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Hyperexpression of two Aspergillus niger xylanase genes in Escherichia coli and characterization of the gene products

机译:黑曲霉中两个木聚糖酶基因在大肠杆菌中的超表达及其基因产物的表征

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摘要

The analysis of individual gene product should enable to clarify the role of a particular enzyme in a complex xylanase system of A. niger. The two genes encoding precursors of co-produced endo-1,4-β-D-xylanases, xynA1 and xynB, were isolated from Aspergillus niger SCTCC 400264 (SCTCC, China) by using RT-PCR technique and then successfully expressed in Escherichia coli BL21. The nucleotide sequences of the xynA1 and xynB genes revealed that they were only 52.5% homology to each other. Characterization of the recombinant enzymes revealed the different properties: the specific activity of recombinant XYNA1 was 16.58 U/mg compared to 1201.7 U/mg for recombinant XYNB; The optimum temperature and pH of the recombinant XYNA1 were 35 ?oC and 3.0, respectively, whereas the corresponding values for the recombinant XYNB were 55 ?oC and 5.0, respectively; The recombinant XYNB showed much more thermostability than recombinant XYNA1; The recombinant XYNB showed 94% of maximal activity after incubating in water for 60 min at 60 ?oC compared to no activity for recombinant XYNA1. Various metal ions had different effects on activity between the two recombinant xylanases.
机译:对单个基因产物的分析应能够阐明特定酶在黑曲霉复杂木聚糖酶系统中的作用。使用RT-PCR技术从黑曲霉SCTCC 400264(SCTCC,China)中分离出了编码共同产生的内源1,4-β-D-木聚糖酶前体xynA1和xynB的两个基因,然后在大肠杆菌中成功表达BL21。 xynA1和xynB基因的核苷酸序列显示它们彼此只有52.5%的同源性。重组酶的表征揭示了不同的特性:重组XYNA1的比活性为16.58 U / mg,而重组XYNB的比活性为1201.7 U / mg。重组XYNA1的最适温度和pH分别为35℃和3.0,而重组XYNB的相应温度分别为55℃和5.0。重组XYNB比重组XYNA1具有更高的热稳定性;重组XYNB在60°C的水中孵育60分钟后显示最大活性的94%,而重组XYNA1没有活性。两种重组木聚糖酶之间,各种金属离子对活性的影响不同。

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