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Separation of human plasma proteins HSA and HIgG using high-capacity macroporous gel-filled membranes

机译:使用大容量大孔凝胶填充膜分离人血浆蛋白HSA和HIgG

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This paper discusses the separation of human serum albumin(HSA),the most abundant protein present in plasma from human immunoglobulin G(HIgG)by membrane chromatography using a novel macroporous gel-filled membrane(designated Q Type 2).The membrane was prepared by anchoring a quaternary ammonium salt macroporous gel within the pores of a non-woven,polypropylene fabric.Factors affecting HSA binding were examined and operating conditions suitable for separating it from human plasma were identified.At an optimized condition,the HSA binding capacity of this novel membrane under saturating conditions was in the range of 290-300 mg/ml.This was not only significantly higher than binding capacities reported for other chromatographic membranes,but also higher than binding capacities of conventional gel based chromatographic media.The protein binding capacity was also largely insensitive to the superficial velocity,indicating the dominance of convective protein transport to and from the binding sites.The suitability of using this membrane for plasma fractionation was demonstrated by the separation of a simulated feed solution consisting of HSA and HIgG.
机译:本文讨论了使用新型大孔凝胶填充膜(命名为Q型2)通过膜色谱从人免疫球蛋白G(HIgG)中分离血浆中最丰富的蛋白质人血清白蛋白(HSA)的方法。将季铵盐大孔凝胶固定在聚丙烯无纺布的孔中。研究了影响HSA结合的因素,并确定了将其与人血浆分离的操作条件。在优化条件下,该新型产品的HSA结合能力饱和条件下膜的结合能力在290-300 mg / ml范围内。这不仅大大高于其他色谱膜报道的结合能力,而且也高于常规基于凝胶的色谱介质的结合能力。对表面速度基本不敏感,表明对流蛋白与结合蛋白之间的运输占主导地位通过分离由HSA和HIgG组成的模拟进料溶液,证明了使用该膜进行血浆分离的适用性。

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