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首页> 外文期刊>Diagnostic microbiology and infectious disease >Construction of internal control for the quantitative assay of Aspergillus fumigatus using real-time nucleic acid sequence-based amplification.
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Construction of internal control for the quantitative assay of Aspergillus fumigatus using real-time nucleic acid sequence-based amplification.

机译:使用基于实时核酸序列的扩增法构建烟曲霉定量测定的内部对照。

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摘要

We have developed a scheme for quantitative real-time (RTi) nucleic acid sequence-based amplification (NASBA) for the detection of Aspergillus fumigatus using internal control (IC) RNA. Construction of IC RNA began with the synthesis of nontarget sequences from Clavibacter michiganensis subsp. sepedonicus by a primary polymerase chain reaction (PCR) step, followed by a secondary PCR step using chimeric primers to produce a chimeric sequence including a T7 promoter region. Finally, chimeric IC RNAs were constructed by the use of in vitro transcription. The assay detected A. fumigatus within a range of 10(4) to 10(8) copies/mL of RNA and 10(0) to 10(8) cells. When the assay was performed with the target and IC RNA in 1 reaction in a single tube, there was little interference of the IC RNA in the measurement of the amount of target. The amount of RNA calculated using the assay was not significantly different from the amount of input RNA as indicated by Bland-Altman analysis. The IC RNA we constructed can be used in RTi-NASBA for quantitative detection of Aspergillus with good precision and accuracy.
机译:我们已经开发了一种基于内部控制(IC)RNA的实时定量(RTi)核酸序列扩增(NASBA)方案,用于检测烟曲霉。 IC RNA的构建始于从密歇根氏杆菌属亚种合成非靶序列。初次聚合酶链反应(PCR)步骤,然后使用嵌合引物进行次要PCR步骤,以产生包含T7启动子区域的嵌合序列。最后,通过使用体外转录构建嵌合IC RNA。该检测方法检测到的烟曲霉的RNA和10(0)至10(8)细胞的范围在10(4)至10(8)个拷贝/ mL。当在单个试管中对1个反应中的靶标和IC RNA进行测定时,在靶标量的测量中IC RNA几乎没有干扰。如通过Bland-Altman分析所表明的,使用该测定法计算的RNA的量与输入的RNA的量没有显着差异。我们构建的IC RNA可用于RTi-NASBA中,以良好的精度和准确度定量检测曲霉。

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