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脂肪酶载体的蓝图:使用疏水可控孔径玻璃作为模型系统。

Blueprint for a lipase support: Use of hydrophobic controlled-pore glasses as model systems.

作者信息

Bosley J A, Clayton J C

机构信息

Unilever Research, Colworth Laboratory, Sharnbrook, Bedford MK44 1LQ, United Kingdom.

出版信息

Biotechnol Bioeng. 1994 Apr 25;43(10):934-8. doi: 10.1002/bit.260431006.

DOI:10.1002/bit.260431006
PMID:18615440
Abstract

For the commercial exploitation of lipase biocatalysis to be successful, it is essential that effective supports are selected for lipase immobilization. In this study hydrophobic controlled-pore glasses have been used as model systems for the immobilization of Rhizomucor miehei lipase. The effect of pore diameter and surface chemistry on enzyme efficiency in a typical esterification reaction under essentially nonaqueous conditions has been examined. It has been found that pore diameters of at least 35 nm are needed for the lipase to be able to utilize the internal volume of the support particles in the immobilization process. Despite the small size of the substrates in the esterification reaction, even larger pores (>100 nm) are required for the lipase efficiency to become independent of pore diameter; below 100 nm lipase activity and efficiency are markedly reduced. It has also been shown that the chemical nature of the hydrophobic surface plays an important part in catalyst design. Although lipase will adsorb readily to a wide range of hydrophobic groups, the highest catalyst activities are obtained when the glass surface is derivatized to give long alkyl chains; the presence of unsaturated derivatives gonerally leads to a reduction in activity. (c) 1994 John Wiley & Sons, Inc.

摘要

为使脂肪酶生物催化的商业开发取得成功,选择有效的载体用于脂肪酶固定化至关重要。在本研究中,疏水性可控孔径玻璃已被用作固定化米黑根毛霉脂肪酶的模型体系。研究了孔径和表面化学性质对在基本非水条件下典型酯化反应中酶效率的影响。已发现,在固定化过程中,脂肪酶要能够利用载体颗粒的内部体积,孔径至少需要35纳米。尽管酯化反应中底物尺寸较小,但为使脂肪酶效率与孔径无关,仍需要更大的孔径(>100纳米);低于100纳米时,脂肪酶活性和效率会显著降低。研究还表明,疏水表面的化学性质在催化剂设计中起着重要作用。虽然脂肪酶能很容易地吸附到多种疏水基团上,但当玻璃表面衍生出长烷基链时,可获得最高的催化剂活性;不饱和衍生物的存在通常会导致活性降低。(c)1994约翰·威利父子公司

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