Summary
Environmental sampling was performed during trypsinization and passage of 3T-6 cell cultures that contained a mean of 4.3×107 colony forming units (CFU) per ml supernatant ofA. laidlawii. The lip of the culture flask and the outside of the used pipet were always heavily contaminated. The outside of the culture flask (3/7), the work surface (8/12) and the outside of a pan of disinfectant (4/5) were regularly contaminated with mycoplasmas. Airborne mycoplasmas were detected eight of 32 times (25%) by settling plates; simultaneous forced-air samplers by two different methods were always negative. The technician’s hands were contaminated two of 15 samples. When hands were contaminated, more contamination was detected in the environment. Droplets ofA. laidlawii andM. orale inoculated onto work surfaces survived drying for a minimum of 3 days, even in laminar airflow cabinets. Twenty-five of 31 (80.6%) cell culture technicians carriedM. salivarium in their throats; only two carriedM. orale. It is concluded that mycoplasma-infected cultures are the most common source of further infection. Recommendations for prevention and control of mycoplasmal infection are listed.
This is a preview of subscription content, log in via an institution to check access.
Similar content being viewed by others
References
Barile, M. F., H. E. Hopps, M. W. Grabowski, D. B. Riggs, and R. A. delGuidice. 1973. The identification and sources of mycoplasmas isolated from contaminated cell cultures. Ann. N.Y. Acad. Sci. 225: 251–264.
Barile, M. F., and J. Kern. 1971. Isolation ofMycoplasma arginini from commercial bovine sera and its implication in contaminated cell cultures. Proc. Soc. Exp. Biol. Med. 138: 432–437.
Edward, D. G. FF. 1969. Mycoplasmas as contaminants and their detection. Prog. Immunobiol. Stand. 3: 17–22.
O’Connell, R. G., R. G. Wittler, and J. E. Faber. 1964. Aerosols as a source of widespread mycoplasma contamination of tissue cultures. Appl. Microbiol. 12: 337–342.
McGarrity, G. J., and L. L. Coriell. 1973. Detection of anaerobic mycoplasmas in cell cultures. In Vitro 9: 17–18.
Clyde, W. A. 1964. Mycoplasma species identification based upon growth inhibition by specific antisera. J. Immunol. 94: 958–965.
Stanbridge, E. 1971. Mycoplasmas and cell cultures. Bacteriol. Rev. 35: 206–227.
Kundsin, R. B. 1968. Aerosols of mycoplasmas, L forms, and bacteria: comparison of particle size, viability, and lethality of ultraviolet radiation. Appl. Microbiol. 16: 143–146.
Wright, D. N., G. D. Bailey, and M. T. Hatch. 1968. Survival of airborne mycoplasma as affected by relative humidity. J. Bacteriol. 95: 251–252.
Shepard, M. C., and C. D. Lunceford. 1965. Effect of pH on human mycoplasma strains. J. Bacteriol. 89: 265–270.
McGarrity, G. J., and L. L. Coriell. 1971. Procedures to reduce contamination of cell cultures. In Vitro 6: 257–265.
McGarrity, G. J. 1975. Control of microbiological contamination. Procedure 16183. TCA Manual 1: 181–184.
Author information
Authors and Affiliations
Additional information
These studies were supported in part by Contract No. 1-GM-2112 from the National Institute of General Medical Sciences, Contract No. 1-CB-23868 from the National Cancer Institute, General Research Support Grant 5-S01-RRO5582 from Research Resources, National Institutes of Health, and by a Grant-in-Aid from the State of New Jersey.
Rights and permissions
About this article
Cite this article
McGarrity, G.J. Spread and control of mycoplasmal infection of cell cultures. In Vitro Cell.Dev.Biol.-Plant 12, 643–648 (1976). https://doi.org/10.1007/BF02797464
Issue Date:
DOI: https://doi.org/10.1007/BF02797464