Detection of Mycoplasma Contamination Directly from Culture Supernatant Using Polymerase Chain Reaction

Pisal, R. V.; Hrebíková, H.; Chvátalová, J.; Kunke, D.; Filip, S.; Mokrý, Jaroslav

doi:10.14712/fb2016062050203

Folia Biologica > Archive > 2016, Vol. 62 > Issue 5 > Detection of Mycoplasma Contamination…

Fol. Biol. 2016, 62, 203-206

https://doi.org/10.14712/fb2016062050203

Detection of Mycoplasma Contamination Directly from Culture Supernatant Using Polymerase Chain Reaction

R. V. Pisal¹, H. Hrebíková¹, J. Chvátalová¹, D. Kunke¹, S. Filip², Jaroslav Mokrý¹

¹Department of Histology and Embryology, Charles University – Faculty of Medicine in Hradec Králové, Czech Republic
²Department of Oncology and Radiotherapy, Charles University – Faculty of Medicine in Hradec Králové, Czech Republic

Received February 2016
Accepted June 2016

Ensuring mycoplasma-free cell culture is of prime importance as they severely affect cellular characteristics leading to experimental artefacts and spurious results. Various methods persist for mycoplasma detection; out of the whole array of methods polymerase chain reaction (PCR) is the most favoured one because it is highly sensitive, specific and quick. The PCR-based detection procedure involves three steps: cell culture supernatant collection, DNA isolation, and PCR. We have modified this procedure so that cell culture supernatant can directly be used for PCR without the need for DNA extraction. This modification makes the procedure quicker and more sensitive because loss of mycoplasma DNA is prevented and this loss becomes more significant when the level of mycoplasma contamination is very low.