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Optimization of a phenol extraction-based protein preparation method amenable to downstream 2DE and MALDI-MS based analysis of bacterial proteomes

机译:适于下游2DE和基于MALDI-MS的细菌蛋白质组分析的基于酚提取的蛋白质制备方法的优化

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摘要

2DE is one of the most efficient and widely used methods for resolving complex protein mixtures. For efficient analysis of complex samples, high-resolution separation of proteins on 2D gel is essential, and for that purpose good sample preparation is crucial. In this study, we have improvized a method for preparing bacterial total cellular proteome, from a strategy applied earlier to recalcitrant plant tissues, which gave high-quality resolution on 2DE. The method involving phenol extraction followed by methanol/ammonium acetate precipitation was first optimized for the chemolithotrophic proteobacteria Tetrathiobacter kashmirensis WT001 and Pseudaminobacter salicylatoxidans KCT001 that did not yield quality protein preps in conventional trichloroacetic acid/acetone precipitation method. Subsequently, to validate its general applicability, the method was evaluated against the trichloroacetic acid/acetone precipitation method for two other model bacteria, i.e. Escherichia coli DH5α and Mycobacterium smegmatis mc26. Identification of at least four proteins each from the outer membrane, periplasm, and cytoplasm of T. kashmirensis by MALDI-MS not only proved the efficiency of the method in extracting proteins from the different cellular compartments but also the amenability of the obtained protein spots toward MALDI-MS based identification.
机译:2DE是解决复杂蛋白质混合物的最有效和广泛使用的方法之一。为了高效地分析复杂的样品,在2D凝胶上高分辨率分离蛋白质至关重要,为此,良好的样品制备至关重要。在这项研究中,我们改进了一种用于制备细菌总细胞蛋白质组的方法,该方法是从较早应用于顽plant植物组织的策略开始的,该策略在2DE上具有高质量的分辨率。首先优化了化学上的营养型变形杆菌克什米尔WT001和水产假单胞菌水杨酸过氧化钾KCT001的方法,其中涉及酚的提取,然后甲醇/乙酸铵沉淀的方法没有传统的三氯乙酸/丙酮沉淀法制备高质量的蛋白质。随后,为了验证其通用性,针对三种其他模式细菌,即大肠杆菌DH5α和耻垢分枝杆菌mc26,针对三氯乙酸/丙酮沉淀法对该方法进行了评估。通过MALDI-MS从克什米尔犬的外膜,周质和细胞质中鉴定出至少四种蛋白质,不仅证明了该方法从不同细胞区室提取蛋白质的效率,而且证明了获得的蛋白质斑点对蛋白质的适应性基于MALDI-MS的识别。

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