Quantitative assessment of phytopathogenic fungi in various substrates using a DNA macroarray

生物 大丽花黄萎病 聚合酶链反应 茄丝核菌 尖孢镰刀菌 DNA提取 索拉尼镰刀菌 实时聚合酶链反应 计算生物学 微生物学 植物 遗传学 基因
作者
Bart Lievens,Margreet Brouwer,A. Vanachter,C. André Lévesque,Bruno P.A. Cammue,Bart P. H. J. Thomma
出处
期刊:Environmental Microbiology [Wiley]
卷期号:7 (11): 1698-1710 被引量:129
标识
DOI:10.1111/j.1462-2920.2005.00816.x
摘要

Summary Detection, identification and quantification of plant pathogens are the cornerstones of preventive plant disease management. To detect multiple pathogens in a single assay, DNA array technology currently is the most suitable technique. However, for sensitive detection, polymerase chain reaction (PCR) amplification before array hybridization is required. To evaluate whether DNA array technology can be used to simultaneously detect and quantify multiple pathogens, a DNA macroarray was designed and optimized for accurate quantification over at least three orders of magnitude of the economically important vascular wilt pathogens Verticillium albo‐atrum and Verticillium dahliae . A strong correlation was observed between hybridization signals and pathogen concentrations for standard DNA added to DNA from different origins and for infested samples. While accounting for specific criteria like amount of immobilized detector oligonucleotide and controls for PCR kinetics, accurate quantification of pathogens was achieved in concentration ranges typically encountered in horticultural practice. Subsequently, quantitative assessment of other tomato pathogens ( Fusarium oxysporum , Fusarium solani , Pythium ultimum and Rhizoctonia solani ) in environmental samples was performed using DNA array technology and correlated to measurements obtained using real‐time PCR. As both methods of quantification showed a very high degree of correlation, the reliability and robustness of the DNA array technology is shown.
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