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Comparison of Five Commercial Molecular Assays for Mycoplasma Testing of Cellular Therapy Products

支原体 重复性 琼脂 连续稀释 微生物学 生殖支原体 生物 检出限 病毒学 色谱法 医学 化学 细菌 病理 替代医学 沙眼衣原体 遗传学
作者
Arthur H. Totten,Anna Julia Adams,Hyunmi Halas,James E. T. Gebo,Amanda D. East,Anna F. Lau
出处
期刊:Journal of Clinical Microbiology [American Society for Microbiology]
卷期号:61 (2) 被引量:5
标识
DOI:10.1128/jcm.01498-22
摘要

Testing of cellular therapy products for Mycoplasma is a regulatory requirement by the United States Food and Drug Administration (FDA) to ensure the sterility and safety of the product prior to release for patient infusion. The risk of Mycoplasma contamination in cell culture is high. Gold standard testing follows USP 63 which requires a 28-day agar and broth cultivation method that is impractical for short shelf-life biologics. Several commercial molecular platforms have been marketed for faster raw material and product release testing; however, little performance data are available in the literature. In this study, we performed a proof-of-principle analysis to evaluate the performance of five commercial molecular assays, including the MycoSEQ Mycoplasma detection kit (Life Technologies), the MycoTOOL Mycoplasma real-time detection kit (Roche), the VenorGEM qOneStep kit (Minerva Biolabs), the ATCC universal Mycoplasma detection kit, and the Biofire Mycoplasma assay (bioMérieux Industry) using 10 cultured Mollicutes spp., with each at four log-fold dilutions (1,000 CFU/mL to 1 CFU/mL) in biological duplicates with three replicates per condition (n = 6) to assess limit of detection (LOD) and repeatability. Additional testing was performed in the presence of tumor infiltrating lymphocytes (TILs). Based on LOD alone, the Biofire Mycoplasma assay was most sensitive followed by the MycoSEQ and MycoTOOL which were comparable. We showed that not all assays were capable of meeting the ≤10 CFU/mL LOD to replace culture-based methods according to European and Japanese pharmacopeia standards. No assay interference was observed when testing in the presence of TILs.

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