Kit used for detecting swine salmonella antibody
A kit, Salmonella technology, applied in the direction of measuring devices, instruments, scientific instruments, etc., to achieve the effect of easy operation, good repeatability, and reduce the rate of missed detection
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Embodiment 1
[0044] Example 1 Construction of pET-32a-fljB prokaryotic expression plasmid
[0045] Primer design and synthesis, designed primers to amplify the fljB gene, for the same conserved region of the same target gene, the inventor designed multiple pairs of primers:
[0046] F0 F: CGCGGATCCATGGCACAAGTAATCAACACTAACAG (SEQ ID NO. 5)
[0047] F0 R: CCGCTCGAGTTAACGTAACAGAGACAGCACGTT (SEQ ID NO. 6)
[0048] F1 F: CGCGGATCCATGGCACAAGTAATCAACACTAACAGT (SEQ ID NO. 1)
[0049] F1 R: CCGCTCGAGTTAACGTAACAGAGACAGC (SEQ ID NO. 2)
[0050] F2 F: CGCGGATCCATGGCACAAGTAATCAACAC (SEQ ID NO. 7)
[0051] F2 R: CCGCTCGAGTTAACGTAACAGAGACAGC (SEQ ID NO. 8)
[0052] From the electropherogram of the amplified product, see figure 1 , the F2 primer was not amplified, although both F0 and F1 were amplified, but after sequencing, it was found that there were many mutations in F0, such as figure 2 , and finally the inventors selected all correct F1 primers for sequencing as amplification primers.
[005...
Embodiment 2
[0060] Example 2 Prokaryotic expression and purification of recombinant protein
[0061] 1. For the colony pET-32a-fljB with the correct sequence in Example 1, pick a single colony and inoculate it in liquid LB medium containing Amp+, shake overnight at 37°C. Take the overnight culture and inoculate it in the liquid LB medium containing Amp+ in an amount of 2%, shake it at 37°C until the A600 value is 0.5-1.0, add IPTG to the final concentration of 1mM, shake it at 30°C and 37°C respectively, and At different times of culture (0, 3, 6, 10 h), take 1 mL of the bacterial solution from the culture and transfer it to a centrifuge tube, centrifuge at 10,000 r / min for 5 min, collect the bacterial pellet, resuspend the pellet and ultrasonically break it, and then 4000 r / min Min and then centrifuged for 10 min, respectively take 10 μL of supernatant and precipitate, add 90 μL 2×loading buffer and 10 μL 1mol / L DTT to suspend and mix, boil for 5 min, and perform SDS-PAGE electrophoresis...
Embodiment 3
[0065] The establishment of embodiment 3 ELISA and condition optimization
[0066] 1. Reagents for ELISA detection
[0067] (1) Coating solution: 0.05mol / L carbonate buffer solution, stored at 4°C.
[0068] (2) Sample diluent: phosphate-Tween buffer containing 1% bovine serum albumin (BSA).
[0069] (3) Blocking solution: phosphate-Tween buffer containing 5% bovine serum albumin (BSA).
[0070] (4) Enzyme-labeled secondary antibody: goat anti-pig IgG / HRP.
[0071] (5) Substrate buffer (phosphate-citrate buffer (PBS, pH5.0): 0.2mol Na 2 HPO 4 12H 2 O25.7mL, 0.1mol citric acid 24.3mL, deionized water 50mL.
[0072] (6) TMB substrate chromogenic solution: 0.01g TMB dry powder was dissolved in 1mL DMSO, and 9.9mL substrate buffer was added to 30μL H 2 o 2 , and then add 100 μL of TMB dissolved in DMSO.
[0073] (7) stop solution (2M H 2 SO 4 ): distilled water 178.3mL, add concentrated 2M H 2 SO 4 21.7mL.
[0074] (8) 0.05% PBST: Add 0.5 mL of Tween-20 to 1 L of PBS...
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