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Single-Cell Phenotyping within Transparent Intact Tissue through Whole-Body Clearing

机译:通过全身清除在透明完整组织内的单细胞表型

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摘要

Understanding the structure-function relationships at cellular, circuit, and organ-wide scale requires 3D anatomical and phenotypical maps, currently unavailable for many organs across species. At the root of this knowledge gap is the absence of a method that enables whole-organ imaging. Herein, we present techniques for tissue clearing in which whole organs and bodies are rendered macromoleculepermeable and optically transparent, thereby exposing their cellular structure with intact connectivity. We describe PACT (passive clarity technique), a protocol for passive tissue clearing and immunostaining of intact organs; RIMS (refractive index matching solution), a mounting media for imaging thick tissue; and PARS (perfusion-assisted agent release in situ), a method for whole-body clearing and immunolabeling. We show that in rodents PACT, RIMS, and PARS are compatible with endogenous-fluorescence, immunohistochemistry, RNA single-molecule FISH, long-term storage, and microscopy with cellular and subcellular resolution. These methods are applicable for high-resolution, highcontent mapping and phenotyping of normal and pathological elements within intact organs and bodies.
机译:要了解细胞,电路和器官范围内的结构-功能关系,需要3D解剖图和表型图,目前跨物种的许多器官都无法使用。这种知识鸿沟的根源在于缺乏一种能够进行全器官成像的方法。在本文中,我们介绍了用于组织清除的技术,其中使整个器官和身体都具有大分子可渗透性和光学透明性,从而以完整的连接性暴露其细胞结构。我们描述了PACT(被动清除技术),一种用于完整组织的被动组织清除和免疫染色的协议; RIMS(折射率匹配解决方案),一种用于对厚组织成像的安装介质; PARS(灌注辅助剂原位释放),一种全身清除和免疫标记的方法。我们显示,在啮齿动物中,PACT,RIMS和PARS与内源性荧光,免疫组织化学,RNA单分子FISH,长期储存以及具有细胞和亚细胞分辨率的显微镜相兼容。这些方法适用于完整器官和体内正常和病理元素的高分辨率,高含量作图和表型分析。

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