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将二硫键引入泡盛曲霉糖化酶对其热稳定性和催化活性的影响

Effect on thermostability and catalytic activity of introducing disulfide bonds into Aspergillus awamori glucoamylase.

作者信息

Li Y, Coutinho P M, Ford C

机构信息

Department of Zoology, Iowa State University, Ames 50011, USA.

出版信息

Protein Eng. 1998 Aug;11(8):661-7. doi: 10.1093/protein/11.8.661.

DOI:10.1093/protein/11.8.661
PMID:9749918
Abstract

Two additional disulfide bonds and three combined thermostabilizing mutations were introduced into Aspergillus awamori glucoamylase to test their effects on enzyme thermostability and catalytic properties. The single cysteine mutations N20C, A27C, T72C and A471C were made and combined to produce the double cysteine mutations N20C/ A27C and T72C/A471C. The double cysteine mutants were expressed efficiently in Saccharomyces cerevisiae, and disulfide bonds formed spontaneously after fermentation. At 50 degrees C, the single mutants N20C and A27C had decreased specific activity, whereas the specific activity of the double mutants N20C/A27C and T72C/A471C were similar to wild-type glucoamylase. The N20C/A27C mutation increased thermostability, with an increased activation free energy of 1.5 kJ/mol at 65 degrees C, while the single mutation A27C only slightly increased thermostability and N20C decreased it. The other disulfide bond-forming mutation T72C/A471C did not affect thermostability at pH 4.5. The N20C/A27C mutation was separately combined with two other thermostabilizing mutations, G137A and S436P. Thermostabilities of all of the combined mutated glucoamylases were additive. N20C/A27C/G137A glucoamylase had higher specific activity than wild-type glucoamylase from 45 to 67.5 degrees C. The disulfide bond between positions 20 and 27 connects the C-terminus of helix 1 and the following beta-turn, suggesting that this region is important for glucoamylase thermostability.

摘要

在泡盛曲霉葡萄糖淀粉酶中引入了另外两个二硫键和三个组合的热稳定突变,以测试它们对酶热稳定性和催化特性的影响。构建了单半胱氨酸突变体N20C、A27C、T72C和A471C,并将它们组合以产生双半胱氨酸突变体N20C/A27C和T72C/A471C。双半胱氨酸突变体在酿酒酵母中高效表达,发酵后自发形成二硫键。在50℃时,单突变体N20C和A27C的比活性降低,而双突变体N20C/A27C和T72C/A471C的比活性与野生型葡萄糖淀粉酶相似。N20C/A27C突变提高了热稳定性,在65℃时活化自由能增加了1.5 kJ/mol,而单突变体A27C仅略微提高了热稳定性,N20C则降低了热稳定性。另一个形成二硫键的突变T72C/A471C在pH 4.5时不影响热稳定性。N20C/A27C突变分别与另外两个热稳定突变G137A和S436P组合。所有组合突变的葡萄糖淀粉酶的热稳定性是相加的。N20C/A27C/G137A葡萄糖淀粉酶在45至67.5℃范围内比野生型葡萄糖淀粉酶具有更高的比活性。20位和27位之间的二硫键连接螺旋1的C末端和随后的β-转角,表明该区域对葡萄糖淀粉酶的热稳定性很重要。

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