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Techniques for Single-Molecule mRNA Imaging in Living Cells

机译:活细胞中单分子mRNA成像的技术

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摘要

Typical measurement of macromolecules in a biological sample typically averages the result over all the cells or molecules within the sample, and while these types of measurements provide very useful information, they completely miss heterogeneity among the components within the sample that could be a very important aspect of the sample's function. These techniques are also limited in their ability to examine intracellular spatial orientation of molecular activity, which is often a critical component to the regulation of biological processes, particularly in cells with unique spatial relationships, such as neurons. This makes a strong case for single-cell and single-molecule analysis that allows similar novel insight into complex molecular machinery that would not be possible when pooling heterogeneous molecular states. mRNA has proven to be quite tractable to molecular analysis in single cells. Almost two decades of single-molecule studies of mRNA processing both in situ and in live cells have been facilitated by microscopy of mRNA. This has been made possible by multiplexing fluorophores in situ hybridization probes or fluorescent RNA-tag-binding protein probes. The purpose of this chapter is to describe the approaches that have made single-molecule mRNA imaging accessible, as well as to give an overview of the state of the art for techniques that are available to track mRNA in real time in living cells, highlighting the application to neuroscience.
机译:生物样品中大分子的典型测量通常平均结果对样品内的所有细胞或分子,而这些类型的测量提供了非常有用的信息,它们完全错过了样本内的组件之间的异质性,这可能是一个非常重要的方面样本的功能。这些技术也受到检查分子活性细胞内空间取向的能力,这通常是生物过程调节的关键组分,特别是在具有独特的空间关系的细胞中,例如神经元。这对单细胞和单分子分析产生了强烈的案例,其允许在汇集异质分子状态时对复杂的分子机械进行类似的新颖洞察力。已证明MRNA在单细胞中的分子分析非常易于。通过MRNA的显微镜促进了几乎二十二十年来原位和活细胞的mRNA处理的单分子研究。这是通过在原位杂交探针或荧光RNA标签结合蛋白探针中复用荧光团来实现的。本章的目的是描述使单分子mRNA成像的方法可获得的方法,并概述了用于在活细胞实时跟踪mRNA的技术的技术的概述,突出显示应用于神经科学。

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