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通过扩展显微镜技术追踪联会复合体的分子结构。

Tracking down the molecular architecture of the synaptonemal complex by expansion microscopy.

机构信息

Department of Biotechnology and Biophysics Biocenter, University of Würzburg, Am Hubland, 97074, Würzburg, Germany.

Department of Cell and Developmental Biology Biocenter, University of Würzburg, Am Hubland, 97074, Würzburg, Germany.

出版信息

Nat Commun. 2020 Jun 26;11(1):3222. doi: 10.1038/s41467-020-17017-7.

Abstract

The synaptonemal complex (SC) is a meiosis-specific nuclear multiprotein complex that is essential for proper synapsis, recombination and segregation of homologous chromosomes. We combined structured illumination microscopy (SIM) with different expansion microscopy (ExM) protocols including U-ExM, proExM, and magnified analysis of the proteome (MAP) to investigate the molecular organization of the SC. Comparison with structural data obtained by single-molecule localization microscopy of unexpanded SCs allowed us to investigate ultrastructure preservation of expanded SCs. For image analysis, we developed an automatic image processing software that enabled unbiased comparison of structural properties pre- and post-expansion. Here, MAP-SIM provided the best results and enabled reliable three-color super-resolution microscopy of the SCs of a whole set of chromosomes in a spermatocyte with 20-30 nm spatial resolution. Our data demonstrate that post-expansion labeling by MAP-SIM improves immunolabeling efficiency and allowed us thus to unravel previously hidden details of the molecular organization of SCs.

摘要

联会复合体(SC)是一种减数分裂特异性核多蛋白复合物,对于同源染色体的正确联会、重组和分离至关重要。我们将结构照明显微镜(SIM)与不同的扩展显微镜(ExM)方案(包括 U-ExM、proExM 和放大分析蛋白质组学(MAP))相结合,研究 SC 的分子组织。与通过未扩展 SC 的单分子定位显微镜获得的结构数据进行比较,使我们能够研究扩展 SC 的超微结构保存情况。对于图像分析,我们开发了一种自动图像处理软件,能够在扩展前后进行结构特性的无偏比较。在这里,MAP-SIM 提供了最佳结果,并能够以 20-30nm 的空间分辨率可靠地对整个染色体组的精母细胞的 SC 进行三色超分辨率显微镜观察。我们的数据表明,MAP-SIM 的扩展后标记提高了免疫标记效率,使我们能够揭示 SC 分子组织的先前隐藏细节。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5f41/7320163/eb2ace299108/41467_2020_17017_Fig1_HTML.jpg

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