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毕赤酵母中重组人生长激素的合成、纯化表达系统及基质辅助激光解吸电离飞行时间质谱结构分析

Expression system for synthesis and purification of recombinant human growth hormone in Pichia pastoris and structural analysis by MALDI-ToF Mass Spectrometry.

作者信息

Calik Pinar, Orman Mehmet Ali, Celik Eda, Halloran S Mitchell, Calik Güzide, Ozdamar Tunçer H

机构信息

Chemical Engineering Department, Industrial Biotechnology and Metabolic Engineering Laboratory, Middle East Technical University, 06531 Ankara, Turkey.

出版信息

Biotechnol Prog. 2008 Jan-Feb;24(1):221-6. doi: 10.1021/bp070294t. Epub 2008 Jan 11.

DOI:10.1021/bp070294t
PMID:18186643
Abstract

An expression system in Pichia pastoris for the production and purification of recombinant human growth hormone (rHGH) was designed and implemented. hGH cDNA sequence was cloned into pPICZalphaA vector under the control of AOX1 promoter, which included a polyhistidine-tag on the amino terminal end to enable affinity purification and a target site for Factor Xa protease such that protease cleavage in vitro would produce rhGH without any non-native N- and C-termini. Analyses of the affinity-purified rhGH product by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS) showed a spectral peak at m/z 23699. Purified product digested with Factor Xa protease had a molecular mass of 22132 kDa. The molecular mass difference before and after Factor Xa protease digestion expectedly corresponds to the 12 amino acids in the rhGH amino terminus, which includes the EcoRI digestion site (Glu-Phe), the 6xHis tag for affinity purification, and the Factor Xa protease recognition sequence (Ile-Glu-Gly-Arg), a result that also indicates that the signal peptide was properly processed by P. pastoris. N-Terminal sequence analysis of the Factor Xa protease trimmed recombinant product confirmed the mature hGH sequence. Thus, the system designed functioned with its intended purpose effectively in expression, cleavage, and purification of the recombinant product.

摘要

设计并构建了一种用于生产和纯化重组人生长激素(rHGH)的毕赤酵母表达系统。将hGH cDNA序列克隆到受AOX1启动子控制的pPICZalphaA载体中,该载体在氨基末端包含一个多组氨酸标签以实现亲和纯化,以及一个凝血因子Xa蛋白酶的切割位点,这样体外蛋白酶切割将产生没有任何非天然N端和C端的rhGH。通过基质辅助激光解吸/电离飞行时间质谱(MALDI-TOF MS)对亲和纯化的rhGH产物进行分析,结果显示在m/z 23699处有一个光谱峰。用凝血因子Xa蛋白酶消化后的纯化产物分子量为22132 kDa。凝血因子Xa蛋白酶消化前后的分子量差异符合rhGH氨基末端的12个氨基酸,其中包括EcoRI切割位点(Glu-Phe)、用于亲和纯化的6xHis标签以及凝血因子Xa蛋白酶识别序列(Ile-Glu-Gly-Arg),这一结果也表明信号肽已被毕赤酵母正确加工。对凝血因子Xa蛋白酶处理后的重组产物进行N端序列分析,证实了成熟hGH序列。因此,所设计的系统在重组产物的表达、切割和纯化方面有效地实现了预期目的。

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