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MTT Cell Proliferation and Cytotoxicity Assay Kit– MSE Supplies LLC

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MTT Cell Proliferation and Cytotoxicity Assay Kit - MSE Supplies LLC

MTT Cell Proliferation and Cytotoxicity Assay Kit

SKU: E-CK-A341-1000

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MTT Cell Proliferation and Cytotoxicity Assay Kit

 

Introduction

Elabscience® MTT Cell Proliferation and Cytotoxicity Assay Kit is a rapid and highly sensitive kit widely used in cell proliferation and cytotoxicity detection.

MTT is 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide which can be reduced by some dehydrogenases in mitochondria to form a crystalline dark purple product formazan. Formazan can be completely dissolved by DMSO and its absorbance is near 570 nm wavelength. The more and faster the cells proliferate, the darker the color is, and the more cytotoxic, the lighter the color is. For the same cells, there is a linear relationship between the depth darkness of color and the number of cells.

 

Product Details

Properties

Application Viability/Proliferation/Cytotoxicity
Detection method Colorimetric Method
Sample type Cell samples
Detection instrument Microplate reader
Other reagents required DMSO
Storage 2~8°C, shading light
Shipping Ice bag
Expiration date 6 months

 

Staining Procedure

  1. Reagent Preparation
    MTT (5×) is concentrated, please diluted with MTT Diluent Buffer to 1×MTT working solution before use. For example: take 100 μL MTT (5×), add to 400 μL MTT Diluent Buffer, and the mixture is 1×MTT working solution.
  2. Add 100 μL of cell suspension per well to the 96 well microplate, and set blank wells (do not seed cells but add 100 μL of culture medium).
    Note: For cell proliferation test, add 100 μL (about 2,000 cells) cell suspension to each well. For cell cytotoxicity test, add 100 μL (about 5,000 cells) cell suspension to each well. The number of cells used in each well depends on the size of the cell and the rate of cell proliferation, etc.
  3. Culture the cells according to the experimental design.
  4. Add 50 μL of 1×MTT working solution to each well and incubate for 1~4 h.
    Note: MTT incubation conditions are the same as cell culture conditions.
  5. Remove the supernatant carefully, add 150 μL DMSO to each to dissolve the formazan format on the last step, shake the well with a flat shaker.
  6. Measure the OD value with microplate reader at 570 nm.
  7. Calculation
    [Note]:
    ODsample: the OD value of sample well.
    ODcontrol: the OD value of control well.
    ODblank: the OD value of blank well.

 

Storage

Store at 2~8°C for half a year, MTT (5×) should be stored in dark.

 

Notes

  1. This kit is for research use only.
  2. For your safety and health, please take safety precautions and follow the procedures of laboratory reagent operation. Wear laboratory clothes and disposable gloves during operation, and avoid direct contact with the human body or inhalation of the body.
  3. For maximal assay performance, this reagent should be used within 6 months. Avoid freeze/thaw cycles.
  4. MTT is yellow and needs to be stored in dark. Long-term illumination will lead to failure. Do not use when the color turns grey green. MTT may solidify at 4°C or lower temperature. It can be incubated in water bath at 20~25°C until it is completely melted before use.
  5. Pay attention to mixing during cell seeding to avoid unequal number of cells per well due to cell sedimentation.
  6. The incubation time of MTT is generally 1~4 hours. It is recommended to take a preliminary experiment to explore the optimal number of cells and the incubation time of MTT.
  7. When using a 96-well plate for cell culture, pay attention to the result error caused by water evaporation. It is recommended to discard the outer circle of wells and add PBS, water or culture medium to prevent water evaporation. In addition, the 96-well plate can also be placed in the incubator near the water.
  8. Make sure that there is no bubble in each well when measuring the OD value with the microplate reader, otherwise it will interfere with the determination.
  9. The detection of this kit relies on the dehydrogenase catalyzed reaction, so reducing agents (such as some antioxidants) will interfere with the detection. If there are reducing agents in the system, try to remove them. Or replace the fresh medium before adding MTT to remove the influence of the reagent.
  10. Suspension cells must be centrifuged and absorb supernatant before adding DMSO