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软质成熟奶酪中肠致病性大肠杆菌的检测与生长

Detection and growth of enteropathogenic Escherichia coli in soft ripened cheese.

作者信息

Fantasia L D, Mestrandrea L, Schrade J P, Yager J

出版信息

Appl Microbiol. 1975 Feb;29(2):179-85. doi: 10.1128/am.29.2.179-185.1975.

Abstract

The organism most frequently encountered during the 1971 outbreak of enteropathogenic Escherichia coli (EPEC) in soft ripened cheese was a strain that failed to ferment lactose broth within 48 h. Since existing methods for E. coli are dependent upon fermentation of this sugar, such strains can remain undetected, particularly when present in low numbers. Therefore a cultural testing procedure was developed to insure isolation of both lactose-positive and -negative strains. This method used GN broth, modified by substituting lactose and arabinose for glucose and D-mannitol, as an enrichment medium. MacConkey agar, used as a plating medium, was modified by substituting arabinose for half the lactose. The cultural procedure was used in conjunction with a fluorescent antibody method to screen cheese for the presence of presumptive enteropathogenic E. coli. Suspected isolates were subjected to further biochemical and serological testing and identified as members of specific serogroups. These methods were used for the analysis of over 2,000 wheels of cheese; over 10% of the samples tested were found to contain strains belonging to six different serogroups associated with diarrheal diseases. No attempt was made to confirm pathogenicity by in vivo tests. Enumeration of E. coli in cheese showed that numbers increased during storage. Cheese with less than 10 organisms/g initially increased to over 10-5 at room temperature and over 10-3 at 4 C within 10 days. With higher initial counts, levels up to 10-9 were found at 4 C. These studies showed that the high levels of E. coli encountered in these products cannot be used as a direct indicator of post-processing contamination.

摘要

1971年软质成熟奶酪爆发肠道致病性大肠杆菌(EPEC)疫情期间,最常遇到的菌株是在48小时内无法发酵乳糖肉汤的菌株。由于现有的大肠杆菌检测方法依赖于这种糖的发酵,此类菌株可能仍未被检测到,尤其是数量较少时。因此,开发了一种培养检测程序,以确保分离出乳糖阳性和阴性菌株。该方法使用通过用乳糖和阿拉伯糖替代葡萄糖和D-甘露糖醇进行改良的GN肉汤作为增菌培养基。用作平板培养基的麦康凯琼脂通过用阿拉伯糖替代一半乳糖进行改良。该培养程序与荧光抗体法结合使用,以筛查奶酪中是否存在推定的肠道致病性大肠杆菌。对疑似分离株进行进一步的生化和血清学检测,并鉴定为特定血清群的成员。这些方法用于分析2000多个奶酪轮;超过10%的测试样品被发现含有属于与腹泻病相关的六个不同血清群的菌株。未尝试通过体内试验确认致病性。奶酪中大肠杆菌的计数表明,储存期间数量会增加。初始菌数少于10个/克的奶酪在室温下10天内增加到超过10⁵,在4℃下增加到超过10³。初始菌数较高时,在4℃下可发现菌数高达10⁹。这些研究表明,这些产品中遇到的高水平大肠杆菌不能用作加工后污染的直接指标。

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