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展示基因工程化细胞表面蛋白的大肠杆菌细胞的固定与稳定化

Fixation and stabilization of Escherichia coli cells displaying genetically engineered cell surface proteins.

作者信息

Freeman A, Abramov S, Georgiou G

机构信息

Department of Molecular Microbiology and Biotechnology, Faculty of Life Sciences, Tel-Aviv University, Tel-Aviv 69978, Israel.

出版信息

Biotechnol Bioeng. 1996 Dec 5;52(5):625-30. doi: 10.1002/(SICI)1097-0290(19961205)52:5<625::AID-BIT10>3.0.CO;2-E.

DOI:10.1002/(SICI)1097-0290(19961205)52:5<625::AID-BIT10>3.0.CO;2-E
PMID:18629936
Abstract

A large biotechnological potential is inherent in the display of proteins (e.g., enzymes, single-chain antibodies, on the surface of bacterial cells) (Georgiou et al., 1993). Applications such as immobilized whole-cell biocatalysts or cellular adsorbents require cell fixation to prevent disintegration, stabilization of the anchored protein from leakage, denaturation or proteolysis, and total loss of cell viability, preventing medium and potential product contamination with cells. In this article we describe the adaptation of a simple two-stage chemical crosslinking procedure based on "bi-layer encagement" (Tor et al., 1989) for stabilizing Escherichia coli cells expressing an Lpp-OmpA (46-159)-beta-lactamase fusion that displays beta-lactamase on the cell surface. Bilayer crosslinking and coating the bacteria with a polymeric matrix is accomplished by treating the cells first with either glutaraldehyde or polyglutaraldehyde, followed by secondary crosslinking with polyacrylamide hydrazide. These treatments resulted in a 5- to 25-fold reduction of the thermal inactivation rate constant at 55 degrees C of surface anchored beta-lactamase and completely prevented the deterioration of the cells for at least a week of storage at 4 degrees C. The stabilization procedure developed paves the way to scalable biotechnological applications of E. coli displaying surface anchored proteins as whole-cell biocatalysts and adsorbents.

摘要

蛋白质在细菌细胞表面展示(如酶、单链抗体)具有巨大的生物技术潜力(Georgiou等人,1993年)。固定化全细胞生物催化剂或细胞吸附剂等应用需要细胞固定,以防止细胞解体,稳定锚定蛋白,防止其泄漏、变性或被蛋白水解,并防止细胞完全丧失活力,从而避免培养基和潜在产物被细胞污染。在本文中,我们描述了一种基于“双层包裹”(Tor等人,1989年)的简单两阶段化学交联程序的改进方法,用于稳定表达Lpp-OmpA(46-159)-β-内酰胺酶融合蛋白的大肠杆菌细胞,该融合蛋白在细胞表面展示β-内酰胺酶。双层交联和用聚合物基质包被细菌是通过先用戊二醛或聚戊二醛处理细胞,然后用聚丙烯酰胺酰肼进行二次交联来完成的。这些处理使表面锚定的β-内酰胺酶在55℃下的热失活速率常数降低了5至25倍,并在4℃下至少储存一周的时间内完全防止了细胞的降解。所开发的稳定程序为将展示表面锚定蛋白的大肠杆菌作为全细胞生物催化剂和吸附剂的可扩展生物技术应用铺平了道路。

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