SKU: AFG-VGS-07

AffiVET® Avian Marek's Disease Virus Antibody Elisa Kit

Vendor AffiGEN
Regular price CHF 385.00
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Avian Marek's disease virus antibody ELISA kit    

1. Usage

This kit is used to detect Avian Marek's disease virus(MDV) antibody in chicken serum, to assess antibody condition by Avian Marek's disease vaccine in chicken farm and assist diagnosis of serological infected chicken.

2. Principle

The Avian Marek's disease antibody ELISA kit is based on an indirect enzymatic immunoassay (Indirect ELISA).The purified MDV antigen is coated on plates. When testing, add the diluted serum sample, after incubation, if the serum sample contains specific antibodies against MD virus, they will bind to the antigen coated on plates. Wash the unbound antibodies and other components. Then add a specific enzyme conjugate, it will combine the antigen-antibody combination on plates. After incubation and washing, discard the uncombined enzyme conjugate; add the TMB substrate. A colorimetric reaction will appear, add stop solution, measured OD value by a spectrophotometer (450 nm).

3. Reagents

1

MD antigen coated microtiter strips

1/2 pieces

7

Stop solution

6/11 mL

2

EnzymeConjugate

11/21 mL

8

Negative control

0.8/1.6 mL

3

10× washing solution

50/100 mL

9

Positivecontrol

0.8/1.6 mL

4

Substrate A solution

6/11 mL

10

Serum dilution plate

1/2 pieces

5

SubstrateBsolution

6/11 mL

11

Adhesive film

2/4 pieces

6

Sample dilution

50/100 mL

12

Instruction

1 piece

4.Materials required but not provided

1) Micropipettors and disposable tips: 0.5μL~10μL、10μL~100μL、100μL~1000μL

2) 37 ℃ Incubator

3) Measuring cylinder: 500 ml

4) 96 wells microplate reader

5) Distilled water or deionied water

6) Bottle or microplate washing machine 

5. Sample preparation

Take animal whole blood, make serum according to regular methods, the serum should be clear, have no hemolysis.

6. Preparation of washing buffer

Return washing solution to room temperature before use, if there is salty crystals, shake to make the crystals dissolve, then use distilled water or deionized water to dilute it at 10 times. The diluted washing solution can store for 1 week at 4 ℃.

7. Sample dilution

At serum dilution plate, dilute serum at 1:99 with sample dilution (for example: 495μL sample diluent + 5μL serum)

Notice: Negative control and Positive control do not need dilute. Exchange tip after taking sample every time, record the situation of the sample on plate accurately. Shake the sample evenly before adding it.

8. Notes

1) All reagents should be adjusted to the room temperature and shake evenly before using, store at 2-8 ℃after using

2) Do not exchange the reagents from the kits of different lot numbers to use. Avoid reagent pollution when using.

3) Substrate and stop solution may have excitant to skin and eyes, pay attention when using.

4) Do not expose TMB (Substrate B) to light and avoid it contact with antioxidants.

5) The wells should avoid damp or touching water after unsealing (Put the un-using microplate back to bag with dehydrator in 2~8 ℃soon )

6) Deal all waste reasonable before dumping to avoid pollution.

7) Strictly adhere to instruction to get best result. All procedure including pipetting, timing and washing etc. must be accurate.

8) Serum dilution plate is disposable, do not use for second time; the MAX volume of it is 300μL/well.

9. ELISA procedure

1) Take pre-coated microplate (Can unseal for several time use as per sample quantity), add 100μL diluted serum to a well, meanwhile set 1 wells for Negative control, Positive control and blank control wells separately. Add 100μL Negative/Positive control to its wells, only add 100μL sample dilution in the blank control well. Shake softly (do not spill),incubate at 37℃ for 30 min.

2) Pour the liquid out of the wells, add 300 μL diluted washing solution to each well, static for 1 min, pour out. Repeat 3 times, then pat to dry on absorbent paper.

3) Add 100 μL Enzyme Conjugate to each well, andincubate at 37℃ for 30 min.

4) Repeat the step 2(washing). Remember pat to dry on absorbent paper at last.

5) Add 50 μL substrate A, then substrate B (50 μL) to each well, mix properly,react for 10 min at 37℃ in dark.

6) Add 50 μL stop solution in each well, and measure the result within 10 min.

10. Results

Set zero for the blank well, and test the A450nm (630 nm as a reference) value on the microplate-reader. The conditions for the test to be tenable are that the positive control wells’ A450nm value is greater than or equal to 0.6, and the negative control wells’ A450nm value is less than 0.15. If the test is invalid, the operation is in doubt, retest and observe all the reagents carefully.

If the sample’s A450 value is greater than 0.2+ absorbance of negative control mean, it is judged to be positive; and if less than 0.2+ absorbance of negative control mean, negative. If absorbance of negative control mean is less than 0.05, calculate as 0.05

Specifications: 96 wells/kit or 96*2 wells/kit.

Expiry date:12 months.

Storage: Storing at 2-8℃, in the dark.