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Microscale tools for measuring spatiotemporal chemical gradients in biological systems

机译:用于测量生物系统中时空化学梯度的微观工具

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Chemical gradients drive many processes in biology, ranging from nerve signal transduction to ovulation. At present, microscopy is the primary tool used to understand these gradients. Microscopy has provided many important breakthroughs in our understanding of the fundamental biology, but is limited due to the need to incorporate fluorescent molecules into a biological system. As a result, there is a need to develop tools that can measure chemical gradient formation in biological systems that do not require fluorescent modification of the molecules in question, can be multiplexed to measure more than one molecule and is compatible with a variety of biological sample types, including in vitro cell cultures and ex vivo tissue slices. Work from our group centered on the development of microscale tools to measure chemical gradients will be presented. In this project, we have developed a microfluidic interface that allows for sampling from underneath a tissue slice or in vitro cell culture system. The sampling system can resolve up to 19 different ports and can be interfaced with either electrochemical or fluorescence-based detection methods. Using these two detection methods, we are capable of analyzing the release of either small molecule metabolites or proteins and peptides using immunoassays.
机译:化学梯度在生物学中驱动许多过程,从神经信号转导到排卵。目前,显微镜是用于理解这些渐变的主要工具。显微镜在我们对基本生物学的理解中提供了许多重要的突破,但由于需要将荧光分子掺入生物系统中,因此受到限制。结果,需要开发能够在不需要荧光修饰所讨论的分子的生物系统中测量化学梯度形成的工具,可以多路复用以测量多种分子,并与各种生物样品相容类型,包括体外细胞培养物和离体组织切片。我们集团的工作以微观工具的开发为中心,以衡量化学梯度。在该项目中,我们开发了一种微流体界面,允许从组织切片或体外细胞培养系统下面采样。采样系统可以解决高达19个不同的端口,并且可以用电化学或基于荧光的检测方法接口。使用这两种检测方法,我们能够使用免疫测定分析小分子代谢物或蛋白质和肽的释放。

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