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牛棒状杆菌在组织培养条件和培养基中的生长

Corynebacterium bovis Growth in Tissue Culture Conditions and Media.

作者信息

Kleymann Alyssa M, Zawadzki Nicholas A, Fong Derek L, Fink Michael K, Habenicht Lauren M, Leszczynski Jori K, Anderson Steven M, Schurr Michael J, Manuel Christopher A

机构信息

1Office of Laboratory Animal Resources, University of Colorado Denver Anschutz Medical Campus, Aurora, Colorado.

2Department of Immunology and Microbiology, University of Colorado Denver Anschutz Medical Campus, Aurora, Colorado.

出版信息

J Am Assoc Lab Anim Sci. 2024 Nov 1;63(6):655-661. doi: 10.30802/AALAS-JAALAS-24-050.

Abstract

A common concern in preclinical cancer research is the introduction of Corynebacterium bovis into immunodeficient mouse colonies through cancer cell lines. C. bovis is a known contaminant of patient-derived xenograft tumors passaged horizontally between immunodeficient mice. However, it is unclear if C. bovis can grow in mammalian tissue culture conditions or tissue culture media. We hypothesized that C. bovis would not grow under tissue culture conditions or media, diminishing the risk of transmission from tumor cell lines cultured in vitro. Three C. bovis isolates, CUAMC1, HAC, and ATCC-7715, were used to test our hypothesis in 3 of the most common media used to grow human cancer cell lines including RPMI 1640 + 10% FBS (RPMI), DMEM/high glucose + 10% FBS (DMEM), and DMEM/F-12 + 10% FBS (DMEM/F12). Our results confirmed propagation of each C. bovis isolate in DMEM/F12 media under tissue culture conditions after 72 h. However, these results also demonstrate diminished viability of each C. bovis isolate in RPMI and DMEM after 72 h. To assess whether antibiotics could halt the growth of C. bovis under tissue culture conditions in DMEM/F12, penicillin-streptomycin (pen/strep) was added to the experimental media. This treatment was effective in eliminating all viable C. bovis in the culture system after 72 h. Our data suggest that C. bovis growth under tissue culture conditions is possible and growth in tissue culture media is nuanced. These results highlight the importance of pathogen surveillance for tumor cell lines propagated in vitro and demonstrate the need for further investigation into C. bovis growth requirements.

摘要

临床前癌症研究中的一个常见问题是通过癌细胞系将牛棒状杆菌引入免疫缺陷小鼠群体。牛棒状杆菌是免疫缺陷小鼠之间水平传代的患者来源异种移植肿瘤的已知污染物。然而,尚不清楚牛棒状杆菌是否能在哺乳动物组织培养条件或组织培养基中生长。我们假设牛棒状杆菌在组织培养条件或培养基下不会生长,从而降低体外培养的肿瘤细胞系传播的风险。使用三种牛棒状杆菌分离株CUAMC1、HAC和ATCC - 7715,在用于培养人类癌细胞系的三种最常用培养基中测试我们的假设,包括RPMI 1640 + 10%胎牛血清(RPMI)、DMEM/高糖 + 10%胎牛血清(DMEM)和DMEM/F - 12 + 10%胎牛血清(DMEM/F12)。我们的结果证实,在组织培养条件下,72小时后每种牛棒状杆菌分离株在DMEM/F12培养基中均有增殖。然而,这些结果也表明,72小时后每种牛棒状杆菌分离株在RPMI和DMEM中的活力下降。为了评估抗生素是否能在DMEM/F12的组织培养条件下阻止牛棒状杆菌的生长,将青霉素 - 链霉素(pen/strep)添加到实验培养基中。该处理在72小时后有效消除了培养系统中所有存活的牛棒状杆菌。我们的数据表明,牛棒状杆菌在组织培养条件下生长是可能的,并且在组织培养基中的生长情况较为微妙。这些结果突出了对体外培养的肿瘤细胞系进行病原体监测的重要性,并表明需要进一步研究牛棒状杆菌的生长需求。

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