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Evaluation of Styrene-Divinylbenzene Beads as a Support to Immobilize Lipases

机译:苯乙烯-二乙烯基苯珠的评估以固定化脂肪酶。

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摘要

A commercial and very hydrophobic styrene-divinylbenzene matrix, MCI GEL® CHP20P, has been compared to octyl-Sepharose® beads as support to immobilize three different enzymes: lipases from Thermomyces lanuginosus (TLL) and from Rhizomucor miehie (RML) and Lecitase® Ultra, a commercial artificial phospholipase. The immobilization mechanism on both supports was similar: interfacial activation of the enzymes versus the hydrophobic surface of the supports. Immobilization rate and loading capacity is much higher using MCI GEL® CHP20P compared to octyl-Sepharose® (87.2 mg protein/g of support using TLL, 310 mg/g using RML and 180 mg/g using Lecitase® Ultra). The thermal stability of all new preparations is much lower than that of the standard octyl-Sepharose® immobilized preparations, while the opposite occurs when the inactivations were performed in the presence of organic co-solvents. Regarding the hydrolytic activities, the results were strongly dependent on the substrate and pH of measurement. Octyl-Sepharose® immobilized enzymes were more active versus p-NPB than the enzymes immobilized on MCI GEL® CHP20P, while RML became 700-fold less active versus methyl phenylacetate. Thus, the immobilization of a lipase on this matrix needs to be empirically evaluated, since it may present very positive effects in some cases while in other cases it may have very negative ones.
机译:已将商业和疏水性很强的苯乙烯-二乙烯基苯基质MCI GEL ® CHP20P与辛基-Sepharose ®珠进行了比较,以固定三种不同的酶:嗜热单胞菌的脂肪酶(TLL)和Rhizomucor miehie(RML)和Lecitase ® Ultra(一种商用人工磷脂酶)。两种载体上的固定机理相似:酶相对于载体的疏水表面的界面活化。与辛基-Sepharose ®相比,使用MCI GEL ® CHP20P的固定率和负载量要高得多(TLL为87.2 mg蛋白/ g载体,RML为310 mg / g和使用Lecitase ® Ultra的180 mg / g)。所有新制剂的热稳定性都比标准的辛基-琼脂糖固定化制剂低,而当在有机助溶剂存在下进行灭活时,则相反。关于水解活性,结果在很大程度上取决于底物和测量的pH。与p-NPB相比,辛基琼脂糖固定化酶比固定在MCI GEL CHP20P上的酶更具活性,而RML的活性则比苯乙酸甲酯低700倍。因此,必须凭经验评估脂肪酶在该基质上的固定化,因为在某些情况下它可能会产生非常积极的影响,而在其他情况下可能会产生非常不利的影响。

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