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系统且定量的消化效率和特异性比较揭示了胰蛋白酶质量对基于 MS 的蛋白质组学的影响。

Systematic and quantitative comparison of digest efficiency and specificity reveals the impact of trypsin quality on MS-based proteomics.

机构信息

Leibniz-Institut für Analytische Wissenschaften - ISAS - e.V., Dortmund, Germany.

出版信息

J Proteomics. 2012 Feb 2;75(4):1454-62. doi: 10.1016/j.jprot.2011.11.016. Epub 2011 Nov 30.

Abstract

Trypsin is the most frequently used proteolytic enzyme in mass spectrometry-based proteomics. Beside its good availability, it also offers some major advantages such as an optimal average peptide length of ~14 amino acids, and typically the presence of at least two defined positive charges at the N-terminus as well as the C-terminal Arg/Lys, rendering tryptic peptides well suited for CID-based LC-MS/MS. Here, we conducted a systematic study of different types of commercially available trypsin in order to qualitatively and quantitatively compare cleavage specificity, efficiency as well as reproducibility and the potential impact on quantitation and proteome coverage. We present a straightforward strategy applied to complex digests of human platelets, comprising (1) digest controls using a monolithic column HPLC-setup, (2) SCX enrichment of semitryptic/nonspecific peptides, (3) targeted MRM analysis of corresponding full cleavage/missed cleavage peptide pairs as well as (4) LC-MS analyses of complete digests with a three-step data interpretation. Thus, differences in digest performance can be readily assessed, rendering these procedures extremely beneficial to quality control not only the trypsin of choice, but also to effectively compare as well as optimize different digestion conditions and to evaluate the reproducibility of a dedicated digest protocol for all kinds of quantitative proteome studies.

摘要

胰蛋白酶是基于质谱的蛋白质组学中最常用的蛋白水解酶。除了良好的可用性外,它还具有一些主要优势,例如平均肽长度约为 14 个氨基酸,通常在 N 末端和 C 末端 Arg/Lys 处具有至少两个定义的正电荷,使得胰蛋白酶肽非常适合基于 CID 的 LC-MS/MS。在这里,我们对不同类型的商业可得的胰蛋白酶进行了系统研究,以便定性和定量比较切割特异性、效率以及重现性,以及对定量和蛋白质组覆盖度的潜在影响。我们提出了一种直接应用于人血小板复杂消化物的策略,包括 (1) 使用整体柱 HPLC 装置进行消化对照,(2) SCX 对半切割/非特异性肽的富集,(3) 对相应的全切割/缺失切割肽对进行靶向 MRM 分析,以及 (4) 对完整消化物进行 LC-MS 分析,通过三步数据解释。因此,可以轻松评估消化性能的差异,这些程序不仅对选择的胰蛋白酶的质量控制非常有益,而且还可以有效地比较和优化不同的消化条件,并评估专用消化方案的重现性,用于各种定量蛋白质组学研究。

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