Rapid Detection of Cercospora beticola in Sugar Beet and Mutations Associated with Fungicide Resistance Using LAMP or Probe-Based qPCR

被引:17
作者
Shrestha, Subidhya [1 ,2 ]
Neubauer, Jonathan [2 ]
Spanner, Rebecca [1 ,2 ]
Natwick, Mari [2 ]
Rios, Joshua [2 ]
Metz, Nicholas [1 ,2 ,3 ]
Secor, Gary A. [1 ]
Bolton, Melvin D. [1 ,2 ]
机构
[1] North Dakota State Univ, Dept Plant Pathol, Fargo, ND 58108 USA
[2] ARS, USDA, Northern Crop Sci Lab, Fargo, ND 58102 USA
[3] Colorado State Univ, Soil & Crop Sci, Ft Collins, CO 80523 USA
基金
美国农业部;
关键词
benzimidazole; Cercospora beticola; Cercospora leaf spot (CLS); DMI; fungicide; G143A; loop-mediated isothermal amplification (LAMP); probe-based qPCR; sugar beet; LEAF-SPOT; MYCOSPHAERELLA-GRAMINICOLA; TIME; SENSITIVITY; MODEL; GUIDELINES; EVOLUTION; TOLERANT; STRAINS;
D O I
10.1094/PDIS-09-19-2023-RE
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
Cercospora leaf spot (CLS), caused by the fungal pathogen Cercospora beticola, is the most destructive disease of sugar beet worldwide. Although growing CLS-tolerant varieties is helpful, disease management currently requires timely application of fungicides. However, overreliance on fungicides has led to the emergence of fungicide resistance in many C. beticola populations, resulting in multiple epidemics in recent years. Therefore, this study focused on developing a fungicide resistance detection "toolbox" for early detection of C. beticola in sugar beet leaves and mutations associated with different fungicides in the pathogen population. A loop-mediated isothermal amplification (LAMP) method was developed for rapid detection of C. heticola in infected sugar beet leaves. The LAMP primers specific to C. beticola (Cb-LAMP) assay was able to detect C. beticola in inoculated sugar beet leaves as early as 1 day postinoculation. A quinone outside inhibitor (QoI)-LAMP assay was also developed to detect the G143A mutation in cytochrome b associated with Qol resistance in C. beticola. The assay detected the mutation in C. beticola both in vitro and in planta with 100% accuracy. We also developed a probe-based quantitative PCR (qPCR) assay for detecting an E198A mutation in 13-tubulin associated with benzimidazole resistance and a probe-based qPCR assay for detection of mutations in cytochrome P450-dependent sterol 14a-demethylase (Cyp51) associated with resistance to sterol demethylation inhibitor fungicides. The primers and probes used in the assay were highly efficient and precise in differentiating the corresponding fungicide-resistant mutants from sensitive wild-type isolates.
引用
收藏
页码:1654 / 1661
页数:8
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