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首页> 外文期刊>Electrophoresis: The Official Journal of the International Electrophoresis Society >Manipulation of protein fingerprints during on-column fluorescent labeling: Protein fingerprinting of six Staphylococcus species by capillary electrophoresis
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Manipulation of protein fingerprints during on-column fluorescent labeling: Protein fingerprinting of six Staphylococcus species by capillary electrophoresis

机译:柱上荧光标记过程中蛋白质指纹的操纵:毛细管电泳对六个葡萄球菌的蛋白质指纹

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摘要

Bacterial proteomes were analyzed by use of electrophoretically mediated microanalysis (EMMA) and field-enhanced stacking. A water-soluble protein fraction was injected onto a capillary. Next, a fluorogenic reagent was injected and allowed to react with the protein mixture, producing fluorescent products that were separated by submicellar capillary electrophoresis and detected by laser-induced fluorescence. By use of a low-ionic strength sample buffer and a brief electrophoretic step, slow moving anionic proteins were stacked at the reagent-sample interface and were preferentially labeled. By reversing the order of sample injection and labeling reagent, fast moving cationic proteins were preferentially labeled. By adjustment of the sample buffer pH, proteins with different isoelectric points were selectively labeled. Electrophoresis fingerprints were generated for the water-soluble protein fraction from six Staphylococcus species. The protein patterns produced were species-specific and were used to construct a phylogenetic tree. [References: 19]
机译:通过使用电泳介导的微量分析(EMMA)和现场增强堆叠技术对细菌蛋白质组进行了分析。将水溶性蛋白质部分注入毛细管中。接下来,注入一种荧光试剂,使其与蛋白质混合物反应,生成荧光产物,该产物通过胶束下的毛细管电泳分离,并通过激光诱导的荧光进行检测。通过使用低离子强度的样品缓冲液和短暂的电泳步骤,将缓慢移动的阴离子蛋白堆叠在试剂-样品界面处,并进行了优先标记。通过颠倒样品进样和标记试剂的顺序,优先标记快速移动的阳离子蛋白。通过调节样品缓冲液的pH,选择性标记具有不同等电点的蛋白质。电泳指纹图谱来自六个葡萄球菌物种的水溶性蛋白质部分。产生的蛋白质模式是物种特异性的,并用于构建系统发育树。 [参考:19]

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