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三种方法分离和富集低分子量蛋白质用于 SELDI-TOF-MS 差异分析的比较。

Comparison of three methods for fractionation and enrichment of low molecular weight proteins for SELDI-TOF-MS differential analysis.

机构信息

Clinical Chemistry, GIGA Research, University of Liège, CHU, B36, B-4000 Liège 1, Belgium.

出版信息

Talanta. 2010 Jun 30;82(1):245-54. doi: 10.1016/j.talanta.2010.04.029. Epub 2010 Apr 22.

Abstract

In most diseases, the clinical need for serum/plasma markers has never been so crucial, not only for diagnosis, but also for the selection of the most efficient therapies, as well as exclusion of ineffective or toxic treatment. Due to the high sample complexity, prefractionation is essential for exploring the deep proteome and finding specific markers. In this study, three different sample preparation methods (i.e., highly abundant protein precipitation, restricted access materials (RAM) combined with IMAC chromatography and peptide ligand affinity beads) were investigated in order to select the best fractionation step for further differential proteomic experiments focusing on the LMW proteome (MW inferior to 40,000 Da). Indeed, the aim was not to cover the entire plasma/serum proteome, but to enrich potentially interesting tissue leakage proteins. These three methods were evaluated on their reproducibility, on the SELDI-TOF-MS peptide/protein peaks generated after fractionation and on the information supplied. The studied methods appeared to give complementary information and presented good reproducibility (below 20%). Peptide ligand affinity beads were found to provide efficient depletion of HMW proteins and peak enrichment in protein/peptide profiles.

摘要

在大多数疾病中,血清/血浆标志物的临床需求从未如此重要,不仅用于诊断,还用于选择最有效的治疗方法,以及排除无效或有毒的治疗方法。由于样品复杂性高,预分级对于探索深度蛋白质组和寻找特定标志物至关重要。在这项研究中,研究了三种不同的样品制备方法(即高丰度蛋白质沉淀、限制访问材料(RAM)与 IMAC 色谱和肽配体亲和珠相结合),以选择最佳分级步骤,用于进一步进行专注于低分子量蛋白质组(分子量低于 40000Da)的差异蛋白质组学实验。实际上,目标不是涵盖整个血浆/血清蛋白质组,而是富集潜在有趣的组织渗漏蛋白。这三种方法在其重现性、分级后 SELDI-TOF-MS 肽/蛋白质峰的生成以及提供的信息方面进行了评估。研究方法似乎提供了互补的信息,并且具有良好的重现性(低于 20%)。肽配体亲和珠被发现能够有效地去除高分子量蛋白质,并在蛋白质/肽图谱中富集峰。

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