首页> 外文期刊>Journal of proteomics >Strategy for purification and mass spectrometry identification of SELDI peaks corresponding to low-abundance plasma and serum proteins.
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Strategy for purification and mass spectrometry identification of SELDI peaks corresponding to low-abundance plasma and serum proteins.

机译:纯化和质谱鉴定与低丰度血浆和血清蛋白相对应的SELDI峰的策略。

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Analysis by SELDI-TOF-MS of low abundance proteins makes it possible to select peaks as candidate biomarkers. Our aim was to define a purification strategy to optimise identification by MS of peaks detected by SELDI-TOF-MS from plasma or serum, regardless of any treatment by a combinatorial peptide ligand library (CPLL). We describe 2 principal steps in purification. First, choosing the appropriate sample containing the selected peak requires setting up a databank that records all the m/z peaks detected from samples in different conditions. Second, the specific purification process must be chosen: separation was achieved with either chromatographic columns or liquid-phase isoelectric focusing, both combined when appropriate with reverse-phase chromatography. After purification, peaks were separated by gel electrophoresis and the candidate proteins were analyzed by nano-liquid-chromatography-MS/MS. We chose 4m/z peaks (9400, 13,571, 13,800 and 15,557) selected for their differential expression between two conditions, as examples to explain the different strategies of purification, and we successfully identified 3 of them. Despite some limitations, our strategy to purify and identify peaks selected from SELDI-TOF-MS analysis was effective.
机译:通过SELDI-TOF-MS分析低丰度蛋白质,可以选择峰作为候选生物标记。我们的目标是定义一种纯化策略,以最优化通过MS对从血浆或血清中SELDI-TOF-MS检测到的峰进行质谱鉴定,而不考虑通过组合肽配体库(CPLL)进行的任何处理。我们描述了纯化中的2个主要步骤。首先,选择包含所选峰的合适样品需要建立一个数据库,该数据库记录在不同条件下从样品中检测到的所有m / z峰。其次,必须选择特定的纯化过程:使用色谱柱或液相等电聚焦进行分离,并在适当时将其与反相色谱法结合使用。纯化后,通过凝胶电泳分离峰,并通过纳米液相色谱-MS / MS分析候选蛋白。我们选择了4m / z峰(9400、13571、13800和15557)作为两个条件之间的差异表达,以举例说明不同的纯化策略,我们成功鉴定了其中的3个。尽管有一些限制,但我们用于纯化和鉴定从SELDI-TOF-MS分析中选择的峰的策略仍然有效。

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