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H7抗血清-山梨醇发酵培养基:一种用于检测与出血性结肠炎相关的大肠杆菌O157:H7的单管筛选培养基。

H7 antiserum-sorbitol fermentation medium: a single tube screening medium for detecting Escherichia coli O157:H7 associated with hemorrhagic colitis.

作者信息

Farmer J J, Davis B R

出版信息

J Clin Microbiol. 1985 Oct;22(4):620-5. doi: 10.1128/jcm.22.4.620-625.1985.

Abstract

Escherichia coli serotype O157:H7 has been isolated from outbreaks and sporadic cases of hemorrhagic colitis. There is convincing evidence that it can cause this diarrheal disease. Because of the interest in hemorrhagic colitis, it has become desirable to detect this particular strain in human feces, which usually contains many other strains of E. coli. Two characteristics of the incriminated E. coli O157:H7 strain have made its isolation and identification easier. It does not ferment D-sorbitol rapidly, in contrast to about 95% of other E. coli strains. In addition, the strain has H antigen 7, but only about 10% of other E. coli strains have this particular antigen. To screen for E. coli O157:H7 we devised H7 antiserum-sorbitol fermentation medium (18 g of enteric fermentation base, 10 g of D-sorbitol, 4 g of agar, 10 ml of Andrade indicator, 989 ml of water; all ingredients were mixed, autoclaved, and cooled; 1 ml of E. coli H7 antiserum was then added). Colonies to be screened were inoculated into this medium. Strains of E. coli O157:H7 gave a characteristic pattern; they did not ferment sorbitol and were immobilized in the semisolid medium because of the reaction of their flagella with the flagella antiserum. Almost all other strains of E. coli gave a different pattern; they fermented sorbitol or were not immobilized by the H7 serum or both. Strains which were presumptive positives (sorbitol negative, H7 positive) were then tested in E. coli O157 serum by slide or tube agglutination. The number of strains which were presumptive positive by H7-sorbitol medium but then were not found to be O157 was less than 1%. A second approach has been helpful in deciding which colonies to screen in H7-sorbitol medium. MacConkey-sorbitol agar (22.2 g MacConkey agar base [which contains no sugar], 10 g of D-sorbitol, 1,000 ml of water) was designed as a plating medium. Stools were plated on MacConkey agar to estimate the number of E. coli colonies and also plated on MacConkey-sorbitol agar to estimate the number of sorbitol-negative colonies of E. coli. These two approaches have proved useful for isolating and identifying E. coli O157:H7 form human feces and from feces of animals infected in the laboratory with this strain. The results suggest that media may be formulated in a similar fashion for detecting other specific strains of E. coli.

摘要

大肠杆菌O157:H7血清型已从出血性结肠炎的暴发疫情和散发病例中分离出来。有确凿证据表明它可引发这种腹泻病。鉴于对出血性结肠炎的关注,检测人类粪便中这种特定菌株变得很有必要,因为人类粪便中通常含有许多其他大肠杆菌菌株。被怀疑的大肠杆菌O157:H7菌株的两个特性使其分离和鉴定变得更容易。与约95%的其他大肠杆菌菌株不同,它不能快速发酵D-山梨醇。此外,该菌株具有H抗原7,但只有约10%的其他大肠杆菌菌株具有这种特定抗原。为筛选大肠杆菌O157:H7,我们设计了H7抗血清-山梨醇发酵培养基(18克肠道发酵基础培养基、10克D-山梨醇、4克琼脂、10毫升安德拉德指示剂、989毫升水;将所有成分混合、高压灭菌并冷却;然后加入1毫升大肠杆菌H7抗血清)。将待筛选的菌落接种到该培养基中。大肠杆菌O157:H7菌株呈现出特征性模式;它们不发酵山梨醇,并且由于其鞭毛与鞭毛抗血清的反应而在半固体培养基中被固定。几乎所有其他大肠杆菌菌株呈现出不同的模式;它们发酵山梨醇或不被H7血清固定或两者皆有。然后通过玻片或试管凝集试验在大肠杆菌O157血清中对推定阳性菌株(山梨醇阴性、H7阳性)进行检测。通过H7-山梨醇培养基推定阳性但后来未被发现为O157的菌株数量不到1%。第二种方法有助于确定在H7-山梨醇培养基中筛选哪些菌落。麦康凯-山梨醇琼脂(22.2克麦康凯琼脂基础培养基[不含糖]、10克D-山梨醇、1000毫升水)被设计为一种平板培养基。将粪便接种在麦康凯琼脂上以估计大肠杆菌菌落数量,同时接种在麦康凯-山梨醇琼脂上以估计大肠杆菌山梨醇阴性菌落数量。这两种方法已被证明可用于从人类粪便以及实验室感染该菌株的动物粪便中分离和鉴定大肠杆菌O157:H7。结果表明,可以以类似方式配制培养基来检测其他特定的大肠杆菌菌株。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ebd5/268479/bb6b8e1f78f9/jcm00111-0173-a.jpg

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