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甘氨酸对携带R因子的大肠杆菌K12耐药性的消除作用。

Eliminatory action of glycine on drug resistance of Escherichia coli K12 harboring an R factor.

作者信息

Tomoeda M, Inuzuka M, Hayashi M

出版信息

Jpn J Microbiol. 1976 Feb;20(1):27-32. doi: 10.1111/j.1348-0421.1976.tb00904.x.

Abstract

Glycine, known to inhibit the synthesis of a peptidoglycan component of the bacterial cell wall, was effective in eliminating drug resistance of Escherichia coli K12 JE2100 strain harboring theR100-1 factor although in lower frequencies than that of sodium dodecyl sulfate (SDS). The action of glycine was found to be less effective on the same R factor in JE177 strain, and not effective on the F factor in W6. Infection of R factors from R+ cells to R- cells was found to take place in the glycine broth as efficiently as in broth without glycine. This might result in lowering the apparent efficiency of the action of glycine on those plasmids. The segregation patterns of drug-susceptible clones obtained by the glycine treatment were different from those obtained after the SDS treatment. These results coupled with other evidences suggest that the mode of action of glycine on R+ cells maybe different from those of other curing agents and may involve mechanisms other than selection of R- or drug susceptible segregantsthat are present in R+ culture.

摘要

已知甘氨酸可抑制细菌细胞壁肽聚糖成分的合成,它能有效消除携带R100 - 1因子的大肠杆菌K12 JE2100菌株的耐药性,不过其频率低于十二烷基硫酸钠(SDS)。研究发现,甘氨酸对JE177菌株中相同R因子的作用效果较差,对W6菌株中的F因子则无作用。结果表明,R⁺细胞中的R因子向R⁻细胞的转移在甘氨酸肉汤中与在不含甘氨酸的肉汤中一样高效。这可能导致甘氨酸对这些质粒作用的表观效率降低。经甘氨酸处理获得的药物敏感克隆的分离模式与经SDS处理后获得的不同。这些结果与其他证据表明,甘氨酸对R⁺细胞的作用方式可能与其他消除剂不同,可能涉及除选择R⁻或R⁺培养物中存在的药物敏感分离株之外的机制。

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