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拟南芥中替代性且有效的蛋白质组学分析

Alternative and effective proteomic analysis in Arabidopsis.

作者信息

Espagne Christelle, Martinez Aude, Valot Benoît, Meinnel Thierry, Giglione Carmela

机构信息

Protein Maturation, Cell Fate and Therapeutics, Institut des Sciences du Végétal UPR2355, Centre National de la Recherche Scientifique, Gif-sur-Yvette, France.

出版信息

Proteomics. 2007 Oct;7(20):3788-99. doi: 10.1002/pmic.200700346.

DOI:10.1002/pmic.200700346
PMID:17828791
Abstract

Various functional genomics platforms are required to define the phenotype associated with a mutant. Global protein analyses may be included in any study. We describe here a rapid method of protein sample preparation and analysis, suitable for all laboratories and using Arabidopsis plantlets as the starting material. This reliable and reproducible method for high yield protein extraction from small amounts of material can be used on even the most recalcitrant tissues. The proteins extracted are suitable for many types of protein analysis, including nondenaturing investigations. This method was validated by a rigorous 2-DE approach, coupled with unambiguous LC-MS/MS identifications featuring strong sequence coverage (average of 26% with eight different peptides/spot protein). The reproducibility of the method was demonstrated by multiple protein identifications from identical series of spots. An interactive map (http://www.isv.cnrsgif.fr/gel2d/), including 435 protein variants showed that (i) 38% of the proteins were yet unreported, (ii) reduced subfractionation, (iii) had frequent protein modifications (average of two spots/protein entry), and (iv) underwent no major proteolytic events other than leader peptide cleavage. Finally, a simple mobility shift method for the large subunit of RuBisCo (LS) in the first dimension made it possible to characterize previously masked protein spots.

摘要

需要各种功能基因组学平台来定义与突变体相关的表型。任何研究都可能包括全局蛋白质分析。我们在此描述一种快速的蛋白质样品制备和分析方法,适用于所有实验室,并以拟南芥幼苗作为起始材料。这种从少量材料中高产提取蛋白质的可靠且可重复的方法,甚至可用于最难处理的组织。提取的蛋白质适用于多种类型的蛋白质分析,包括非变性研究。该方法通过严格的二维电泳(2-DE)方法进行了验证,并结合了具有强序列覆盖率(平均26%,每个斑点蛋白有八个不同肽段)的明确的液相色谱-串联质谱(LC-MS/MS)鉴定。通过对相同系列斑点的多次蛋白质鉴定证明了该方法的可重复性。一个包含435种蛋白质变体的交互式图谱(http://www.isv.cnrsgif.fr/gel2d/)显示:(i)38%的蛋白质尚未被报道;(ii)亚分级减少;(iii)存在频繁的蛋白质修饰(平均每个蛋白质条目有两个斑点);(iv)除了前导肽切割外,没有发生重大的蛋白水解事件。最后,一种用于在第一维中对核酮糖-1,5-二磷酸羧化酶/加氧酶(RuBisCo)大亚基(LS)进行简单迁移率偏移的方法,使得鉴定先前被掩盖的蛋白质斑点成为可能。

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