研究从转基因烟草根部渗出的重组蛋白。

Environmental biosafety research Pub Date : 2008-10-01 Epub Date: 2008-10-07 DOI:10.1051/ebr:2008020
Francesca Pizzuti, Lorenza Daroda
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引用次数: 10

摘要

植物制成的药物(PMPs)具有众多优点,包括生产成本低廉、生物安全性高以及可进行农业规模生产,这一点已得到广泛认可。与此同时,最大限度地降低与这项新技术相关的任何潜在风险(包括可能向环境中释放生物活性蛋白)也非常重要。为了解决这个问题,我们研究了表达两种重组单链可变片段(scFv)抗体(分别为 scFvB9 和 scFvH10)的转基因烟草和烟草植物。ScFvB9 是针对番茄斑萎病毒(TSWV)的糖蛋白 G1 提出的,而 scFvH10 则是针对人类肿瘤相关抗原 tenascin-C 提出的。这两种抗体都是以分泌途径为靶标,使用的是N-末端的信号肽,该信号肽来自粗壮相思豆多聚半乳糖醛酸酶抑制蛋白(PGIP),scFvH10还带有C-末端的KDEL四肽,用于保留在内质网(ER)中。我们建立了无菌水培培养基,以便研究 scFvB9 和 scFvH10 是否存在于根系渗出液中。对从不同植物组织中提取的细胞间液进行了 Western 印迹分析,结果显示存在 scFvB9。在水培培养基中也证明了 scFvB9 的成功分泌,而在叶片、茎或根的细胞质中检测不到 scFvH10,也没有分泌到水培培养基中。我们的结果表明,scFvH10 不会从转基因植物的根部释放或扩散,这表明 KDEL 信号可能有助于提高生产 PMPs 的作物的环境生物安全性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Investigating recombinant protein exudation from roots of transgenic tobacco.

It is widely acknowledged that plant-made pharmaceuticals (PMPs) offer numerous benefits, including inexpensive production, biological safety and the facility for production at agricultural scale. At the same time, it is important to minimize any potential risk associated with this new technology, including the potential release of bioactive proteins into the environment. To address this issue, we studied transgenic Nicotiana benthamiana and Nicotiana tabacum plants expressing two recombinant single-chain variable fragment (scFv) antibodies, respectively scFvB9 and scFvH10. ScFvB9 was raised against glycoprotein G1 of Tomato spotted wilt virus (TSWV), and scFvH10 was raised against human tumor-associated antigen tenascin-C. Both antibodies were targeted to the secretory pathway using the N-terminal signal peptide from Phaseolus vulgaris polygalacturonase-inhibiting protein (PGIP), and scFvH10 carried in addition a C-terminal KDEL tetrapeptide for retention in the endoplasmic reticulum (ER). Sterile hydroponic cultures were established, allowing us to investigate whether scFvB9 and scFvH10 were present in root exudates. Intercellular fluids extracted from different plant tissues were analyzed by western blotting revealing the presence of scFvB9. Successful secretion of scFvB9 in hydroponic medium was also demonstrated, whereas no scFvH10 could be detected in the leaf, stem or root apoplast, nor secreted into the hydroponic medium. Our results show that scFvH10 release or diffusion from the roots of transgenic plants was not occurring, suggesting that the KDEL signal might contribute to the environmental biosafety of crops producing PMPs.

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