Correlative microscopy approach for biology using X-ray holography, X-ray scanning diffraction and STED microscopy

Bernhardt, Marten; Nicolas, Jan-David; Osterhoff, Markus; Mittelstädt, Haugen; Reuß, Matthias; Harke, Benjamin; Wittmeier, Andrew; Sprung, Michael; Köster, Sarah; Salditt, Tim

doi:10.1038/s41467-018-05885-z

Cited by 43 publications

(46 citation statements)

References 67 publications

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“…STED microscopy has already been successfully combined to transmission electron microscopy to correlate protein localization with cell ultrastructure (Watanabe et al, 2011), or to atomic force microscopy to investigate protein aggregation at high spatial resolution (Cosentino et al, 2019). Recently, STED has been performed together with synchrotron scanning diffraction microscopy to inform about diffraction patterns in cells (Bernhardt et al, 2018). These correlative approaches however cannot be transposed to the imaging of metals in cells since they require steps of chemical fixation known to disrupt the metal-binding equilibrium in cells (Roudeau et al, 2014;Perrin et al, 2015).…”

Section: Discussionmentioning

confidence: 99%

Correlating STED and synchrotron XRF nano-imaging unveils the co-segregation of metals and cytoskeleton proteins in dendrites

Domart

Cloetens

Roudeau

et al. 2019

Preprint

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Zinc and copper are involved in neuronal differentiation and synaptic plasticity but the molecular mechanisms behind these processes are still elusive due in part to the difficulty of imaging trace metals at the synapse level. We correlate stimulated emission depletion (STED) microscopy of proteins and synchrotron X-ray fluorescence (SXRF) imaging of trace metals, both performed with 40 nm spatial resolution, on primary rat hippocampal neurons. We achieve a detection limit for trace metals in the zeptogram level per pixel. We reveal the colocalization at the nanoscale of zinc and tubulin in dendrites with a molecular ratio of about one zinc atom per tubulin-αβ dimer. We observe the co-segregation of copper and F-actin within the nano-architecture of dendritic spines. Overall, the combination of STED superresolution microscopy and SXRF nano-imaging indicates new functions for zinc and copper in the regulation of the synaptic cytoskeleton associated to memory formation.

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Section: Discussionmentioning

confidence: 99%

Correlating STED and synchrotron XRF nano-imaging unveils the co-segregation of metals and cytoskeleton proteins in dendrites

Domart

Cloetens

Roudeau

et al. 2019

Preprint

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“…In a broad sense, correlative microscopy refers to any combination of microscopy techniques (Karreman et al, 2016), microscopic X-ray computed tomography of excised tissue (Karreman et al, 2017), transmission electron microscopy (TEM) (Fuest et al, 2018), atmospheric or environmental scanning electron microscopy (SEM) (Peckys and de Jonge, 2015;Sato et al, 2019), cathodoluminescence of nanoparticles in SEM (Glenn et al, 2012), cryo-electron tomography (Tao et al, 2018), array tomography of electron microscopy (Burel et al, 2018;Collman et al, 2015;Micheva and Smith, 2007), X-ray holography, X-ray scanning diffraction (Bernhardt et al, 2018), X-ray fluorescence imaging and mass spectrometry imaging (Decelle et al, 2020). Some authors emphasized this integration of information from multiple imaging methods, by proposing a "morphomics" notation (Lucocq et al, 2015).…”

Section: Correlative Microscopymentioning

confidence: 99%

Correlating cell function and morphology by performing fluorescent immunocytochemical staining on the light-microscope stage

Kawano

Kakazu

Iwabuchi

et al. 2020

Preprint

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ABSTRACTBackgroundCorrelation of fluorescence signals from functional changes in live cells with those from immunocytochemical indicators of their morphology following chemical fixation can be highly informative with regard to function-structure relationship. Such analyses can be technically challenging because they need consistently aligning the images between imaging sessions. Existing solutions include introducing artificial spatial landmarks and modifying the microscopes. However, these methods can require extensive changes to the experimental systems.New methodHere we introduce a simple approach for aligning images. It is based on two procedures: performing immunocytochemistry while a specimen stays on a microscope stage (on-stage), and aligning images using biological structures as landmarks after they are observed with transmitted-light optics in combination with fluorescence-filter sets.ResultsWe imaged a transient functional signal from a fluorescent Ca2+ indicator, and mapped it to neurites based on immunocytochemical staining of a structural marker. In the same preparation, we could identify presynaptically silent synapses, based on a lack of labeling with an indicator for synaptic vesicle recycling and on positive immunocytochemical staining for a structural marker of nerve terminals. On-stage immunocytochemistry minimized lateral translations and eliminated rotations, and transmitted-light images of neurites were sufficiently clear to enable spatial registration, effective at a single-pixel level.Comparison with existing methodsThis method aligned images with minimal change or investment in the experimental systems.ConclusionsThis method facilitates information retrieval across multiple imaging sessions, even when functional signals are transient or local, and when fluorescent signals in multiple imaging sessions do not match spatially.

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“…Multi-scale imaging does not necessarily need to be performed with a single imaging method. Indeed, the added benefit from combining two different modalities can be greater than the sum of the two [73]. We have primarily used visible light fluorescence microscopy for this purpose as it is a very well established imaging method that offers a distinct, highly specific contrast that does not exploit the electron density.…”

Section: Future Directionsmentioning

confidence: 99%

“…Recently, we have introduced a novel approach of parallel STED or confocal microscopy recordings together with X-ray scanning diffraction and X-ray holography, all integrated into a single synchrotron endstation [73,171]. Here we have made use of this setup to image adult cardiomyocytes.…”

Section: Correlative Microscopymentioning

confidence: 99%

“…4.8(C) is now a map of all cellular components that were traversed by the Xray beam. The anisotropic scattering due to the aligned myofibrils is apparent from the example scattering pattern shown in The image was recorded using a custom-built STED/ confocal microscope that was setup next to the X-ray beam including a motorized sample translation stage to combine STED or confocal imaging with X-ray diffraction of X-ray holography [73,171]. (B) Single image from the stack, stack average and a maximum projection through the entire stack.…”

Section: Correlative Microscopy 75mentioning

confidence: 99%

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Multiscale X-Ray Analysis of Biological Cells and Tissues by Scanning Diffraction and Coherent Imaging

Nicolas¹

2019

Göttingen Series in X-Ray Physics

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The Göttingen series in x-ray physics is intended as a collection of research monographs in x-ray science, carried out at the Institute for X-ray Physics at the Georg-August-Universität in Göttingen, and in the framework of its related research networks and collaborations. It covers topics ranging from x-ray microscopy, nano-focusing, wave propagation, image reconstruction, tomography, short x-ray pulses to applications of nanoscale x-ray imaging and biomolecular structure analysis. In most but not all cases, the contributions are based on Ph.D. dissertations. The individual monographs should be enhanced by putting them in the context of related work, often based on a common long term research strategy, and funded by the same research networks. We hope that the series will also help to enhance the visibility of the research carried out here and help others in the field to advance similar projects.

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Correlative microscopy approach for biology using X-ray holography, X-ray scanning diffraction and STED microscopy

Cited by 43 publications

References 67 publications

Correlating STED and synchrotron XRF nano-imaging unveils the co-segregation of metals and cytoskeleton proteins in dendrites

Correlating STED and synchrotron XRF nano-imaging unveils the co-segregation of metals and cytoskeleton proteins in dendrites

Correlating cell function and morphology by performing fluorescent immunocytochemical staining on the light-microscope stage

Multiscale X-Ray Analysis of Biological Cells and Tissues by Scanning Diffraction and Coherent Imaging

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