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首页> 外文期刊>Transgenic research >Translational fusion of chloroplast-expressed human papillomavirus type 16 L1 capsid protein enhances antigen accumulation in transplastomic tobacco
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Translational fusion of chloroplast-expressed human papillomavirus type 16 L1 capsid protein enhances antigen accumulation in transplastomic tobacco

机译:叶绿体表达的人乳头瘤病毒16型L1衣壳蛋白的翻译融合增强了转质体烟草中的抗原积累

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摘要

Human Papillomavirus (HPV) is the causal agent of cervical cancer, one of the most common causes of death for women. The major capsid L1 protein self-assembles in Virus Like Particles (VLPs), which are highly immunogenic and suitable for vaccine production. In this study, a plastid transformation approach was assessed in order to produce a plant-based HPV-16 L1 vaccine. Transplastomic plants were obtained after transformation with vectors carrying a chimeric gene encoding the L1 protein either as the native viral (L1(v) gene) or a synthetic sequence optimized for expression in plant plastids (L1(pt) gene) under control of plastid expression signals. The L1 mRNA was detected in plastids and the L1 antigen accumulated up to 1.5% total leaf proteins only when vectors included the 5'-UTR and a short N-terminal coding segment (Downstream Box) of a plastid gene. The half-life of the engineered L1 protein, determined by pulse-chase experiments, is at least 8 h. Formation of immunogenic VLPs in chloroplasts was confirmed by capture ELISA assay using antibodies recognizing conformational epitopes and by electron microscopy.
机译:人乳头瘤病毒(HPV)是宫颈癌的病因,宫颈癌是女性最常见的死亡原因之一。主要的衣壳L1蛋白在病毒样颗粒(VLP)中自组装,具有很高的免疫原性,适合疫苗生产。在这项研究中,评估了质体转化方法,以生产基于植物的HPV-16 L1疫苗。使用带有编码L1蛋白的嵌合基因的载体转化后,获得质体转化的植物,该嵌合基因可以作为原生病毒(L1(v)基因),也可以在质体表达的控制下优化用于在植物质体中表达的合成序列(L1(pt)基因)信号。仅当载体包含质体基因的5'-UTR和短N端编码片段(下游框)时,才能在质体中检测到L1 mRNA,并且L1抗原积累的叶蛋白总量高达1.5%。通过脉冲追踪实验确定的工程L1蛋白的半衰期至少为8小时。叶绿体中免疫原性VLP的形成通过使用识别构象表位的抗体的捕获ELISA分析和电子显微镜确认。

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