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重组人抑肽素在毕赤酵母中的高效表达及其生物活性

[High level expression of recombinant human kallistatin in Pichia pastoris and its bioactivity].

作者信息

Huang Xiaoping, Wang Xiao, Dong Hao, Zhao Xiaofeng, Li Zhaofa, Wang Qizhao, Xu Ruian, Diao Yong

机构信息

Institute of Molecular Medicine, Huaqiao University, Quanzhou, China.

出版信息

Sheng Wu Gong Cheng Xue Bao. 2010 Feb;26(2):249-55.

Abstract

In order to research the bioactivity of kallistatin (Kal), we obtained the recombinant Kal using Pichia pastoris expression system. Kal cDNA was amplified from pAAV-Kal and inserted into pPIC9 vector to generate a recombinant vector of pPIC9-Kal. Then, pPIC9-Kal was linearized and transformed into Pichia pastoris strain GS115 (His4) by electroporation. The positive transformants were selected by MD plate and confirmed by PCR. High level of Kal was obtained in BMMY medium (pH 7.0) after 96 hours induction of 29 degrees C and 2% methanol, with the highest yield of 14 mg/L in shake flask culture. Kal protein was purified from the supernatant with Phenyl Superose and Heparin Sepharose FF chromatograph. The recombinant Kal had a molecular weight of 58 kDa with 98% purity, showing by SDS-PAGE. Moreover, it had a high peroxidase activity (163+/-4) U/(mgmin), which could protect LX-2 cell against oxidation of H2O2. Recombinant Kal also effectively inhibited HUVEC proliferation. In this report, we successfully established the expression system using Pichia pastoris and obtained the bioactive recombinant human Kal. It lays a foundation for its further anti-cancer therapy.

摘要

为了研究抑癌素(Kal)的生物活性,我们使用毕赤酵母表达系统获得了重组Kal。从pAAV-Kal中扩增Kal cDNA,并将其插入pPIC9载体中以产生pPIC9-Kal重组载体。然后,将pPIC9-Kal线性化并通过电穿孔转化到毕赤酵母菌株GS115(His4)中。通过MD平板筛选阳性转化子并通过PCR进行确认。在29℃和2%甲醇诱导96小时后,在BMMY培养基(pH 7.0)中获得了高水平的Kal,摇瓶培养中最高产量为14 mg/L。用苯基琼脂糖和肝素琼脂糖FF色谱从上清液中纯化Kal蛋白。通过SDS-PAGE显示,重组Kal的分子量为58 kDa,纯度为98%。此外,它具有较高的过氧化物酶活性(163±4)U/(mg·min),可以保护LX-2细胞免受H2O2的氧化。重组Kal还能有效抑制人脐静脉内皮细胞(HUVEC)的增殖。在本报告中,我们成功建立了毕赤酵母表达系统并获得了具有生物活性的重组人Kal。这为其进一步的抗癌治疗奠定了基础。

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