T-2 Toxin (T-2) ELISA Kit

For reference only. Please follow the manual included in your kit for instructions.

Catalog Number
RDT-E004
RDT-E004
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Product Description

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The T-2 Toxin (T-2) ELISA Kit (RDT-E004) is an enzyme-linked immunosorbent assay for quantitative detection of T-2 in Food samples with a standard range of 0.05-4.05ppb. This kit uses the Traditional ELISA format for colorimetric detection of natural T-2 in samples including Beans,Corn,Oats,Peanuts,Feed. The kit is easy to use and comes with a pre-coated microplate and all necessary reagents and buffers. The standard curve generated in the experiment is used to calculate the concentration of T-2 in samples. For research use only.

Product Specifications

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Product Name
T-2 Toxin (T-2) ELISA Kit
Catalog Number
RDT-E004
Detection Range
0.05-4.05ppb
Species Reactivity
Food
Species
Food
Assay Length
45 minutes
Experimental Method
Competitive Inhibition
Detection Method
Colorimetric
Sample Type
Beans,Corn,Oats,Peanuts,Feed
Storage
2-8°C,Avoid freeze
Shelf Life
12 monthes

Product Details

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Intended Use

For the quantitative detection of T-2 Toxin (T-2) concentration in beans, corn, oats, peanuts, and feed samples.

Assay Principle

This kit uses Competitive-ELISA as the method for the quantitative detection. It can detect T-2 Toxin (T-2) in samples, such as grain, peanut, etc. This kit is composed of ELISA Microtiter plate, HRP conjugate, antibody working solution, standard and other supplementary reagents. The microplate provided in this kit has been pre-coated with coupled antigen. During the reaction, T-2 in the samples or standard competes with coupled antigen on the solid phase supporter for sites of anti-T-2 antibody. Then Horseradish Peroxidase (HRP) conjugate is added to each micro plate well, and substrate reagent is added for color development. There is a negative correlation between the OD value of samples and the concentration of T-2. The concentration of T-2 in the samples can be calculated by comparing the OD of the samples to the standard curve.

Application Data

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Reagents and Materials Provided

Reagent Quantity
ELISA Microtiter plate 96 wells
Standard Liquid 1 mL each (ppb=ng/mL=ng/g) (0ppb, 0.05ppb, 0.15ppb, 0.45ppb, 1.35ppb, 4.05ppb)
HRP Conjugate 5.5 mL
Antibody Working Solution 5.5 mL
Substrate Reagent A 6 mL
Substrate Reagent B 6 mL
Stop Solution 6 mL
20×Concentrated Wash Buffer 40 mL
Plate Sealer 3
Sealed Bag 1
Manual 1
Note:

All reagent bottle caps should be tightly closed to prevent evaporation and microbial contamination.

Materials Required but not Supplied

  1. Equipment: Microplate reader, Printer, Homogenizer, Vortex mixer, Centrifuge, Graduated pipette, Balance (sensibility 0.01 g), Funnel, Filter paper.
  2. Micropipettes: single-channel 20-200 µL, 100-1000 µL, and multi-channel 300 µL.
  3. Reagents: Methanol.

Storage

  1. Store the kit at 2-8℃. Do not freeze any kit components.
  2. Return any unused microwells to their original foil bag and reseal them together with the desiccant provided. Continue to store at 2-8℃.
  3. Shelf life is approximately 12 months from date of manufacture. Check packaging for expiry date.

Sample Preparation

  • Beans, corn, oats, peanuts, feed:
  • Homogenize the sample, use Homogenizer.
  • Weigh 1±0.05 g of homogenate sample in to 50 mL centrifuge tube, add 20 mL of 60% Methanol (Solution 1), vortex mixer for 5 min, centrifuge at 4000 rpm for 5 min at room temperature (or filter by quantitative analysis filter paper).
  • Take 1 mL of the supernatant to another centrifuge tube, and dilute with deionized water (for example, supernatant (V): deionized water (V) =1:5).
  • Take 50 μL for analysis.
Note: Sample dilution factor: 120, detection limit: 6 ppb

Reagent Preparation

Solution preparation:
Prepare solutions according to the number of samples. Avoid using all components in the kit at once.
Solution 1: 60% Methanol
Methanol (V): deionized water (V) =3:2.
Solution 2: Wash Buffer
Dilute the 20×Concentrated Wash Buffer with deionized water. (20×Concentrated Wash Buffer (V): Deionized water (V) =1:19).
Notes:
  • Bring all reagents and samples to room temperature before use.
  • Turn on the microplate reader 30 min in advance to preheat the instrument and set the testing parameters.
  • All experimental apparatus should be clean, and disposable pipette should be used and changed frequently to avoid cross-contamination during the experiment.

Assay Procedure

Bring all reagents and samples to room temperature (25℃) before use. All reagents should be mixed thoroughly by gently swirling before pipetting. Avoid foaming. Any unused Microtiter plate wells should be resealed as soon as possible and stored at 2-8℃.

  1. Number: number the samples and standards in order (multiple wells), and keep a record of the plate layout. Standards and Samples must be tested in duplicate.
  2. Add Sample: add 50 μL of Standard or Sample to each well, then add 50 uL HRP Conjugate, then 50 μL of Antibody Working Solution to each well, and cover the plate with plate sealer. Oscillate gently for 5 s to mix thoroughly, then incubate at 25℃ for 30 min in the dark.
  3. Wash: Carefully remove the plate sealer, then remove the liquid from each well. Immediately add 300 μL of Wash Buffer (Solution 2) to each well and wash. Repeat wash procedure 5 times, 30 s intervals each time. Invert the plate and pat it against a thick sheet of absorbent paper (If there are bubbles in the wells, clean pipette tips can be used to pop them).
  4. Color Development: add 50 μL of Substrate Reagent A to each well, and then add 50 μL of Substrate Reagent B. Gently oscillate for 5 s to mix thoroughly. Incubate at 25℃ for 15 min in the dark (The reaction time can be extended according to the amount of color change).
  5. Stop Reaction: add 50 μL of Stop Solution to each well. Gently oscillate to mix thoroughly.
  6. OD Measurement: determine the optical density (OD value) of each well at 450 nm (reference wavelength 630 nm) with a microplate reader. This step should be performed no later than 10 min after the reaction has been stopped.

Calculation of Results

Absorbance (%) = A/A₀×100%

  • A: Average absorbance of standard or sample
  • A₀: Average absorbance of 0 ppb Standard
  • Drawing and calculation of standard curve
  • Create a standard curve by plotting the absorbance percentage of each standard on the y-axis against the log concentration on the x-axis to draw a semi-logarithmic plot. Add the average absorbance value of each sample to the standard curve to calculate the corresponding concentration. If samples have been diluted, the concentration calculated from the standard curve must be multiplied by the dilution factor.
  • We recommend using professional software for fast and accurate analysis of large numbers of samples.

Product Data

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Reaction conditions (Incubation time and temperature)

25℃; 30 min, 15 min

Detection limit

Beans, Corn, Oats, Peanuts, Feed--- 6 ppb

Cross-reactivity

Sample recovery rate

110%±15%

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