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一种在高度多重化平台中富集 N 端蛋白质组的快速、稳健方法。

iNrich, Rapid and Robust Method to Enrich N-Terminal Proteome in a Highly Multiplexed Platform.

机构信息

Center for Theragnosis, Korea Institute of Science and Technology, Seoul 02792, Republic of Korea.

Department of Life Science and Research Institute for Natural Sciences, Hanyang University, Seoul 04763, Republic of Korea.

出版信息

Anal Chem. 2020 May 5;92(9):6462-6469. doi: 10.1021/acs.analchem.9b05653. Epub 2020 Apr 21.

Abstract

The field of terminal proteomics is limited in that it is optimized for large-scale analysis via multistep processes involving liquid chromatography. Here, we present an integrated N-terminal peptide enrichment method (iNrich) that can handle as little as 25 μg of cell lysate via a single-stage encapsulated solid-phase extraction column. iNrich enables simple, rapid, and reproducible sample processing, treatment of a wide range of protein amounts (25 μg ∼ 1 mg), multiplexed parallel sample preparation, and in-stage sample prefractionation using a mixed-anion-exchange filter. We identified ∼5000 N-terminal peptides (Nt-peptides) from only 100 μg of human cell lysate including Nt-formyl peptides. Multiplexed sample preparation facilitated quantitative and robust enrichment of N-terminome with dozens of samples simultaneously. We further developed the method to incorporate isobaric tags such as a tandem mass tag (TMT) and used it to discover novel peptides during ER stress analysis. The iNrich facilitated high-throughput N-terminomics and degradomics at a low cost using commercially available reagents and apparatus, without requiring arduous procedures.

摘要

端肽组学领域受到限制,因为它通过涉及液相色谱的多步过程进行了优化,适用于大规模分析。在这里,我们提出了一种集成的 N 端肽富集方法(iNrich),通过单个阶段的封装固相萃取柱,仅使用 25μg 的细胞裂解物即可处理。iNrich 能够实现简单、快速和可重复的样品处理,处理范围广泛的蛋白量(25μg∼1mg),可进行多重平行样品制备,并可使用混合阴离子交换过滤器在同一阶段进行样品预分级。我们从仅 100μg 的人细胞裂解物中鉴定出了约 5000 个 N 端肽(Nt-肽),包括 Nt 甲酰化肽。多重样品制备促进了 N 端组学的定量和稳健富集,可同时对数十个样品进行富集。我们进一步开发了该方法,将等压标签(如串联质量标签(TMT))整合其中,并在 ER 应激分析过程中使用它来发现新的肽。iNrich 利用市售试剂和仪器以较低的成本实现了高通量的 N 端组学和降解组学,而无需繁琐的程序。

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