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Comparison of in-gel protein separation techniques commonly used for fractionation in mass spectrometry-based proteomic profiling

机译:凝胶蛋白质分离技术的比较常用于大规模光谱法蛋白质组学分析中的分馏

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摘要

Fractionation of complex samples at the cellular, subcellular, protein or peptide level is an indispensable strategy to improve the sensitivity in mass spectrometry-based proteomic profiling. This study revisits, evaluates, and compares the most common gel-based protein separation techniques i.e., 1-D SDS PAGE, preparative 1-D SDS PAGE, isoelectric focusing in immobilized pH gradients (IEF-IPG), and 2-D PAGE in their performance as fractionation approaches in nanoLC-ESI-MS/MS analysis of a mixture of protein standards and mitochondrial extracts isolated from rat liver. This work demonstrates that all the above techniques provide complementary protein identification results, but 1-D SDS PAGE and IEF-IPG had the highest number of identifications. The IEF-IPG technique resulted in the highest average number of detected peptides per protein. The 2-D PAGE was evaluated as a protein fractionation approach. This work shows that the recovery of proteins and resulting proteolytic digests is highly dependent on the total volume of the gel matrix. The performed comparison of the fractionation techniques demonstrates the potential of a combination of orthogonal 1-D SDS PAGE and IEF-IPG for the improved sensitivity of profiling without significant decrease in throughput.
机译:在细胞,亚细胞,蛋白质或肽水平上对复杂样品进行分级分离是提高基于质谱的蛋白质组学分析灵敏度的必不可少的策略。这项研究回顾,评估和比较了最常见的基于凝胶的蛋白质分离技术,即1-D SDS PAGE,制备型1-D SDS PAGE,固定化pH梯度中的等电聚焦(IEF-IPG)和2-D PAGE。它们在分离蛋白质标准品和从大鼠肝脏中分离的线粒体提取物的混合物的nanoLC-ESI-MS / MS分析中作为分级方法的性能。这项工作证明上述所有技术都可以提供互补的蛋白质鉴定结果,但是1-D SDS PAGE和IEF-IPG的鉴定数量最多。 IEF-IPG技术导致每个蛋白质中检测到的肽段的平均数量最高。二维PAGE被评估为蛋白质分离方法。这项工作表明蛋白质的回收和产生的蛋白水解消化物高度依赖于凝胶基质的总体积。分级技术的比较结果表明,将正交1-D SDS PAGE和IEF-IPG结合使用可提高分析灵敏度,而不会显着降低产量。

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