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首页> 外文期刊>Journal of Clinical Microbiology >Novel, ultrasensitive, Q-beta replicase-amplified hybridization assay for detection of Chlamydia trachomatis.
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Novel, ultrasensitive, Q-beta replicase-amplified hybridization assay for detection of Chlamydia trachomatis.

机译:用于检测沙眼衣原体的新型超灵敏Q-beta复制酶扩增杂交检测方法。

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A sensitive, nonisotopic hybridization assay termed "dual capture" is described. The assay rapidly and specifically detects very low levels of target nucleic acids and organisms. The assay is based on the principles of sandwich hybridization, reversible target capture, and Q-Beta replicase amplification. The assay can be completed in less than 4 h, and in the described model format, it detects Chlamydia trachomatis rRNA or rDNA. Up to 96 samples can be analyzed simultaneously. The assay employs two types of probes: a test-specific capture probe, which mediates the cycling of the target probe complex on and off derivatized magnetic beads, and a replicatable RNA detector molecule containing a sequence complementary to and adjacent to the capture probe site on the target. Following reversible target capture, detection of the signal is accomplished by replication of the detector molecule by Q-Beta replicase in the presence of propidium iodide. A specific assay signal can be detected from as few as 1,000 molecules above the background. In a limited study of 94 urogenital samples the assay detected five of the six culture-positive samples and did not detect the C. trachomatis target in 85 of the 88 culture-negative samples.
机译:描述了称为“双重捕获”的敏感的非同位素杂交测定。该测定法可以快速,特异性地检测极低水平的靶核酸和生物。该测定基于三明治杂交,可逆靶标捕获和Q-Beta复制酶扩增的原理。该测定可以在不到4小时内完成,并且以所述的模型格式,它可以检测沙眼衣原体rRNA或rDNA。可以同时分析多达96个样品。该测定法使用两种类型的探针:一种测试特异性捕获探针,可介导目标探针复合物在衍生的磁珠上和在衍生磁珠上的循环;一种可复制的RNA检测器分子,其包含与捕获探针位点互补并相邻的序列。目标。在可逆的靶标捕获之后,通过在碘化丙锭存在下通过Q-β复制酶复制检测器分子来完成信号的检测。可以从高于背景的低至1,000个分子中检测到特定的测定信号。在一项针对94个泌尿生殖道样本的有限研究中,该检测方法检测到了六个培养阳性样本中的五个,而未检测到88个培养阴性样本中的85个沙眼衣原体靶标。

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