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冷冻置换脑组织的复水用于包埋前免疫电镜。

Rehydration of Freeze Substituted Brain Tissue for Pre-embedding Immunoelectron Microscopy.

机构信息

Department of Physiology and Neurobiology, University of Connecticut, 75 North Eagleville Rd. Unit 3156, Storrs, CT 06269-3156, USA.

Connecticut Institute for the Brain and Cognitive Sciences, University of Connecticut, 337 Mansfield Rd. Unit 1272, Storrs, CT 06269-1272, USA.

出版信息

Microsc Microanal. 2023 Sep 29;29(5):1694-1704. doi: 10.1093/micmic/ozad077.

Abstract

Electron microscopy (EM) volume reconstruction is a powerful tool for investigating the fundamental structure of brain circuits, but the full potential of this technique is limited by the difficulty of integrating molecular information. High quality ultrastructural preservation is necessary for EM reconstruction, and intact, highly contrasted cell membranes are essential for following small neuronal processes through serial sections. Unfortunately, the antibody labeling methods used to identify most endogenous molecules result in compromised morphology, especially of membranes. Cryofixation can produce superior morphological preservation and has the additional advantage of allowing indefinite storage of valuable samples. We have developed a method based on cryofixation that allows sensitive immunolabeling of endogenous molecules, preserves excellent ultrastructure, and is compatible with high-contrast staining for serial EM reconstruction.

摘要

电子显微镜(EM)体积重建是研究大脑回路基本结构的有力工具,但该技术的全部潜力受到整合分子信息的难度限制。EM 重建需要高质量的超微结构保存,而完整、高对比度的细胞膜对于通过连续切片跟踪小神经元过程至关重要。不幸的是,用于识别大多数内源性分子的抗体标记方法会导致形态学受损,尤其是细胞膜。冷冻固定可以产生更好的形态保存,并且具有允许无限期储存有价值样品的额外优点。我们开发了一种基于冷冻固定的方法,该方法可以对内源性分子进行敏感的免疫标记,同时保持出色的超微结构,并与用于连续 EM 重建的高对比度染色兼容。

相似文献

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Cryopreparation of biological specimens for immunoelectron microscopy.用于免疫电子显微镜的生物样本冷冻制备
Ann Anat. 2009 Jun;191(3):231-47. doi: 10.1016/j.aanat.2008.11.004. Epub 2009 Jan 20.

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