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从玉米种子中回收重组I型α1胶原蛋白的工艺整合。

Process integration for recovery of recombinant collagen type I α1 from corn seed.

作者信息

Setina Christopher M, Haase Jason P, Glatz Charles E

机构信息

Koch Industries - Flint Hills Resources, 510 S.16th Street, suite 104, Ames, IA, 50010.

Dow Chemical Co., 7600 Metro Blvd., Edina, MN, 55439.

出版信息

Biotechnol Prog. 2016 Jan-Feb;32(1):98-107. doi: 10.1002/btpr.2191. Epub 2015 Nov 17.

DOI:10.1002/btpr.2191
PMID:26518757
Abstract

Because of safety concerns and product consistency issues with the use of animal-derived collagen, several recombinant protein expression hosts have been considered for recombinant collagen corn seed. Full length, triple-helical, recombinant collagen (rCIα1) is expressed as a fusion with a foldon domain, which must later be removed. Here we have examined integration of purification and foldon removal by comparing advantages of removal before or after purification, using salt precipitation as the main purification step. Because expression levels in available maize lines are low, Pichia-produced recombinant collagens, both with and without foldon, were added to corn seed germ at the extraction step. Salt precipitation of an acidic corn seed extract yielded 100% of the collagen without foldon at >70% purity without the pepsin pretreatment. With pepsin pretreatment, yield was 94.0% with purity of 76.5%. Analysis of the protein molecular weight distribution of the pre- and post-treatment extracts showed that the corn proteins are largely resistant to pepsin proteolysis, explaining why little benefit was obtained by pepsin treatment. In the absence of pepsin treatment, the recovery of rCIα1 with foldon was still above 90% but the purity was only 44%. This still represented at about 13-fold purification with a 2.7-fold volume reduction which would reduce the pepsin requirement for post-recovery foldon cleavage.

摘要

由于使用动物源胶原蛋白存在安全问题和产品一致性问题,人们考虑了几种重组蛋白表达宿主来生产重组胶原蛋白玉米种子。全长三螺旋重组胶原蛋白(rCIα1)以与折叠域融合的形式表达,随后必须去除该折叠域。在这里,我们通过比较纯化前或纯化后去除折叠域的优势,以盐沉淀作为主要纯化步骤,研究了纯化和去除折叠域的整合情况。由于现有玉米品系中的表达水平较低,在提取步骤中,将毕赤酵母生产的含或不含折叠域的重组胶原蛋白添加到玉米种子胚中。酸性玉米种子提取物的盐沉淀在未进行胃蛋白酶预处理的情况下,可产生纯度>70%的100%无折叠域胶原蛋白。经过胃蛋白酶预处理后,产量为94.0%,纯度为76.5%。对处理前后提取物的蛋白质分子量分布分析表明,玉米蛋白对胃蛋白酶水解具有很大抗性,这解释了胃蛋白酶处理为何益处不大。在未进行胃蛋白酶处理的情况下,含折叠域的rCIα1回收率仍高于90%,但纯度仅为44%。这仍代表约13倍的纯化,体积减少2.7倍,这将减少回收后折叠域切割所需的胃蛋白酶量。

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