Diarrheogenic escherichia coli detection kit and detection and typing method thereof
A detection kit, Escherichia coli technology, applied in biochemical equipment and methods, material excitation analysis, microbial determination/inspection, etc., can solve the problems of low accuracy, low detection efficiency, single detection object, etc. Simple, high sensitivity, avoid false positive effect
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Embodiment 1
[0112] Embodiment 1 Preparation of Diarrheal Escherichia coli Detection Kit
[0113] 1. Synthesize primers and probes for nine genes of stp, sth, lt, aggR, eaeA, escV, stx1, stx2 and ipaH, namely SEQ ID NO: 1-SEQ ID NO: 27, wherein each probe sequence 3' Both ends are connected with DABCYL, and the fluorescent groups corresponding to each probe sequence are as follows:
[0114] SEQ ID NO:3 corresponds to HEX, SEQ ID NO:6 corresponds to FAM, SEQ ID NO:9 corresponds to ROX, SEQ ID NO:12 corresponds to Cy5,
[0115] SEQ ID NO:15 corresponds to Cy5, SEQ ID NO:18 corresponds to HEX, SEQ ID NO:21 corresponds to ROX, SEQ ID NO:24 corresponds to ROX, and SEQ ID NO:27 corresponds to FAM;
[0116] The Homo-tag sequence (SEQ ID NO:28) was synthesized and prepared into a stock solution with a concentration of 50 μM;
[0117] 2. Separately prepare PCR buffer, MgCl 2 solution, dNTP solution, rTaq enzyme solution;
[0118] 3. Take the PCR reaction eight tubes, add PCR buffer, MgCl 2 sol...
Embodiment 2
[0127] 1. Synthesize primers and probes for nine genes of stp, sth, lt, aggR, eaeA, escV, stx1, stx2 and ipaH, namely SEQ ID NO:1-SEQ ID NO:27, wherein each probe sequence 3' Both ends are connected with BHQ, and the fluorescent groups corresponding to each probe sequence are as follows:
[0128] SEQ ID NO:3 corresponds to FAM, SEQ ID NO:6 corresponds to ROX, SEQ ID NO:9 corresponds to Cy5, SEQ ID NO:12 corresponds to HEX,
[0129] SEQ ID NO:15 corresponds to FAM, SEQ ID NO:18 corresponds to FAM, SEQ ID NO:21 corresponds to Cy5, SEQ ID NO:24 corresponds to HEX, and SEQ ID NO:27 corresponds to ROX;
[0130]The Homo-tag sequence (SEQ ID NO:28) was synthesized and prepared into a stock solution with a concentration of 50 μM;
[0131] 2. Separately prepare PCR buffer, MgCl 2 solution, dNTP solution, rTaq enzyme solution;
[0132] 3. Take the PCR reaction eight tubes, add PCR buffer, MgCl 2 solution, dNTP solution, and rTaq enzyme solution, so that they meet the following final...
Embodiment 3
[0140] Example three specificity analysis
[0141] Obtained 204 strains related to Enterobacter, cocci, Vibrio and other bacteria, using the detection kit of Example 1 to carry out specificity experiments and using positive strains as a control, the situation of the detected strains is shown in Table 1, and the detection results were all negative.
[0142] Table 1 Specificity analysis results
[0143]
[0144]
[0145] The results in Table 1 show that the detection kit of Example 1 has good detection specificity, no non-specific amplification occurs, and the occurrence of false positives caused by non-specificity is avoided.
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