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Highly Efficient Enzyme Reactors Containing Trypsin and Endoproteinase LysC Immobilized on Porous Polymer Monolith Coupled to MS Suitable for Analysis of Antibodies

机译:包含胰蛋白酶和内蛋白酶LysC的高效酶反应器,固定在与MS偶联的适于分析抗体的多孔聚合物整料上

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Capillary enzymatic microreactors containing trypsin and endoproteinase LysC immobilized on a porous polymer monolith have been prepared and used for the characterization and identification of proteins such as cytochrome c, bovine serum albumin, and high-molecular weight human immunoglobulin G. The hydrophilicity of diol functionalities originating from the hydrolyzed poly (glycidyl methacrylate-co-ethylene dimethacrylate) monolith was not sufficient to avoid adsorption of hydrophobic albumin in a highly aqueous mobile phase. Therefore, this monolith was first hydrophilized via photografting of poly(ethylene glycol) methacrylate followed by photografting of a 4-vinyl-2,2-dimethylazlactone to provide the pore surface with reactive functionalities required for immobilization. This new approach reduced the undesired nonspecific adsorption of proteins and peptides and facilitated control of both the enzyme immobilization and protein digestion processes. The enzymatic reactors were coupled off-line with MALDI/TOF MS and/or on-line with ESI/TOF MS. Experimental conditions for digestion were optimized using cytochrome c and bovine serum albumin as model proteins. The optimized reactors were then integrated into a multidimensional system comprised of a monolithic capillary enzyme reactor, an in-line nanoLC separation of peptides using a poly(lauryl methacrylate-co-ethylene dimethacrylate) monolithic column, and ESI/TOF MS. With the use of this system, immunoglobulin G was digested at room temperature in 6 min to an extent similar to that achieved with soluble enzyme at 37 deg C after 24 h.
机译:已经制备了固定在多孔聚合物整料上的包含胰蛋白酶和内蛋白酶LysC的毛细管酶微反应器,并将其用于表征和鉴定蛋白质,例如细胞色素c,牛血清白蛋白和高分子量人免疫球蛋白G。二醇官能团的亲水性源自水解的聚(甲基丙烯酸缩水甘油酯-共聚二甲基丙烯酸乙二酯)的整体结构不足以避免疏水性白蛋白在高水性流动相中的吸附。因此,首先通过聚甲基丙烯酸乙二醇酯的光接枝,然后4-乙烯基-2,2-二甲基氮杂内酯的光接枝,为孔表面提供固定化所需的反应性官能团,使该整料亲水化。这种新方法减少了不希望的蛋白质和多肽的非特异性吸附,并促进了酶固定和蛋白质消化过程的控制。酶反应器与MALDI / TOF MS离线偶联和/或与ESI / TOF MS联机偶联。使用细胞色素c和牛血清白蛋白作为模型蛋白优化了消化的实验条件。然后将优化的反应器整合到一个多维系统中,该系统包括一个整体式毛细管酶反应器,使用聚(甲基丙烯酸月桂酯-共聚二甲基丙烯酸乙二酯)整体柱和ESI / TOF MS进行的肽的在线纳米LC分离。使用该系统,免疫球蛋白G在室温下在6分钟内被消化,其程度类似于24小时后在37摄氏度下用可溶性酶达到的程度。

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