Detection of race 1 strains of Ralstonia solanacearum in field samples in Taiwan using a BIO-PCR method |
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Authors: | Chih-Hung Lin Shih-Tien Hsu Kuo-Ching Tzeng Jaw-Fen Wang |
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Affiliation: | (1) Department of Plant Pathology, National Chung Hsing University, Taichung, Taiwan, 40227, Republic of China;(2) AVRDC—The World Vegetable Center, P.O. Box 42, Shanhua, Tainan, Taiwan, 74199, Republic of China |
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Abstract: | Bacterial wilt caused by race 1 strains of Ralstonia solanacearum is endemic on tomato produced in diverse agro-ecosystems in Taiwan. Using a new BIO-PCR protocol developed in this study, R. solanacearum was detected in soil, weed, and water samples collected from eight fields with different disease histories and cropping systems located in major tomato production areas. The sensitivity of the BIO-PCR was 1.9 CFU ml−1 and 17 CFU g−1 of soil for pure suspension and infested soil, respectively. The positive detection frequency of the BIO-PCR method was 66.6, 39.6, 23.1, and 31.8% for all tested samples of soil, weed rhizosphere soil, weed root, and water, respectively, and was higher than plating on MSM-1 medium. Detection of R. solanacearum from field soil indicated that spatial distribution of the pathogen in the field was not even regardless of the presence or absence of the disease and the different agro-ecosystems where the sampled fields were located, and the degree of unevenness was higher when tomato was absent from the field. Weed rhizosphere soils could be good sampling targets to monitor the pathogen in the field, because a higher positive detection proportion and population of R. solanacearum were found in the rhizosphere rather than the root of the collected weed samples. Symptomless weeds and contaminated irrigation, standing, or drainage waters were found to be important for the over-season survival and dissemination of R. solanacearum. |
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Keywords: | Spatial distribution Sampling Selective medium Soil Weed Water |
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