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首页> 外文期刊>Journal of Biotechnology >Exploitation of the S-layer self-assembly system for site directed immobilization of enzymes demonstrated for an extremophilic laminarinase from Pyrococcus furiosus
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Exploitation of the S-layer self-assembly system for site directed immobilization of enzymes demonstrated for an extremophilic laminarinase from Pyrococcus furiosus

机译:S层自组装系统用于酶的定点固定化的研究证明了激烈热球菌的嗜极端性laminarinase

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摘要

A fusion protein based on the S-layer protein SbpA from Bacillus sphaericus CCM 2177 and the enzyme laminarinase (LamA) from Pyrococcus furiosus was designed and overexpressed in Escherichia coli. Due to the construction principle, the S-layer fusion protein fully retained the self-assembly capability of the S-layer moiety, while the catalytic domain of LamA remained exposed at the outer surface of the formed protein lattice. The enzyme activity of the S-layer fusion protein monolayer obtained upon recrystallization on silicon wafers, glass slides and different types of polymer membranes was determined colorimetrically and related to the activity of sole LamA that has been immobilized with conventional techniques. LamA aligned within the S-layer fusion protein lattice in a periodic and orientated fashion catalyzed twice the glucose release from the laminarin polysaccharide substrate in comparison to the randomly immobilized enzyme. In combination with the good shelf-life and the high resistance towards temperature and diverse chemicals, these novel composites are regarded a promising approach for site-directed enzyme immobilization.
机译:设计了基于球形芽孢杆菌CCM 2177的S层蛋白SbpA和激烈热球菌的层板酶(LamA)的融合蛋白,并在大肠杆菌中过表达。由于构造原理,S层融合蛋白完全保留了S层部分的自组装能力,而LamA的催化结构域仍然暴露在形成的蛋白晶格的外表面。通过比色法确定在硅片,载玻片和不同类型的聚合物膜上重结晶后获得的S层融合蛋白单层的酶活性,并与已用常规技术固定的唯一LamA的活性有关。与随机固定的酶相比,以周期性和定向方式排列在S层融合蛋白晶格内的LamA催化从层粘连蛋白多糖底物中释放的葡萄糖两倍。这些新的复合材料与良好的保质期以及对温度和各种化学药品的高耐受性相结合,被认为是定点酶固定化的有前途的方法。

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