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首页> 外文期刊>Analytical chemistry >Improved Protein Coverage in Bottom-Up Proteomes Analysis Using Fluoroalcohol-Mediated Supramolecular Biphasic Systems With Mixed Amphiphiles for Sample Extraction, Fractionation, and Enrichment
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Improved Protein Coverage in Bottom-Up Proteomes Analysis Using Fluoroalcohol-Mediated Supramolecular Biphasic Systems With Mixed Amphiphiles for Sample Extraction, Fractionation, and Enrichment

机译:利用氟醇介导的超分子双相体系,改善蛋白质覆盖,用于使用含氟醇介导的共分子双相体系,用于样品萃取,分级和富集

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摘要

A new class of supramolecular biphasic systems containing fluoroalcohol-induced coacervates (FAiC) provides concomitant fractionation of complex protein mixtures, high solubilizing power for extraction of various types of proteins, especially those with high hydrophobicity (such as membrane proteins), and enrichment of low-abundance proteins. Subsequently, the use of FAiC biphasic systems (BPS) in the bottom-up proteomics workflow resulted in significantly higher coverage for the whole proteome, various subproteomes, especially those embedded or associated with membranes, post-translationally modified proteins, and low-abundance proteins (LAPs) as compared to the conventional methodologies. In this work, we used a new type of FAiC-BPS composed of mixed amphiphiles, a zwitterionic surfactant 3-(N,N-dimethylmyristyl ammonia) propane sulfonate (DMMAPS), a quaternary ammonium salt (QUATS), and hexafluoroisopropanol (HFIP) as the coacervator for extraction, fractionation, and enrichment of yeast proteome in bottom-up proteomics. The coverage of the lower-abundance proteins (abundance below 2000 molecules/cell) improved by more than 100% using DMMAPS and DMMAPS + QUATS systems as compared to the conventional methods using urea or detergent solutions for protein solubilization. Additionally, these coacervate systems show increased coverage of integral membrane proteins and proteins with alpha-helices by up to 24 and 555%, respectively.
机译:一类新的含氟醇诱导凝聚物(FAiC)的超分子双相体系同时提供复杂蛋白质混合物的分馏、提取各种类型蛋白质的高溶解能力,尤其是那些具有高疏水性的蛋白质(如膜蛋白),以及富集低丰度蛋白质。随后,与传统方法相比,在自下而上的蛋白质组学工作流程中使用FAiC双相系统(BPS)大大提高了整个蛋白质组、各种亚组的覆盖率,尤其是嵌入或与膜相关的亚组、翻译后修饰蛋白质和低丰度蛋白质(LAPs)。在这项工作中,我们使用了一种新型的FAiC BPS,其由混合两亲物、两性离子表面活性剂3-(N,N-二甲基肉豆蔻氨)丙烷磺酸盐(DMMAP)、季铵盐(QUATS)和六氟异丙醇(HFIP)组成,作为自底向上蛋白质组学中酵母蛋白质组的提取、分离和富集的凝聚剂。与使用尿素或洗涤剂溶液溶解蛋白质的传统方法相比,使用DMMAP和DMMAP+QUATS系统的低丰度蛋白质(丰度低于2000个分子/细胞)的覆盖率提高了100%以上。此外,这些凝聚体系显示完整膜蛋白和α螺旋蛋白的覆盖率分别增加了24%和555%。

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