Kit for detecting eight staphylococcus aureus drug-resistance genes and detection method
A drug-resistant gene and Staphylococcus technology, which is applied in the field of high-resolution melting curve HRM analysis and fluorescent PCR, can solve the problems that the research of multiple fluorescent PCR detection has not been reported, so as to avoid cross-contamination, simplify the detection process, and shorten the detection time Effect of Cycle Time and Inspection Cost
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Embodiment 1
[0066] Use fluorescent PCR of the present invention in conjunction with HRM analysis technology to detect eight kinds of drug-resistant genes of Staphylococcus aureus
[0067] DNA extraction and PCR reaction
[0068] Take 1.5 mL of the culture and centrifuge at 10,000 rpm for 2 min; add 500 μL of TE buffer to the precipitate, resuspend it by pipetting repeatedly, add 30 μL of 10% SDS and 15 μL of proteinase K, mix well, and incubate at 37°C for 1 h; L NaCl, mix well, then add 80ul CTAB / NaCl solution, mix well and then incubate at 65°C for 10min; add an equal volume of phenol / chloroform / isoamyl alcohol and mix well, centrifuge for 4-5min, transfer the supernatant to a Add 0.8 times the volume of isopropanol to a new tube, and mix gently until the DNA precipitates; after the precipitate is washed with 1 mL of 70% ethanol, add TE solution to dissolve the precipitate, and then take 1 μL of the extract and add it to the following reaction system:
[0069]
[0070] Carry out PCR...
Embodiment 2
[0076] The present invention can simultaneously detect eight kinds of drug-resistant gene kits of Staphylococcus aureus, wherein the reaction system in the non-labeled fluorescent PCR amplification process consists of the following components:
[0077]
[0078] Wherein said upstream primers include:
[0079] The upstream primer of methicillin-resistant gene mecA: GCAATCGCTAAAGAACTA
[0080] erythromycin resistance gene ermc upstream primer: TGCCATTGAAATAGACCA
[0081] TetM upstream primer for tetracycline resistance gene: AAAATCCGCACCCCTCTAC
[0082] Aminoglycoside resistance gene aph3 upstream primer: AAAATACCGCTGCGTAAA
[0083] Disinfectant resistance gene qacA / qacB upstream primer: GGGTCGTGTTATTAGGCA
[0084] Vancomycin resistance gene vanA upstream primer: TGAATCGGCAAGACAATA
[0085] Mupirocin resistance gene mupA upstream primer: TCACGAATACGCACCAAG
[0086] The upstream primer of drug resistance accessory gene femB: CGAATCGTGGTCCAGTAA
[0087] Described downstrea...
Embodiment 3
[0099] A detection method of the present invention comprises the following steps:
[0100] A, according to eight kinds of Staphylococcus aureus drug-resistant gene design primer pairs;
[0101] B. After extracting the sample DNA, use the designed primer pair to perform fluorescent PCR amplification;
[0102] C. Use a fluorescent quantitative PCR instrument with an HRM module to perform HRM analysis on the PCR amplification product, determine the Tm value of the amplification product, and then determine the result;
[0103] Wherein the fluorescent PCR amplification reaction system in step B is made up of the following components:
[0104]
[0105]
[0106] Wherein said upstream primers include:
[0107] The upstream primer of methicillin-resistant gene mecA: GCAATCGCTAAAGAACTA
[0108] erythromycin resistance gene ermc upstream primer: TGCCATTGAAATAGACCA
[0109] TetM upstream primer for tetracycline resistance gene: AAAATCCGCACCCCTCTAC
[0110] Aminoglycoside resist...
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