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凝胶电泳/电洗脱分级器与过滤辅助样品制备相结合,用于深度蛋白质组学分析。

Gel electrophoresis/electroelution sorting fractionator combined with filter-aided sample preparation for deep proteomic analysis.

机构信息

Proteomics Group, System Biology Department, Center for Genetic Engineering and Biotechnology, Havana, Cuba.

China-Cuba Biotechnology Joint Innovation Center (CCBJIC), Yongzhou Zhong Gu Biotechnology, Hunan Province, P. R. China.

出版信息

J Sep Sci. 2022 May;45(10):1784-1796. doi: 10.1002/jssc.202100992. Epub 2022 Apr 21.

DOI:10.1002/jssc.202100992
PMID:35306742
Abstract

Sample preparation and protein fractionation are important issues for proteomic studies. Protein extraction procedures strongly affect the performance of fractionation methods by provoking protein dispersion in several fractions. The most notable exception is the gel-based electrophoretic protein fractionation due to its resolution and effectiveness of sodium dodecyl sulfate as a solubilizing agent, while its main limitation lies in the poor recovery of the gel-trapped proteins. We created a fractionator device to separate complex mixture of proteins and peptides that is based on the continuous gel electrophoresis/electroelution sorting of these molecules. In an unsupervised process, complex mixtures of proteins or peptides are fractionated into the gel while separated fractions are simultaneously and sequentially electroeluted to the solution containing wells. The performance of the device was studied for protein fractionation in terms of reproducibility, protein recovery, and loading capacity. In a setup free of sodium dodecyl sulfate, complex peptide mixtures can also be fractionated. More than 11,700 proteins were identified in the whole-cell lysate of the CaSki cell line by using the fractionator combined with the filter-aided sample preparation method and mass spectrometry analysis. Fractionator-based proteome characterization increased 1.7-fold the number of identified proteins compared to the unfractionated sample analysis.

摘要

样品制备和蛋白质分级分离是蛋白质组学研究中的重要问题。蛋白质提取程序通过将蛋白质分散到几个部分中,强烈影响分级分离方法的性能。凝胶电泳的蛋白质分级分离是最显著的例外,因为其分辨率和十二烷基硫酸钠作为溶解剂的有效性,但其主要限制在于凝胶捕获的蛋白质的回收率差。我们创建了一种分馏器设备,用于分离基于这些分子的连续凝胶电泳/电洗脱排序的复杂蛋白质和肽混合物。在无监督的过程中,复杂的蛋白质或肽混合物在凝胶中被分级分离,而分离的部分则同时并连续地电洗脱到含有孔的溶液中。该设备的性能根据重复性、蛋白质回收率和加载容量来研究蛋白质分级分离。在没有十二烷基硫酸钠的设置中,也可以对复杂的肽混合物进行分级分离。通过使用分馏器结合过滤辅助样品制备方法和质谱分析,在 CaSki 细胞系的全细胞裂解物中鉴定出超过 11700 种蛋白质。与未分级的样品分析相比,基于分馏器的蛋白质组学特征分析增加了 1.7 倍鉴定出的蛋白质数量。

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