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Multiplexed Quantification of Nucleic Acids with Large Dynamic Range Using Multivolume Digital RT-PCR on a Rotational SlipChip Tested with HIV and Hepatitis C Viral Load

机译:用HIV和丙型肝炎病毒载量测试多变数字RT-PCR大动态范围的核酸的多重定量核酸

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摘要

In this paper, we are working toward a problem of great importance to global health: determination of viral HIV and hepatitis C (HCV) loads under point-of-care and resource limited settings. While antiretroviral treatments are becoming widely available, viral load must be evaluated at regular intervals to prevent the spread of drug resistance and requires a quantitative measurement of RNA concentration over a wide dynamic range (from 50 up to 10^6 molecules/mL for HIV and up to 108 molecules/mL for HCV). “Digital” single molecule measurements are attractive for quantification, but the dynamic range of such systems is typically limited or requires excessive numbers of compartments. Here we designed and tested two microfluidic rotational SlipChips to perform multivolume digital RT-PCR (MV digital RT-PCR) experiments with large and tunable dynamic range. These designs were characterized using synthetic control RNA and validated with HIV viral RNA and HCV control viral RNA. The first design contained 160 wells of each of four volumes (125 nL, 25 nL, 5 nL, and 1 nL) to achieve a dynamic range of 5.2 × 10^2 to 4.0 × 10^6 molecules/mL at 3-fold resolution. The second design tested the flexibility of this approach, and further expanded it to allow for multiplexing while maintaining a large dynamic range by adding additional wells with volumes of 0.2 nL and 625 nL and dividing the SlipChip into five regions to analyze five samples each at a dynamic range of 1.8 × 10^3 to 1.2 × 10^7 molecules/mL at 3-fold resolution. No evidence of cross-contamination was observed. The multiplexed SlipChip can be used to analyze a single sample at a dynamic range of 1.7 × 10^2 to 2.0 × 10^7 molecules/mL at 3-fold resolution with limit of detection of 40 molecules/mL. HIV viral RNA purified from clinical samples were tested on the SlipChip, and viral load results were self-consistent and in good agreement with results determined using the Roche COBAS AmpliPrep/COBAS TaqMan HIV-1 Test. With further validation, this SlipChip should become useful to precisely quantify viral HIV and HCV RNA for high-performance diagnostics in resource-limited settings. These microfluidic designs should also be valuable for other diagnostic and research applications, including detecting rare cells and rare mutations, prenatal diagnostics, monitoring residual disease, and quantifying copy number variation and gene expression patterns. The theory for the design and analysis of multivolume digital PCR experiments is presented in other work by Kreutz et al.
机译:在本文中,我们正在努力解决一个对全球健康至关重要的问题:在现场护理和资源有限的情况下确定病毒性HIV和丙型肝炎(HCV)的载量。虽然抗逆转录病毒疗法的广泛使用,但必须定期评估病毒载量以防止耐药性的蔓延,并且需要在广泛的动态范围内对RNA浓度进行定量测量(对于HIV和HIV,从50至10 ^ 6分子/ mL) HCV最高可达108分子/ mL)。 “数字”单分子测量对于定量分析很有吸引力,但是此类系统的动态范围通常受到限制或需要过多的隔室。在这里,我们设计并测试了两个微流体旋转滑动芯片,以进行动态范围大且可调的多体积数字RT-PCR(MV数字RT-PCR)实验。这些设计使用合成的对照RNA进行表征,并用HIV病毒RNA和HCV对照病毒RNA进行验证。第一个设计包含160个孔,每个孔有四个容积(125 nL,25 nL,5 nL和1 nL),以3倍的分辨率实现5.2×10 ^ 2至4.0×10 ^ 6分子/ mL的动态范围。第二个设计测试了这种方法的灵活性,并通过添加额外的体积分别为0.2 nL和625 nL的孔并将滑动芯片划分为五个区域以分别分析五个样品,从而进一步扩展了该方法以允许多路复用,同时保持较大的动态范围。在3倍分辨率下,动态范围为1.8×10 ^ 3到1.2×10 ^ 7分子/ mL。没有观察到交叉污染的证据。多重SlipChip可用于以1.7×10 ^ 2至2.0×10 ^ 7分子/ mL的动态范围以3倍的分辨率分析单个样品,检测限为40个分子/ mL。从临床样本中纯化的HIV病毒RNA在SlipChip上进行了测试,病毒载量结果是自洽的,并且与使用Roche COBAS AmpliPrep / COBAS TaqMan HIV-1测试确定的结果非常吻合。经过进一步验证,这种滑动芯片应可用于精确定量病毒HIV和HCV RNA,从而在资源有限的环境中进行高性能诊断。这些微流体设计对于其他诊断和研究应用也应该是有价值的,包括检测稀有细胞和稀有突变,产前诊断,监测残留疾病以及定量拷贝数变异和基因表达模式。 Kreutz等人在其他工作中提出了用于多体积数字PCR实验设计和分析的理论。

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