Super-Resolution Imaging of Tight and Adherens Junctions: Challenges and Open Questions

The tight junction (TJ) and the adherens junction (AJ) bridge the paracellular cleft of epithelial and endothelial cells. In addition to their role as protective barriers against bacteria and their toxins they maintain ion homeostasis, cell polarity, and mechano-sensing. Their functional loss leads to pathological changes such as tissue inflammation, ion imbalance, and cancer. To better understand the consequences of such malfunctions, the junctional nanoarchitecture is of great importance since it remains so far largely unresolved, mainly because of major difficulties in dynamically imaging these structures at sufficient resolution and with molecular precision. The rapid development of super-resolution imaging techniques ranging from structured illumination microscopy (SIM), stimulated emission depletion (STED) microscopy, and single molecule localization microscopy (SMLM) has now enabled molecular imaging of biological specimens from cells to tissues with nanometer resolution. Here we summarize these techniques and their application to the dissection of the nanoscale molecular architecture of TJs and AJs. We propose that super-resolution imaging together with advances in genome engineering and functional analyses approaches will create a leap in our understanding of the composition, assembly, and function of TJs and AJs at the nanoscale and, thereby, enable a mechanistic understanding of their dysfunction in disease.

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Super-Resolved Fluorescence Imaging of Peripheral Nerve

10.21203/rs.3.rs-141500/v1 ◽

2021 ◽

Author(s):

Iván Coto Hernández ◽

Suresh Mohan ◽

Nate Jowett

Keyword(s):

Peripheral Nerve ◽

Imaging Techniques ◽

Super Resolution ◽

Stimulated Emission ◽

Biomedical Science ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Unmyelinated Axons ◽

Histopathologic Evaluation ◽

Resolution Imaging

Abstract Traditional histopathologic evaluation of peripheral nerve employs brightfield microscopy with diffraction limited resolution of ~ 250 nm. Though electron microscopy yields nanoscale resolution of the nervous system, it is resource-intensive and incompatible with life. Super-resolution microscopy (SRM) comprises a set of imaging techniques permitting unprecedented resolution of fluorescent objects using visible light. The advent of SRM has transformed biomedical science in establishing non-toxic means for investigation of nanoscale cellular structures. Herein, sciatic nerve sections from GFP-variant expressing mice, and regenerating human nerve from cross-facial autografts labelled with a myelin-specific fluorescent dye were imaged by super-resolution radial fluctuation microscopy, stimulated emission depletion microscopy, and structured illumination microscopy. Super-resolution imaging of axial cryosections of murine sciatic nerves demonstrated robust visualization of myelinated and unmyelinated axons. Super-resolution imaging of axial cryosections of human cross-facial nerve grafts demonstrated enhanced resolution of small-calibre thinly-myelinated regenerating motor axons. The utility of SRM in imaging of mammalian cranial and peripheral nerves is demonstrated. The increase in contrast and structural clarity achievable with super-resolution techniques enables visualization of unmyelinated axons, regenerating axons, cytoskeleton ultrastructure, and neuronal appendages using light microscopes.

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Comparing Super-Resolution Microscopy Techniques to Analyze Chromosomes

International Journal of Molecular Sciences ◽

10.3390/ijms22041903 ◽

2021 ◽

Vol 22 (4) ◽

pp. 1903

Author(s):

Ivona Kubalová ◽

Alžběta Němečková ◽

Klaus Weisshart ◽

Eva Hřibová ◽

Veit Schubert

Keyword(s):

Single Molecule ◽

Imaging Techniques ◽

Chromatin Condensation ◽

Super Resolution ◽

Stimulated Emission ◽

Wide Field ◽

Structured Illumination Microscopy ◽

Metaphase Chromosomes ◽

Localization Microscopy ◽

Super Resolution Microscopy

The importance of fluorescence light microscopy for understanding cellular and sub-cellular structures and functions is undeniable. However, the resolution is limited by light diffraction (~200–250 nm laterally, ~500–700 nm axially). Meanwhile, super-resolution microscopy, such as structured illumination microscopy (SIM), is being applied more and more to overcome this restriction. Instead, super-resolution by stimulated emission depletion (STED) microscopy achieving a resolution of ~50 nm laterally and ~130 nm axially has not yet frequently been applied in plant cell research due to the required specific sample preparation and stable dye staining. Single-molecule localization microscopy (SMLM) including photoactivated localization microscopy (PALM) has not yet been widely used, although this nanoscopic technique allows even the detection of single molecules. In this study, we compared protein imaging within metaphase chromosomes of barley via conventional wide-field and confocal microscopy, and the sub-diffraction methods SIM, STED, and SMLM. The chromosomes were labeled by DAPI (4′,6-diamidino-2-phenylindol), a DNA-specific dye, and with antibodies against topoisomerase IIα (Topo II), a protein important for correct chromatin condensation. Compared to the diffraction-limited methods, the combination of the three different super-resolution imaging techniques delivered tremendous additional insights into the plant chromosome architecture through the achieved increased resolution.

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Super-Resolution Imaging in Fluid Mechanics Using New Illumination Approaches

Annual Review of Fluid Mechanics ◽

10.1146/annurev-fluid-010719-060059 ◽

2020 ◽

Vol 52 (1) ◽

pp. 369-393

Author(s):

Minami Yoda

Keyword(s):

Fluid Mechanics ◽

Total Internal Reflection ◽

Imaging Techniques ◽

Super Resolution ◽

Internal Reflection ◽

Interfacial Flows ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Entire Volume ◽

Resolution Imaging

Quantifying submillimeter flows using optical diagnostic techniques is often limited by a lack of spatial resolution and optical access. This review discusses two super-resolution imaging techniques, structured illumination microscopy and total internal reflection fluorescence or microscopy, which can visualize bulk and interfacial flows, respectively, at spatial resolutions below the classic diffraction limits. First, we discuss the theory and applications of structured illumination for optical sectioning, i.e., imaging a thin slice of a flow illuminated over its entire volume. Structured illumination can be used to visualize the interior of multiphase flows such as sprays by greatly reducing secondary scattering. Second, the theory underlying evanescent waves is introduced, followed by a review of how total internal reflection microscopy has been used to visualize interfacial flows over the last 15 years. Both techniques, which are starting to be used in fluid mechanics, could significantly improve quantitative imaging of microscale and macroscale flows.

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Laser-free super-resolution microscopy

Philosophical Transactions of The Royal Society A Mathematical Physical and Engineering Sciences ◽

10.1098/rsta.2020.0144 ◽

2021 ◽

Vol 379 (2199) ◽

Author(s):

Kirti Prakash

Keyword(s):

Single Molecule ◽

Super Resolution ◽

Stimulated Emission ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Correlative Imaging ◽

Deep Blue ◽

Meiotic Chromosomes ◽

Set Up ◽

Super Resolution Microscopy

We report that high-density single-molecule super-resolution microscopy can be achieved with a conventional epifluorescence microscope set-up and a mercury arc lamp. The configuration termed as laser-free super-resolution microscopy (LFSM) is an extension of single-molecule localization microscopy (SMLM) techniques and allows single molecules to be switched on and off (a phenomenon termed as ‘blinking’), detected and localized. The use of a short burst of deep blue excitation (350–380 nm) can be further used to reactivate the blinking, once the blinking process has slowed or stopped. A resolution of 90 nm is achieved on test specimens (mouse and amphibian meiotic chromosomes). Finally, we demonstrate that stimulated emission depletion and LFSM can be performed on the same biological sample using a simple commercial mounting medium. It is hoped that this type of correlative imaging will provide a basis for a further enhanced resolution. This article is part of the Theo Murphy meeting issue ‘Super-resolution structured illumination microscopy (part 1)’.

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Effect of light polariztion on pattern illumination super-resolution imaging

Journal of Innovative Optical Health Sciences ◽

10.1142/s1793545816410017 ◽

2016 ◽

Vol 09 (03) ◽

pp. 1641001 ◽

Cited By ~ 2

Author(s):

Caimin Qiu ◽

Jianling Chen ◽

Zexian Hou ◽

Chaoxian Xu ◽

Shusen Xie ◽

...

Keyword(s):

Polarized Light ◽

Super Resolution ◽

Stimulated Emission ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Excitation Light ◽

Imaging Technology ◽

Circularly Polarized Light ◽

Resolution Imaging ◽

The Right

Far-field fluorescence microscopy has made great progress in the spatial resolution, limited by light diffraction, since the super-resolution imaging technology appeared. And stimulated emission depletion (STED) microscopy and structured illumination microscopy (SIM) can be grouped into one class of the super-resolution imaging technology, which use pattern illumination strategy to circumvent the diffraction limit. We simulated the images of the beads of SIM imaging, the intensity distribution of STED excitation light and depletion light in order to observe effects of the polarized light on imaging quality. Compared to fixed linear polarization, circularly polarized light is more suitable for SIM on reconstructed image. And right-handed circular polarization (CP) light is more appropriate for both the excitation and depletion light in STED system. Therefore the right-handed CP light would be the best candidate when the SIM and STED are combined into one microscope. Good understanding of the polarization will provide a reference for the patterned illumination experiment to achieve better resolution and better image quality.

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Superresolving the kidney—a practical comparison of fluorescence nanoscopy of the glomerular filtration barrier

Analytical and Bioanalytical Chemistry ◽

10.1007/s00216-020-03084-8 ◽

2020 ◽

Author(s):

Lucia C. S. Wunderlich ◽

Florian Ströhl ◽

Stefan Ströhl ◽

Oliver Vanderpoorten ◽

Luca Mascheroni ◽

...

Keyword(s):

Glomerular Filtration ◽

Single Molecule ◽

Super Resolution ◽

Stimulated Emission ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Glomerular Filtration Barrier ◽

Maximum Resolution ◽

Filtration Barrier ◽

Super Resolution Microscopy

AbstractImmunofluorescence microscopy is routinely used in the diagnosis of and research on renal impairments. However, this highly specific technique is restricted in its maximum resolution to about 250 nm in the lateral and 700 nm in the axial directions and thus not sufficient to investigate the fine subcellular structure of the kidney’s glomerular filtration barrier. In contrast, electron microscopy offers high resolution, but this comes at the cost of poor preservation of immunogenic epitopes and antibody penetration alongside a low throughput. Many of these drawbacks were overcome with the advent of super-resolution microscopy methods. So far, four different super-resolution approaches have been used to study the kidney: single-molecule localization microscopy (SMLM), stimulated emission depletion (STED) microscopy, structured illumination microscopy (SIM), and expansion microscopy (ExM), however, using different preservation methods and widely varying labelling strategies. In this work, all four methods were applied and critically compared on kidney slices obtained from samples treated with the most commonly used preservation technique: fixation by formalin and embedding in paraffin (FFPE). Strengths and weaknesses, as well as the practicalities of each method, are discussed to enable users of super-resolution microscopy in renal research make an informed decision on the best choice of technique. The methods discussed enable the efficient investigation of biopsies stored in kidney banks around the world.

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

10.1101/821298 ◽

2019 ◽

Author(s):

Fabian U. Zwettler ◽

Marie-Christin Spindler ◽

Sebastian Reinhard ◽

Teresa Klein ◽

Andreas Kurz ◽

...

Keyword(s):

Synaptonemal Complex ◽

Single Molecule ◽

Super Resolution ◽

Structural Data ◽

Molecular Organization ◽

Molecular Architecture ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Automatic Image Processing ◽

Ultrastructure Preservation

AbstractThe 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 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 expansion factor determination. 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.

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Unraveling the Nanoscopic Organization and Function of Central Mammalian Presynapses With Super-Resolution Microscopy

Frontiers in Neuroscience ◽

10.3389/fnins.2020.578409 ◽

2021 ◽

Vol 14 ◽

Author(s):

Lia G. Carvalhais ◽

Vera C. Martinho ◽

Elisabete Ferreiro ◽

Paulo S. Pinheiro

Keyword(s):

Imaging Techniques ◽

Rapid Evolution ◽

Super Resolution ◽

Synaptic Function ◽

Stimulated Emission ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Axon Terminals ◽

Optical Reconstruction ◽

And Function

The complex, nanoscopic scale of neuronal function, taking place at dendritic spines, axon terminals, and other minuscule structures, cannot be adequately resolved using standard, diffraction-limited imaging techniques. The last couple of decades saw a rapid evolution of imaging methods that overcome the diffraction limit imposed by Abbe’s principle. These techniques, including structured illumination microscopy (SIM), stimulated emission depletion (STED), photo-activated localization microscopy (PALM), and stochastic optical reconstruction microscopy (STORM), among others, have revolutionized our understanding of synapse biology. By exploiting the stochastic nature of fluorophore light/dark states or non-linearities in the interaction of fluorophores with light, by using modified illumination strategies that limit the excitation area, these methods can achieve spatial resolutions down to just a few tens of nm or less. Here, we review how these advanced imaging techniques have contributed to unprecedented insight into the nanoscopic organization and function of mammalian neuronal presynapses, revealing new organizational principles or lending support to existing views, while raising many important new questions. We further discuss recent technical refinements and newly developed tools that will continue to expand our ability to delve deeper into how synaptic function is orchestrated at the nanoscopic level.

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Faculty Opinions recommendation of Two-photon instant structured illumination microscopy improves the depth penetration of super-resolution imaging in thick scattering samples.

Faculty Opinions – Post-Publication Peer Review of the Biomedical Literature ◽

10.3410/f.725269134.793520068 ◽

2016 ◽

Author(s):

Christopher Janetopoulos

Keyword(s):

Super Resolution ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Two Photon ◽

Resolution Imaging

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Super-resolution imaging of fluorescent dipoles via polarized structured illumination microscopy

Nature Communications ◽

10.1038/s41467-019-12681-w ◽

2019 ◽

Vol 10 (1) ◽

Cited By ~ 16

Author(s):

Karl Zhanghao ◽

Xingye Chen ◽

Wenhui Liu ◽

Meiqi Li ◽

Yiqiong Liu ◽

...

Keyword(s):

Hippocampal Neurons ◽

Fluorescent Protein ◽

Imaging Modality ◽

Super Resolution ◽

Vital Role ◽

Molecular Structures ◽

Polarization Microscopy ◽

Structured Illumination ◽

Structured Illumination Microscopy ◽

Resolution Imaging

Abstract Fluorescence polarization microscopy images both the intensity and orientation of fluorescent dipoles and plays a vital role in studying molecular structures and dynamics of bio-complexes. However, current techniques remain difficult to resolve the dipole assemblies on subcellular structures and their dynamics in living cells at super-resolution level. Here we report polarized structured illumination microscopy (pSIM), which achieves super-resolution imaging of dipoles by interpreting the dipoles in spatio-angular hyperspace. We demonstrate the application of pSIM on a series of biological filamentous systems, such as cytoskeleton networks and λ-DNA, and report the dynamics of short actin sliding across a myosin-coated surface. Further, pSIM reveals the side-by-side organization of the actin ring structures in the membrane-associated periodic skeleton of hippocampal neurons and images the dipole dynamics of green fluorescent protein-labeled microtubules in live U2OS cells. pSIM applies directly to a large variety of commercial and home-built SIM systems with various imaging modality.

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