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Purification and basic biochemical characterization of 19 recombinant plant peroxidase isoenzymes produced in Pichia pastoris

机译:巴斯德毕赤酵母中产生的19种重组植物过氧化物酶同工酶的纯化和基本生化特性

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The plant enzyme horseradish peroxidase (HRP) is used in several important industrial and medical applications, of which especially biosensors and diagnostic kits describe an emerging field. Although there is an increasing demand for high amounts of pure enzyme preparations, HRP is still isolated from the plant as a mixture of different isoenzymes with different biochemical properties. Based on a recent next generation sequencing approach of the horseradish transcriptome, we produced 19 individual HRP isoenzymes recombinantly in the yeast Pichia pastoris. After optimizing a previously reported 2-step purification strategy for the recombinant isoenzyme HRP C1A by substituting an unfavorable size exclusion chromatography step with an anion exchange step using a monolithic column, we purified the 19 HRP isoenzymes with varying success. Subsequent basic biochemical characterization revealed differences in catalytic activity, substrate specificity and thermal stability of the purified HRP preparations. The preparations of the isoenzymes HRP A2A and HRP A2B were found to be highly interesting candidates for future applications in diagnostic kits with increased sensitivity.
机译:植物酶辣根过氧化物酶(HRP)在几种重要的工业和医学应用中使用,尤其是生物传感器和诊断试剂盒描述了一个新兴领域。尽管对大量纯酶制剂的需求不断增长,但HRP仍是从植物中分离出来的,它们是具有不同生化特性的不同同工酶的混合物。基于辣根转录组的新一代测序方法,我们在巴斯德毕赤酵母中重组产生了19种HRP同工酶。通过使用整体柱通过阴离子交换步骤取代尺寸排阻色谱步骤不利于重组重组酶HRP C1A的先前报道的两步纯化策略后,我们成功地纯化了19种HRP同工酶。随后的基本生化特征表明,纯化的HRP制剂在催化活性,底物特异性和热稳定性方面存在差异。发现同工酶HRP A2A和HRP A2B的制备是高度感兴趣的候选物,可用于将来在诊断试剂盒中以更高的灵敏度应用。

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