Weldon School of Biomedical Engineering, Purdue University, West Lafayette, IN, USA.
School of Mechanical Engineering, Purdue University, West Lafayette, IN, USA.
Anal Chim Acta. 2022 Apr 22;1203:339702. doi: 10.1016/j.aca.2022.339702. Epub 2022 Mar 9.
In 2019 the COVID-19 pandemic, caused by SARS-CoV-2, demonstrated the urgent need for rapid, reliable, and portable diagnostics. The COVID-19 pandemic was declared in January 2020 and surges of the outbreak continue to reoccur. It is clear that early identification of infected individuals, especially asymptomatic carriers, plays a huge role in preventing the spread of the disease. The current gold standard diagnostic for SARS-CoV-2 is quantitative reverse transcription polymerase chain reaction (qRT-PCR) test based on the detection of the viral RNA. While RT-PCR is reliable and sensitive, it requires expensive centralized equipment and is time consuming (∼2 h or more); limiting its applicability in low resource areas. The FDA issued Emergency Use Authorizations (EUAs) for several COVID-19 diagnostics with an emphasis on point-of care (PoC) testing. Numerous RT-PCR and serological tests were approved for use at the point of care. Abbott's ID NOW, and Cue Health's COVID-19 test are of particular interest, which use isothermal amplification methods for rapid detection in under 20 min. We look to expand on the range of current PoC testing platforms with a new rapid and portable isothermal nucleic acid detection device. We pair reverse transcription loop mediated isothermal amplification (RT-LAMP) with a particle imaging technique, particle diffusometry (PD), to successfully detect SARS-CoV-2 in only 35 min on a portable chip with integrated heating. A smartphone device is used to image the samples containing fluorescent beads post-RT-LAMP and correlates decreased diffusivity to positive samples. We detect as little as 30 virus particles per μL from a RT-LAMP reaction in a microfluidic chip using a portable heating unit. Further, we can perform RT-LAMP from a diluted unprocessed saliva sample without RNA extraction. Additionally, we lyophilize SARS-CoV-2-specific RT-LAMP reactions that target both the N gene and the ORF1ab gene in the microfluidic chip, eliminating the need for cold storage. Our assay meets specific target product profiles outlined by the World Health Organization: it is specific to SARS-CoV-2, does not require cold storage, is compatible with digital connectivity, and has a detection limit of less than 35 × 10 viral particles per mL in saliva. PD-LAMP is rapid, simple, and attractive for screening and use at the point of care.
2019 年,由严重急性呼吸系统综合征冠状病毒 2(SARS-CoV-2)引发的 COVID-19 大流行,突显了对快速、可靠和便携诊断的迫切需求。COVID-19 大流行于 2020 年 1 月宣布,疫情爆发仍在持续。很明显,早期识别感染者,特别是无症状携带者,在阻止疾病传播方面发挥着巨大作用。目前,针对 SARS-CoV-2 的金标准诊断方法是基于病毒 RNA 检测的定量逆转录聚合酶链反应(qRT-PCR)测试。虽然 RT-PCR 可靠且灵敏,但它需要昂贵的集中式设备且耗时(约 2 小时或更长时间);限制了其在资源匮乏地区的适用性。食品和药物管理局(FDA)发布了几项 COVID-19 诊断的紧急使用授权(EUA),重点是即时护理(PoC)检测。许多 RT-PCR 和血清学检测被批准在即时护理点使用。雅培的 ID NOW 和 Cue Health 的 COVID-19 检测尤其受到关注,它们使用等温扩增方法在不到 20 分钟内进行快速检测。我们希望通过一种新的快速便携等温核酸检测设备来扩展当前 PoC 检测平台的范围。我们将逆转录环介导等温扩增(RT-LAMP)与粒子成像技术,即粒子扩散度测定(PD)相结合,成功地在带有集成加热功能的便携式芯片上仅在 35 分钟内检测到 SARS-CoV-2。智能手机设备用于对 RT-LAMP 反应后含有荧光珠的样品进行成像,并将扩散度降低与阳性样品相关联。我们使用便携式加热单元在微流控芯片中从 RT-LAMP 反应中检测到低至 30 个病毒颗粒/μL。此外,我们可以在没有 RNA 提取的情况下对稀释的未处理唾液样本进行 RT-LAMP。此外,我们在微流控芯片中冻干针对 SARS-CoV-2 的 N 基因和 ORF1ab 基因的特异性 RT-LAMP 反应,消除了对冷藏的需求。我们的检测符合世界卫生组织(WHO)规定的特定目标产品概况:它是针对 SARS-CoV-2 的,不需要冷藏,兼容数字连接,在唾液中的检测限低于 35×10 个病毒颗粒/mL。PD-LAMP 快速、简单,非常适合即时护理点的筛查和使用。
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