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鞘蛛科蜘蛛 Cupiennius salei 的多组分毒液:应用不同策略的生物分析研究。

Multicomponent venom of the spider Cupiennius salei: a bioanalytical investigation applying different strategies.

机构信息

Department of Chemistry and Biochemistry, University of Bern, Switzerland.

出版信息

FEBS J. 2012 Aug;279(15):2683-94. doi: 10.1111/j.1742-4658.2012.08650.x. Epub 2012 Jun 18.

DOI:10.1111/j.1742-4658.2012.08650.x
PMID:22672445
Abstract

The multicomponent venom of the spider Cupiennius salei was separated by three different chromatographic strategies to facilitate subsequent analysis of peptidic venom components by tandem mass spectrometry (MALDI-TOF-MS and ESI-MS), Edman degradation and amino acid analysis: (a) desalting of the crude venom by RP-HPLC only, (b) chromatographic separation of the crude venom into 42 fractions by RP-HPLC, and (c) multidimensional purification of the crude venom by size exclusion and cation exchange chromatography and RP-HPLC. A total of 286 components were identified in the venom of C. salei by mass spectrometry and the sequence of 49 new peptides was determined de novo by Edman degradation and tandem mass spectrometry; 30 were C-terminally amidated. The novel peptides were assigned to two main groups: (a) short cationic peptides and (b) Cys-containing peptides with the inhibitor cystine knot motif. Bioinformatics revealed a limited number of substantial similarities, namely with the peptides CpTx1 from the spider Cheiracantium punctorium and U3-ctenitoxin-Asp1a from the South American fishing spider (Ancylometes sp.) and with sequences from a Lycosa singoriensis venom gland transcriptome analysis. The results clearly indicate that the quality of the data is strongly dependent on the chosen separation strategy. The combination of orthogonal analytical methods efficiently excludes alkali ion and matrix adducts, provides indispensable information for an unambiguous identification of isomasses, and results in the most comprehensive repertoire of peptides identified in the venom of C. salei so far.

摘要

蜘蛛 Cupiennius salei 的多组分毒液通过三种不同的色谱策略进行分离,以方便随后通过串联质谱(MALDI-TOF-MS 和 ESI-MS)、Edman 降解和氨基酸分析对肽毒液成分进行分析:(a)仅通过 RP-HPLC 脱盐粗毒液,(b)通过 RP-HPLC 将粗毒液分离成 42 个馏分,(c)通过尺寸排阻和阳离子交换色谱以及 RP-HPLC 对粗毒液进行多维纯化。通过质谱鉴定了 C. salei 毒液中的 286 种成分,并通过 Edman 降解和串联质谱从头确定了 49 种新肽的序列;30 种是 C 末端酰胺化的。这些新肽被分配到两个主要组:(a)短阳离子肽和(b)含半胱氨酸的肽,具有抑制剂半胱氨酸结基序。生物信息学显示,实质性相似性的数量有限,即与蜘蛛 Cheiracantium punctorium 的 CpTx1 肽和南美钓鱼蜘蛛(Ancylometes sp.)的 U3-ctenitoxin-Asp1a 肽以及 Lycosa singoriensis 毒液腺转录组分析的序列有相似性。结果清楚地表明,数据的质量强烈依赖于所选的分离策略。正交分析方法的组合有效地排除了碱离子和基质加合物,为明确鉴定等质量体提供了不可或缺的信息,并产生了迄今为止在 C. salei 毒液中鉴定出的最全面的肽谱。

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