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Integrated Sample Preparation Methodology for Proteomics: Analysis of Native Proteins

机译:蛋白质组学的综合样品制备方法:天然蛋白质分析

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An innovative sample preparation strategy is reported for protein identification in complex mixtures based on integration of affinity chromatographic selection and accelerated trypsin digestion using a continuous flow immobilized enzyme reactor (cf-IMER). Affinity selected glycoproteins were released to a cf-IMER column which converted native proteins to peptides in 5 min at elevated temperature. Digestion with the cf-IMER was compared to the traditional 16 h solution-based trypsin digestion of reduced and alkylated proteins. With immobilized antibody selection of Lewis x (Le~x) glycan bearing glycoproteins from plasma, 66 proteins were identified in total with the two methods while approximately 1/3 of the total proteins and peptides were only observed with the cf-IMER. This suggests that proteomics based on protein identification by reduction and alkylation with solution-based trypsin digestion alone may not be identifying large numbers of proteins or peptides present at detectable levels in samples. Furthermore, except for proteins containing a high content of disulfide bonds, the majority of proteins did not require reduction and alkylation steps for their identification. The validity of the proposed proteolysis was evaluated in several ways by analyses of a model protein and yeast lysates where the reproducibility of quantification was essentially the same with both cf-IMER and solution-based proteolysis.
机译:据报道,基于亲和色谱选择和使用连续流固定化酶反应器(cf-IMER)加速胰蛋白酶消化的整合,一种用于复杂混合物中蛋白质鉴定的创新样品制备策略。亲和力选定的糖蛋白被释放到cf-IMER色谱柱上,该色谱柱在高温下5分钟内将天然蛋白转化为肽。将cf-IMER的消化与传统的基于16 h溶液的胰蛋白酶消化的还原和烷基化蛋白质进行了比较。通过从血浆中固定化选择带有Lewis x(Le〜x)聚糖的糖蛋白的抗体,两种方法共鉴定出66种蛋白,而仅使用cf-IMER观察到总蛋白和肽的约1/3。这表明基于仅通过基于溶液的胰蛋白酶消化的还原和烷基化进行蛋白质鉴定的蛋白质组学可能无法鉴定样品中可检测水平的大量蛋白质或肽。此外,除了含有高含量二硫键的蛋白质外,大多数蛋白质不需要还原和烷基化步骤即可鉴定。通过分析模型蛋白和酵母裂解物,以几种方式评估了提出的蛋白水解的有效性,其中定量重现性与cf-IMER和基于溶液的蛋白水解基本相同。

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