CyQUANT XTT Cell Viability Assay Protocol | Thermo Fisher Scientific

Metabolic activity-based cell viability assay

XTT is a two-reagent kit that consists of the XTT reagent and the Electron Coupling Reagent. This is a colorimetric assay used to assess cell viability as a function of cell number based on metabolic activity. The water-soluble XTT is converted to an orange-colored formazan product with an absorbance read at 450 nm and 660 nm.

This protocol can be used for:

Quantification of cell number based on metabolic activity in microplate readers capable of absorbance measurements

This protocol should not be used for:

Fluorescence microscopy

You will need the following for this protocol:

Cells growing in culture
CyQUANT XTT Cell Viability Assay (Cat. No. X12223)
Cell culture medium
96- or 364-well plate
Microplate reader
CO₂ incubator

Protocol

1. Seed cells in a 96-well plate containing 100 μL/well of culture medium with compounds to be tested. Culture in a CO₂ incubator for 24–48 hours

2. Add 1 mL of Electron Coupling Reagent to 6 mL of XTT Reagent; vortex to mix. Once prepared, this working solution should be used promptly

liquid being added to cell culture plate

3. Add 70 µL of the working solution to each well

4. Incubate at 37°C for 4 hours in a CO₂ incubator

5. Read absorbance at 450 nm and 660 nm

Protocol tips

Immediately use the XTT/Electron Coupling Reagent after preparation
Freeze/thaw cycles will affect assay performance, as a result single-use vials are provided to ensure stability and should be kept at –20ºC until use
Washing is not required after staining
To correct for background absorbance, include at least three wells with only complete culture medium without cells
A cell titration experiment using a range of cells from 10³–10⁵ cells/well can be used to generate a standard curve

XTT has increased signal-to-background compared to MTT

Click image to enlarge

Figure 1. A549 cells were assayed using either the CyQUANT XTT Cell Viability Assay or a commercially available MTT according to their respective manufacturers’ protocols. The signal-to-background ratio for the MTT assay product is calculated as the absorbance of the sample at 540 nm divided by the absorbance of the blank at 540 nm.

For Research Use Only. Not for use in diagnostic procedures.