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首页> 外文期刊>Biotechnology Letters >Two simple and rapid methods for the detection of polymer-degrading enzymes on high-resolution, alkaline, cold, in situ-native (HiRACIN)-RAGE and high-resolution, in situ-inhibited native (HiRISIN)-PAGE
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Two simple and rapid methods for the detection of polymer-degrading enzymes on high-resolution, alkaline, cold, in situ-native (HiRACIN)-RAGE and high-resolution, in situ-inhibited native (HiRISIN)-PAGE

机译:两种简单,快速的方法,可在高分辨率,碱性,冷,原位(HiRACIN)-RAGE和高分辨率,原位抑制的天然(HiRISIN)-PAGE上检测聚合物降解酶

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摘要

Two sensitive, high-resolution and exceedingly versatile methods for the detection of isoenzymes of polymer-degrading enzymes on high-resolution, alkaline, cold, in situ-native (HiRACIN)-PAGE and high-resolution in situ-inhibited, native (HiRISIN)-PAGE are described. Extracellular crude extracts contaiing xylanases and carboxymethylcellulases from Scopulariopsis sp. and glucoamylases from Aspergillus niger were subjected to non-denaturing PAGE containing substrates in the resolving gel. In case of HiRACIN-PAGE, the enzymes were prevented from degrading their respective substrates during run by carring out electrophoresis at 4 deg C and the pH of running and resolving gel buffer systems were increased from 8.5 to 10.6. In case of HiRISIN-PAGE, adding competitive inhibitor of the enzyme, cellobiose, in the resolving gel prevents the degradation of polymer during the run. These techniques were successfully applied, for the first time, to visualize four, three and four sharp and distinct bands of xylanases, glucoamylases and CMCases, respectively.
机译:在高分辨率,碱性,冷,原位(HiRACIN)-PAGE和高分辨率原位抑制的天然(HiRISIN)上检测聚合物降解酶同工酶的两种灵敏,高分辨率且用途广泛的方法描述)-PAGE。含有木瓜酶和木糖酶的胞外粗提物。将来自黑曲霉的糖化酶和葡糖淀粉酶在分离凝胶中进行含非变性PAGE的底物。在HiRACIN-PAGE的情况下,通过在4摄氏度进行电泳,可防止酶在运行过程中降解其各自的底物,并且运行和分离的凝胶缓冲液系统的pH从8.5增加到10.6。在HiRISIN-PAGE的情况下,在分辨凝胶中加入竞争性的纤维二糖酶抑制剂可防止聚合物在运行过程中降解。这些技术首次成功地用于分别可视化木聚糖酶,葡糖淀粉酶和CMCase的四个,三个和四个清晰而独特的条带。

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