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植物中富含半胱氨酸肽的肽组学鉴定

Peptidomic Identification of Cysteine-Rich Peptides from Plants.

作者信息

Hemu Xinya, Serra Aida, Darwis Dina A, Cornvik Tobias, Sze Siu Kwan, Tam James P

机构信息

School of Biological Sciences, Nanyang Technological University, Singapore, Singapore.

出版信息

Methods Mol Biol. 2018;1719:379-393. doi: 10.1007/978-1-4939-7537-2_26.

DOI:10.1007/978-1-4939-7537-2_26
PMID:29476526
Abstract

Plant cysteine-rich peptides (CRPs) constitute a majority of plant-derived peptides with high molecular diversity. This protocol describes a rapid and efficient peptidomic approach to identify a whole spectrum of CRPs in a plant extract and decipher their molecular diversity and bioprocessing mechanism. Cyclotides from C. ternatea are used as the model CRPs to demonstrate our methodology. Cyclotides exist naturally in both cyclic and linear forms, although the linear forms (acyclotide) are generally present at much lower concentrations. Both cyclotides and acyclotides require linearization of their backbone prior to fragmentation and sequencing. A novel and practical three-step chemoenzymatic treatment was developed to linearize and distinguish both forms: (1) N-terminal acetylation that pre-labels the acyclotides; (2) conversion of Cys into pseudo-Lys through aziridine-mediated S-alkylation to reduce disulfide bonds and to increase the net charge of peptides; and (3) opening of cyclic backbones by the novel asparaginyl endopeptidase butelase 2 that cleaves at the native bioprocessing site. The treated peptides are subsequently analyzed by liquid chromatography coupled to mass spectrometry using electron transfer dissociation fragmentation and sequences are identified by matching the MS/MS spectra directly with the transcriptomic database.

摘要

植物富含半胱氨酸的肽(CRPs)构成了具有高分子多样性的大多数植物源肽。本方案描述了一种快速有效的肽组学方法,用于鉴定植物提取物中的全谱CRPs,并解读其分子多样性和生物加工机制。来自蝶豆的环肽用作模型CRPs来证明我们的方法。环肽以环状和线性形式天然存在,尽管线性形式(无环肽)的浓度通常要低得多。环肽和无环肽在片段化和测序之前都需要将其主链线性化。开发了一种新颖且实用的三步化学酶处理方法来线性化和区分这两种形式:(1)N端乙酰化,预先标记无环肽;(2)通过氮丙啶介导的S-烷基化将半胱氨酸转化为假赖氨酸,以减少二硫键并增加肽的净电荷;(3)通过新型天冬酰胺内肽酶butelase 2打开环状主链,该酶在天然生物加工位点进行切割。随后,使用电子转移解离片段化通过液相色谱-质谱联用分析处理后的肽,并通过将MS/MS谱图直接与转录组数据库匹配来鉴定序列。

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