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Complementary use of MALDI and ESI for the HPLC-MS/MS analysis of DNA-binding proteins

机译:MALDI和ESI在DNA结合蛋白的HPLC-MS / MS分析中的补充使用

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Proteins from Escherichia coli were isolated based on their ability to bind DNA and digested in-solution with trypsin; the resulting peptides were separated using HPLC and subsequently analyzed using MALDI TOF/TOF and ESI Q-TOF instruments. Various properties of the peptides observed with the two ionization techniques were compared taking into account the differences between the mass analyzers. This empirical analysis of a data set containing hundreds of peptides and thousands of individual amino acids supports some of the currently held notions regarding the complementary nature of the two ionization processes. Specifically, ESI tends to favor the identification of hydrophobic peptides whereas MALDI tends to lead to the identification of basic and aromatic species. Findings from the present study suggest that ESI and MALDI may be complementary due to the biases of the two ionization techniques for certain classes of amino acids. From a practical standpoint, these biases indicate that, for the present at least, analyses must be performed on both types of instruments in order to gain the most information possible out of a given set of samples in a proteomics study.
机译:根据结合蛋白质的能力从大肠杆菌中分离蛋白质,并用胰蛋白酶在溶液中消化;使用HPLC分离得到的肽,随后使用MALDI TOF / TOF和ESI Q-TOF仪器进行分析。考虑到质量分析仪之间的差异,比较了用两种电离技术观察到的肽的各种特性。对包含数百个肽和数千个单个氨基酸的数据集进行的经验分析支持了一些目前持有的关于两个电离过程的互补性质的观念。具体而言,ESI倾向于有利于疏水肽的鉴定,而MALDI倾向于导致碱性和芳香族物质的鉴定。来自本研究的发现表明,由于两种电离技术对某些类型的氨基酸的偏倚,ESI和MALDI可能是互补的。从实际的角度来看,这些偏见表明,至少就目前而言,必须对两种类型的仪器都进行分析,以便从蛋白质组学研究中的给定样本集中获得尽可能多的信息。

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