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首页> 外文期刊>Amino acids >The use of native gels for the concomitant determination of protein sequences and modifications by mass spectrometry with subsequent conformational and functional analysis of native proteins following electro-elution
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The use of native gels for the concomitant determination of protein sequences and modifications by mass spectrometry with subsequent conformational and functional analysis of native proteins following electro-elution

机译:使用天然凝胶通过质谱同时测定蛋白质序列和修饰,随后在电洗脱后进行天然蛋白质的构象和功能分析

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The protocol consists of running a native gel with in-gel digestion by proteases, subsequent mass spec-trometrical determination of protein sequence and modifications, followed by electro-elution and conformational analysis using melting point and circular dichroism. Finally, the eluted protein is tested for preserved function. Herein, C1 esterase inhibitor is applied on a native gel; in-gel digestion by proteases is carried out and peptides are identified by nano-LC-ESI-CID/ETD-MS/MS using an ion trap for generation of peptide sequences and protein modifications. Protein from replicate bands from the same gel is electro-eluted and used for determination of the melting point and used for circular dichroism analysis. Additional bands from the native gel are either in-gel digested with asparaginase to generate deamidation or PNGase F for deglycosylation, followed by mass spectrometry, conformational and functional studies. Preserved conformation and function of the C1 esterase inhibitor was shown. This protocol can be completed in 1 week.
机译:该方案包括运行天然凝胶,并通过蛋白酶在凝胶中进行消化,随后对蛋白质序列和修饰进行质谱测定,然后使用熔点和圆二色性进行电洗脱和构象分析。最后,测试洗脱的蛋白质的保留功能。在此,将C1酯酶抑制剂应用于天然凝胶。进行蛋白酶在凝胶中的消化,并使用离子阱通过纳米LC-ESI-CID / ETD-MS / MS鉴定肽,以生成肽序列和蛋白质修饰。来自同一凝胶的重复条带中的蛋白质被电洗脱并用于确定熔点,并用于圆二色性分析。来自天然凝胶的其他条带要么用天冬酰胺酶在凝胶中消化以产生脱酰胺作用,要么用PNGase F进行去糖基化,然后进行质谱,构象和功能研究。显示了C1酯酶抑制剂的保留构象和功能。该协议可以在1周内完成。

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