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Integrated microfluidic bioprocessors for infectious disease detection.

机译:集成的微流体生物处理器,可用于传染病检测。

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摘要

The emergence of micro-Total Analysis Systems has revolutionized the world of molecular diagnostics by enabling sensitive multi-step fluidic processes to be performed and reliably integrated in a single platform. In particular, microfluidic systems now provide the tools and components to enable quantitative detection of biomarkers relevant to pathogen identification and disease characterization. In this thesis, these advances are exploited to develop an integrated microfluidic platform for automated, rapid and sensitive genetic identification of infectious food-borne bacterial and respiratory viral pathogens.My first goal was the integration of improved sample purification, preconcentration and injection technology with a polymerase chain reaction-capillary electrophoresis (PCR-CE) microdevice. By introducing an in-line affinity capture system utilizing an in situ photopolymerized oligonucleotide capture gel, double-stranded PCR amplicons generated in an integrated PCR reactor were selectively captured, purified and injected with 100% efficiency for high resolution CE separation. The superior performance of this integrated platform was demonstrated in a quantitative genetic analysis of E. coli. This integrated system exhibits a six-fold improvement in resolution of a multiplex analysis of Escherichia coli O157/E. coli K12 and is able to detect E. coli O157 in a 500-fold higher background of E. coli K12.To enable the parallel detection of multiple infectious pathogens, an improved purification method relying on biotin-streptavidin interaction was developed for universal product capture. This technique has the advantage of eliminating the complications associated with designing sequence-specific oligonucleotide capture probes for multiple targets. This process was integrated into a new 4-unit array PCR-CE microchip designed for automated product amplification, capture, and analysis. Coupled with a portable laser-induced fluorescence rotary scanner, the system can simultaneously detect as few as ten copies per reactor of influenza A & B, human metapneumovirus (hMPV), and coronavirus samples from cloned plasmid standards within 2.5 hours. Furthermore, the ability of the system to process RNA samples was demonstrated by performing RT-PCR analyses of an influenza B/hMPV co-infection model case, with respective detection limits of 50 and 100 copies/reactor.This thesis concludes with a discussion of proposed methods for nucleic acid isolation from biological samples that will provide a complete sample-in to answer-out diagnostic device and method for pathogen detection. When fully developed, this technology will be a significant advancement in infectious disease detection and surveillance both inside and outside clinical settings.
机译:微型总分析系统的出现彻底改变了分子诊断领域,它使敏感的多步流体过程得以执行并可靠地集成在单个平台中。尤其是,微流控系统现在提供了工具和组件,可以定量检测与病原体识别和疾病特征相关的生物标记。本文利用这些进展开发了一种集成的微流控平台,用于对食源性传染性细菌和呼吸道病毒病原体进行自动,快速和灵敏的遗传鉴定。我的第一个目标是将改进的样品纯化,预浓缩和注射技术与聚合酶链反应毛细管电泳(PCR-CE)微型设备。通过引入利用原位光聚合寡核苷酸捕获凝胶的在线亲和捕获系统,可以选择性地捕获,纯化和注入集成PCR反应器中生成的双链PCR扩增子,以100%的效率进行高分辨率CE分离。大肠杆菌的定量遗传分析证明了该集成平台的优越性能。该集成系统在大肠杆菌O157 / E的多重分析中显示出六倍的分辨率提高。大肠杆菌K12能够在大肠杆菌K12的500倍以上背景中检测到O157大肠杆菌。为了能够并行检测多种传染性病原体,开发了一种依靠生物素-链霉亲和素相互作用的改良纯化方法以实现通用产品捕获。该技术具有消除与设计用于多个靶标的序列特异性寡核苷酸捕获探针相关的复杂性的优点。此过程已集成到新的4单元阵列PCR-CE微芯片中,该芯片设计用于自动产物扩增,捕获和分析。结合便携式激光诱导荧光旋转扫描仪,该系统可以在2.5小时内从克隆质粒标准中同时检测出每个反应器甲型和乙型流感,人间质肺炎病毒(hMPV)和冠状病毒样本少至十个拷贝。此外,通过对B / hMPV流感共同感染模型病例进行RT-PCR分析,证明了该系统处理RNA样品的能力,分别检测限为50和100个拷贝/反应器。提出了从生物样品中分离核酸的方法,该方法将提供完整的样品输入以应答诊断设备和病原体检测方法。全面开发后,该技术将在临床环境内外的传染病检测和监视方面取得重大进步。

著录项

  • 作者

    Thaitrong, Numrin.;

  • 作者单位

    University of California, Berkeley.;

  • 授予单位 University of California, Berkeley.;
  • 学科 Biology Molecular.Chemistry Analytical.Engineering Biomedical.
  • 学位 Ph.D.
  • 年度 2010
  • 页码 87 p.
  • 总页数 87
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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