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Enzyme Immobilization onto Ultrahigh Specific Surface Cellulose Fibers via Amphiphilic (PEG) Spacers and Electrolyte (PAA) Grafts

机译:通过两亲(PEG)间隔物和电解质(PAA)移植物将酶固定到超高比表面纤维素纤维上

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Our group has investigated the incorporation of proteins in fibers by two approaches. One involves physical encapsulation of proteins in the bulk of ultrafine and porous fibers and the other bound proteins to fiber surfaces with reactive spacers and functional grafts. This paper reports two examples from the seco'nd approach. Both involve the addition of covalently bonded polymeric chains to ultra-fine cellulose fiber surfaces. One tethers enzyme proteins by covalently bonds via amphiphilic PEG spacers that carry reactive end groups. The other adds polyelectrolyte PAA grafts that are sufficiently polar to attract enzymes via secondary forces. Both surface polymer systems are compatible with aqueous and organic media. Lipase (E.C. 3.1,1.3, from Candida rugosa) enzyme was used. PEG was introduced by reacting cellulose with PEG diacylchloride followed by amide covalent bond formation between COOH of PEG and amine (NH2) of the lipase. PAA (0.76-40.9 mmol of COOH per g cellulose) was grafted via eerie ion initiated polymerization. On the PEG attached cellulose, reactive COOH end groups ranging from 0.2 to 1.0 mmol per g cellulose.
机译:我们的小组通过两种方法调查了纤维中蛋白质的掺入。一种涉及在大量超细和多孔纤维中的物理包封蛋白质和其他结合的蛋白质与具有反应间隔物和功能移植物的纤维表面。本文报告了Seco'nd方法的两个例子。两者都涉及向超细纤维素纤维表面加入共价键合的聚合物链。通过共价键合通过携带反应端基团的两亲的PEG间隔物共价键合一致的酶蛋白。另一个添加了足够极性的聚电解质Paa移植物,以通过二次力吸收酶。两个表面聚合物系统与水性和有机介质相容。使用脂肪酶(例如3.1,1.3,来自Candida Rugosa)酶。通过使纤维素与PEG二琥酰氯化物反应,然后在脂肪酶的COOH和胺(NH2)之间的酰胺共价键形成酰胺的酰胺共价键形成引入PEG。通过Eerie离子引发的聚合接枝Paa(0.76-40.9mmol每G纤维素)。在PEG附着的纤维素上,每G纤维素的反应性CoOH端基范围为0.2-1.0mmol。

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