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MBCs for Staphylococcus aureus as determined by macrodilution and microdilution techniques.

机译:通过宏观稀释和微量稀释技术测定的金黄色葡萄球菌的MBC。

摘要

MBC testing of clindamycin, methicillin, cephalothin, gentamicin, and vancomycin with 67 clinical isolates of Staphylococcus aureus was examined by both standard macrodilution tubes and commercial microdilution trays. Standard macrodilution failed to give reproducible (99.9% killing) MBC results, even when a strictly defined protocol was followed. Continuous shaking during incubation resulted in regrowth of more colonies than did stationary incubation. Vortexing of incubated tubes before subculture resulted in regrowth of more colonies than did careful transfer of the contents to sterile tubes before vortexing and subculture. No significant difference in MBCs was demonstrated by the use of log-phase versus stationary-phase inocula. Use of the multiprong inoculator for subculture from commercial microdilution trays was unsatisfactory because, although antibiotics evaluated were inactivated by subculture to a pH 5.5 agar plate coated with a beta-lactamase solution, the volume of broth transferred by the prongs was small and inconsistent, ranging from 0 to 3 microliter. Subcultures of commercial microdilution panels with a 1-microliter loop, 10-microliter pipette, and 100-microliter pipette were also evaluated. Results of MBC testing were most reproducible when the entire 100-microliter volume was aspirated from commercial microdilution wells after stirring and the contents of each well were spread over a separate sheep blood agar plate.
机译:通过标准的大型稀释管和市售微量稀释盘,对67株金黄色葡萄球菌临床分离株进行了克林霉素,甲氧西林,头孢菌素,庆大霉素和万古霉素的MBC检测。即使采用严格定义的方案,标准的宏观稀释法也无法提供可再现的(99.9%的杀死率)MBC结果。孵育过程中连续摇动导致的菌落再生比固定培养更多。与在涡旋和继代培养之前小心地将内含物转移到无菌试管中相比,在传代培养前对培养管进行涡旋培养会导致更多的菌落再生。对数相和固定相接种均未显示MBC的显着差异。使用多叉接种器从商业微量稀释托盘进行继代培养并不令人满意,因为尽管评估的抗生素是通过继代培养到涂有β-内酰胺酶溶液的pH 5.5琼脂平板上而失活的,但是通过插脚转移的肉汤体积很小且不一致,范围从0到3微升。还评估了带有1微升定量环,10微升移液器和100微升移液器的商业微稀释板的亚培养物。搅拌后从商业微量稀释孔中吸出全部100微升体积,并将每个孔的内容物铺在单独的羊血琼脂平板上,MBC测试结果最可重复。

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