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首页> 外文期刊>Environmental Science: Water Research & Technology >Propidium monoazide pretreatment on a 3D-printed microfluidic device for efficient PCR determination of live versus dead' microbial cells
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Propidium monoazide pretreatment on a 3D-printed microfluidic device for efficient PCR determination of live versus dead' microbial cells

机译:在3D打印的微流控设备上进行单叠氮化丙锭预处理,以有效PCR测定活微生物与死微生物

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摘要

Waterborne microbial pathogen detection via nucleic acid analysis on portable microfluidic devices is a growing area of research, development, and application. Traditional polymerase chain reaction (PCR)-based nucleic acid analysis detects total extracted DNA, but cannot differentiate live and dead cells. A propidium monoazide (PMA) pretreatment step before PCR can effectively exclude DNA from nonviable cells, as PMA can selectively diffuse through compromised cell membranes and intercalate with DNA to form DNA-PMA complex upon light exposure. The complex strongly inhibits the amplification of the bound DNA in PCR, and thus, only cells with intact cell membranes are detected. Herein, this study reports the development of a microfluidic device to carry out PMA pretreatment ` on-chip'. Chip design was guided by computer simulations, and prototypes were fabricated using a high-resolution 3D printer. The optimized design utilizes split and recombine mixers for initial PMA-sample mixing and a serpentine flow channel containing herringbone structures for dark and light incubation. On-chip PMA pretreatment to differentiate live and dead bacterial cells in buffer and natural pond water samples was successfully demonstrated.
机译:通过便携式微流控设备上的核酸分析对水性微生物病原体进行检测是研究,开发和应用领域中不断增长的领域。基于传统聚合酶链反应(PCR)的核酸分析可检测提取的总DNA,但无法区分活细胞和死细胞。 PCR之前的单叠氮化丙啶(PMA)预处理步骤可以有效地将DNA从不活的细胞中排除,因为PMA可以选择性地通过受损的细胞膜扩散并与DNA嵌入,从而在曝光后形成DNA-PMA复合物。该复合物强烈抑制PCR中结合DNA的扩增,因此,仅检测到具有完整细胞膜的细胞。本文中,这项研究报告了微流体装置的开发,该装置可进行“片上” PMA预处理。芯片设计以计算机仿真为指导,并使用高分辨率3D打印机制造原型。优化的设计利用分体式和复合式混合器进行初始PMA样品混合,并采用蛇形流动通道(包含人字形结构)进行暗光和暗光孵育。成功地证明了片上PMA预处理可区分缓冲液和天然池塘水样品中的活细菌和死细菌细胞。

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