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采用被动免疫溶血法对大肠杆菌不耐热肠毒素进行直接血清学检测。

Direct serological assay for the heat-labile enterotoxin of Escherichia coli, using passive immune hemolysis.

作者信息

Evans D J, Evans D G

出版信息

Infect Immun. 1977 May;16(2):604-9. doi: 10.1128/iai.16.2.604-609.1977.

Abstract

Sheep erythrocytes sensitized with the heat-labile enterotoxin (LT) of Escherichia coli exhibited passive immune hemolysis (PIH) when exposed to specific antitoxin and complement. Thus, PIH serves as the basis for an in vitro serological assay for LT that is sufficiently specific and sensitive to differentiate LT-positive and LT-negative E. coli isolates. The PIH assay for E. coli LT has been performed with the standard Microtiter system and also by a tube method employing the spectrophotometric determination of hemoglobin release. The spectrophotometric method enhances the sensitivity, accuracy, and objectivity of the PIH assay. The increased sensitivity of the spectrophotometric method also facilitates the identification of LT-positive cultures employing polymyxin "mini-extracts" of whole overnight (18 h) broth cultures of 2.0% Casamino Acid-0.6% yeast extract-salts medium rather than mini-extracts of cells derived from 3.5-h subcultures. Thus, large numbers of E. coli isolates can be individually tested for LT in less than 24 h after broth inoculation by a rapid in vitro assay which requires anti-LT serum as the only specific reagent.

摘要

用大肠杆菌不耐热肠毒素(LT)致敏的绵羊红细胞在暴露于特异性抗毒素和补体时会出现被动免疫溶血(PIH)。因此,PIH可作为一种体外LT血清学检测方法的基础,该方法具有足够的特异性和敏感性,能够区分LT阳性和LT阴性大肠杆菌分离株。大肠杆菌LT的PIH检测已通过标准微量滴定系统进行,也通过采用分光光度法测定血红蛋白释放的试管法进行。分光光度法提高了PIH检测的灵敏度、准确性和客观性。分光光度法提高的灵敏度还便于使用2.0%酪蛋白氨基酸-0.6%酵母提取物-盐培养基的全夜(18小时)肉汤培养物的多粘菌素“微量提取物”,而不是3.5小时传代培养物的细胞微量提取物来鉴定LT阳性培养物。因此,通过一种快速体外检测方法,在肉汤接种后不到24小时内,就可以对大量大肠杆菌分离株单独进行LT检测,该方法仅需要抗LT血清作为唯一的特异性试剂。

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