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在果蝇 S2 细胞中表达具有生物活性的人凝血因子 IX:昆虫酶对人维生素 K 依赖性蛋白的 γ-羧化作用。

Expression of biologically active human clotting factor IX in Drosophila S2 cells: γ-carboxylation of a human vitamin K-dependent protein by the insect enzyme.

机构信息

Department of Genetics, Tarbiat Modares University, Tehran, Iran.

出版信息

Biotechnol Prog. 2012 Jan-Feb;28(1):45-51. doi: 10.1002/btpr.723. Epub 2011 Oct 19.

DOI:10.1002/btpr.723
PMID:22012919
Abstract

The Drosophila γ-glutamyl carboxylase (dγC) has substrate recognition properties similar to that of the vertebrate γ-carboxylase (γC), and its carboxylated product yield, in vitro, was shown to be more than that obtained with the human enzyme. However, whether the Drosophila enzyme is able to γ-carboxylate the human vitamin K-dependent (VKD) proteins, such as the human coagulation factor IX (hFIX), as synthesized in cultured Drosophila cells was not known. To examine this possibility, the Drosophila Schnider (S2) cell line was transfected with a metallothionein promoter-regulated hFIX-expressing plasmid. After induction with copper ion, expression efficiency of the active hFIX was analyzed by performing enzyme-linked immunosorbent assey (ELISA) and coagulation test on the culture supernatant of the transfected S2 cells during 72 h of postinduction. In comparison with Chinese hamster ovary cell line, S2 cells showed higher (≈ 12-fold) expression level of the hFIX. The γ-carboxylation of the Drosophila-derived hFIX was confirmed by evaluation of the expressed protein, after being precipitated with barium citrate. The biological activity of the S2 cell-derived hFIX indicated the capability of S2 cells to fulfill the required γ-carboxylation of the expressed hFIX. Coexpression of the human γ-glutamyl carboxylases (hγC) was also shown to improve both expression and γ-carboxylation of the hFIX. This is the first in vivo data to describe the ability of the dγC to recognize the human-based propeptide as substrate, which is an essential step for production of biologically active γ-carboxylated VKD proteins.

摘要

果蝇 γ-谷氨酰羧化酶(dγC)具有与脊椎动物 γ-羧化酶(γC)相似的底物识别特性,其体外羧化产物的产量高于人源酶。然而,果蝇酶是否能够对在培养的果蝇细胞中合成的人类维生素 K 依赖性(VKD)蛋白,如人凝血因子 IX(hFIX)进行 γ-羧化,尚不清楚。为了研究这种可能性,用金属硫蛋白启动子调控的 hFIX 表达质粒转染果蝇 Schnider(S2)细胞系。用铜离子诱导后,通过在诱导后 72 小时内对转染的 S2 细胞培养上清液进行酶联免疫吸附测定(ELISA)和凝血试验,分析活性 hFIX 的表达效率。与中国仓鼠卵巢细胞系相比,S2 细胞显示出更高(≈12 倍)的 hFIX 表达水平。用柠檬酸钡沉淀表达的蛋白质后,证实了果蝇来源的 hFIX 的 γ-羧化。S2 细胞衍生的 hFIX 的生物学活性表明 S2 细胞能够完成表达的 hFIX 所需的 γ-羧化。人 γ-谷氨酰羧化酶(hγC)的共表达也显示出提高 hFIX 的表达和 γ-羧化的作用。这是首次描述 dγC 能够识别人类前肽作为底物的体内数据,这是产生具有生物活性的 γ-羧化 VKD 蛋白的必要步骤。

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