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Optimization and Standardization of Thermal Treatment as a Plasma Prefractionation Method for Proteomic Analysis

机译:作为蛋白质组学分析的等离子体预分馏方法的热处理的优化和标准化

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摘要

Prefractionation is a prerequisite step for deep plasma proteomics. Highly abundant proteins, particularly human serum albumin (HSA) and immunoglobulin G (IgG), typically interfere with investigation of proteins with lower abundance. A relatively simple preparation method based on high temperature can precipitate thermolabile proteins, providing a strategic window to access the thermostable plasma subproteome. This study aimed to optimize thermal treatment as a reliable prefractionation method and to compare it with two commercial kits, including HSA and IgG immunodepletion (IMDP) and combinatorial peptide ligand libraries (CPLL), using untreated plasma as a control condition. By varying the temperature and the incubation period, the optimal condition was found as treatment at 95°C for 20 min, which maintained about 1% recovery yield of soluble proteins. Consistency and reproducibility of thermal treatment-derived plasma subproteome were checked by two-dimensional electrophoresis. The coefficient of variation regarding protein spot numbers was less than 10% among three independent specimens. Highly abundant protein depletion of the thermal treatment was evaluated by immunoblotting against HSA and IgG as compared to the untreated plasma, IMDP, and CPLL. Multidimensional comparison based on 489 unique peptides derived from the label-free quantitative mass spectrometry revealed that the thermal treatment, IMDP, and CPLL provided distinct sets of plasma subproteome compared to untreated plasma, and these appeared to be complementary to each other. Comparing the characteristics of the three procedures suggested that thermal treatment was more cost-effective and less time-consuming than IMDP and CPLL. This study proposes the use of thermal treatment as a reliable and cost-effective method for plasma prefractionation which provides benefits to large-scale proteomic projects and biomarker studies.
机译:预分离是深层血浆蛋白质组学的必要步骤。高度丰富的蛋白质,特别是人血清白蛋白(HSA)和免疫球蛋白G(IgG),通常会干扰蛋白质丰度较低的研究。一种基于高温的相对简单的制备方法可以沉淀热不稳定的蛋白质,从而为进入热稳定的血浆亚蛋白质组提供了战略窗口。这项研究旨在优化热处理作为一种可靠的预分离方法,并将其与两种商业试剂盒进行比较,包括HSA和IgG免疫耗竭(IMDP)和组合肽配体库(CPLL),并使用未处理的血浆作为对照条件。通过改变温度和孵育时间,发现最佳条件是在95°C处理20分钟,从而保持了约1%的可溶性蛋白质回收率。通过二维电泳检查源自热处理的血浆亚蛋白质组的一致性和可重复性。在三个独立的样本中,有关蛋白质斑点数量的变异系数小于10%。与未处理的血浆,IMDP和CPLL相比,通过针对HSA和IgG的免疫印迹评估了热处理中高度丰富的蛋白质消耗。基于源自无标记定量质谱的489种独特肽的多维比较显示,与未经处理的血浆相比,热处理,IMDP和CPLL提供了不同的血浆亚蛋白质组集,并且它们看起来是互补的。比较这三个程序的特性,表明热处理比IMDP和CPLL更具成本效益且耗时更少。这项研究提出使用热处理作为血浆预分离的可靠且具有成本效益的方法,这为大规模蛋白质组计划和生物标记研究提供了好处。

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