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从增菌培养物中免疫层析检测B族链球菌抗原。

Immunochromatographic detection of the group B streptococcus antigen from enrichment cultures.

作者信息

Matsui Hidehito, Kimura Juri, Higashide Masato, Takeuchi Yoshio, Okue Kuniyuki, Cui Longzhu, Nakae Taiji, Sunakawa Keisuke, Hanaki Hideaki

机构信息

Research Center for Infections and Antimicrobials, Kitasato Institute for Life Sciences, Kitasato University, Shirokane, Minato-Ku, Tokyo, Japan.

出版信息

Clin Vaccine Immunol. 2013 Sep;20(9):1381-7. doi: 10.1128/CVI.00171-13. Epub 2013 Jul 3.

Abstract

Group B Streptococcus (GBS; Streptococcus agalactiae) is a leading cause of serious neonatal infections. The Centers for Disease Control and Prevention recommends GBS screening for all pregnant women during the 35th to 37th weeks of gestation. Although GBS screening has been performed mainly by the culture-based method, it takes several days to obtain a reliable result. In this study, we developed a rapid immunochromatographic test (ICT) for the detection of GBS-specific surface immunogenic protein in 15 min using an overnight enrichment culture. The ICT was prepared using two anti-Sip monoclonal antibodies. This ICT was able to detect recombinant Sip levels of 0.5 ng/ml, or about 10(6) CFU/ml of GBS cells, in tests with 9 GBS strains of different serotypes. The cross-reactivity test using 26 species of microorganism showed no detectable false-positive result. Reactivity of the ICT with 229 GBS strains showed one false-negative result that was attributable to the production of truncated Sip. Among 260 enrichment cultures of vaginal swabs, 17 produced red to orange pigments in Granada medium, and they were all GBS and Sip positive. Among 219 pigment-negative cultures, 12 were GBS positive and 10 were Sip positive. Two Sip-negative cultures contained GBS cells below the limit of detection by the ICT. Among 207 GBS-negative cultures, only one was Sip positive, which was attributable to GBS cell debris. Thus, the sensitivity and specificity of the ICT appeared to be 93.1% and 99.6%, respectively. The newly developed ICT is readily applicable to clinical use in the detection of GBS.

摘要

B族链球菌(GBS;无乳链球菌)是严重新生儿感染的主要病因。美国疾病控制与预防中心建议对所有孕妇在妊娠第35至37周进行GBS筛查。尽管GBS筛查主要通过基于培养的方法进行,但获得可靠结果需要数天时间。在本研究中,我们开发了一种快速免疫层析试验(ICT),使用过夜富集培养物在15分钟内检测GBS特异性表面免疫原性蛋白。该ICT使用两种抗Sip单克隆抗体制备。在对9种不同血清型的GBS菌株进行的测试中,这种ICT能够检测到0.5 ng/ml的重组Sip水平,或约10⁶CFU/ml的GBS细胞。使用26种微生物进行的交叉反应试验未显示可检测到的假阳性结果。该ICT与229株GBS菌株的反应性显示有一个假阴性结果,这归因于截短型Sip的产生。在260份阴道拭子富集培养物中,17份在格拉纳达培养基中产生红色至橙色色素,它们均为GBS且Sip阳性。在219份色素阴性培养物中,12份GBS阳性,10份Sip阳性。两份Sip阴性培养物中含有低于ICT检测限的GBS细胞。在207份GBS阴性培养物中,只有一份Sip阳性,这归因于GBS细胞碎片。因此,该ICT的敏感性和特异性分别似乎为93.1%和99.6%。新开发的ICT很容易应用于GBS检测的临床应用。

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