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Hybridisation mix synthesis in a spiral lab-on-chip device for fast-track microarray genotyping of human pathogens

机译:杂交混合合成在螺旋实验室装置中,用于人病原体的快速轨道微阵列基因分型

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DNA microarrays can provide bacterial identification, which is crucial for targeted therapy. However they lack rapidness, because of multiple analysis steps. Therefore a fast one-step method for synthesising a hybridisation-ready reagent out of initial bacterial DNA is required. This work presents the combination and acceleration of PCR and fluorescent labelling within a disposable microfluidic chip, fabricated by injection moulding. The utilised geometry consists of a spiral meander with 40 turns, representing a cyclic-flow PCR system. The used reaction chemistry includes Cy3-conjugated primers and a high-yield polymerase leading to a one-step process accelerated by cyclic-flow PCR. Three different bacterial samples (Staphylococcus aureus, Escherichia coli and Pseudomonas aeruginosa) were processed and the bacterial DNA was successfully amplified and labelled with detection limits down to 102 cells per reaction. The specificity of species identification was comparable to the approach of separate PCR and labelling. Furthermore the overall processing time was decreased from 6 hours to 1.5 hours. We showed that a disposable polycarbonate chip, fabricated by injection moulding is suitable for the significant acceleration of DNA microarray assays. The reaction output lead to high-sensitivity bacterial identification in a short time, which is crucial for an early and targeted therapy against infectious diseases.
机译:DNA微阵列可以提供细菌鉴定,这对于靶向治疗至关重要。然而,由于多种分析步骤,它们缺乏速度。因此,需要一种快速的一步法,用于在初始细菌DNA中结合杂交的杂交试剂。该工作介绍了一次性微流体芯片内PCR和荧​​光标记的组合和加速,通过注塑制造。利用的几何形状由螺旋曲线组成,螺旋曲线40匝,代表循环流动PCR系统。二手反应化学包括Cy3 - 缀合的引物和高产聚合酶,其导致通过环状流动PCR加速的一步法。加工了三种不同的细菌样品(金黄色葡萄球菌,大肠杆菌和假单胞菌铜绿假单胞菌),并将细菌DNA成功扩增并用检测限为每次反应的102个细胞。物种鉴定的特异性与单独的PCR和标记的方法相当。此外,总处理时间从6小时到1.5小时降低。我们表明,通过注塑制造的一次性聚碳酸酯芯片适用于DNA微阵列测定的显着加速度。反应输出在短时间内导致高敏感性细菌鉴定,这对于对传染病的早期和靶向治疗至关重要。

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