Fluorescence imaging of beta cell primary cilia

Li, Zipeng A.; Cho, Jung Hoon; Woodhams, Louis G.; Hughes, Jing W.

doi:10.3389/fendo.2022.1004136

Cited by 9 publications

(9 citation statements)

References 82 publications

(70 reference statements)

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“…Cilia across spatial scales were tracked by morphology and their identification aided by immunogold labeling of ciliary protein markers. Preservation of ciliary structures was excellent as most cilia axonemes remained intact, exhibiting similar lengths (4-10 µm) and diameters (200-300 nm at base) as previously characterized by us and others 9,11,14,15 . We found moderate magnification (20-35,000x) to give a good overview of the entire ciliary structure.…”

Section: Resultssupporting

confidence: 71%

“…These primary antibodies were used in conjunction with standard gold-conjugated secondary antibodies specific for mouse and rabbit IgG. Table 1 lists the source and labeling conditions of all primary antibodies, typically used at 5-to 10-fold higher concentrations as for immunofluorescence imaging 8,[11][12][13] . Some but not all primary antibodies were tested in both mouse and human islets -species indicated in figures.…”

Section: Resultsmentioning

confidence: 99%

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Immuno-Scanning Electron Microscopy of Islet Primary Cilia

Sviben,

Polino,

Melena

et al. 2024

Preprint

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The definitive demonstration of protein localization on primary cilia has been a challenge for cilia biologists. Primary cilia are solitary thread-like projections that contain specialized protein composition, but as the ciliary structure overlays the cell membrane and other cell parts, the identity of ciliary proteins are difficult to ascertain by conventional imaging approaches like immunofluorescence microscopy. Surface scanning electron microscopy combined with immuno-labeling (immuno-SEM) bypasses some of these indeterminacies by unambiguously showing protein expression in the context of the 3D ultrastructure of the cilium. Here we apply immuno-SEM to specifically identify proteins on the primary cilia of mouse and human pancreatic islets, including post-translationally modified tubulin, intraflagellar transport (IFT) 88, the small GTPase Arl13b, as well as subunits of axonemal dynein. Key parameters in sample preparation, immuno-labeling, and imaging acquisition are discussed to facilitate similar studies by others in the cilia research community.

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Section: Resultssupporting

confidence: 71%

Section: Resultsmentioning

confidence: 99%

Immuno-Scanning Electron Microscopy of Islet Primary Cilia

Sviben,

Polino,

Melena

et al. 2024

Preprint

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“…In human islets, primary cilia were first described in beta cells, in 1964 in a case of insulinoma (13), whereas validation in non-diseased islet tissues took decades to follow (14)(15)(16). More recently, islet primary cilia were found to have glucoseregulated motility, suggesting that primary cilia are not simply static sensory organelles (16,17). These findings have fueled growing interest in islet primary cilia in diabetes research, paralleled by an increasing need to understand the basic structure and composition of these cellular projections.…”

Section: Introductionmentioning

confidence: 99%

Scanning electron microscopy of human islet cilia

Polino

Sviben²,

Melena³

et al. 2023

Preprint

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Human islet primary cilia are vital glucose-regulating organelles whose structure remains uncharacterized. Scanning electron microscopy (SEM) is a useful technique for studying the surface morphology of membrane projections like primary cilia, but conventional sample preparation does not reveal the sub-membrane axonemal structure which holds key implications for cilia function. To overcome this challenge, we combined SEM with membrane-extraction techniques to examine cilia in native human islets. Our data show well-preserved cilia subdomains which demonstrate both expected and unexpected ultrastructural motifs. Morphometric features were quantified when possible, including axonemal length and diameter, microtubule conformations and chirality. We further describe a novel ciliary ring, a structure that may be a specialization in human islets. Key findings are correlated with fluorescence microscopy and interpreted in the context of cilia function as a cellular sensor and communications locus in pancreatic islets.

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“…Besides Click-iT chemistry and SNAP/HALO tag technology, low-molecular weight reagents for labelling other cellular structures (primarily cytoskeleton—SiR and SPY probes; ref. 43 ) are available, though the spectrum of applications is limited. Our approach will benefit from the current effort to introduce other labelling strategies which aim to minimize the size of the labelling reagents and thus increase the permeability through Lowicryl resin, including detection with scFv antibody fragments, nanobodies 44 , 45 , proximity labelling with biotin 46 or DAB precipitation-based probes (reviewed in ref.…”

Section: Discussionmentioning

confidence: 99%

In-section Click-iT detection and super-resolution CLEM analysis of nucleolar ultrastructure and replication in plants

Franek,

Koptašíková,

Mikšátko

et al. 2024

Nat Commun

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Correlative light and electron microscopy (CLEM) is an important tool for the localisation of target molecule(s) and their spatial correlation with the ultrastructural map of subcellular features at the nanometre scale. Adoption of these advanced imaging methods has been limited in plant biology, due to challenges with plant tissue permeability, fluorescence labelling efficiency, indexing of features of interest throughout the complex 3D volume and their re-localization on micrographs of ultrathin cross-sections. Here, we demonstrate an imaging approach based on tissue processing and embedding into methacrylate resin followed by imaging of sections by both, single-molecule localization microscopy and transmission electron microscopy using consecutive CLEM and same-section CLEM correlative workflow. Importantly, we demonstrate that the use of a particular type of embedding resin is not only compatible with single-molecule localization microscopy but shows improvements in the fluorophore blinking behavior relative to the whole-mount approaches. Here, we use a commercially available Click-iT ethynyl-deoxyuridine cell proliferation kit to visualize the DNA replication sites of wild-type Arabidopsis thaliana seedlings, as well as fasciata1 and nucleolin1 plants and apply our in-section CLEM imaging workflow for the analysis of S-phase progression and nucleolar organization in mutant plants with aberrant nucleolar phenotypes.

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Fluorescence imaging of beta cell primary cilia

Cited by 9 publications

References 82 publications

Immuno-Scanning Electron Microscopy of Islet Primary Cilia

Immuno-Scanning Electron Microscopy of Islet Primary Cilia

Scanning electron microscopy of human islet cilia

In-section Click-iT detection and super-resolution CLEM analysis of nucleolar ultrastructure and replication in plants

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