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Development of Beet necrotic yellow vein virus‐based vectors for multiple‐gene expression and guide RNA delivery in plant genome editing

机译:植物基因组中的多基因表达的BEET坏死黄静脉病毒 - 基于BEET坏死的黄静脉病毒的载体

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Many plant viruses with monopartite or bipartite genomes have been developed as efficient expression vectors of foreign recombinant proteins. Nonetheless, due to lack of multiple insertion sites in these plant viruses, it is still a big challenge to simultaneously express multiple foreign proteins in single cells. The genome of Beet necrotic yellow vein virus (BNYVV) offers an attractive system for expression of multiple foreign proteins owning to a multipartite genome composed of five positive‐stranded RNAs. Here, we have established a BNYVV full‐length infectious cDNA clone under the control of the Cauliflower mosaic virus 35S promoter. We further developed a set of BNYVV‐based vectors that permit efficient expression of four recombinant proteins, including some large proteins with lengths up to 880 amino acids in the model plant Nicotiana benthamiana and native host sugar beet plants. These vectors can be used to investigate the subcellular co‐localization of multiple proteins in leaf, root and stem tissues of systemically infected plants. Moreover, the BNYVV‐based vectors were used to deliver NbPDS guide RNAs for genome editing in transgenic plants expressing Cas9, which induced a photobleached phenotype in systemically infected leaves. Collectively, the BNYVV‐based vectors will facilitate genomic research and expression of multiple proteins, in sugar beet and related crop plants.
机译:许多植物病毒具有单氨酸或二分离基因组的病毒已成为外国重组蛋白的有效表达载体。尽管如此,由于这些植物病毒中缺乏多种插入位点,因此在单细胞中同时表达多种外来蛋白质仍然是一个很大的挑战。甜菜坏死黄静脉病毒(BNYVV)的基因组提供了一种有吸引力的系统,用于表达多种外来蛋白质,其具有由五个正链RNA组成的多重基因组。在这里,我们在Cauliflower马赛克病毒35s启动子的控制下建立了BNYVV全长传染cDNA克隆。我们进一步开发了一系列基于BNYVV的载体,其允许有效表达四种重组蛋白质,包括一些大蛋白质,其中一些大蛋白质在模型植物尼古利亚纳·尼沙米纳和天然宿主甜菜植物中长达880个氨基酸。这些载体可用于研究在系统感染植物的叶片,根和干组织中的多种蛋白质的亚细胞共定位。此外,基于BNYVV的载体用于在表达CAS9的转基因植物中递送NBPDS指导RNA用于基因组编辑,其在系统感染的叶片中诱导光漂白的表型。集体,基于BNYVV的载体将促进甜菜和相关作物植物中多种蛋白质的基因组研究和表达。

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