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Expression of an alkalo-tolerant fungal xylanase enhanced by directed evolution in Pichia pastoris and Escherichia coli

机译:巴斯德毕赤酵母和大肠杆菌中定向进化增强了耐碱真菌木聚糖酶的表达

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The alkaline stability of the xylanase from Thermomyces lanuginosus was further improved by directed evolution using error-prone PCR mutagenesis. Positive clones were selected by their ability to produce zones of clearing on pH 9 and 12 xylan agar plates. Variant NC38 was able to withstand harsh alkaline conditions retaining 84% activity after exposure at pH 10 for 90min at 60 super(o)C, while the parent enzyme had 22% activity after 60min. The alkaline stable variant NC38 was cloned into pBGP1 under the control GAP promoter and pET22b(+) for expression in Pichia pastoris and Escherichia coli BL21, respectively. Best extracellular expression of the recombinant xylanase was observed in P. pastoris (261.7+ /-0.61Uml super(-) super(1)) whereas intracellular activity was observed in E. coli (47.9+/-0.28Uml super(-) super(1)) was low. Total activity obtained in P. pastoris was 545-fold higher than E. coli. The mutated alkaline stable xylanase from P. pastoris was secreted into the culture medium with little or no contamination by host proteins, which favours the application of this enzyme in the pulp and paper industry.
机译:通过使用易错PCR诱变的定向进化进一步提高了来自嗜热嗜热丝菌的木聚糖酶的碱性稳定性。通过在pH 9和12木聚糖琼脂平板上产生澄清区的能力来选择阳性克隆。变体NC38能够承受苛刻的碱性条件,在60℃下于pH 10下暴露90分钟后,仍能保持84%的活性,而亲本酶在60分钟后具有22%的活性。将碱性稳定变体NC38克隆到控制GAP启动子和pET22b(+)的pBGP1中,分别在巴斯德毕赤酵母和大肠杆菌BL21中表达。在巴斯德毕赤酵母中观察到重组木聚糖酶的最佳细胞外表达(261.7+ /-0.61Uml super(-)超级(1)),而在大肠杆菌中观察到细胞内活性(47.9 +/- 0.28Uml super(-)超级(-) (1))低。巴斯德毕赤酵母中获得的总活性比大肠杆菌高545倍。来自巴斯德毕赤酵母的突变的碱性稳定的木聚糖酶被分泌到培养基中,几乎没有或没有宿主蛋白质的污染,这有利于该酶在制浆造纸工业中的应用。

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