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为高质量的全哺乳动物大脑光学和超微结构研究保存细胞外空间。

Preserving extracellular space for high-quality optical and ultrastructural studies of whole mammalian brains.

机构信息

Department of Molecular and Cellular Biology and Center for Brain Science, Harvard University, Cambridge, MA, USA.

出版信息

Cell Rep Methods. 2023 Jul 5;3(7):100520. doi: 10.1016/j.crmeth.2023.100520. eCollection 2023 Jul 24.

Abstract

Analysis of brain structure, connectivity, and molecular diversity relies on effective tissue fixation. Conventional tissue fixation causes extracellular space (ECS) loss, complicating the segmentation of cellular objects from electron microscopy datasets. Previous techniques for preserving ECS in mammalian brains utilizing high-pressure perfusion can give inconsistent results owing to variations in the hydrostatic pressure within the vasculature. A more reliable fixation protocol that uniformly preserves the ECS throughout whole brains would greatly benefit a wide range of neuroscience studies. Here, we report a straightforward transcardial perfusion strategy that preserves ECS throughout the whole rodent brain. No special setup is needed besides sequential solution changes, and the protocol offers excellent reproducibility. In addition to better capturing tissue ultrastructure, preservation of ECS has many downstream advantages such as accelerating heavy-metal staining for electron microscopy, improving detergent-free immunohistochemistry for correlated light and electron microscopy, and facilitating lipid removal for tissue clearing.

摘要

分析大脑结构、连接和分子多样性依赖于有效的组织固定。传统的组织固定会导致细胞外空间(ECS)的损失,从而使电子显微镜数据集的细胞对象分割变得复杂。以前利用高压灌注来保持哺乳动物大脑 ECS 的技术由于血管内静水压的变化而导致结果不一致。一种更可靠的固定方案,可以在整个大脑中均匀地保存 ECS,将极大地有益于广泛的神经科学研究。在这里,我们报告了一种简单的心脏灌流策略,可以在整个啮齿动物大脑中保存 ECS。除了顺序改变溶液外,不需要特殊的设置,而且该方案具有很好的重现性。除了更好地捕获组织超微结构外,ECS 的保存还有许多下游优势,例如加速电子显微镜的重金属染色,改进用于相关光和电子显微镜的无去污剂免疫组织化学,以及便于组织透明化时的脂质去除。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/48c9/10391564/0e16e1198a8f/fx1.jpg

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