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METHOD FOR MEASURING THE SIZE DISTRIBUTION OF AIRBORNE RHINOVIRUS

机译:测量空气鼻病毒尺寸分布的方法

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About 50% of viral-induced respiratory illnesses are caused by the human rhino virus (HRV). Measurements of the concentrations and sizes of bioaerosols are critical for research on building characteristics, aerosol transport, and mitigation measures. We developed a quantitative reverse transcription-coupled polymerase chain reaction (RT-PCR) assay for HRV and verified that this assay detects HRV in nasal lavage samples. A quantitation standard was used to determine a detection limit of 5 fg of HRV RNA with a linear range over 1000-fold. To measure the size distribution of HRV aerosols, volunteers with a head cold spent two hours in a ventilated research chamber. Airborne particles from the chamber were collected using an Andersen Six-Stage Cascade Impactor. Each stage of the impactor was analyzed by quantitative RT-PCR for HRV. For the first two volunteers with confirmed HRV infection, but with mild symptoms, we were unable to detect HRV on any stage of the impactor.
机译:大约50%的病毒诱导的呼吸疾病是由人犀牛病毒(HRV)引起的。生物溶胶浓度和尺寸的测量对于研究建筑特征,气溶胶运输和缓解措施至关重要。我们开发了用于HRV的定量逆转录偶联聚合酶链反应(RT-PCR)测定,并验证该测定检测鼻灌洗样品中的HRV。定量标准用于确定具有1000倍超过1000倍的线性范围的5FG的检测限。为了测量HRV气溶胶的大小分布,志愿者在通风的研究室中花了两个小时。使用Andersen六级级联撞击器收集来自腔室的空气颗粒。通过定量RT-PCR进行影响,分析了撞击器的每个阶段。对于具有证实的HRV感染的前两名志愿者,但症状轻微,我们无法在撞击器的任何阶段检测HRV。

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