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Gateway-compatible vectors for functional analysis of proteins in cell type specific manner

机译:网关兼容载体,用于细胞类型特定方式蛋白质的功能分析

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Genetically encoded fluorescent proteins are often used to label proteins and study protein function and localization in vivo. Traditional cloning methods mediated by restriction digestion and ligation are time-consuming and sometimes difficult due to the lack of suitable restriction sites. Invitrogen developed the Gateway cloning system based on the site-specific DNA recombination, which allows for digestion-free cloning. Most gateway destination vectors available for use in plants employ either the 35S or ubiquitin promoters, which confer high-level, ubiquitous expression. There are far fewer options for moderate, cell-type specific expression. Here we report on the construction of a Gateway-compatible cloning system (SWU vectors) to rapidly tag various proteins and express them in a cell-type specific manner in plants. We tested the SWU vectors using the HISTONE (H2B) coding sequence in stable transgenic plants. The SWU vectors are a valuable tool for low cost, high efficiency functional analysis of proteins of interest in specific cell types in the Arabidopsis root.
机译:遗传编码的荧光蛋白通常用于标记蛋白质和研究体内的蛋白质功能和定位。由限制消化和结扎介导的传统克隆方法是耗时的,有时由于缺乏合适的限制性位点而有时困难。 Invitrogen基于特异性DNA重组开发了网关克隆系统,其允许无消化的克隆。可用于植物的大多数网关目的地向量使用35s或泛素启动子,其赋予高水平的普遍表达。适度,单元格类型特定表达式的选项越来越少。在这里,我们报告了网关兼容的克隆系统(SWU向量)的构建,以快速标记各种蛋白质并以植物中的细胞类型特异性方式表达它们。我们使用稳定的转基因植物中使用组蛋白(H2B)编码序列来测试SWU载体。 SWU向量是拟南芥根中特定细胞类型的低成本,高效功能性分析的有价值的工具。

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