Cronobacter sakazakii strain detecting method, kit and primer
A technology of Cronobacter and a kit, which is applied in the field of microbial detection, can solve the problems of long detection time and achieve the effects of short detection time, simple result judgment, and improved detection efficiency
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Embodiment 1
[0026] PCR detection method of Cronobacter strains
[0027] Step 1, primer synthesis
[0028] Synthesize primers capable of PCR amplifying the conserved sequence in the Cronobacter gyrB gene sequence (synthesized by Shanghai Sangon Bioengineering Technology Service Co., Ltd.), the primer sequence is as follows:
[0029] SEN2-L: 5'-ATGGATAAAGAGGGCTACAG-3' (SEQ ID NO: 1),
[0030] SEN2-R: 5'-CGCCTGATTCTTACGGTTAC-3' (SEQ ID NO: 2).
[0031] Step 2, the system and reaction parameters of the PCR detection method
[0032] Using the above primers, using the genomic DNA of the standard strain of Cronobacter genus as a template, the PCR reaction system and reaction procedures were established and optimized. After single factor, multifactor experiments and hybridization experiments, it was found that the following reaction systems and reaction procedures can be A single amplification product of about 438bp was obtained. The PCR reaction system is: 1×PCR reaction buffer, 10-15mmol / L ...
Embodiment 2
[0045] Detection of artificial contamination of Cronobacter sakazakii standard strain ATCC25944
[0046] Preparation of artificially contaminated samples: Mix 10mL of milk with 89mL of liquid TSB medium, add 1mL of diluted Kronobacter sakazakii ATCC2594 pure culture solution (7CFU / mL), at 37°C, 150r / min Under culture for 12h. Samples were taken every 2 hours, genomic DNA was extracted by water boiling, and PCR detection was carried out according to the optimized conditions. The PCR detection method for Cronobacter strains established in Example 1 was used for PCR detection, and the bacteria could be detected 8 hours after artificial contamination.
[0047]
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