Abstract
Abstract The detection efficiency of the PCR methods for Xanthomonas euvesicatoria pv. perforans (Xep) was determined. Xep specific primer set; HpaF-f/HpaF-r was compared with the previously reported Bs-XpF/Bs-XpR primers in multiplex PCR reaction and singleplex PCR for detection of Xep were tested. The improvement of PCR amplification efficacy was investigated by adding PCR additives or either 5% DMSO or 1 M betaine. Adding both PCR additives gave the same lowest detection limit of Xep detection in both multiplex and singleplex PCR at 100 fg. However, multiplex PCR gave no equal amplification rate for both sets of primers and also showed cross-amplification to X. vesicatoria. Then singleplex PCR with both PCR additives was further tested in a tomato seed lot. The artificially inoculated tomato seeds with various concentrations of Xep from 1.05 x 105 to 101 CFU/ml were tested with singleplex PCR. The lowest detection limit was 101 CFU/ml of the 5 replications of each inoculated seed. One artificially inoculated tomato seed from each bacterial cell suspension was mixed with 2,000 healthy seeds making 0.05% (1/2,000) contaminated tomato seeds sample and further tested with singleplex PCR, results showed the detection limit of 101 CFU/ml in 0.05% Xep contaminated seed lot. Keywords: PCR additives, Seed, Bacterial leaf spot, Tomato, Conventional PCR
Published Version
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