关键词: 唐菖蒲伯克霍尔德菌, 荧光 PCR, 检测, 培养

Abstract: Objective To establish a fluorescent quantitative PCR ( q-PCR) method for detection of Burkholderia gladioli (B. gladioli) in laboratory mouse. Method the q-PCR method was established with the primers, probe and plasmid of B. gladioli which were synthesized according to the sequence published by Group Standard. And the linearity, sensitivity, repeatability and specificity of the method were verified. 110 samples of mice were tested for B. gladioli by the q-PCR method and bacterial culture method. Result The established q-PCR method for B. gladioli showed good linearity with correlation coefficient R 2 0. 998, and high sensitivity with a detection limit of 1 × 10 2 copies/ 5 μL. The assay could test specifically for B. gladioli with no cross reaction for Staphylococcus aureus, Klebsiella pneumoniae, Klebsiella oxytoca, Pseudomonas aeruginosa and Pasteurella pneumotropica. 110 samples were collected from euthanized mice and tested by bacterial culture and the q-PCR method respectively. The result with the two method were all negative, which were completely consistent. Conclusion The established q-PCR method had good performance and could be used for the detection of B. gladioli in laboratory mouse. 

Key words: Burkholderia gladioli, q-PCR, test, culture