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首页> 外文期刊>Journal of Clinical Microbiology >Improved plaque assays for Rickettsia prowazekii in Vero 76 cells.
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Improved plaque assays for Rickettsia prowazekii in Vero 76 cells.

机译:改进了Vero 76细胞中立氏立克次体的噬斑测定。

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摘要

Typhus group rickettsiae, including Rickettsia prowazekii and R. typhi, produce visible plaques on primary chick embryo fibroblasts and low-passage mouse embryo fibroblasts but do not form reproducible plaques on continuous cell culture lines. We tested medium overlay modifications for plaque formation of typhus group rickettsiae on the continuous fibroblast cell line Vero76. A procedure involving primary overlay with medium at pH 6.8, which was followed 2 to 3 days later with secondary overlay at neutral pH containing 1 microgram of emetine per ml and 20 micrograms of NaF per ml, resulted in visible plaques at 7 to 10 days postinfection. A single-step procedure involving overlay with medium containing 50 ng of dextran sulfate per ml also resulted in plaque formation within 8 days postinfection. These assays represent reproducible and inexpensive methods for evaluating the infectious titers of typhus group rickettsiae, cloning single plaque isolates, and testing the susceptibilities of rickettsiae to antibiotics.
机译:斑疹伤寒群立克次体,包括立克次氏菌和鼠伤寒立克次体,在原代鸡胚成纤维细胞和低传代小鼠胚胎成纤维细胞上产生可见的噬菌斑,但在连续细胞培养线上不形成可复制的噬菌斑。我们测试了连续覆盖的成纤维细胞系Vero76上斑疹伤寒立克次体斑形成的培养基覆盖修饰。该过程涉及在pH 6.8的条件下进行初次覆盖,然后在2至3天后在中性pH下进行二次覆盖,其中每毫升含1微克依替丁和每毫升20微克NaF,在感染后7至10天产生可见的菌斑。涉及覆盖每毫升含50 ng硫酸葡聚糖的培养基的单步操作程序也导致感染后8天内形成噬菌斑。这些测定法代表了可再现且廉价的方法,用于评估斑疹伤寒组立克次体的感染滴度,克隆单个噬菌斑分离物以及测试立克次体对抗生素的敏感性。

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