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使用……的重组甘精胰岛素生产工艺

Recombinant Glargine Insulin Production Process Using .

作者信息

Hwang Hae-Gwang, Kim Kwang-Jin, Lee Se-Hoon, Kim Chang-Kyu, Min Cheol-Ki, Yun Jung-Mi, Lee Su Ui, Son Young-Jin

机构信息

Department of Pharmacy, Sunchon National University, Suncheon 57922, Republic of Korea.

Research Institute of Life and Pharmaceutical Sciences, Sunchon National University, Suncheon 57922, Republic of Korea.

出版信息

J Microbiol Biotechnol. 2016 Oct 28;26(10):1781-1789. doi: 10.4014/jmb.1602.02053.

DOI:10.4014/jmb.1602.02053
PMID:27363479
Abstract

Glargine insulin is a long-acting insulin analog that helps blood glucose maintenance in patients with diabetes. We constructed the pPT-GI vector to express prepeptide glargine insulin when transformed into JM109. The transformed cells were cultured by fed-batch fermentation. The final dry cell mass was 18 g/l. The prepeptide glargine insulin was 38.52% of the total protein. It was expressed as an inclusion body and then refolded to recover the biological activity. To convert the prepeptide into glargine insulin, citraconylation and trypsin cleavage were performed. Using citraconylation, the yield of enzymatic conversion for glargine insulin increased by 3.2-fold compared with that without citraconylation. After the enzyme reaction, active glargine insulin was purified by two types of chromatography (ion-exchange chromatography and reverse-phase chromatography). We obtained recombinant human glargine insulin at 98.11% purity and verified that it is equal to the standard of human glargine insulin, based on High-performance liquid chromatography analysis and Matrix-assisted laser desorption/ionization Time-of-Flight Mass Spectrometry. We thus established a production process for high-purity recombinant human glargine insulin and a method to block Arg (B31)-insulin formation. This established process for recombinant human glargine insulin may be a model process for the production of other human insulin analogs.

摘要

甘精胰岛素是一种长效胰岛素类似物,可帮助糖尿病患者维持血糖水平。我们构建了pPT - GI载体,将其转化到JM109中时可表达甘精胰岛素前体肽。通过补料分批发酵培养转化后的细胞。最终干细胞质量为18 g/L。甘精胰岛素前体肽占总蛋白的38.52%。它以包涵体形式表达,然后复性以恢复生物活性。为了将前体肽转化为甘精胰岛素,进行了柠康酰化和胰蛋白酶切割。使用柠康酰化,与未进行柠康酰化相比,甘精胰岛素的酶促转化产量提高了3.2倍。酶反应后,通过两种色谱法(离子交换色谱法和反相色谱法)纯化活性甘精胰岛素。基于高效液相色谱分析和基质辅助激光解吸/电离飞行时间质谱,我们获得了纯度为98.11%的重组人甘精胰岛素,并验证其与重组人甘精胰岛素标准品相当。因此,我们建立了高纯度重组人甘精胰岛素的生产工艺以及一种阻止精氨酸(B31)-胰岛素形成的方法。这种已建立的重组人甘精胰岛素生产工艺可能是生产其他人类胰岛素类似物的模型工艺。

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