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使用稳定同位素富集蛋白和直接联用的高效液相色谱-电感耦合等离子体质谱法定量监测金属在蛋白质之间的转移。

Use of stable isotopically enriched proteins and directly coupled high-performance liquid chromatography inductively coupled plasma mass spectrometry for quantitatively monitoring the transfer of metals between proteins.

作者信息

Mason Andrew Z, Moeller Rhonda, Thrippleton Kelly A, Lloyd Douglas

机构信息

Department of Biological Sciences and Institute for Integrated Research in Materials, Environments, and Society, California State University, Long Beach, Long Beach, CA 90840, USA.

出版信息

Anal Biochem. 2007 Oct 1;369(1):87-104. doi: 10.1016/j.ab.2007.06.015. Epub 2007 Jun 15.

DOI:10.1016/j.ab.2007.06.015
PMID:17673155
Abstract

Studies have shown that metallothionein (MT) may play an important role in modulating the activity of certain Zn-regulated enzymes under various oxidoreductive conditions by either donating or removing Zn. To better determine the role of MT in interprotein metal transfer, we describe a procedure that uses stable isotopically enriched (67)Zn(7) metallothionein 2 ((67)Zn(7)-MT-2) to quantitatively determine the stoichiometry of transfer of Zn from the protein to a recipient apo-metalloenzyme, apo-carbonic anhydrase (apo-CA) by directly coupled ion exchange high-performance liquid chromatography inductively coupled plasma mass spectrometry. Quantitatively, the transfer of (67)Zn was consistent with the enzymatic activation of the apo-enzyme as judged by its esterase activity and ability to cleave p-nitrophenyl acetate. Maximum enzyme activation occurred at an MT-2:apo-CA molar ratio of 1, implying the release of a single atom of Zn from MT-2. Preincubation of (67)Zn(7)-MT-2 with an excess of oxidized glutathione (GSSG) increased metal donation fourfold, whereas reduced glutathione (GSH) inhibited donation by approximately 50%. By using multiple recipient and donor proteins having different stable isotopic signatures, the technique has the potential for quantitatively studying the kinetic and thermodynamic aspects of Zn transfer between numerous competing ligands in vitro, an important first step toward understanding the regulatory role of this metal in protein functioning and cellular metabolism in vivo.

摘要

研究表明,金属硫蛋白(MT)可能在各种氧化还原条件下,通过提供或去除锌来调节某些锌调节酶的活性方面发挥重要作用。为了更好地确定MT在蛋白质间金属转移中的作用,我们描述了一种程序,该程序使用稳定同位素富集的(67)Zn(7)金属硫蛋白2((67)Zn(7)-MT-2),通过直接耦合离子交换高效液相色谱-电感耦合等离子体质谱法,定量测定锌从该蛋白质转移到受体脱辅基金属酶——脱辅基碳酸酐酶(apo-CA)的化学计量。从定量角度来看,(67)Zn的转移与脱辅基酶的酶促激活一致,这通过其酯酶活性和切割对硝基苯乙酸的能力来判断。最大酶激活发生在MT-2:apo-CA摩尔比为1时,这意味着从MT-2释放出单个锌原子。(67)Zn(7)-MT-2与过量氧化型谷胱甘肽(GSSG)预孵育使金属提供增加了四倍,而还原型谷胱甘肽(GSH)则抑制提供约50%。通过使用具有不同稳定同位素特征的多种受体和供体蛋白质,该技术有潜力在体外定量研究锌在众多竞争性配体之间转移的动力学和热力学方面,这是理解这种金属在体内蛋白质功能和细胞代谢中调节作用的重要第一步。

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