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Optimization of human serum albumin monoliths for chiral separations and high-performance affinity chromatography

机译:人血清白蛋白单块手性激酶的优化 分离和高效亲和色谱

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摘要

Various organic-based monoliths were prepared and optimized for immobilization of the protein human serum albumin (HSA) as a binding agent for chiral separations and high-performance affinity chromatography. These monoliths contained co-polymers based on glycidyl methacrylate (GMA) and ethylene glycol dimethacrylate (EDMA) or GMA and trimethylolpropane trimethacrylate (TRIM). A mixture of cyclohexanol and 1-dodecanol was used as the porogen, with the ratio of these solvents being varied along with the polymerization temperature to generate a library of monoliths. These monoliths were used with both the Schiff base and epoxy immobilization methods and measured for their final content of HSA. Monoliths showing the highest protein content were further evaluated in chromatographic studies using R/S-warfarin and D/L-tryptophan as model chiral solutes. A 2.6–2.7-fold increase in HSA content was obtained in the final monoliths when compared to similar HSA monoliths prepared according to the literature. The increased protein content made it possible for the new monoliths to provide higher retention and/or two-fold faster separations for the tested solutes when using 4.6 mm i.d. × 50 mm columns. These monoliths were also used to create 4.6 mm i.d. × 10 mm HSA microcolumns that could separate the same chiral solutes in only 1.5–6.0 min. The approaches used in this study could be extended to the separation of other chiral solutes and to the optimization of organic monoliths for use with additional proteins as binding agents.
机译:制备并优化了各种有机基整体料,用于固定人血清白蛋白(HSA)蛋白,作为手性分离和高效亲和色谱的结合剂。这些整体包含基于甲基丙烯酸缩水甘油酯(GMA)和乙二醇二甲基丙烯酸酯(EDMA)或GMA和三羟甲基丙烷三甲基丙烯酸酯(TRIM)的共聚物。环己醇和1-十二烷醇的混合物用作致孔剂,这些溶剂的比例随聚合温度变化而生成整料库。这些整料与Schiff碱和环氧固定方法一起使用,并测量了它们的HSA最终含量。使用R / S-华法林和D / L-色氨酸作为模型手性溶质,在色谱研究中进一步评估了显示最高蛋白质含量的整体。与根据文献制备的类似HSA整体相比,最终整体中HSA含量增加了2.6-2.7倍。当使用4.6 mm i.d.时,增加的蛋白质含量使新的整料能够为测试的溶质提供更高的保留率和/或两倍的更快分离速度。 ×50毫米色谱柱。这些整料也被用来产生4.6mm的内径。 ×10 mm HSA微柱仅需1.5–6.0分钟即可分离相同的手性溶质。这项研究中使用的方法可以扩展到其他手性溶质的分离和有机整料的优化,以与其他蛋白质作为结合剂一起使用。

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