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固定化 L-阿拉伯糖异构酶生产 D-塔格糖的稳定性研究。

Stabilization of immobilized l-arabinose isomerase for the production of d-tagatose from d-galactose.

机构信息

Department for Innovation in Biological, Agro-food and Forest Systems, University of Tuscia, Viterbo, Italy.

出版信息

Biotechnol Prog. 2020 Nov;36(6):e3033. doi: 10.1002/btpr.3033. Epub 2020 Jun 30.

DOI:10.1002/btpr.3033
PMID:32506832
Abstract

The aim of this work was to develop a stable immobilized enzyme biocatalyst for the isomerization of d-galactose to d-tagatose at high temperature. l-Arabinose isomerase from the hyperthermophilic bacterium Thermotoga maritima (TMAI) was produced as a (His) -tagged protein, immobilized on a copper-chelate epoxy support and subjected to several postimmobilization treatments aimed at increasing its operational and structural stability. Treatment with glutaraldehyde and ethylenediamine resulted in a more than twofold increase in the operational stability and in all enzyme subunits linked, directly or indirectly, to the support via covalent bonds. A postimmobilization treatment of the immobilized derivatives with mercaptoethanol for the removal of any remaining copper ions, determined a further increase of the operational biocatalytic activity. Immobilized derivatives subjected to both treatments were used for the bioconversion of 18 g/L d-galactose to d-tagatose at 80°C in a packed bed reactor in three repeated cycles and showed a better operational stability compared with the literature data. This study shows that a postimmobilization stabilization treatment with glutaraldehyde and ethylenediamine can stabilize the multi-subunit structure of an enzyme immobilized on a metal-chelate epoxy support with an increase of its operational stability, results that are not easily achievable with the sole immobilization on epoxy or metal chelate-epoxy supports in the case of complex multimeric enzymes with geometric incongruence with the support.

摘要

这项工作的目的是开发一种稳定的固定化酶生物催化剂,用于在高温下将 d-半乳糖异构化为 d-塔格糖。来自嗜热细菌 Thermotoga maritima(TMAI)的 l-阿拉伯糖异构酶作为(His)标记蛋白生产,固定在铜螯合环氧载体上,并进行了多次固定化后处理,旨在提高其操作和结构稳定性。用戊二醛和乙二胺处理导致操作稳定性提高了两倍以上,并且所有酶亚基都通过共价键直接或间接地与载体相连。用巯基乙醇对固定化衍生物进行固定化后处理,以去除任何残留的铜离子,进一步提高了操作生物催化活性。经过两种处理的固定化衍生物在填充床反应器中用于 18 g/L d-半乳糖在 80°C 下的生物转化,在三个重复循环中,与文献数据相比,显示出更好的操作稳定性。这项研究表明,戊二醛和乙二胺的固定化后稳定处理可以稳定固定在金属螯合环氧载体上的多亚基结构的酶,提高其操作稳定性,这在复杂的多聚体酶与载体的几何不重合的情况下,仅通过环氧或金属螯合环氧载体的固定化是不容易实现的。

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Stabilization of immobilized l-arabinose isomerase for the production of d-tagatose from d-galactose.固定化 L-阿拉伯糖异构酶生产 D-塔格糖的稳定性研究。
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