Detection of TEM beta-lactamase genes by non-isotopic spot hybridisation.

G I Carter, K J Towner, R C Slack
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引用次数: 2

Abstract

A 998 bp fragment of plasmid pBR322, comprising part of the TEM-1 beta-lactamase gene, was labelled with biotin-11-dUTP for use as a DNA probe in a rapid non-isotopic spot hybridisation test. Diluted broth cultures of bacteria producing different beta-lactamases were filtered onto nitrocellulose and lysed in situ. Following pre-hybridisation treatment with proteinase K, hybridisation with the labelled probe was demonstrated using a commercially available streptavidine/polyalkaline phosphatase-based detection system. The probe was highly specific, reacting only with strains producing either the TEM-1 or structurally similar TEM-2 enzyme. An inoculum of 3-4 X 10(6) cells gave optimum positive discrimination. When 90 recent ampicillin-resistant strains of Escherichia coli isolated from patients with urinary tract infections were screened using the system, 72% gave a positive hybridisation signal.

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非同位素斑点杂交法检测透射电镜β -内酰胺酶基因。
用生物素-11- dutp标记了质粒pBR322的998 bp片段,该片段包含TEM-1 β -内酰胺酶基因的一部分,用于快速非同位素斑点杂交试验的DNA探针。产生不同β -内酰胺酶的细菌的稀释肉汤培养物被过滤到硝化纤维素上并原位裂解。在用蛋白酶K进行预杂交处理后,使用市售的链亲和胺/多碱性磷酸酶检测系统证明了与标记探针的杂交。该探针具有高度特异性,仅与产生TEM-1或结构相似的TEM-2酶的菌株反应。接种3-4 × 10(6)个细胞获得最佳阳性鉴别。对近期从尿路感染患者中分离到的90株氨苄西林耐药大肠杆菌进行筛选,结果显示,72%的菌株杂交阳性。
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