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Development of Viral Vectors Based on Citrus leaf blotch virus to Express Foreign Proteins or Analyze Gene Function in Citrus Plants

机译:基于柑橘叶片斑点病毒表达外源蛋白质或分析柑橘植物基因功能的病毒载体的开发

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Viral vectors have been used to express foreign proteins in plants or to silence endogenous genes. This methodology could be appropriate for citrus plants that have long juvenile periods and adult plants that are difficult to transform. We developed viral vectors based on Citrus leaf blotch virus (CLBV) by duplicating a minimum promoter (92 bp) either at the 3′ untranslated region (clbv3′pr vector) or at the intergenic region between the movement and coat protein (CP) genes (clbvINpr vector). The duplicated fragment (–42/+50) around the transcription start site of the CP subgenomic RNA (sgRNA) had the full promoter activity and induced synthesis of a new sgRNA in infected plants. Agroinoculation with these vectors resulted in systemic infection of Nicotiana benthamiana and the resulting virions systemically infected citrus plants. A clbvINpr vector carrying the green fluorescent protein (GFP) gene expressed GFP in citrus plants and triggered gfp silencing in gfp-transgenic citrus plants, and vectors carrying fragments of the phytoene desaturase or the magnesium chelatase genes incited a silencing phenotype in citrus plants. These silenced phenotypes persisted in successive flushes. Because CLBV infections are symptomless in most citrus species, the effective silencing induced by CLBV-derived vectors will be helpful to analyze citrus gene function.
机译:病毒载体已用于在植物中表达外源蛋白质或沉默内源基因。该方法可能适用于幼年长的柑橘类植物和难以转化的成年植物。我们通过在3'非翻译区(clbv3'pr载体)或运动与外壳蛋白(CP)基因之间的基因间区域复制最小启动子(92 bp),开发了基于柑桔叶斑点病毒(CLBV)的病毒载体(clbvINpr向量)。 CP亚基因组RNA(sgRNA)转录起始位点周围的重复片段(–42 / + 50)具有完整的启动子活性,并在受感染植物中诱导了新sgRNA的合成。用这些载体进行农杆菌接种会导致本氏烟草的系统感染,并导致病毒体被系统感染的柑橘类植物感染。带有绿色荧光蛋白(GFP)基因的clbvINpr载体在柑桔植物中表达GFP,并在转基因的柑桔植物中引发gfp沉默,而带有八氢番茄红素去饱和酶或镁螯合酶基因片段的载体在柑桔植物中引发了沉默表型。这些沉默的表型在连续的潮红中持续存在。由于在大多数柑橘类物种中,CLBV感染无症状,因此,由CLBV衍生的载体诱导的有效沉默将有助于分析柑橘类基因的功能。

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