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Biontex's Detection of Mycoplasma in Cell Culture FAQ

Regarding the performance of the kits there is no difference. The MycoSPY® kit is a classical PCR kit with single components (Taq-Polymerase, PCR Buffer with dNTPs, Primer Mix), which have to be mixed before PCR. There is no loading buffer and tracking dye for gel electrophoresis included. MycoSPY® Master Mix kit is easier to handle and to ship. The lyophilisized Mastermix contains all necessary components premixed for PCR and subsequent gel electrophoresis. After reconstitution with water (included in the kit) the working flow is very simple (see MycoSPY® Master Mix). The Mastermix Kit is more stable and can therefore be shipped at room temperature. 

► Many commercial PCR-based mycoplasma test kits include a positive control and internal control. What is the difference?

Most kits for PCR-based detection of mycoplasmas contain a plasmid as positive control that encodes for the 16S rRNA of mycoplasmas. This ensures the functionality of the primers. This plasmid produces a DNA amplicon of equal or similar size to that expected if mycoplasma contamination were present. Therefore, the PCR with the positive control must be carried out in a separate tube. An internal control is usually included additionally, to make sure that the PCR is not inhibited by proteins and cell debris from the cell culture supernatant. The internal control produces a DNA amplicon of a different length from a mycoplasma-contaminated cell sample. Therefore the internal control can be carried out in each approach.

The internal control included in the MycoSPY® Master Mix kit and the MycoSPY® kit is a plasmid, which encodes for a shortened form of the 16S rRNA of mycoplasmas. The internal control thus serves as a positive control and ensures for each PCR approach that no inhibitors are present from the cell culture supernatant. It thus excludes false-negative results.

Both the MycoSPY® Master Mix kit and the MycoSPY® kit detect at least 80 copies of a mycoplasma genome. The internal control reduces the sensitivity slightly. Since mycoplasmas reproduce relatively quickly after contamination of a cell culture, this sensitivity is easily sufficient.
We therefore recommend adding the internal control in every PCR to ensure the absence of any existing inhibitor (proteins, cell debris) originating from the cell culture supernatant. 

It is not necessary to avoid conventional antibiotics such as penicillin, streptomycin or gentamicin, as these do not inhibit the assay of MycoSPY® Master Mix Kit the or the MycoSPY® kit.

Yes. We recommend storage at-20°C without additives (e.g. DMSO). After thawing, the cell culture supernatants should be prepared as described in the manual.

We recommend cultivating the cells for at least 48–72 hours or until at least 80% coverage of the growth area is achieved. For suspension cells, cell density should be approximately in the range of the cell number recommended for subculturing. Since the mycoplasmas are detected in the cell culture supernatant, the medium should not be changed in the interim.

We recommend performing the PCR for mycoplasmas (e.g. with MycoSPY® or MycoSPY® Master Mix) least every 1-2 months, particularly when cells are cultured in the presence of antibiotics (e.g. pen/strep). These antibiotics prevent the discovery of unsterile working techniques but allow mycoplasma contamination of cell cultures.

 

NOTE: This guide is for Biontex products only.