isotope-labeled substrate ((13)C(2)-enriched oxalate) in MIMS provides a method to characterize the catalytic reaction in cell suspensions by detecting the mass peak for product (13)CO(2) (m/z 45), avoiding inaccuracies due to endogenous (12)CO(2).

摘要

膜进样质谱(MIMS)利用扩散穿过可渗透膜来检测溶液中不带电荷的小分子分子量的物质。我们在这里指出,MIMS 可用于确定草酸盐脱羧酶(OxDC)的催化特性,以枯草芽孢杆菌中的 OxDC 为例。脱羧酶活性通过非氧化反应产生二氧化碳和甲酸盐,但伴随着同时发生的氧化酶活性,该活性消耗草酸盐和氧气,并产生二氧化碳和过氧化氢。MIMS 用于测量 OxDC 催化作用的应用涉及实时和连续检测各自质量峰的离子电流中的氧气和产物 CO(2)。使用 MIMS 测量产物 CO(2)获得的脱羧酶活性的稳态催化常数与基于与甲酸脱氢酶偶联反应的传统终点测定法获得的常数相当,并且使用 MIMS 测量 O(2)的消耗也估计了氧化酶活性。MIMS 中使用同位素标记的底物((13)C(2)富集草酸盐)提供了一种通过检测产物(13)CO(2)(m/z 45)的质量峰来表征细胞悬浮液中催化反应的方法,避免了由于内源性(12)CO(2) 而导致的不准确性。

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