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Refolding of Lactate Dehydrogenase by Zeolite Beta

机译:Beta型沸石对乳酸脱氢酶的重折叠

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摘要

We used zeolite beta as an adsorbing matrix to refold recombinant lactate dehydrogenase(LDH)protein collected as an insoluble aggregate from a bacterial expression system.The adsorption isotherm revealed that 1 g of zeolite adsorbed 200 mg of denatured LDH solubi-lized with a buffer containing 6 M of guanidine hydrochloride.The pH of the buffer had little effect on the adsorption,but this property was abolished by preincubation of the zeolite with polyethylene glycol(PEG)in a weight ratio of 1:10.These data suggest that the adsorption of LDH depends on the hydrophobicity of the zeolite surface,and that the adsorption of PEG to zeolite is sufficient to release LDH from its surface.LDH was thus released by refolding buffer containing PEG and arginine,and soluble LDH was obtained in its active enzymatic form.The addition of arginine dramatically increased the yield of LDH in a dose-dependent manner.The overall refolding efficiency was optimized to 35%.
机译:我们使用β沸石作为吸附基质,将细菌表达系统中收集的重组乳酸脱氢酶(LDH)蛋白作为不溶性聚集物进行重折叠。吸附等温线显示1 g沸石吸附了200 mg变性LDH并用缓冲液溶解6 M的盐酸胍。缓冲液的pH值对吸附几乎没有影响,但是通过将沸石与聚乙二醇(PEG)重量比为1:10进行预温育,该性能被取消。这些数据表明, LDH取决于沸石表面的疏水性,而PEG对沸石的吸附足以从其表面释放LDH,因此通过重折叠包含PEG和精氨酸的缓冲液释放LDH,并以活性酶形式获得可溶性LDH。精氨酸的添加以剂量依赖的方式显着提高了LDH的产量,总重折叠效率优化为35%。

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