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由Genenase I切割并激活的工程化重组肝细胞生长因子的生成。

Generation of engineered recombinant hepatocyte growth factor cleaved and activated by Genenase I.

作者信息

Hayata Daichika, Fukuta Kazuhiro, Matsumoto Kunio, Adachi Eri, Hanada Keigo, Adachi Kiichi, Nakamura Toshikazu

机构信息

Saito Laboratory, Research & Development, Kringle Pharma, Inc., 7-7-15 Saitoasagi, Ibaraki, Osaka 567-0085, Japan.

出版信息

J Biotechnol. 2008 Feb 29;133(4):478-85. doi: 10.1016/j.jbiotec.2007.11.006. Epub 2007 Nov 22.

DOI:10.1016/j.jbiotec.2007.11.006
PMID:18178280
Abstract

Hepatocyte growth factor (HGF) is biosynthesized as a biologically inactive, single-chain form (pro-HGF). Its activation is associated with cleavage at Arg494-Val495 into a two-chain mature form composed of disulfide-linked alpha- and beta-chains. Because serum is a major source of HGF activator (the predominant serine protease responsible for the processing of pro-HGF), serum-free production of recombinant, two-chain HGF had not been established. In this study, to enable serum-free production of two-chain HGF, we generated engineered human pro-HGFs that can be specifically cleaved and activated by Genenase I. Since Genenase I specifically cleaves the C-terminus of the His-Tyr sequence, which does not exist in human HGF, Arg494 (the C-terminus of the HGF alpha-chain) was replaced by His-Tyr, Ala-Ala-His-Tyr, Pro-Gly-His-Tyr, or Pro-Gly-Ala-Ala-His-Tyr. Genenase I cleaved engineered pro-HGFs specifically at the replaced amino acid sequences, forming a disulfide-linked two-chain form. The cleavage was most efficient in the case of the Pro-Gly-Ala-Ala-His-Tyr sequence, and cleaved HGFs displayed biological activities identical to those of wild-type HGF. Considering a potential medical application of HGF, the present technique is valuable because it enables the production of recombinant, two-chain HGF entirely without serum and extends the choice of host cells and organisms for recombinant production.

摘要

肝细胞生长因子(HGF)以生物学上无活性的单链形式(前HGF)进行生物合成。其激活与在精氨酸494 - 缬氨酸495处切割成由二硫键连接的α链和β链组成的双链成熟形式有关。由于血清是HGF激活剂(负责前HGF加工的主要丝氨酸蛋白酶)的主要来源,因此尚未建立无血清生产重组双链HGF的方法。在本研究中,为了实现无血清生产双链HGF,我们构建了可被Genenase I特异性切割和激活的工程化人源前HGF。由于Genenase I特异性切割人HGF中不存在的组氨酸 - 酪氨酸序列的C末端,因此将精氨酸494(HGFα链的C末端)替换为组氨酸 - 酪氨酸、丙氨酸 - 丙氨酸 - 组氨酸 - 酪氨酸、脯氨酸 - 甘氨酸 - 组氨酸 - 酪氨酸或脯氨酸 - 甘氨酸 - 丙氨酸 - 丙氨酸 - 组氨酸 - 酪氨酸。Genenase I在替换的氨基酸序列处特异性切割工程化前HGF,形成二硫键连接的双链形式。在脯氨酸 - 甘氨酸 - 丙氨酸 - 丙氨酸 - 组氨酸 - 酪氨酸序列的情况下切割效率最高,切割后的HGF显示出与野生型HGF相同的生物学活性。考虑到HGF潜在的医学应用,本技术具有重要价值,因为它能够完全在无血清条件下生产重组双链HGF,并扩展了用于重组生产的宿主细胞和生物体的选择范围。

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