Olaquindox (OQX) ELISA Test KitThe Olaquindox (OQX) ELISA Test Kit is based on a competitive colorimetric ELISA assay.The Olaquindox has been coated in the plate wells. During the analysis, sample is added along with the Olaquindox antibody. If the Olaquindox residue is present in the
The Olaquindox (OQX) ELISA Test Kit is based on a competitive colorimetric ELISA assay.
The Olaquindox has been coated in the plate wells. During the analysis, sample is added along with the Olaquindox antibody. If the Olaquindox residue is present in the sample, it will compete for the Olaquindox antibody, thereby preventing the antibody attached to the well, last, take coloration with TMB substrate. The samples A value is an inverse relationship with OQX residue content. Lastly, compared with the standard curve can be concluded the OQX residues in sample.
| Manufacturer | Shandong xinyu Biotechnology Co., LTD |
|---|---|
| Trademark | Xinyubio |
| Production lot number | EOQX(FA)240710 |
| Analyte | Olaquindox |
| Sample type | feed,etc |
| Method | Enzyme-linked immunosorbent assay (ELISA) |
| Package | 96T |
| Limit of detection | 0.6ppb |
| Storage | The kit should be stored in a dry, dark place at a temperature of 2-8 ° C. Do not freeze. |
| Shelf life | The package is valid for 6 months |
The sample to be tested, enzyme-linked immunosorbent assay (ELISA) reagents, and antibody working solution are added sequentially for detection, without the need for separate pre mixing and transfer
the same sample can be extracted and diluted once, and vomiting toxin, zearalenone, and aflatoxin B1 can be detected simultaneously
Samples with strong acidity and alkalinity do not require adjustment of pH value, and can be directly detected after dilution
with high repeatability, the variation within the board is less than 5%, and the overall recovery rate can reach over 90%,
1.Sample Diluent 50 ml*2
2.Enzyme conjugate 20ml
3.Stop Solution 15ml
4.Premix Microtiter plate 96 wells
5.Standard substance (Calibrators) 1.5ml * 5
6.Chromogen TMB solution 15ml
7.Reaction Microtiter plate 96 wells
8.Microtiter plate cover 2 pcs
9.Quality inspection report 1 pc
10.Instruction 1 pc
Balance (accuracy: 0.01g)
centrifuge
pulverizer
oscillator
50ml centrifugal tube or conical bottle
10~100μL、50-1000 μL pipette and pipette tips
Microplate reader
Note: The above pictures are for reference only.For the actual product, please check Provided Materials and Reagent or consult the sales manager.
Weigh 5g samples through 20 mesh screens
Add 25ml of 70% methanol
Vortex oscillation for 3 minu
Centrifuge at 4000 RPM for 5 min
Take 100 μl of sample supernatant
Add 50 μl of sample solution, ELISA reagent, and antibody working solution separately
Wash the ELISA plate 4 times
Add 100 μl of substrate/chromogen
Add 100 μl of stop solution
Values are read using an enzyme marker
1. Take 2kg of representative samples for grinding, so that more than 95% of the samples can pass through a 20 mesh sieve. Mix evenly for sampling.
2. Preparation of extraction solution (70% methanol): According to the dosage, mix methanol and distilled water in a 7:3 volume ratio.
3. Weigh 10g ± 0.1g of the above sample into a clean container with a lid, and add 50mL of 70% methanol (the ratio of sample to 70% methanol is 1:5 (w: v)).
4. Fully shake and extract for 3 minutes, let it stand and take the supernatant. Centrifuge at 4000 rpm for 5 minutes.
5. Take 100 μl of supernatant and add 900 μl of Olaquindox sample diluent (10 fold dilution), mix well and wait for testing.
1. Premixing: take appropriate amount of premixed Flat noodles as required, add 60 μ L of Olaquindox
calibrator/sample to
be tested into the micropore and record its position. Add 120 μl of Olaquindox enzyme-linked immunosorbent
assay (ELISA) reagent to each well, pipette and mix well or shake horizontally.
(A ratio of 1:2 is sufficient for the pre mixing of calibration sample/test sample and enzyme reagent.
To make a re
well, mix 100 μl of calibration sample/test sample with 200 μl of enzyme, and add 100 μl to
each of the two detection plate wells.)
2. Sample addition: Add 100 μl of pre mixed liquid to the detection plate hole. Cover with cover film and incubate at 25 ℃ for 15 minutes.
3. Washing plate: shake off the solution in the micropores, fill with distilled water, repeat 4 times, and pat dry on absorbent paper.
4. Color development: Add 100 μl of color development solution to each well, cover with a cover film, and incubate at 25 ℃ in the dark for 5 minutes.
5. Termination: Add 100 μl of termination solution to each well, and immediately read the absorbance value at 450/630nm dual wavelength.
Doing replicate holes for the calibration product and the measured sample can improve the accuracy of thedetection.
Replace the pipette tip when drawing different reagents to prevent cross-contamination.
When using the pipette, be careful to avoid drawing in bubbles and affecting the volume of the added liquid. The way of drawing once and dispensing twice is easy to splatter after dispensing the liquid, so it is recommended to use the way of drawing twice and dispensing once to add the liquid vertically to the center of the micropores.
The liquid should be dispensed quickly and should not form water droplets.
The transfer of the mixed liquid in the pre-mixing plate to the detection plate starts the reaction. To reduce the error, please control the time difference between the transfer of different micropores (increase the transfer speed,control the number of single-sample tests. It is better to use a multi-channel pipette to test 4 strips at a time;it is better to use a single-channel pipette to test 2 strips at a time).
Do not use expired kits, and do not mix different batches of reagents.
Please keep the kit properly. Freezing, room temperature, and high temperature conditions will accelerate the aging of the kit. In use, please avoid cross-contamination of different reagents. If an abnormality of the reagent is found, such as the chromogenic solution turning blue, or the reagent being turbid, do not use it.
This method is only for the rapid preliminary screening of samples. For confirmation, please refer to methods such as liquid chromatography.
| Name | Xinyu Microplate reader |
|---|---|
| Model number | TruthersReader-01 |
| Light source | halogen lamp |
| Number of optical channels | single channel fiber optic detection |
| Filter | Standard with four filters: 405nm, 450nm, 492nm, and 630nm, up to 8 filters can be placed |
| Measurement object | 96 well standard enzyme-linked immunosorbent assay plate |
| Measurement mode and speed | single wavelength 2s/second, dual wavelength 5s/second |
| Vibration function | three types of vibration modes: high, medium, and low |
| Wavelength range | 400-750nm |
| Repeatability | ≤ 0.1% |
| Stability | ≤ ± 0.005 |
| Volume | 384mm * 271mm * 190mm |
| Weight | 7.6kg |
| Name | xinyu Fully automatic ELISA workstation |
|---|---|
| Trademark | TRUTHERS |
| Model number | SC-100E |
| Sampling channel | single channel |
| Sample size | 60-84, adjustable |
| Sample CV | 6% |
| Incubation temperature | 37℃ ±1℃ ° |
| Washing machine | 8 channels, 3 liquid buckets |
| microplate reader | 8 channels |
+8618554033120
zhuliyuan@xinyubio.com
