{"title":"关于鉴别肠炎起病性肠道细菌用lysine - indom - motility (LIM)培养基","authors":"Hideo Igarashi, K. Ohta, Hiroshi ZEN-YOJI","doi":"10.3412/JSB.24.338","DOIUrl":null,"url":null,"abstract":"Many differential media have been devised for the identification of Shigellae, Salmonellae, and other enteric pathogens. None of them, however, had been designed for the determination of the activity of lysine decarboxylase, indole production, and motility of these organisms in a single tube of medium.The present investigation was undertaken with an objective to reduce the man-hour and to simplify the conventional tedious procedures when a large number of samples were involved. The medium developed in it met those criteria and was named lysine-indole-motility (LIM) medium.1) Composition and usage: LIM medium was composed of 10.0g of polypeptone (Daigo Eiyo Chemicals Co.), 3.0g of yeast extract (Difco), 1.0g of glucose, 10.0g of L-lysine monohydrochloride, 0.5g of L-tryptophan, 0.02g of bromcresol purple, 3.0g of agar, and 1, 000ml of distilled water. After these components were dissolved by heating at 100°C, pH was adjusted to 6.7±0.1. The resulting medium was dispensed into 10×100mm tubes in 3∼4ml amounts and sterilized at 121°C for 15 minutes. After the sterilization, the medium was cooled immediately by putting it into cold water. At use, organisms were picked up from a suspicious colony and stabbed into the middle of the medium. After 24 hours incubation at 37°C, reading was made.2) Results of comparative study: Comparison of results was made between LIM medium and some known differential media. A total of 120 Salmonella strains, 166 Shigella strains, and 87 strains of the other enteric pathogen were used. There was a complete agreement on results. Therefore, the sensitivity and accuracy of the medium were demonstrated. Furthermore, in routine diagnostic use, all the enteric pathogens could be tested easily with the new medium in combination with triple sugar iron (TSI) agar.","PeriodicalId":14812,"journal":{"name":"Japanese journal of bacteriology","volume":"11 1","pages":"338-344"},"PeriodicalIF":0.0000,"publicationDate":"1969-07-25","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"腸炎起病性腸内細菌鑑別用Lysine-Indole-Motility (LIM)培地について\",\"authors\":\"Hideo Igarashi, K. Ohta, Hiroshi ZEN-YOJI\",\"doi\":\"10.3412/JSB.24.338\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"Many differential media have been devised for the identification of Shigellae, Salmonellae, and other enteric pathogens. None of them, however, had been designed for the determination of the activity of lysine decarboxylase, indole production, and motility of these organisms in a single tube of medium.The present investigation was undertaken with an objective to reduce the man-hour and to simplify the conventional tedious procedures when a large number of samples were involved. The medium developed in it met those criteria and was named lysine-indole-motility (LIM) medium.1) Composition and usage: LIM medium was composed of 10.0g of polypeptone (Daigo Eiyo Chemicals Co.), 3.0g of yeast extract (Difco), 1.0g of glucose, 10.0g of L-lysine monohydrochloride, 0.5g of L-tryptophan, 0.02g of bromcresol purple, 3.0g of agar, and 1, 000ml of distilled water. After these components were dissolved by heating at 100°C, pH was adjusted to 6.7±0.1. The resulting medium was dispensed into 10×100mm tubes in 3∼4ml amounts and sterilized at 121°C for 15 minutes. After the sterilization, the medium was cooled immediately by putting it into cold water. At use, organisms were picked up from a suspicious colony and stabbed into the middle of the medium. After 24 hours incubation at 37°C, reading was made.2) Results of comparative study: Comparison of results was made between LIM medium and some known differential media. A total of 120 Salmonella strains, 166 Shigella strains, and 87 strains of the other enteric pathogen were used. There was a complete agreement on results. Therefore, the sensitivity and accuracy of the medium were demonstrated. 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引用次数: 0
摘要
许多鉴别培养基已被设计用于鉴定志贺氏菌、沙门氏菌和其他肠道病原体。然而,没有一种方法被设计用于测定赖氨酸脱羧酶的活性、吲哚的产生和这些生物在单管培养基中的运动性。进行本调查的目的是在涉及大量样本时减少工时并简化传统的繁琐程序。其中培养的培养基符合上述标准,命名为赖氨酸-吲哚-活性(LIM)培养基。1)组成和使用:LIM培养基由10.0g多蛋白胨(Daigo Eiyo Chemicals Co.)、3.0g酵母浸膏(Difco)、1.0g葡萄糖、10.0g l -赖氨酸单盐酸、0.5g l -色氨酸、0.02g溴甲酚紫、3.0g琼脂和1000 ml蒸馏水组成。这些成分在100℃下加热溶解后,调整pH至6.7±0.1。将得到的培养基按3 ~ 4ml的量分配到10×100mm管中,在121°C下灭菌15分钟。灭菌后,立即将培养基放入冷水中冷却。在使用时,从可疑的菌落中取出生物并刺入培养基的中间。37℃孵育24小时后,进行读数。2)对比研究结果:将LIM培养基与一些已知的差示培养基进行结果比较。共检测沙门氏菌120株,志贺氏菌166株,其他肠道病原菌87株。结果是完全一致的。因此,证明了该介质的灵敏度和准确性。此外,在常规诊断中,新培养基与三糖铁(TSI)琼脂结合可方便地检测所有肠道病原体。
Many differential media have been devised for the identification of Shigellae, Salmonellae, and other enteric pathogens. None of them, however, had been designed for the determination of the activity of lysine decarboxylase, indole production, and motility of these organisms in a single tube of medium.The present investigation was undertaken with an objective to reduce the man-hour and to simplify the conventional tedious procedures when a large number of samples were involved. The medium developed in it met those criteria and was named lysine-indole-motility (LIM) medium.1) Composition and usage: LIM medium was composed of 10.0g of polypeptone (Daigo Eiyo Chemicals Co.), 3.0g of yeast extract (Difco), 1.0g of glucose, 10.0g of L-lysine monohydrochloride, 0.5g of L-tryptophan, 0.02g of bromcresol purple, 3.0g of agar, and 1, 000ml of distilled water. After these components were dissolved by heating at 100°C, pH was adjusted to 6.7±0.1. The resulting medium was dispensed into 10×100mm tubes in 3∼4ml amounts and sterilized at 121°C for 15 minutes. After the sterilization, the medium was cooled immediately by putting it into cold water. At use, organisms were picked up from a suspicious colony and stabbed into the middle of the medium. After 24 hours incubation at 37°C, reading was made.2) Results of comparative study: Comparison of results was made between LIM medium and some known differential media. A total of 120 Salmonella strains, 166 Shigella strains, and 87 strains of the other enteric pathogen were used. There was a complete agreement on results. Therefore, the sensitivity and accuracy of the medium were demonstrated. Furthermore, in routine diagnostic use, all the enteric pathogens could be tested easily with the new medium in combination with triple sugar iron (TSI) agar.
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