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首页> 外文期刊>Journal of Clinical Microbiology >Use of an immunoperoxidase method for identification of Bacteroides fragilis.
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Use of an immunoperoxidase method for identification of Bacteroides fragilis.

机译:免疫过氧化物酶方法用于鉴定脆弱拟杆菌的用途。

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摘要

An indirect immunoperoxidase (IP) slide test was evaluated for the laboratory identification of Bacteroides fragilis. Antigen-antibody complexes were detected with goat anti-rabbit immunoglobulin G-peroxidase conjugate with 3-amino-9-ethyl-carbazole as the peroxidase substrate. Ninety-one percent of 44 B. fragilis strains tested were IP positive (3+ to 4+ reactions) with greater than or equal to 1:160 dilutions of rabbit antiserum produced against whole cells of B. fragilis ATCC 23745. The antiserum was species specific. No cross-reactions were observed with 35 Bacteroides strains of other species or with a variety of facultative or aerobic gram-negative bacilli. Four B. fragilis strains were IP negative. One of these (VPI 2393) was the deoxyribonucleic acid (DNA) homology group II reference strain. The other three were clinical isolates. IP-negative and representative IP-positive strains were tested for DNA homology with the type strains for DNA homology groups I and II (VPI 2553 and VPI 2393). Two of the three clinical isolates were classified as DNA homology group II, and the remaining strain was classified as a group I. Capsular material known to be unique to B. fragilis was common to both DNA homology groups as indicated by reactions with purified anticapsular antiserum. The IP technique provides a suitable alternative to fluorescent microscopy for the rapid immunological identification of B. fragilis.
机译:评价了间接免疫过氧化物酶(IP)玻片试验,用于实验室鉴定脆弱的拟杆菌。用带有3-氨基-9-乙基咔唑作为过氧化物酶底物的山羊抗兔免疫球蛋白G-过氧化物酶偶联物检测抗原-抗体复合物。测试的44脆弱类B.菌株中有91%呈IP阳性(3+至4+反应),且针对脆弱类B. ATCC 23745的全细胞产生的兔抗血清稀释度大于或等于1:160。具体。与35个其他种类的拟杆菌属菌株或各种兼性或需氧革兰氏阴性杆菌均未观察到交叉反应。四种脆弱的芽孢杆菌菌株均为IP阴性。其中之一(VPI 2393)是脱氧核糖核酸(DNA)同源性II组参考菌株。其他三个是临床分离株。测试了IP阴性和代表性IP阳性菌株的DNA同源性,以及I和II组DNA同源性的类型菌株(VPI 2553和VPI 2393)。三个临床分离株中的两个被分类为DNA同源性II组,其余的菌株被分类为I组。已知与脆弱型芽孢杆菌相对应的荚膜材料在两个DNA同源性组中都是相同的,这与纯化的抗荚膜抗血清反应表明。 IP技术提供了一种合适的荧光显微镜替代方法,用于快速免疫鉴定脆弱的芽孢杆菌。

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