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3D-FISH 和超分辨率结构光照明显微镜在研究三维核构象中的潜力:通过 3D(免疫)-FISH 可视化定义的染色体结构的 3D 结构光照明显微镜为研究核构象开辟了新的视角。

The potential of 3D-FISH and super-resolution structured illumination microscopy for studies of 3D nuclear architecture: 3D structured illumination microscopy of defined chromosomal structures visualized by 3D (immuno)-FISH opens new perspectives for studies of nuclear architecture.

机构信息

Biocenter, Department Biology II, Ludwig Maximilians University (LMU), Martinsried, Germany.

出版信息

Bioessays. 2012 May;34(5):412-26. doi: 10.1002/bies.201100176.

Abstract

Three-dimensional structured illumination microscopy (3D-SIM) has opened up new possibilities to study nuclear architecture at the ultrastructural level down to the ~100 nm range. We present first results and assess the potential using 3D-SIM in combination with 3D fluorescence in situ hybridization (3D-FISH) for the topographical analysis of defined nuclear targets. Our study also deals with the concern that artifacts produced by FISH may counteract the gain in resolution. We address the topography of DAPI-stained DNA in nuclei before and after 3D-FISH, nuclear pores and the lamina, chromosome territories, chromatin domains, and individual gene loci. We also look at the replication patterns of chromocenters and the topographical relationship of Xist-RNA within the inactive X-territory. These examples demonstrate that an appropriately adapted 3D-FISH/3D-SIM approach preserves key characteristics of the nuclear ultrastructure and that the gain in information obtained by 3D-SIM yields new insights into the functional nuclear organization.

摘要

三维结构照明显微镜(3D-SIM)为在超微结构水平上研究核架构提供了新的可能性,可达到~100nm 的范围。我们使用 3D-SIM 结合三维荧光原位杂交(3D-FISH),呈现了初步结果并评估了其潜力,用于对特定核靶点进行拓扑分析。我们的研究还涉及到一个担忧,即 FISH 产生的伪影可能会抵消分辨率的提高。我们研究了 3D-FISH 前后 DAPI 染色 DNA 的拓扑结构、核孔和核纤层、染色体区室、染色质域和单个基因座。我们还观察了着丝粒的复制模式以及 Xist-RNA 在失活 X 染色体区域内的拓扑关系。这些例子表明,经过适当调整的 3D-FISH/3D-SIM 方法可以保留核超微结构的关键特征,并且通过 3D-SIM 获得的信息增益可以深入了解核功能组织。

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