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通过深度蛋白质组测序进行人类变体和异构体的全球检测。

Global detection of human variants and isoforms by deep proteome sequencing.

机构信息

Computational Systems Biochemistry Research Group, Max Planck Institute of Biochemistry, Martinsried, Germany.

Morgridge Institute for Research, Madison, WI, USA.

出版信息

Nat Biotechnol. 2023 Dec;41(12):1776-1786. doi: 10.1038/s41587-023-01714-x. Epub 2023 Mar 23.

Abstract

An average shotgun proteomics experiment detects approximately 10,000 human proteins from a single sample. However, individual proteins are typically identified by peptide sequences representing a small fraction of their total amino acids. Hence, an average shotgun experiment fails to distinguish different protein variants and isoforms. Deeper proteome sequencing is therefore required for the global discovery of protein isoforms. Using six different human cell lines, six proteases, deep fractionation and three tandem mass spectrometry fragmentation methods, we identify a million unique peptides from 17,717 protein groups, with a median sequence coverage of approximately 80%. Direct comparison with RNA expression data provides evidence for the translation of most nonsynonymous variants. We have also hypothesized that undetected variants likely arise from mutation-induced protein instability. We further observe comparable detection rates for exon-exon junction peptides representing constitutive and alternative splicing events. Our dataset represents a resource for proteoform discovery and provides direct evidence that most frame-preserving alternatively spliced isoforms are translated.

摘要

一项普通的 shotgun 蛋白质组学实验可从单个样本中检测到大约 10000 个人类蛋白质。然而,单个蛋白质通常是通过代表其总氨基酸一小部分的肽序列来鉴定的。因此,平均 shotgun 实验无法区分不同的蛋白质变体和同工型。因此,需要更深入的蛋白质组测序来全面发现蛋白质同工型。使用六种不同的人类细胞系、六种蛋白酶、深度分级和三种串联质谱碎裂方法,我们从 17717 个蛋白质组中鉴定出 100 万个独特肽段,中位数序列覆盖率约为 80%。与 RNA 表达数据的直接比较为大多数非同义变异的翻译提供了证据。我们还假设,未检测到的变异可能是由突变诱导的蛋白质不稳定性引起的。我们还观察到代表组成性和选择性剪接事件的外显子-外显子连接肽的可比检测率。我们的数据集代表了蛋白质变体发现的资源,并提供了直接证据,证明大多数保持框架的选择性剪接同工型都被翻译。

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