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大肠杆菌侵袭潜力的识别方法

Methodology for recognition of invasive potential of Escherichia coli.

作者信息

Mehlman I J, Eide E L, Sanders A C, Fishbein M, Aulisio C C

出版信息

J Assoc Off Anal Chem. 1977 May;60(3):546-62.

PMID:323215
Abstract

Surveillance for dysentery-related invasive potential in bacteria using the Sereny keratoconjunctivitis test is restricted by expense, time factor, and necessity for confirmation. Primary screening of isolates in a standardized mammalian cell culture system is recommended. Bacteria are grown 20 hr in veal infusion, washed, and resuspended in 20% heat-inactivated fetal bovine serum (FBS) supplemented with 0.12% brain heart infusion and 0.1% bile salts. The HeLa culture is grown 20 hr as a monolayer in chamber slides with 90% minimal essential medium (MEM)-10% FBS. The host culture is infected at a ratio of 10 bacteria/mammalian cell for 3 hr at 35 degrees C. The infection medium is replaced with MEM-FBS supplemented with 300 microng lysozyme and 5 microng gentamycin/ml. The infected monolayer is incubated 5 hr at 35 degrees C to permit intracellular multiplication. Specimens are washed, fixed with methanol, and stained successively with May-Grunwald and Giemsa dyes. Bacteria occur within the cytoplasm if invasion has occurred. The criterion for a positive test is that 1% of the host cells possesses at least 5 bacteria in 2 of 3 trials. Invasiveness is correlated with and possibly preconditioned by cytotoxic principle(s). Infectivity rates vary from 0 to 30%. The cytopathic effect is noted in 5-50% of HeLa cells. Positive results must be confirmed by the Sereny test.

摘要

使用塞雷尼角膜结膜炎试验监测细菌中与痢疾相关的侵袭潜力受到费用、时间因素和确认必要性的限制。建议在标准化的哺乳动物细胞培养系统中对分离株进行初步筛选。将细菌在小牛肉浸液中培养20小时,洗涤后,重悬于含有0.12%脑心浸液和0.1%胆盐的20%热灭活胎牛血清(FBS)中。HeLa细胞培养物在含有90%最低限度基本培养基(MEM)-10%FBS的腔室载玻片上单层培养20小时。以10个细菌/哺乳动物细胞的比例在35℃下感染宿主培养物3小时。将感染培养基替换为补充有300微克溶菌酶和5微克庆大霉素/毫升的MEM-FBS。将感染的单层在35℃下孵育5小时以允许细胞内增殖。标本洗涤后,用甲醇固定,先后用美蓝-吉姆萨染料染色。如果发生侵袭,细菌会出现在细胞质内。阳性试验的标准是在3次试验中的2次中,1%的宿主细胞至少含有5个细菌。侵袭性与细胞毒性原理相关且可能由其作为前提条件。感染率从0%到30%不等。在5%-50%的HeLa细胞中观察到细胞病变效应。阳性结果必须通过塞雷尼试验确认。

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