| Literature DB >> 25884200 |
Alet van Tonder1, Annie M Joubert2, A Duncan Cromarty3.
Abstract
BACKGROUND: The tetrazolium-based MTT assay has long been regarded as the gold standard of cytotoxicity assays as it is highly sensitive and has been miniaturised for use as a high-throughput screening assay. However, various reports refer to interference by different test compounds, including the glycolysis inhibitor 3-bromopyruvate, with the conversion of the dye to coloured formazan crystals. This study assessed the linear range and reproducibility of three commonly used cell enumeration assays; the neutral red uptake (NRU), resazurin reduction (RES) and sulforhodamine B (SRB) assays, in comparison to the MTT assay. Interference between the MTT assay and three glycolysis inhibitors, 2-deoxyglucose, 3-bromopyruvate and lonidamine, was investigated.Entities:
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Year: 2015 PMID: 25884200 PMCID: PMC4349615 DOI: 10.1186/s13104-015-1000-8
Source DB: PubMed Journal: BMC Res Notes ISSN: 1756-0500
A summary of the advantages and disadvantages of the four cell enumeration assays
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| 1. Cell enumeration independent of enzymatic conversion of dye [ | 1. Some reports of test compound interference [ |
| 2. Few wash steps involved [ | ||
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| 1. Gold standard for cytotoxicity testing | 1. Conversion to formazan crystals depends on metabolic rate and number of mitochondria resulting in many known interferences [ |
| 2. Suitable for high-throughput screening and miniaturisation [ | 2. Numerous wash steps required [ | |
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| 1. Few wash steps involved [ | 1. Conversion to resorufin depend on enzymatic conversion [ |
| 2. Follow-up assays can be performed on same cells as assay is not cytotoxic [ | 2. Absorbance-based method less sensitive than fluorescence-based method | |
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| 1. Cell enumeration dependent on protein content thus no test compound interference [ | 1. Numerous wash steps involved, but fixation required [ |
| 2. Highly reproducible | 2. Less sensitive with non-adherent cells |
Figure 1The linear range of the four cell enumeration assays using MDA-MB-231 cells. Four different cell enumeration assays were performed after 24 and 72 h incubation periods at six increasing starting cell densities. The solid line represents the linear least squares fit of the data. The dashed lines represent the 95% confidence bands. Graphs for 24 h incubation period depicts cell density up to 10 000 cells/well and 72 h incubation period depicts cell density up to 5 000 cells/well (n = 4).
The coefficient of determination (r ) of the four cytotoxicity assays
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| MCF-7 | 24 hours incubation | 0.901 | 0.711 | 0.999 | 0.992 |
| MDA-MB-231 | 0.979 | 0.975 | 0.998 | 0.999 | |
| MCF-12A | 0.846 | 0.903 | 0.976 | 0.999 | |
| MCF-7 | 72 hours incubation | 0.994 | 0.762 | 0.915 | 0.999 |
| MDA-MB-231 | 0.958 | 0.878 | 0.843 | 0.973 | |
| MCF-12A | 0.986 | 0.990 | 0.887 | 0.985 | |
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The neutral red, MTT, resazurin reduction and SRB assays were performed after 24 or 72 hour incubation on three cell lines (n = 4).
Figure 2The effect of 3-bromopyruvate on the growth of MCF-7 cells. The graphs represent results obtained after 24 and 72 hours incubation as assayed by the four cell enumeration assays. Note that the error bars are smaller in the 72 hour incubation graphs and in many of the data points fall within the symbol (n = 3).
The IC concentrations of 3-bromopyruvate calculated for MCF-7 cells after 24 or 72 hour incubation
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| 24 hour Incubation | 54.1 ± 1.6 | - | - | 86.4 ± 1.2 |
| 72 hour incubation | 60.9 ± 1.3 | 98.5 ± 1.1 | 105.9 ± 1.1 | 74.4 ± 1.1 |
Where no values are given these could not be calculated as the assay reported relative cell survival of greater than 50% at the tested concentrations (n = 4).
Results are indicated as mean ± SEM.
Figure 3Interference of three glycolysis inhibitors with the MTT assay in a cell-free system. After 4 hours incubation with (A) 2-deoxyglucose, (B) 3-bromopyruvate and (C) lonidamine interference was seen for the MTT assay (n = 3).