Detection of Vibrio cholerae by isothermal cross-priming amplification combined with nucleic acid detection strip analysis

• A new isothermal cross-priming amplification method was developed to detect all V. cholerae.
• The efficiency and accuracy of detection were improved by using nucleic acid detection strips.
• The method exhibits higher sensitivity and convenience than LAMP method.
• The sensitivity of the method is similar with real-time PCR in artificially contaminated samples detection.

Vibrio cholerae is a water- and food-borne human pathogen, and V. cholerae serotypes O1 and O139 have attracted attention because of their severe pathogenesis. However, non-O1, non-O139 cholera vibrios (NCVs) were also recently recognized as having virulence properties. In this study, we developed a cross-priming amplification (CPA) method for the detection of all serotypes of V. cholerae. The specificity of the CPA method was tested using a panel of 60 different bacterial strains. All of the V. cholerae strains showed positive results, and 41 other types of bacteria gave negative results. The limit of detection of the CPA method was 79.28 fg of genomic DNA, 4.2 × 102 CFU/ml for bacteria in pure culture, and 5.6 CFU per 25 g of sample with pre-enrichment. This method showed a higher sensitivity than the loop-mediated isothermal amplification (LAMP) method did and was more convenient to perform. These results indicate that the CPA method can be used for the rapid preliminary screening of V. cholerae.