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叶片中高水平瞬时产生人碱性成纤维细胞生长因子的蛋白酶抗性突变形式。

High-level transient production of a protease-resistant mutant form of human basic fibroblast growth factor in leaves.

作者信息

Macauyag Edjohn Aaron, Kajiura Hiroyuki, Ohashi Takao, Misaki Ryo, Fujiyama Kazuhito

机构信息

International Center for Biotechnology, Osaka University, Suita, Osaka 565-0871, Japan.

Institute for Open and Transdisciplinary Research Initiatives (OTRI), Osaka University, Suita, Osaka 565-0871, Japan.

出版信息

Plant Biotechnol (Tokyo). 2022 Sep 25;39(3):291-301. doi: 10.5511/plantbiotechnology.22.0628a.

Abstract

The human basic fibroblast growth factor (bFGF) is a protein that plays a pivotal role in cellular processes like cell proliferation and development. As a result, it has become an important component in cell culture systems, with applications in biomedical engineering, cosmetics, and research. Alternative production techniques, such as transient production in plants, are becoming a feasible option as the demand continues to grow. High-level bFGF production was achieved in this study employing an optimized -mediated transient expression system, which yielded about a 3-fold increase in production over a conventional system. This yield was further doubled at about 185 µg g FW using a mutant protease-resistant version that degraded/aggregated at a three-fold slower rate in leaf crude extracts. To achieve a pure product, a two-step purification technique was applied. The capacity of the pure protease-resistant bFGF (PRbFGF) to stimulate cell proliferation was tested and was found to be comparable to that of -produced bFGF in HepG2 and CHO-K1 cells. Overall, this study demonstrates a high-level transient production system of functional PRbFGF in leaves as well as an efficient tag-less purification technique of leaf crude extracts.

摘要

人碱性成纤维细胞生长因子(bFGF)是一种在细胞增殖和发育等细胞过程中起关键作用的蛋白质。因此,它已成为细胞培养系统中的重要组成部分,在生物医学工程、化妆品和研究领域都有应用。随着需求持续增长,诸如在植物中瞬时表达等替代生产技术正成为一种可行的选择。在本研究中,采用优化的介导瞬时表达系统实现了bFGF的高水平生产,与传统系统相比,产量提高了约3倍。使用在叶片粗提物中降解/聚集速度慢三倍的突变型蛋白酶抗性版本,在约185μg g FW时产量进一步翻倍。为了获得纯产品,应用了两步纯化技术。测试了纯蛋白酶抗性bFGF(PRbFGF)刺激细胞增殖的能力,发现在HepG2和CHO-K1细胞中其与产生的bFGF相当。总体而言,本研究展示了叶片中功能性PRbFGF的高水平瞬时生产系统以及叶片粗提物的高效无标签纯化技术。

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