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Molecular characterization and development of diagnostic methods for the rapid detection of Cercospora beticola isolates with resistance to fungicides.

机译:分子特征和诊断方法的开发,可快速检测对杀真菌剂具有抗性的番茄锥孢菌。

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摘要

Cercospora leaf spot (CLS), caused by Cercospora beticola Sacc., is the most destructive foliar disease of sugar beet (Beta vulgaris L.) and various strategies are used for disease management such as the application of fungicides. Fungicide resistance has been reported in C. beticola and was associated with either mutations in the beta-tubulin and cytochrome b genes or an overexpression of the C14alpha--demethylase (Cyp51) gene. Molecular characterization was conducted on various fungicide-targeted sites to develop assays for the rapid detection of C. beticola resistance. A PCR-RFLP assay was developed for the rapid detection of benzimidazole resistance in C. beticola isolates due to a single nucleotide polymorphic (SNP) site on the beta-tubulin gene. The assay involving an in vitro digestion with a BstUI restriction enzyme found ~37% C. beticola benzimidazole-resistant isolates from the High Plains. A baseline analysis was performed on 66 C. beticola isolates to determine the genetic diversity of the Cyp51 gene and found three mutations that were unrelated to DMI resistance. We investigated the potential role of a silent mutation at codon 170 as a mechanism of C. beticola DMI resistance. However, results did not support the hypothesis that the silent mutation at codon 170 was associated with C. beticola DMI resistance mechanism. Molecular analysis of two C. beticola DMI-resistant isolates found no mutation suggesting DMI resistance may not be directly caused by a mutation in the Cyp51 gene. Genetic analysis of the cytochrome b gene (the site of action for quinone outside inhibitor fungicides) found identical partial sequences from 84 C. beticola isolates. Two C. beticola QoI-resistant isolates had a SNP in the cytochrome b gene and was predicted to lead to an amino acid substitution at position 143 (G143A). A PCR-RFLP assay was developed involving an in vitro digestion with a Fnu4HI restriction enzyme for the rapid detection of C. beticola QoI-resistance. Molecular analysis of 173 C. beticola isolates for mating-type idiomorphs distribution revealed ~80% had a MAT1-1 idiomorph and ~20% had a MAT1-2 idiomorph. This was a departure from an equal proportion of mating-type genes as reported for isolates from the Red River Valley region of the United States, Western Europe, parts of Iran, and New Zealand. Results indicated a sexual cycle was likely absent in the C. beticola population from the High Plains. Linkage disequilibrium was present between mating-type idiomorphs and C. beticola benzimidazole sensitivity (resistant or sensitive), indicating asexual reproduction may be dominant in the High Plains region.
机译:由锥状孢子虫(Cercospora beticola Sacc。)引起的锥状孢子叶斑病(CLS)是甜菜(Beta vulgaris L.)最具破坏性的叶面疾病,并且用于疾病管理的各种策略例如杀真菌剂的应用。杀虫剂的抗药性已在锥虫中被报道,并且与β-微管蛋白和细胞色素b基因的突变或C14alpha-脱甲基酶(Cyp51)基因的过表达有关。在针对杀真菌剂的各种位点上进行了分子表征,以开发用于快速检测锥状弯曲杆菌抗性的测定法。由于β-微管蛋白基因上有一个单核苷酸多态性(SNP)位点,因此开发了一种PCR-RFLP测定法,用于快速检测锥虫中的苯并咪唑耐药性。涉及用BstUI限制酶进行体外消化的测定法,从高原地区发现了〜37%的耐锥虫锥虫对苯并咪唑的分离株。对66个锥虫的分离株进行了基线分析,以确定Cyp51基因的遗传多样性,并发现了与DMI抗性无关的三个突变。我们调查了密码子170沉默突变作为C. beticola DMI抗性机制的潜在作用。但是,结果不支持这样的假设,即密码子170处的沉默突变与棉铃虫DMI抗性机制有关。两种对小麦弯曲杆菌DMI抗性分离株的分子分析发现,没有突变表明DMI抗性可能不是由Cyp51基因突变直接引起的。对细胞色素b基因(抑制剂杀真菌剂外醌的作用部位)的遗传分析发现来自84个锥虫的分离部分序列相同。两种对锥虫的QoI耐药的分离株在细胞色素b基因中具有SNP,预计会导致在位置143(G143A)处发生氨基酸取代。开发了一种PCR-RFLP检测方法,该方法涉及用Fnu4HI限制性内切酶进行体外消化,以快速检测线虫的QoI耐药性。针对交配型独特型分布对173个锥虫的分离株进行的分子分析显示,约80%的具有MAT1-1独特型,而约20%的具有MAT1-2独特型。这与来自美国,西欧,伊朗部分地区和新西兰的红河谷地区分离株报道的同等比例的交配型基因背离。结果表明,来自高平原的锥虫中可能没有性生活周期。交配型独特型和C. beticola benzimidazole敏感性(抗性或敏感性)之间存在连锁不平衡,表明无性繁殖可能在高原地区占主导地位。

著录项

  • 作者

    Obuya, James O.;

  • 作者单位

    University of Wyoming.;

  • 授予单位 University of Wyoming.;
  • 学科 Agronomy.;Agriculture.;Plant pathology.
  • 学位 Ph.D.
  • 年度 2014
  • 页码 204 p.
  • 总页数 204
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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