Abstract
In this paper we show how to obtain a three-dimensional model of virus-infected cells by serial sectioning of resin embedded samples and transmission electron microscopic imaging. The method bases on sample fixation by high pressure freezing and processing by freeze substitution with the goal to preserve the structures of interest close to the natural state, as previously described (Walther et al., High pressure freezing for scanning transmission electron tomography analysis of cellular organelles. In: Mossman BT, Taatjes DJ (eds) Cell imaging techniques, vol 931, Methods in molecular biology. Humana Press, Totowa, NJ, pp 525–535, 2013). Advantages of serial sectioning compared to that of other tomographic methods are as follows: No special and expensive additional equipment is required. Relatively large volumes, such as whole cells, can be three-dimensionally reconstructed in a reasonable amount of time. Serial sectioning is a non-destructive method; the sections can be stored, re-imaged, or processed for immunogold labeling when more specific data are requested or when new scientific questions are raised (e.g., higher magnifications, protein distributions). We have recently used this method to obtain a three-dimensional model of the complete assembly complex of an HCMV infected cell, which allowed a detailed insight into this virally induced compartment (Schauflinger et al., Cell Microbiol 15(2):305–314, 2013).
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References
Baumeister W (2004) Mapping molecular landscapes inside cells. Biol Chem 385:865–872
Hohmann-Marriott MF, Sousa AA, Azari AA et al (2009) Nanoscale 3D cellular imaging by axial scanning transmission electron tomography. Nat Methods 6:729–731
Knott G, Marchman H, Wall D et al (2008) Serial section scanning electron microscopy of adult brain tissue using focused ion beam milling. J Neurosci 28:2959–2964
Denk W, Horstmann H (2004) Serial block-face scanning electron microscopy to reconstruct three-dimensional tissue nanostructure. PLoS Biol 2:1900–1909
Villinger C, Gregorius H, Kranz C et al (2012) FIB/SEM tomography with TEM-like resolution for 3D imaging of high-pressure frozen cells. Histochem Cell Biol 138:549–556
Sjöstrand FS (1958) Ultrastructure of retinal rod synapses of the guinea pig eye as revealed by three-dimensional reconstructions from serial sections. J Ultrastruct Res 2:122
Walther P, Ziegler A (2002) Freeze substitution of high-pressure frozen samples: the visibility of biological membranes is improved when the substitution medium contains water. J Microsc 208:3–10
Merchán-Pérez A, Rodriguez JR, Alonso-Nanclares L et al (2009) Counting synapses using FIB/SEM microscopy: a true revolution for ultrastructural volume reconstruction. Front Neuroanat 3:1–14
Schauflinger M, Villinger C, Mertens T et al (2013) Analysis of human cytomegalovirus secondary envelopment by advanced electron microscopy. Cell Microbiol 15(2):305–314
Walther P, Schmid E, Höhn K (2013) High pressure freezing for scanning transmission electron tomography analysis of cellular organelles. In: Mossman BT, Taatjes DJ (eds) Cell imaging techniques, vol 931, Methods in molecular biology. Humana, Totowa, NJ, pp 525–535
Buser C, Walther P (2008) Freeze-substitution: the addition of water to polar solvents enhances the retention of structure and acts at temperatures around −60 °C. J Microsc 230:268–277
Schauflinger M, Fischer D, Schreiber A et al (2011) The tegument protein UL71 of human cytomegalovirus is involved in late envelopment processes and affects multivesicular bodies. J Virol 85:3821–3832
Kremer JR, Mastronarde DN, McIntosh JR (1996) Computer visualization of three-dimensional image data using IMOD. J Struct Biol 116:71–76
McDonald K (2007) Cryopreparation methods for electron microscopy of selected model systems. In: McIntosh JR (ed) Cellular electron microscopy, vol 79, Methods in cell biology. Academic, San Diego, CA, pp 23–56
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Schauflinger, M., Villinger, C., Walther, P. (2013). Three-Dimensional Visualization of Virus-Infected Cells by Serial Sectioning: An Electron Microscopic Study Using Resin Embedded Cells. In: Bailer, S., Lieber, D. (eds) Virus-Host Interactions. Methods in Molecular Biology, vol 1064. Humana Press, Totowa, NJ. https://doi.org/10.1007/978-1-62703-601-6_16
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DOI: https://doi.org/10.1007/978-1-62703-601-6_16
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Publisher Name: Humana Press, Totowa, NJ
Print ISBN: 978-1-62703-600-9
Online ISBN: 978-1-62703-601-6
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