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Yersinia pestis detection by loop-mediated isothermal amplification combined with magnetic bead capture of DNA

机译:通过环介导的等温扩增结合磁珠捕获DNA检测鼠疫耶尔森氏菌

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摘要

We developed a loop-mediated isothermal amplification (LAMP) assay for the detection of Y. pestis by targeting the 3a sequence on chromosome. All 11 species of the genus Yersinia were used to evaluate the specificity of LAMP and PCR, demonstrating that the primers had a high level of specificity. The sensitivity of LAMP or PCR was 2.3 or 23 CFU for pure culture, whereas 2.3 × 10 4 or 2.3 × 10 6 CFU for simulated spleen and lung samples. For simulated liver samples, the sensitivity of LAMP was 2.3 × 10 6 CFU, but PCR was negative at the level of 2.3 × 10 7 CFU. After simulated spleen and lung samples were treated with magnetic beads, the sensitivity of LAMP or PCR was 2.3 × 10 3 or 2.3 × 10 6 CFU, whereas 2.3 × 10 5 or 2.3 × 10 7 CFU for magnetic bead-treated liver samples. These results indicated that some components in the tissues could inhibit LAMP and PCR, and liver tissue samples had a stronger inhibition to LAMP and PCR than spleen and lung tissue samples. LAMP has a higher sensitivity than PCR, and magnetic bead capture of DNAs could remarkably increase the sensitivity of LAMP. LAMP is a simple, rapid and sensitive assay suitable for application in the field or poverty areas.
机译:我们开发了一种环介导的等温扩增(LAMP)测定法,通过靶向染色体上的3a序列来检测鼠疫耶尔森氏菌。耶尔森氏菌属的所有11个物种均用于评估LAMP和PCR的特异性,证明引物具有很高的特异性。对于纯培养物,LAMP或PCR的灵敏度为2.3或23 CFU,而对于模拟的脾脏和肺部样品,其灵敏度为2.3×10 4或2.3×10 6 CFU。对于模拟肝样品,LAMP的灵敏度为2.3×10 6 CFU,但PCR值为2.3×10 7 CFU。用磁珠处理模拟的脾脏和肺部样本后,LAMP或PCR的灵敏度为2.3×10 3或2.3×10 6 CFU,而磁珠处理的肝脏样本的灵敏度为2.3×10 5或2.3×10 7 CFU。这些结果表明,组织中的某些成分可以抑制LAMP和PCR,并且肝组织样品对LAMP和PCR的抑制作用比脾脏和肺组织样品强。 LAMP的灵敏度高于PCR,DNA的磁珠捕获可以显着提高LAMP的灵敏度。 LAMP是一种简单,快速,灵敏的测定方法,适用于野外或贫困地区。

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