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首页> 外文期刊>Separation and Purification Technology >A preparative hydrophobic interaction chromatography for purification of recombinant nucleocapsid protein of Nipah virus from clarified Escherichia coli homogenate
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A preparative hydrophobic interaction chromatography for purification of recombinant nucleocapsid protein of Nipah virus from clarified Escherichia coli homogenate

机译:制备性疏水相互作用色谱法,用于从澄清的大肠杆菌匀浆中纯化尼帕病毒的重组核衣壳蛋白

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摘要

The downstream processing of the recombinant nucleocapsid (N) protein of Nipah virus (NiV) from Escherichia coli homogenate using a preparative hydrophobic interaction chromatography (HIC) was investigated in the present study. Ammonium sulfate precipitation experiment was performed and it showed that 15% saturation of the salt was the most suitable salt concentration for the binding buffer. Batch binding of the N protein of NiV was performed using Sepharose~(TM) 6 Fast Flow (FF) adsorbents coupling separately with four different types of ligand; phenyl low substitution, phenyl high substitution, butyl and octyl. The phenyl low substitution ligand was selected for subsequent optimization process due to its highest yield and purity of the N protein achieved from the batch binding experiment. The HIC for purification of the N protein of NiV was further scaled-up using a 10 cm column packed with phenyl low substitution Sepharose~(TM) adsorbent. A recovering yield of 81% of the N protein of NiV with a purification factor of 9.3 was achieved from this scaled-up operation. The antigenicity of the purified N protein was still preserved as shown in ELISA analysis.
机译:在本研究中,研究了使用制备性疏水相互作用色谱法从大肠杆菌匀浆中对尼帕病毒(NiV)的重组核衣壳(N)蛋白进行的下游加工。进行了硫酸铵沉淀实验,结果表明盐的15%饱和度是结合缓冲液最合适的盐浓度。使用分别与四种不同类型的配体偶联的SepharoseTM 6 Fast Flow(FF)吸附剂进行NiV N蛋白的批量结合。苯基低取代,苯基高取代,丁基和辛基。由于从批次结合实验中获得的N蛋白的最高收率和纯度,因此选择了苯基低取代基配体用于后续的优化过程。使用装有苯基低取代SepharoseTM吸附剂的10 cm色谱柱进一步放大纯化NiV N蛋白的HIC。通过该放大操作,获得了NiV N蛋白的81%的回收率和9.3的纯化因子。如ELISA分析所示,纯化的N蛋白的抗原性仍然保留。

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