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1
High-performance serial block-face SEM of nonconductive biological samples enabled by focal gas injection-based charge compensation.基于局域气体注入的电荷补偿实现非导电生物样品的高性能串行块面扫描电镜。
J Microsc. 2018 May;270(2):142-149. doi: 10.1111/jmi.12667. Epub 2017 Dec 1.
2
Convolutional neural networks for automated annotation of cellular cryo-electron tomograms.用于细胞冷冻电子断层扫描自动标注的卷积神经网络。
Nat Methods. 2017 Oct;14(10):983-985. doi: 10.1038/nmeth.4405. Epub 2017 Aug 28.
3
PAR1 activation induces rapid changes in glutamate uptake and astrocyte morphology.PAR1 激活诱导谷氨酸摄取和星形胶质细胞形态的快速变化。
Sci Rep. 2017 Mar 3;7:43606. doi: 10.1038/srep43606.
4
β-arrestin-2 is an essential regulator of pancreatic β-cell function under physiological and pathophysiological conditions.β-arrestin-2 是生理和病理条件下胰腺 β 细胞功能的重要调节剂。
Nat Commun. 2017 Feb 1;8:14295. doi: 10.1038/ncomms14295.
5
3D multi-energy deconvolution electron microscopy.三维多能量解卷积电子显微镜。
Nanoscale. 2017 Jan 5;9(2):684-689. doi: 10.1039/c6nr07991a.
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3-D EM exploration of the hepatic microarchitecture - lessons learned from large-volume in situ serial sectioning.三维电子显微镜探索肝脏微观结构 - 从大容量原位连续切片中获得的经验教训。
Sci Rep. 2016 Nov 11;6:36744. doi: 10.1038/srep36744.
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Calcium transport into the cells of the sea urchin larva in relation to spicule formation.与骨针形成相关的海胆幼虫细胞对钙的转运
Proc Natl Acad Sci U S A. 2016 Nov 8;113(45):12637-12642. doi: 10.1073/pnas.1612017113. Epub 2016 Oct 24.
8
Golgi proteins in circulating human platelets are distributed across non-stacked, scattered structures.循环中的人体血小板中的高尔基体蛋白分布于非堆叠、分散的结构中。
Platelets. 2017 Jun;28(4):400-408. doi: 10.1080/09537104.2016.1235685. Epub 2016 Oct 18.
9
Deceleration of probe beam by stage bias potential improves resolution of serial block-face scanning electron microscopic images.通过阶段偏置电位使探测光束减速可提高连续块面扫描电子显微镜图像的分辨率。
Adv Struct Chem Imaging. 2017;2(1):11. doi: 10.1186/s40679-016-0025-y. Epub 2016 Sep 15.
10
Cryo-Electron Tomography: Can it Reveal the Molecular Sociology of Cells in Atomic Detail?冷冻电子断层扫描:能否以原子级细节揭示细胞的分子社会学?
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基于扫描电子探针的 3D 细胞成像技术比较:连续块面扫描电镜与轴向明场扫描透射电镜断层成像。

Comparison of 3D cellular imaging techniques based on scanned electron probes: Serial block face SEM vs. Axial bright-field STEM tomography.

机构信息

Laboratory of Cellular Imaging and Macromolecular Biophysics, NIBIB, NIH, Bethesda, MD, USA.

Department of Physiology and Biophysics, University of Arkansas for Medical Sciences, Little Rock, AR, USA.

出版信息

J Struct Biol. 2018 Jun;202(3):216-228. doi: 10.1016/j.jsb.2018.01.012. Epub 2018 Feb 1.

DOI:10.1016/j.jsb.2018.01.012
PMID:29408702
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8349566/
Abstract

Microscopies based on focused electron probes allow the cell biologist to image the 3D ultrastructure of eukaryotic cells and tissues extending over large volumes, thus providing new insight into the relationship between cellular architecture and function of organelles. Here we compare two such techniques: electron tomography in conjunction with axial bright-field scanning transmission electron microscopy (BF-STEM), and serial block face scanning electron microscopy (SBF-SEM). The advantages and limitations of each technique are illustrated by their application to determining the 3D ultrastructure of human blood platelets, by considering specimen geometry, specimen preparation, beam damage and image processing methods. Many features of the complex membranes composing the platelet organelles can be determined from both approaches, although STEM tomography offers a higher ∼3 nm isotropic pixel size, compared with ∼5 nm for SBF-SEM in the plane of the block face and ∼30 nm in the perpendicular direction. In this regard, we demonstrate that STEM tomography is advantageous for visualizing the platelet canalicular system, which consists of an interconnected network of narrow (∼50-100 nm) membranous cisternae. In contrast, SBF-SEM enables visualization of complete platelets, each of which extends ∼2 µm in minimum dimension, whereas BF-STEM tomography can typically only visualize approximately half of the platelet volume due to a rapid non-linear loss of signal in specimens of thickness greater than ∼1.5 µm. We also show that the limitations of each approach can be ameliorated by combining 3D and 2D measurements using a stereological approach.

摘要

基于聚焦电子探针的显微镜使细胞生物学家能够对真核细胞和组织的 3D 超微结构进行成像,这些细胞和组织的体积很大,从而为细胞结构与细胞器功能之间的关系提供了新的认识。在这里,我们比较了两种这样的技术:结合轴向明场扫描透射电子显微镜(BF-STEM)的电子断层扫描和连续块面扫描电子显微镜(SBF-SEM)。通过应用这两种技术来确定人类血小板的 3D 超微结构,考虑到标本几何形状、标本制备、束损伤和图像处理方法,说明了每种技术的优点和局限性。尽管 STEM 断层扫描在块面平面上提供了约 3nm 的各向同性像素尺寸,而 SBF-SEM 则为约 5nm,在垂直方向上为约 30nm,但这两种方法都可以确定构成血小板细胞器的复杂膜的许多特征。在这方面,我们证明 STEM 断层扫描有利于可视化由狭窄(约 50-100nm)膜腔组成的血小板管腔系统。相比之下,SBF-SEM 能够可视化完整的血小板,每个血小板在最小尺寸上延伸约 2μm,而 BF-STEM 断层扫描由于在厚度大于约 1.5μm 的标本中信号快速非线性损失,通常只能可视化大约一半的血小板体积。我们还表明,通过使用立体学方法结合 3D 和 2D 测量,可以改善每种方法的局限性。