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首页> 外文期刊>FEMS immunology and medical microbiology >DNA probes for the rapid identification of medically important Candida species using a multianalyte profiling system.
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DNA probes for the rapid identification of medically important Candida species using a multianalyte profiling system.

机译:使用多分析物分析系统快速鉴定医学上重要的念珠菌物种的DNA探针。

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Recently, a new flow cytometric technology to detect multiple DNA target sequences in a single microtiter well plate was developed [multianalyte profiling (MAP) System, Luminex Corp., Austin, TX]. DNA probes, directed to the internal transcribed spacer 2 region of ribosomal DNA, were therefore designed to detect and differentiate PCR amplicons from six medically important Candida species using this system. Each probe was covalently linked to one of 100 available microsphere (bead) sets. Biotinylated PCR amplicons were then hybridized to the complementary probe on each bead set. Bound amplicons were detected fluorometrically using a streptavidin-linked reporter dye, R-phycoerythrin. Specific hybridization was noted for all six Candida species probes (mean sample-to-background ratio+/-standard error: Candida albicans, 58.7+/-1.2; Candida tropicalis, 53.2+/-3.8; Candida glabrata, 46.9+/-2.1; Candida parapsilosis, 59.9+/-1.6; Candida krusei, 54.7+/-3.7 vs. 0.9+/-0.03 for all heterologous Candida species DNA targets and vs. 1.0+/-0.1 for samples containing water instead of DNA; P < 0.001). The limit of test sensitivity was 0.5 pg of DNA. A sample could be processed and analyzed within 1 h post-PCR amplification. Therefore, the multianalyte profiling system was rapid, sensitive and specific for the detection and differentiation of the most medically important species of Candida.
机译:最近,开发了一种新的流式细胞术技术,用于检测单个微量滴定孔板中的多个DNA靶序列[多分析物分析(MAP)系统,Luminex Corp.,奥斯汀,德克萨斯州]。因此,针对该核糖体DNA内部转录的间隔区2区域的DNA探针被设计为使用该系统检测和区分来自六个医学上重要的念珠菌物种的PCR扩增子。每个探针共价连接到100个可用的微球(珠子)组之一。然后将生物素化的PCR扩增子与每个磁珠组上的互补探针杂交。使用链霉亲和素连接的报告染料R-藻红蛋白通过荧光检测结合的扩增子。注意到所有六个念珠菌物种探针的特异性杂交(平均样品与背景之比+/-标准误:白色念珠菌,58.7 +/- 1.2;热带念珠菌,53.2 +/- 3.8;光滑念珠菌,46.9 +/- 2.1;副念珠菌为59.9 +/- 1.6;克鲁斯念珠菌为54.7 +/- 3.7对所有异源念珠菌DNA靶标为0.9 +/- 0.03,而用水代替DNA的样品为1.0 +/- 0.1; P <0.001 )。测试灵敏度的极限是0.5 pg DNA。样品可以在PCR扩增后1小时内进行处理和分析。因此,多分析物谱分析系统快速,灵敏且特异于检测和区分医学上最重要的念珠菌。

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