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用于肺炎克雷伯菌荚膜血清分型的间接免疫荧光抗体技术的可重复性

Reproducibility of an indirect immunofluorescent-antibody technique for capsular serotyping of Klebsiella pneumoniae.

作者信息

Murcia A, Rubin S J

出版信息

J Clin Microbiol. 1979 Feb;9(2):208-13. doi: 10.1128/jcm.9.2.208-213.1979.

DOI:10.1128/jcm.9.2.208-213.1979
PMID:372225
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC272993/
Abstract

Reproducibility of capsular serotypes of 55 consecutive clinical isolates of Klebsiella pneumoniae was evaluated by an indirect immunofluorescent-antibody technique previously described by Riser et al. (J. Clin. Pathol. 29: 296-304, 1976) Five colonies per specimen were examined for colony-to-colony variation, day-to-day variation, and reader-to-reader variation. Seventy-two reference strains were tested with each of 18 pools and 72 specific antisera prior to the clinical specimens to determine antiserum specificity and cross-reaction patterns. Lot-to-lot variation was examined with the reference strains. There was minimal lot-to-lot variation among the antisera tested. Ten antiserum pools required supplementation with individual antisera. The patterns of supplementation may vary from lot to lot. Colony-to-colony variation in intensity of immunofluorescence occurred, but there was no variation in serotype. These findings differ from previously reported colonial variation which occurred when API 20E biotypes were determined for individual colonies of K. pneumoniae directly from clinical specimens. Eighteen percent of clinical isolates studied gave cross-reactions when tested with the indicated specific antiserum. All but one of the cross-reactions were resolved with further dilutions. Day-to-day and reader-to-reader variations were minimal. The immunofluorescent-antibody technique is a reliable and reproducible method for capsular serotype determination. Capsular serotypes are less variable than API biotypes since colony-to-colony variation of serotype does not occur.

摘要

采用Riser等人先前描述的间接免疫荧光抗体技术(《临床病理学杂志》29: 296 - 304, 1976)对55株连续的肺炎克雷伯菌临床分离株的荚膜血清型可重复性进行了评估。每个标本检查5个菌落,以确定菌落间变异、逐日变异和不同读取者间的变异。在检测临床标本之前,用18个血清池和72种特异性抗血清分别检测72株参考菌株,以确定抗血清特异性和交叉反应模式。用参考菌株检测批次间变异。所检测的抗血清批次间变异极小。10个抗血清池需要补充个别抗血清。补充模式可能因批次而异。免疫荧光强度存在菌落间变异,但血清型无变异。这些发现与先前报道的直接从临床标本中对肺炎克雷伯菌单个菌落进行API 20E生物型测定时出现的菌落变异不同。在所研究的临床分离株中,18%在用指定的特异性抗血清检测时出现交叉反应。除1例交叉反应外,其余均通过进一步稀释得以解决。逐日变异和不同读取者间变异极小。免疫荧光抗体技术是一种可靠且可重复的荚膜血清型测定方法。由于血清型不存在菌落间变异,荚膜血清型比API生物型变异更少。

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本文引用的文献

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