Fluorescence Staining Technique for detection of Mycoplasma Contamination:
The cultures are stained with
Hoechst 33258, a fluorescent dye that binds specifically to DNA. Because mycoplasmas
contain DNA, they can be detected readily by their characteristic particulate
or filamentous pattern of fluorescence on the cell surface and if the
contamination is more fluorescence pattern is observed in surrounding areas.
Monolayer cell cultures can be fixed and stained directly, but after
centrifugation, the medium from cells growing in suspension will need to be added
to an indicator cell (i.e., another monolayer) known to be free of mycoplasma
but also known to be a good host for mycoplasma and to spread well in culture,
with adequate cytoplasm to reveal any adherent mycoplasma. The cell lines that
can be commonly used include epithelial cell lines from mammals like the Normal
Rat Kidney (NRK), 3T6, Vero cells and A549. Using an indicator cell line is suitable
in the technique as it helps avoid problem of false positives that arise due to
debris during the assay of primary cultures or of cells right after thawing. In
case of more debris, we can filter the medium by a sterile 5µm filter membrane or
centrifuged at about 1000 rpm.
PROTOCOL FOR FLUORESCENCE DETECTION OF MYCOPLASMA CONTAMINATION
Culture cells in the absence of
antibiotics for at least one week, transfer the supernatant medium to an early
log phase-indicator culture, incubate 3–5 days, fix and stain the cells, and
look for fluorescence other than in the nucleus.
Materials:
Sterile or Aseptically Prepared:
- Supernatant of medium that do not contain antibiotics, from a seven day monolayer or centrifuged suspension cell culture
- Petri dishes
- Indicator cells (e.g. NRK, 3T6, Vero cells, A549)
Non-sterile:
- Hoechst 33258 stain, 50ng/ml in BSS without phenol red (BSS-PR) or D-PBSA
- Buffered glycerol mounting mixture (substance used to mount microscopic specimens)
- BSS-PR: Hank's Buffer Saline Solution without Phenol Red
- D-PBSA: Dulbecco’s Phosphate Buffer Saline without Ca2+ and Mg2+
- Deionized water
- Freshly prepared acetic acid - methanol (1:3) used as fixative.
Procedure:
1.
Place the given indicator cells into Petridishes
without the use of antibiotics; use sufficient cells to yield about 60% confluence
(cells growing and coming together to cover the medium) in about 5 days (e.g. 105
A549 or 205 NRK, in 5 ml of medium).
2.
Take 1.5ml of medium from the test culture.
3.
Keep the culture for incubation till 60% confluence
is attained by the cells.
Note: Confluence
of cells should not be attained at the end of assay otherwise the staining will
be inhibited and the resulting visual for mycoplasma could be unclear.
After
every rinsing, the rinse should be discarded properly.
4.
Discard the medium.
5.
Monolayer should be rinsed with BSS-PR or D-PBSA.
6.
Rinse the monolayer again with fresh BSS-PR or
D-PBSA diluted 50:50 with fixative.
7.
Rinse with pure fixative.
8.
Take more fixative ∼0.5 ml/cm2 over the monolayer, and allow
fixation to continue for 10 minutes.
9.
Discard the fixative after the 10 minutes fixation
(of previous step).
10. Monolayer
must be completely dried for storage.
(Samples can
be stored at this stage and can be used later for staining)
11. For
staining directly, the fixative must be washed using deionized water.
12. Hoechst
33258 mixed with BSS-PR or D-PBSA is added to the cells and allowed it to stain
at room temperature for 10 minutes.
13. Rinse the
monolayer with water to remove the stain.
14. Take a coverslip,
one drop buffered glycerol mounting mixture and mount it for observation, blot out
excess mounting mixture from the edge of coverslip.
15. Observe monolayer
under epi-fluorescence microscope with a 330-380nm excitation filter and a Long
pass (LP) 440nm barrier filter.
Analysis:
Observe for extra nuclear
fluorescence. Mycoplasma gives pinpointed or filamentous fluorescence on the
cytoplasm and sometimes in intracellular space also. The location of pinpoints is
close to the limit of resolution with a 50x objective (0.1–1.0µm) usually of
regular size and shape. All cells will may not be infected, so very careful
observation must be done to finally reach a conclusion and confirming any
solution as uninfected.
At few times, a light, uniform
staining on cytoplasm is seen, which could be due to RNA.
If there doubts to interpret the fluorescence
test result, the test should be repeated further after sub-culturing test cells
in absence of antibiotics.
In case of repeated unclear
results, PCR or ELISA can be performed.
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Did you read ?
Maintenance of Sterility in Animal Tissue Culture.
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Did you read ?
Maintenance of Sterility in Animal Tissue Culture.
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