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一种改良的多位点 Gateway 克隆策略,用于植物中基因的整合。

A modified MultiSite gateway cloning strategy for consolidation of genes in plants.

机构信息

Department of Crop Physiology, University of Agricultural Sciences, GKVK Campus, Bangalore 560065, India.

出版信息

Mol Biotechnol. 2013 Feb;53(2):129-38. doi: 10.1007/s12033-012-9499-6.

DOI:10.1007/s12033-012-9499-6
PMID:22274939
Abstract

The genome information is offering opportunities to manipulate genes, polygenic characters and multiple traits in plants. Although a number of approaches have been developed to manipulate traits in plants, technical hurdles make the process difficult. Gene cloning vectors that facilitate the fusion, overexpression or down regulation of genes in plant cells are being used with various degree of success. In this study, we modified gateway MultiSite cloning vectors and developed a hybrid cloning strategy which combines advantages of both traditional cloning and gateway recombination cloning. We developed Gateway entry (pGATE) vectors containing attL sites flanking multiple cloning sites and plant expression vector (pKM12GW) with specific recombination sites carrying different plant and bacterial selection markers. We constructed a plant expression vector carrying a reporter gene (GUS), two Bt cry genes in a predetermined pattern by a single round of LR recombination reaction after restriction endonuclease-mediated cloning of target genes into pGATE vectors. All the three transgenes were co-expressed in Arabidopsis as evidenced by gene expression, histochemical assay and insect bioassay. The pGATE vectors can be used as simple cloning vectors as there are rare restriction endonuclease sites inserted in the vector. The modified multisite vector system developed is ideal for stacking genes and pathway engineering in plants.

摘要

基因组信息为操纵植物基因、多基因性状和多种性状提供了机会。尽管已经开发了许多方法来操纵植物的特性,但技术障碍使得这一过程变得困难。基因克隆载体促进了植物细胞中基因的融合、过表达或下调,并且在不同程度上取得了成功。在这项研究中,我们修改了 gateway MultiSite 克隆载体,并开发了一种杂交克隆策略,该策略结合了传统克隆和 gateway 重组克隆的优势。我们开发了带有 attL 位点侧翼的多个克隆位点的 Gateway 入口(pGATE)载体和带有不同植物和细菌选择标记的特定重组位点的植物表达载体(pKM12GW)。我们构建了一个携带报告基因(GUS)的植物表达载体,通过将靶基因用限制性内切酶介导克隆到 pGATE 载体中,然后进行一轮 LR 重组反应,以预定的模式携带两个 Bt cry 基因。所有三个转基因都在拟南芥中共同表达,这可以通过基因表达、组织化学分析和昆虫生物测定来证明。pGATE 载体可以作为简单的克隆载体使用,因为载体中插入了很少的限制性内切酶位点。开发的改良多定位载体系统非常适合在植物中进行基因叠加和途径工程。

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