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在大肠杆菌中产生的重组人胎盘生长激素的纯化及生化特性分析

Purification and biochemical characterization of recombinant human placental growth hormone produced in Escherichia coli.

作者信息

Igout A, Van Beeumen J, Frankenne F, Scippo M L, Devreese B, Hennen G

机构信息

Biochimie et Laboratoire d'Endocrinologie, Tour de Pathologie, Liege, Belgium.

出版信息

Biochem J. 1993 Nov 1;295 ( Pt 3)(Pt 3):719-24. doi: 10.1042/bj2950719.

DOI:10.1042/bj2950719
PMID:8240283
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1134619/
Abstract

The hGH-V (or hGH-2) gene codes for human placental growth hormone (hPGH). Secretion of hPGH is continuous, in contrast with the pulsed secretion of pituitary growth hormone (hGH) which it progressively replaces in the maternal bloodstream. hGH-V cDNA has previously been cloned and isolated. Analysis of its nucleotide sequence has revealed a 191-residue protein, hPGH, differing from hGH at 13 positions. The calculated pI is more basic than that of the pituitary hormone. Here we have inserted hGH-V cDNA into the pIN-III-ompA3 plasmid in order to produce hPGH in its native form in Escherichia coli D1210. Expression of hGH-V cDNA in E. coli is significantly lower than that of hGH cDNA with the same expression system. The hPGH produced in E. coli was purified in quantities sufficient to allow its biochemical and immunochemical characterization. The molecular mass of the protein was determined by electrospray m.s. The determined mass, 22,320 Da, agrees well with the molecular mass calculated from the translated cDNA sequence, assuming the presence of two disulphide bridges. Having established the technique for producing hPGH with a primary structure identical to the natural, non-glycosylated, 22 kDa isoform, we can now plan the full physicochemical and pharmaceutical characterization of this new hormonal entity.

摘要

hGH-V(或hGH-2)基因编码人胎盘生长激素(hPGH)。与垂体生长激素(hGH)的脉冲式分泌不同,hPGH的分泌是持续的,并且它在母体血液中逐渐取代hGH。hGH-V cDNA此前已被克隆和分离。对其核苷酸序列的分析揭示了一种由191个氨基酸残基组成的蛋白质hPGH,它与hGH在13个位置上存在差异。计算得到的pI比垂体激素的pI更偏碱性。在此,我们将hGH-V cDNA插入pIN-III-ompA3质粒中,以便在大肠杆菌D1210中以其天然形式生产hPGH。在相同的表达系统中,hGH-V cDNA在大肠杆菌中的表达明显低于hGH cDNA。在大肠杆菌中产生的hPGH被大量纯化,足以对其进行生化和免疫化学特性分析。通过电喷雾质谱法测定了该蛋白质的分子量。测定得到的质量为22,320 Da,假设存在两个二硫键,这与根据翻译后的cDNA序列计算得到的分子量非常吻合。在建立了生产具有与天然非糖基化22 kDa异构体相同一级结构的hPGH的技术后,我们现在可以计划对这种新的激素实体进行全面的物理化学和药学特性分析。

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