鉴定病毒感染过程中蛋白酶底物的蛋白质组学方法。

2区 医学 Q1 Medicine Advances in Virus Research Pub Date : 2021-01-01 Epub Date: 2021-04-20 DOI:10.1016/bs.aivir.2021.03.003
Xavier Martiáñez-Vendrell, Marjolein Kikkert
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引用次数: 3

摘要

蛋白酶精确且不可逆地催化肽键的水解,调节许多蛋白质的命运、定位和活性。因此,蛋白水解活性在细胞分化和迁移、免疫和炎症反应、细胞凋亡和存活等基本细胞过程中起着重要作用。在病毒感染过程中,宿主蛋白酶参与了从细胞进入到炎症的发生、进展和消退的几个过程。另一方面,许多病毒编码自己的高度特异性蛋白酶,负责病毒蛋白的蛋白水解加工,但与此同时,裂解宿主蛋白以破坏抗病毒宿主反应并调整蛋白质活性以有利于病毒复制。传统上,蛋白酶底物鉴定是通过假设驱动的方法来解决的,但最近蛋白质组学的进展已经提供了一个工具包,可以揭示在感染期间被病毒或宿主蛋白酶切割的宿主蛋白质的广泛库。在这里,我们回顾了目前可用的基于蛋白质组学的方法,这些方法可以并且已经有助于在病毒-宿主相互作用的背景下系统和公正地鉴定新的蛋白酶底物。在病毒感染过程中特定蛋白酶的作用也将被强调。
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Proteomics approaches for the identification of protease substrates during virus infection.

Proteases precisely and irreversibly catalyze the hydrolysis of peptide bonds, regulating the fate, localization, and activity of many proteins. Consequently, proteolytic activity plays an important role in fundamental cellular processes such as differentiation and migration, immunological and inflammatory reactions, apoptosis and survival. During virus infection, host proteases are involved in several processes, from cell entry to initiation, progression and resolution of inflammation. On the other hand, many viruses encode their own highly specific proteases, responsible for the proteolytic processing of viral proteins, but, at the same time, to cleave host proteins to corrupt antiviral host responses and adjust protein activity to favor viral replication. Traditionally, protease substrate identification has been addressed by means of hypothesis-driven approaches, but recent advances in proteomics have made a toolkit available to uncover the extensive repertoire of host proteins cleaved during infection, either by viral or host proteases. Here, we review the currently available proteomics-based methods that can and have contributed to the systematic and unbiased identification of new protease substrates in the context of virus-host interactions. The role of specific proteases during the course of virus infections will also be highlighted.

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来源期刊
CiteScore
7.10
自引率
0.00%
发文量
7
审稿时长
>12 weeks
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