Cloning, purification and characterization of a cellulase-free xylanase from Geobacillus thermodenitrificans AK53.

M Irfan, H I Guler, A O Belduz, A A Shah, S Canakci
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Abstract

Geobacillus thermodenitrificans AK53 xyl gene encoding xylanase was isolated, cloned and expressed in Escherichia coli. After purifying recombinant xylanase from G. thermodenitrificans AK53 (GthAK53Xyl) to homogeneity by ammonium sulfate precipitation and ion exchange chromatography, biochemical properties of the enzyme were determined. The kinetic studies for GthAK53Xyl showed K M value to be 4.34 mg/mL (for D-xylose) and V max value to be 2028.9 μmoles mg–1 min–1. The optimal temperature and pH for enzyme activity were found out to be 70°C and 5.0, respectively. The expressed protein showed the highest sequence similarity with the xylanases of G. thermodenitrificans JK1 (JN209933) and G. thermodenitrificans T-2 (EU599644). Metal cations Mg2+ and Mn2+ were found to be required for the enzyme activity, however, Co2+, Hg2+, Fe2+ and Cu2+ ions caused inhibitor effect on it. GthAK53Xyl had no cellulolytic activity and degraded xylan in an endo-fashion. The action of the enzyme on xylan from oat spelt produced xylobiose and xylopentose. The reported results are suggestive of a xylanase exhibiting desirable kinetics, stability parameters and metal resistance required for the efficient production of xylobiose at industrial scale.

热反硝化地杆菌AK53无纤维素酶木聚糖酶的克隆、纯化及特性研究
分离、克隆并在大肠杆菌中表达了编码木聚糖酶的热反硝化地杆菌AK53基因。利用硫酸铵沉淀法和离子交换色谱法对G. thermodeniticans AK53重组木聚糖酶(GthAK53Xyl)进行纯化并均匀化后,测定了该酶的生化性能。GthAK53Xyl的动力学研究表明,K - M值为4.34 mg/mL (d -木糖),V最大值为2028.9 μmol mg - 1 min-1。酶活性的最佳温度和pH分别为70℃和5.0℃。表达的蛋白与G. thermodenitricans JK1 (JN209933)和G. thermodenitricans T-2 (EU599644)的木聚糖酶序列相似性最高。该酶的活性需要金属阳离子Mg2+和Mn2+,而Co2+、Hg2+、Fe2+和Cu2+离子对其有抑制作用。GthAK53Xyl无纤维素水解活性,以内方式降解木聚糖。该酶对燕麦中的木聚糖的作用产生木糖糖和木糖戊糖。报告的结果表明,木聚糖酶具有理想的动力学,稳定性参数和金属抗性,需要在工业规模上有效地生产木糖糖。
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