Porcine Japanese B Encephalitis Virus Swine Influenza Test Kit Ab ELISA 192 Wells/Kit GMP

Porcine Japanese B Encephalitis Virus Ab ELISA Kit 192 Wells/Kit GMP

1. Usage

The Porcine Japanese B Encephalitis Virus IgG Antibody ELISA test kit is used for the detection of the porcine encephalitis virus IgG antibodies in swine serum; assessment the immunity conditions against porcine encephalitis virus, serological diagnosis of pig infection in the pig farms and investigation of the epidemiology of the porcine encephalitis virus.

2. Principle

The GreenSpring® Porcine Japanese B Encephalitis Virus IgG antibody ELISA test kit is made from the antigen coated microtiter plate(coated with JEV antigen) and other reagents. It applies the Solid-phase ELISA principle to JEV-IgG in serum, then add enzyme conjugate to specifically bind with complex of coated antigen+JEV-IgG+enzyme labeled anti-pig-IgG antibody on the microplate. With the TMB substrate, it will generate an amount of color. The depth of color is relative with the content of the JEV-IgG, when the value of color is greater than the cut-off value, the pigs are vaccinated well or natural infected exist.

3. The kit components

4. Materials Required But Not Provided

1) Microplate Reader (double-wave length: 450/630 nm).
2) Precise micropipette (single-channel 1-100ul,0.5-10ul,multi-channel 30-300ul)
3) Constant temperature box or water bath box.
4) Oscillator.
5) Disposable tips (10ul, 200ul)
6) Deionized water

5. Sample requirement

1) The samples are porcine serum, which should be collected with no bacteria. The storage time should be less than 1 week at 2-8 ℃, if for long term, it should be kept at -20℃.
2) Avoid to use the samples with severe hemolysis, precipitate, contaminated by bacteria or protein suspension.

6. Preparation

1) Bring ELISA reagents to the room temperature (20-25 ℃) for 30 min to get best results, open the Microplate after return to room temperature and moisture dry.
2) Sample dilute: Dilute sample with the sample diluent solution at 40 times.(eg. 5ul serum sample + 195ul sample diluent solution )
3) Washing solution preparation: Dilute the20×concentrated washing buffer with deionized water at 20 times. (eg.50ml 20×concentrated washing buffer + 950ml deionized water ), if there is crystallization in the 20×concentrated washing buffer, it is normal, dissolve it at 37℃.

7. Test Procedure

1) Take out the coated plates (Can be detached) and record the sample position on a worksheet. Set 2 wells for negative control serum, add undiluted negative control serum, 2 wells for positive control serum, add undiluted positive control serum, 100μL/well. Others are sample wells, add the diluted sample, 100μL/well.
2) Mix gently, cover and incubate at 37℃ for 30 min.
3) Remove adhesive foil. Pour the liquid out of the wells, add the diluted Washing buffer into each well fully, be static for 10s and pour out. Repeat 3 times, at last time pat to dry on absorbent paper.
4) Add 100μL enzyme conjugate into each well.
5) Cover plate with new adhesive foil. Mix gently,Incubate at 37 ℃ for30 min.
6) Repeat step 3(washing).
7) Add substrate 100ul into each well, mix properly,incubate for 10 min at37℃ in the dark with new adhesive foil.
8) Add stop solution 50μL into each well, mix gently and determine the result.
9) Measure the OD value of each well with a photometer at dual-wave length 450nm/630nm.

8. Results

For the assay to be valid, the positive control wells’ average OD value must be greater than or equal to 0.6, and the negative control wells’ average OD value is less than 0.1. Otherwise the test is invalid, need test again.
The result is judged by S/P value,
S/P=(Sample OD450/630- NCx(—))/( PCx(—)- NCx(—)), NCx(—) means Negative control’s average OD450/630 value(calculate as 0.05 for value lower than 0.05), PCx(—) means Positive control’s average OD450/630 value
If S/P≥0.25, it is positive; less than 0.25, it is negative.

9. Precautions and warnings for users

1. This kit is for research use only.
2. Read the instructions carefully before running the test.
3. The experimental garbage should be sterilized with high pressure steam at 121℃ for 30 minutes, or treated with 5.0g/L sodium hypochlorite disinfectant for 30 minutes and then discarded.
4. Microplates removed from refrigeration should be equilibrated, dry at room temperature, and ready to be opened. Return unused microplates to dry foil bags and seal at 4 °C. Unused liquid reagents should be covered and stored with other components at 2-8°C away from light.
5. Samples and reagents should be added using a micropipette and frequently demonstrated for accuracy.
6. When adding wash buffer, it should be filled but not overflowed to avoid free enzyme or cross-contamination between wells.
7. The stop solution is corrosive, immediately rinse with plenty of water when it comes into contact with skin or clothes.

Specifications:96 wells×2.
Expiry date:12 months.
Storage:Store at 2~8℃, in the dark.
Production Date:On outer-packing of the test kit.

Q1: How long will it take for you to ship?
A1: Usually ships within 7 working days.

Q2: Do you support OEM/ODM?
A2: can be supported. We can customize according to your specific needs and specific quantities.

Q3: How is your factory doing in terms of quality control?
A3: We have ISO9001 certification and ISO13485 certification, so far all the production process, we have standard rules, we comply with the relevant behavior and laws of the government.

Q4: Is after-sales service guaranteed?
A4: We provide professional online technical after-sales service. If the product fails during the experiment, we can provide
one-to-one guidance through telephone, video and other forms.

Q5: What is your minimum order quantity?
A5: 1Kit.

Q6: What is the shipping method?
A6: It can be shipped by express (FEDEX, UPS, DHL, EMS, etc.) or by air and ground.Please confirm with us before placing an order.