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Integrated microfluidic platforms for investigating neuronal networks.

机译:集成的微流控平台,用于研究神经元网络。

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摘要

This dissertation describes the development and application of integrated microfluidics-based assay platforms to study neuronal activities in the nervous system in-vitro. The assay platforms were fabricated using soft lithography and micro/nano fabrication including microfluidics, surface patterning, and nanomaterial synthesis. The use of integrated microfluidics-based assay platform allows culturing and manipulating many types of neuronal tissues in precisely controlled microenvironment. Furthermore, they provide organized multi-cellular in-vitro model, long-term monitoring with live cell imaging, and compatibility with molecular biology techniques and electrophysiology experiment. In this dissertation, the integrated microfluidics-based assay platforms are developed for investigation of neuronal activities such as local protein synthesis, impairment of axonal transport by chemical/physical variants, growth cone path finding under chemical/physical cues, and synaptic transmission in neuronal circuit.;Chapter 1 describes the motivation, objectives, and scope for developing in-vitro platform to study various neuronal activities. Chapter 2 introduces microfluidic culture platform for biochemical assay with large-scale neuronal tissues that are utilized as model system in neuroscience research. Chapter 3 focuses on the investigation of impaired axonal transport by beta-Amyloid and oxidative stress. The platform allows to control neuronal processes and to quantify mitochondrial movement in various regions of axons away from applied drugs. Chapter 4 demonstrates the development of microfluidics-based growth cone turning assay to elucidate the mechanism underlying axon guidance under soluble factors and shear flow. Using this platform, the behaviors of growth cone of mammalian neurons are verified under the gradient of inhibitory molecules and also shear flow in well-controlled manner. In Chapter 5, I combine in-vitro multicellular model with microfabricated MEA (multielectrode array) or nanowire electrode array to study electrophysiology in neuronal network. Also, "diode-like" microgrooves to control the number of neuronal processes is embedded in this platform. Chapter 6 concludes with a possible future direction of this work. Interfacing micro/nanotechnology with primary neuron culture would open many doors in fundamental neuroscience research and also biomedical innovation.
机译:本文介绍了基于微流体的集成化检测平台在体外研究神经系统神经元活动的开发和应用。使用软光刻和包括微流控,表面图案化和纳米材料合成在内的微/纳米加工制造了检测平台。集成的基于微流体的分析平台的使用允许在精确控制的微环境中培养和操纵多种类型的神经元组织。此外,它们提供了有组织的多细胞体外模型,通过活细胞成像进行的长期监控以及与分子生物学技术和电生理学实验的兼容性。本文研究了基于微流体的集成化检测平台,以研究神经元活动,例如局部蛋白质合成,化学/物理变异对轴突运输的损伤,化学/物理线索下的生长锥路径发现以及神经回路中突触传递。第1章介绍了开发体外平台以研究各种神经元活动的动机,目标和范围。第2章介绍了用于大规模神经元组织生化测定的微流体培养平台,该平台用作神经科学研究中的模型系统。第3章重点研究β-淀粉样蛋白和氧化应激对轴突运输的损害。该平台允许控制神经元过程,并量化轴突在远离应用药物的各个区域中的线粒体运动。第4章演示了基于微流体的生长锥转向分析技术的发展,以阐明在可溶性因子和剪切流作用下轴突导向的基本机理。使用该平台,可以在抑制分子的梯度下以及以可控的方式剪切流动来验证哺乳动物神经元生长锥的行为。在第5章中,我将体外多细胞模型与微型MEA(多电极阵列)或纳米线电极阵列相结合,以研究神经元网络中的电生理。同样,控制该神经元过程的数量的“二极管状”微槽嵌入该平台中。第六章总结了这项工作的未来方向。将微/纳米技术与原代神经元文化相结合将为基础神经科学研究和生物医学创新打开许多大门。

著录项

  • 作者

    Kim, Hyung Joon.;

  • 作者单位

    University of California, Irvine.;

  • 授予单位 University of California, Irvine.;
  • 学科 Biology Neurobiology.;Engineering Materials Science.;Engineering Biomedical.
  • 学位 Ph.D.
  • 年度 2010
  • 页码 174 p.
  • 总页数 174
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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