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可溶性gp130生物活性片段作为ELP融合蛋白在转基因植物中的功能表达:通过反向转变循环进行纯化。

Functional expression of a biologically active fragment of soluble gp130 as an ELP-fusion protein in transgenic plants: purification via inverse transition cycling.

作者信息

Lin Meng, Rose-John Stefan, Grötzinger Joachim, Conrad Udo, Scheller Jürgen

机构信息

Biochemisches Institut, Christian-Albrechts Universität zu Kiel, Olshausenstr. 40, D-24098 Kiel, Germany.

出版信息

Biochem J. 2006 Sep 15;398(3):577-83. doi: 10.1042/BJ20060544.

DOI:10.1042/BJ20060544
PMID:16716147
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1559449/
Abstract

In murine models of Crohn's disease, rheumatoid arthritis and colon cancer, IL-6 (interleukin-6) signalling via the sIL-6R (soluble IL-6 receptor; termed IL-6 trans-signalling) has been shown to promote the pathology associated with these conditions. These detrimental activities can, however, be selectively blocked by soluble forms of the gp130 (glycoprotein 130) receptor. Although sgp130 (soluble gp130) therefore represents a viable therapeutic modality for the treatment of these conditions, the mass manufacture of such biologics is often expensive. The advent of molecular farming has, however, provided an extremely cost-effective strategy for the engineering of recombinant proteins. Here, we describe the expression and production of a biologically active sgp130 variant that is expressed in transgenic tobacco plants as an ELP (elastin-like peptide)-fusion protein (mini-gp130-ELP). Mini-gp130-ELP consists of the first three domains of gp130 (Ig-like domain and cytokine binding module) fused to 100 repeats of ELP. Expression of mini-gp130-ELP did not affect the growth rate or morphology of the transgenic plants, and purification was achieved using inverse transition cycling. This approach led to an overall yield of 141 microg of purified protein per g of fresh leaf weight. The purified mini-gp130-ELP specifically inhibited sIL-6R-mediated trans-signalling as measured by binding to the IL-6-sIL-6R complex and through its ability to block sIL-6R-mediated activation of STAT3 (signal transducer and activator of transcription 3) phosphorylation and proliferation in human hepatoma cells and murine pre-B-cells. Consequently, the present study validates the potential application of molecular farming in transgenic tobacco plants as a strategy for the expression and purification of therapeutically advantageous biologics such as sgp130.

摘要

在克罗恩病、类风湿性关节炎和结肠癌的小鼠模型中,白细胞介素-6(IL-6)通过可溶性IL-6受体(sIL-6R;称为IL-6转信号传导)发出信号,已被证明会促进与这些病症相关的病理过程。然而,这些有害活动可被糖蛋白130(gp130)受体的可溶性形式选择性阻断。因此,尽管可溶性gp130(sgp130)代表了治疗这些病症的一种可行治疗方式,但大规模生产此类生物制剂通常成本高昂。然而,分子农业的出现为重组蛋白工程提供了一种极具成本效益的策略。在此,我们描述了一种具有生物活性的sgp130变体的表达和生产,该变体在转基因烟草植物中作为弹性蛋白样肽(ELP)融合蛋白(微型gp130-ELP)表达。微型gp130-ELP由gp130的前三个结构域(免疫球蛋白样结构域和细胞因子结合模块)与100个ELP重复序列融合而成。微型gp130-ELP的表达不影响转基因植物的生长速率或形态,并且使用反向转变循环实现了纯化。该方法导致每克鲜叶重的纯化蛋白总产量为141微克。纯化的微型gp130-ELP通过与IL-6-sIL-6R复合物结合以及通过其阻断sIL-6R介导的信号转导和转录激活因子3(STAT3)磷酸化以及人肝癌细胞和小鼠前B细胞增殖的能力,特异性抑制sIL-6R介导的转信号传导。因此,本研究验证了分子农业在转基因烟草植物中的潜在应用,作为表达和纯化治疗上有利的生物制剂(如sgp130)的策略。

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