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通过戊二醛交联吸附在胺化载体上的蛋白质实现酶的稳定化。

Enzyme stabilization by glutaraldehyde crosslinking of adsorbed proteins on aminated supports.

作者信息

López-Gallego Fernando, Betancor Lorena, Mateo Cesar, Hidalgo Aurelio, Alonso-Morales Noelia, Dellamora-Ortiz Gisela, Guisán Jose M, Fernández-Lafuente Roberto

机构信息

Departamento de Biocatálisis, Instituto de Catálisis, CSIC, Campus Universidad Autonoma, Cantoblanco, 28049 Madrid, Spain.

出版信息

J Biotechnol. 2005 Sep 22;119(1):70-5. doi: 10.1016/j.jbiotec.2005.05.021.

Abstract

The stabilization achieved by different immobilization protocols have been compared using three different enzymes (glutaryl acylase (GAC), D-aminoacid oxidase (DAAO), and glucose oxidase (GOX)): adsorption on aminated supports, treatment of this adsorbed enzymes with glutaraldehyde, and immobilization on glutaraldehyde pre-activated supports. In all cases, the treatment of adsorbed enzymes on amino-supports with glutaraldehyde yielded the higher stabilizations: in the case of GOX, a stabilization over 400-fold was achieved. After this treatment, the enzymes could no longer be desorbed from the supports using high ionic strength (suggesting the support-protein reaction). Modification of the enzymes immobilized on supports that did not offer the possibility of react with glutaraldehyde showed the same stability that the non modified preparations demonstrating that the mere chemical modification did not have effect on the enzyme stability. This simple strategy seems to permit very good results in terms of immobilization rate and stability, offering some advantages when compared to the immobilization on glutaraldehyde pre-activated supports.

摘要

已使用三种不同的酶(戊二酰基酰化酶(GAC)、D - 氨基酸氧化酶(DAAO)和葡萄糖氧化酶(GOX))比较了不同固定化方案所实现的稳定性:酶吸附在胺化载体上,用戊二醛处理吸附的酶,以及固定在戊二醛预活化的载体上。在所有情况下,用戊二醛处理氨基载体上吸附的酶可实现更高的稳定性:就GOX而言,实现了超过400倍的稳定性。此处理后,使用高离子强度已无法使酶从载体上解吸(表明载体 - 蛋白质发生了反应)。固定在不具备与戊二醛反应可能性的载体上的酶的修饰显示出与未修饰制剂相同的稳定性,这表明单纯的化学修饰对酶稳定性没有影响。这种简单策略似乎在固定化率和稳定性方面能产生非常好的结果,与固定在戊二醛预活化载体上相比具有一些优势。

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