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A Programmable Digital Microfluidic Assay for the Simultaneous Detection of Multiple Anti-Microbial Resistance Genes

机译:同时检测多种抗微生物基因的可编程数字微流分析

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The rapid emergence of antimicrobial resistant bacteria requires the development of new diagnostic tests. Nucleic acid-based assays determine antimicrobial susceptibility by detecting genes that encode for the resistance. In this study, we demonstrate rapid and simultaneous detection of three genes that confer resistance in bacteria to extended spectrum ???2-lactam and carbapenem antibiotics; CTX-M-15, KPC and NDM-1. The assay uses isothermal DNA amplification (recombinase polymerase amplification, RPA) implemented on a programmable digital microfluidics (DMF) platform. Automated dispensing protocols are used to simultaneously manipulate 45 droplets of nL volume containing sample DNA, reagents, and controls. The droplets are processed and mixed under electronic control on the DMF devices with positive amplification measured by fluorescence. The assay on these devices is significantly improved with a Time to Positivity (TTP) half that of the benchtop assay.
机译:抗菌素耐药细菌的迅速出现要求开发新的诊断测试方法。基于核酸的测定法通过检测编码耐药性的基因来确定抗菌药的敏感性。在这项研究中,我们证明了快速和同时检测三个赋予细菌对广谱2-内酰胺和碳青霉烯类抗生素耐药的基因。 CTX-M-15,KPC和NDM-1。该测定使用在可编程数字微流控(DMF)平台上实施的等温DNA扩增(重组酶聚合酶扩增,RPA)。自动分配方案可用于同时处理45个nL体积的液滴,其中包含样品DNA,试剂和对照。在DMF设备上的电子控制下,对液滴进行处理和混合,并通过荧光测量得到阳性扩增。在这些设备上的检测时间得到了显着改善,正电动时间(TTP)为台式检测时间的一半。

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