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用于肽和蛋白质的元素编码亲和标签。

Element-coded affinity tags for peptides and proteins.

作者信息

Whetstone Paul A, Butlin Nathaniel G, Corneillie Todd M, Meares Claude F

机构信息

Department of Chemistry, University of California, One Shields Avenue, Davis, California 95616, USA.

出版信息

Bioconjug Chem. 2004 Jan-Feb;15(1):3-6. doi: 10.1021/bc034150l.

DOI:10.1021/bc034150l
PMID:14733576
Abstract

Isotope-coded affinity tags (ICAT) represent an important new tool for the analysis of complex mixtures of proteins in living systems [Aebersold, R., and Mann, M. (2003) Nature, 422, 198-207]. We envisage an alternative protein-labeling technique based on tagging with different element-coded metal chelates, which affords affinity chromatography, quantification, and identification of a tagged peptide from a complex mixture. As proof of concept, a synthetic peptide was modified at a cysteine side chain with either a carboxymethyl group or acetamidobenzyl-1,4,7,10-tetraazacyclododecane-N,N',N' ',N' "-tetraacetic acid (AcBD) chelates of terbium or yttrium. A mixture of the three modified peptides in a mole ratio of 100:1.0:0.83 carboxymethyl:AcBD-Tb:AcBD-Y was trypsinized, purified on a new affinity column that binds rare-earth DOTA chelates, and analyzed by LC-MS/MS. Chelate-tagged tryptic peptides eluted cleanly from the affinity column; the tagged peptides chromatographically coeluted during LC-MS analysis, were present in the expected ratio as indicated by MS ion intensity, and were sequence-identified by tandem mass spectrometry. DOTA-rare earth chelates have exceptional properties for use as affinity tags. They are highly polar and water-soluble. Many of the rare earth elements are naturally monoisotopic, providing a variety of simple choices for preparing mass tags. Further, the rare earths are heavy elements, whose mass defects give the masses of tagged peptides exact values not normally shared by molecules that contain only light elements.

摘要

同位素编码亲和标签(ICAT)是分析生物系统中复杂蛋白质混合物的一种重要新工具[Aebersold, R., and Mann, M. (2003) Nature, 422, 198 - 207]。我们设想了一种基于用不同元素编码的金属螯合物进行标记的替代蛋白质标记技术,该技术可实现亲和色谱分析、定量以及从复杂混合物中鉴定标记肽段。作为概念验证,在半胱氨酸侧链上用羧甲基基团或铽或钇的乙酰氨基苄基 - 1,4,7,10 - 四氮杂环十二烷 - N,N',N'',N''' - 四乙酸(AcBD)螯合物对合成肽进行修饰。将三种修饰肽按羧甲基:AcBD - Tb:AcBD - Y的摩尔比为100:1.0:0.83混合后用胰蛋白酶消化,在一种能结合稀土DOTA螯合物的新型亲和柱上进行纯化,并通过LC - MS/MS分析。螯合物标记的胰蛋白酶肽段从亲和柱上干净地洗脱下来;标记肽段在LC - MS分析过程中色谱共洗脱,如MS离子强度所示以预期比例存在,并通过串联质谱进行序列鉴定。DOTA - 稀土螯合物作为亲和标签具有特殊性质。它们具有高极性且水溶性好。许多稀土元素天然为单同位素,为制备质量标签提供了多种简单选择。此外,稀土是重元素,其质量缺陷使标记肽段的质量具有仅含轻元素的分子通常不具备的精确值。

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