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The utilization of the Hmg2 inducible promoter to genetically engineer parasite resistance in tobacco.

机译:Hmg2诱导型启动子在遗传上改造烟草中的寄生虫抗性的用途。

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摘要

The cyst nematode, Globodera tabacum tabacum Behrens, and the parasitic angiosperm, Egyptian broomrape, Orobanche aegyptiaca Pers., are obligate root parasites that cause severe yield and quality loss of many important crop hosts. Although these represent two diverse classes of parasites, they have significant similarities in the modes of parasitism and complex interactions with their hosts. Conventional control methods have had limited success in controlling these parasites. The overall objective of this research was to engineer resistance to the cyst nematode and Egyptian broomrape by expressing genes encoding parasite specific toxins under the control of parasite-responsive promoters using tobacco (Nicotiana tabacum L. cv. Xanthi). For nematode resistance, an anti-feeding strategy was employed utilizing the tomato proteinase inhibitor I (PI-I) gene as a nematode specific toxin. Transgenic tobacco plants were generated that expressed genes encoding an intracellarly retained or secreted form of tomato PI-I under the control of the nematode-inducible promoter, derived from tomato (Lycopersicon esculentum L.) Hmg2 gene. Our goals were to determine the effectiveness of local PI-I expression on nematode resistance and to determine if intracellular or extracellular PI-I deposition enhances resistance. Two constructs were generated that contained either the coding region of the tomato PI-I gene, lacking the signal sequence (EMI), or the coding region of PI-I including the signal sequence (EM2), fused to the nematode-responsive Hmg2 promoter. Transgenic PI-I plants were inoculated with G. t. tabacum cysts and evaluated for nematode interactions. Our results suggest that local expression of intercellular of PI-I significantly reduced cyst production when compared to the nontransformed controls. For broomrape resistance, a well characterized R/avr gene pair, the tobacco N resistance gene and the tobacco mosaic virus replicase (TMV) gene, was utilized to create novel gene-for-gene resistance via a N gene-mediated hypersensitive response (HR) to limit broomrape parasitism. The bean (Phaselous vulgaris L.) chalcone synthase 8 (CHS8) promoter has been characterized as a broomrape-responsive promoter. We introduced the CHS8:TMV replicase gene construct into tobacco plants that contains an endogenous N gene. Transgenic tobacco plants were inoculated with O. aegyptiaca seeds and monitored for parasite attachment and development. The expression of the TMV replicase leads to a significant reduction in broomrape parasitism. These genetic engineering strategies show promise in enhancing resistance to these destructive parasites.
机译:线虫囊肿线虫(Blobens tabacum tabacum)和寄生被子植物埃及b帚(Orobanche aegyptiaca Pers)是专性根系寄生虫,会导致许多重要农作物寄主的严重减产和品质下降。尽管它们代表了两类不同的寄生虫,但它们在寄生虫的模式以及与宿主之间复杂的相互作用方面具有显着的相似性。传统的控制方法在控制这些寄生虫方面取得的成功有限。这项研究的总体目标是通过使用烟草表达表达在寄生虫反应性启动子控制下的寄生虫特异性毒素的基因,从而设计出对囊肿线虫和埃及扫帚的抗药性(烟草(Nicotiana tabacum L. cv。Xanthi))。对于线虫的抗性,采用了抗喂食策略,利用番茄蛋白酶抑制剂I(PI-1)基因作为线虫特异性毒素。产生了转基因烟草植物,其表达的基因编码在线虫诱导型启动子的控制下编码番茄PI-1的细胞内保留或分泌形式,所述启动子来源于番茄(Lycopersicon esculentum L.)Hmg2基因。我们的目标是确定局部PI-1表达对线虫抗药性的有效性,并确定细胞内或细胞外PI-1沉积是否增强抗药性。产生了两个构建体,其包含与信号线响应的Hmg2启动子融合的番茄PI-1基因的编码区,该编码区缺少信号序列(EMI),或者包含信号序列的PI-1的编码区(EM2)。 。将转基因PI-1植物接种G.t。烟草孢囊和线虫相互作用的评估。我们的结果表明,与未转化的对照相比,PI-1的细胞间局部表达显着降低了囊肿的产生。对于b帚抗性,利用特征明确的R / avr基因对,烟草N抗性基因和烟草花叶病毒复制酶(TMV)基因,通过N基因介导的超敏反应(HR)来创建新的基因对基因抗性。 )以限制扫帚寄生。豆(Phaselous vulgaris L.)查尔酮合酶8(CHS8)启动子已被表征为扫帚反应性启动子。我们将CHS8:TMV复制酶基因构建体引入含有内源性N基因的烟草植物中。将转基因烟草植物用埃及古埃及种接种,并监测寄生虫的附着和发育。 TMV复制酶的表达导致扫帚寄生虫的显着减少。这些基因工程策略显示出增强对这些破坏性寄生虫的抵抗力的希望。

著录项

  • 作者

    Winston, Eugenia Michele.;

  • 作者单位

    Virginia Polytechnic Institute and State University.;

  • 授予单位 Virginia Polytechnic Institute and State University.;
  • 学科 Biology Molecular.Agriculture Plant Pathology.Agriculture Plant Culture.
  • 学位 Ph.D.
  • 年度 2003
  • 页码 138 p.
  • 总页数 138
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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