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两步离线等电聚焦:先进行蛋白质分级,再进行肽段分级,并应用于人类血浆蛋白质组分析。

Two-stage Off-Gel isoelectric focusing: protein followed by peptide fractionation and application to proteome analysis of human plasma.

作者信息

Heller Manfred, Michel Philippe E, Morier Patrick, Crettaz David, Wenz Christian, Tissot Jean-Daniel, Reymond Frédéric, Rossier Joel S

机构信息

DiagnoSwiss SA, CH-1870 Monthey, Switzerland.

出版信息

Electrophoresis. 2005 Mar;26(6):1174-88. doi: 10.1002/elps.200410106.

Abstract

This paper presents the recently introduced Off-Gel electrophoresis (OGE) technology as a versatile tool to reproducibly fractionate intact proteins and peptides into discrete liquid fractions. The coupling of two stages of OGE, i.e., the separation of intact proteins in a first-stage followed by fractionation of peptides derived from each protein fraction after proteolysis in a second stage, results in an array of 15 x 15 fractions that are directly amenable to additional peptide fractionation like reverse-phase liquid chromatography (RPC). The analysis of all second-stage peptide fractions from only the first-stage protein fraction representing pH 5.0 -5.15 by on-line reverse-phase LC-tandem mass spectrometry resulted in the identification of 53 proteins (337 peptides), of which 10 were on different immunoglobulin (Ig) chains, with an input of only 1.5 mg human blood plasma proteins. Increasing the protein load to approximately 12 mg increased the number of identified proteins in the same protein fraction to 73 proteins (449 peptides), of which 15 were Ig-related. Immunodepletion of six of the most abundant proteins (albumin, transferrin, haptoglobin, IgG, IgA, and alpha-1-antitrypsin) prior to first-stage OGE with an input of 1.5 mg of protein (equivalent to approximately 10 mg nondepleted plasma) resulted in the identification of 81 proteins (660 peptides), of which three were still Ig fragments. The pI-based separation of peptides appears to be nonuniform based on the theoretically determined pI values of identified peptides. This observation specifically accounts for the neutral zone (pI 5-8) and can be accounted for by the physicochemical properties of the peptides given by their amino acid composition. The power of OGE separation of proteins and peptides is discussed with a focus on the use of the knowledge about the pI of proteins and peptides that assist the validation of correct identifications together with the retention time of peptides on RPC.

摘要

本文介绍了最近引入的离胶电泳(OGE)技术,它是一种通用工具,可将完整蛋白质和肽可重复地分离成离散的液体馏分。两个阶段的OGE联用,即在第一阶段分离完整蛋白质,然后在第二阶段对每个蛋白质馏分经蛋白酶解后得到的肽进行分级分离,产生了一系列15×15的馏分,这些馏分可直接用于如反相液相色谱(RPC)等额外的肽分级分离。仅对代表pH 5.0 - 5.15的第一阶段蛋白质馏分的所有第二阶段肽馏分进行在线反相LC-串联质谱分析,仅输入1.5 mg人血浆蛋白,就鉴定出了53种蛋白质(337个肽),其中10种在不同的免疫球蛋白(Ig)链上。将蛋白质上样量增加到约12 mg,同一蛋白质馏分中鉴定出的蛋白质数量增加到73种(449个肽),其中15种与Ig相关。在第一阶段OGE之前对六种最丰富的蛋白质(白蛋白、转铁蛋白、触珠蛋白、IgG、IgA和α-1-抗胰蛋白酶)进行免疫去除,输入1.5 mg蛋白质(相当于约10 mg未去除血浆),鉴定出81种蛋白质(660个肽),其中三种仍是Ig片段。基于肽的pI值进行的分离似乎并不均匀,这是根据鉴定出的肽的理论计算pI值得出的。这一观察结果特别适用于中性区(pI 5 - 8),可以用肽由其氨基酸组成所赋予的物理化学性质来解释。本文讨论了OGE分离蛋白质和肽的能力,重点是利用有关蛋白质和肽pI的知识,这有助于验证正确的鉴定结果以及肽在RPC上的保留时间。

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