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Fluorogenic LUX Primer for Quantitation of HIV-1 by Real-Time RT-PCR.

机译:用于实时RT-PCR定量HIV-1的荧光LUX引物。

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Measurement of HIV-1 viral load in plasma is an important marker of disease progression and efficacy of antiretroviral therapy. Real-time polymerase chain reaction (PCR) offers an opportunity to develop more affordable alternative viral load assays. This article reports on the development of a novel real-time reverse-transcriptase (RT)-PCR assay for quantitation of HIV-1 RNA copies. This assay utilizes the LightCycler(R) (version2) real-time PCR platform and light upon extension (LUX) primer for specific detection of amplicons. An external standard (ES) for quantitation of viral RNA represents an in vitro transcribed RNA. The LUX assay shows a wide linear (R2 = 0.99) dynamic range from 4 x 106 to 4 x 102 copies/mL. Analytical sensitivity of the assay is 4 x 102 copies/mL of ES RNA. Intra- and inter-assay variability of the LUX assay was less than 0.5log10 copies of ES RNA (i.e., no clinically significant variability was found). Virology quality assurance (VQA) HIV-1 RNA copy controls were used to validate ES and preliminarily evaluate the assay performance. This feasibility study demonstrated that the LUX assay is sensitive, reproducible, and compares well to the Roche Amplicor tests used for characterization of the RNA copy controls. These results suggest further evaluation of the LUX assay using a large cohort of well-characterized samples from HIV-1 positive individuals.
机译:血浆中HIV-1病毒载量的测量是疾病进展和抗逆转录病毒疗法疗效的重要标志。实时聚合酶链反应(PCR)提供了开发更实惠的替代病毒载量测定的机会。本文报道了一种新型实时定量逆转录酶(RT)-PCR检测试剂盒,用于定量HIV-1 RNA拷贝。该测定利用LightCycler(实时版本2)实时PCR平台和延伸引物(LUX)引物对扩增子进行特异性检测。用于定量病毒RNA的外标(ES)代表体外转录的RNA。 LUX测定显示出从4 x 106到4 x 102拷贝/ mL的宽线性(R2 = 0.99)动态范围。该测定法的分析灵敏度为4 x 102拷贝/ mL ES RNA。 LUX测定的测定内和测定间变异性小于0.5log10拷贝的ES RNA(即,未发现临床上显着的变异性)。病毒学质量保证(VQA)HIV-1 RNA复制对照用于验证ES并初步评估测定性能。这项可行性研究表明,LUX检测方法灵敏,可重现,并且与用于表征RNA复制对照的Roche Amplicor检测法相比具有优势。这些结果表明,使用来自HIV-1阳性个体的大量特征明确的样本对LUX分析进行进一步评估。

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