Junctional Adhesion Molecule 3 Expression in the Mouse Airway Epithelium Is Linked to Multiciliated Cells

Mateos-Quiros, Clara Maria; Garrido-Jimenez, Sergio; Álvarez-Hernán, Guadalupe; Diaz-Chamorro, Selene; Barrera-Lopez, Juan Francisco; Francisco-Morcillo, Javier; Román, Ángel; Centeno, Francisco; Carvajal-González, José María

doi:10.3389/fcell.2021.622515

Cited by 7 publications

(11 citation statements)

References 52 publications

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“…Ns = not significantly different (p > 0.05). Mateos-Quiros et al, 2021;Mikhailik et al, 2021;Reula et al, 2021;Smith et al, 2012;Zahid et al, 2020). The lack of a standardized fps for imaging motile cilia is especially problematic because it hinders high-speed video microscopy from being clinically adapted as a diagnostic tool to help uncover motile cilia diseases, such as primary ciliary dyskinesia (Bricmont et al, 2021;Shapiro et al, 2018).…”

Section: Discussionmentioning

confidence: 99%

“…The easiest way to assess motile cilia function is by quantifying CBF via highspeed video microscopy (Francis & Lo, 2013 ; O'Callaghan et al, 2012 ; Sisson et al, 2003 ) and this forms a sizable chunk of the cilia literature. However, no standardized frame rate exists when imaging cilia motility for subsequent CBF calculation, this has resulted in a large range of frames rates used to image cilia motility within the published literature (Abdelhamed et al, 2018 ; Abdelhamed et al, 2020 ; Bustamante‐Marin et al, 2019 ; Chen et al, 2016 ; Hagiwara et al, 2020 ; Hennessy et al, 1986 ; Liu et al, 2021 ; Mateos‐Quiros et al, 2021 ; Mikhailik et al, 2021 ; Reula et al, 2021 ; Smith et al, 2012 ; Zahid et al, 2020 ). The lack of a standardized fps for imaging motile cilia is especially problematic because it hinders high‐speed video microscopy from being clinically adapted as a diagnostic tool to help uncover motile cilia diseases, such as primary ciliary dyskinesia (Bricmont et al, 2021 ; Shapiro et al, 2018 ).…”

Section: Discussionmentioning

confidence: 99%

“…Determination of the optimum sampling rates for cilia video microscopy is also becoming increasingly important with the rapid advancements in digital camera technology (Liang & Wang, 2021; Pauls & Mukasyan, 2017). This has put high‐speed digital imaging within the budget of even the most modest of laboratories, with even consumer‐grade devices (e.g., iPhone) now having the possible frame rates required for cilia imaging (Chen et al, 2016; Mateos‐Quiros et al, 2021). Determining the optimal sampling rate for cilia video microscopy is needed due to the dramatic increase in imaging rates seen in the latest generation of scientific high‐speed video cameras (Etoh et al, 2013), where fps oversampling can greatly increase file sizes needing to be processed and archived (Aiello et al, 2019; Yaffe, 2019).…”

Section: Introductionmentioning

confidence: 99%

“…The most used method to assess motile cilia function is to quantify cilia beat frequency (CBF) via high‐speed video microscopy (Reula et al, 2021 ; Rubbo et al, 2019 ; Shapiro et al, 2018 ). However, a large heterogeneity exists within the published literature as to what frame rate per second (fps) to use when imaging cilia motility for subsequent CBF calculation; with published frame rates varying between 28–500 fps (Abdelhamed et al, 2018 ; Abdelhamed et al, 2020 ; Bustamante‐Marin et al, 2019 ; Chen et al, 2016 ; Hagiwara et al, 2020 ; Liu et al, 2021 ; Mateos‐Quiros et al, 2021 ; Mikhailik et al, 2021 ; Reula et al, 2021 ; Smith et al, 2012 ; Zahid et al, 2020 ). The large variation in sampling rates suggests some studies may be under‐sampling or oversampling cilia motility, which could result in inaccurate quantification of CBF or generation of large volumes of oversampled data requiring analysis and storage.…”

Section: Introductionmentioning

confidence: 99%

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Quantifying cilia beat frequency using high‐speed video microscopy: Assessing frame rate requirements when imaging different ciliated tissues

Scopulovic

Francis

Pandžić

et al. 2022

Physiological Reports

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Motile cilia are found in numerous locations throughout our body and play a critical role in various physiological processes. The most commonly used method to assess cilia motility is to quantify cilia beat frequency (CBF) via video microscopy. However, a large heterogeneity exists within published literature regarding the framerate used to image cilia motility for calculating CBF. The aim of this study was to determine the optimal frame rate required to image cilia motility for CBF assessment, and if the Nyquist theorem may be used to set this rate. One‐second movies of cilia were collected at >600 fps from mouse airways and ependyma at room‐temperature or 37°C. Movies were then down‐sampled to 30–300 fps. CBF was quantified for identical cilia at different framerates by either manual counting or automated MATLAB script. Airway CBF was significantly impaired in 30 fps movies, while ependymal CBF was significantly impaired in both 60 and 30 fps movies. Pairwise comparison showed that video framerate should be at least 150 fps to accurately measure CBF, with minimal improvement in CBF accuracy in movies >150 fps. The automated script was also found to be less accurate for measuring CBF in lower fps movies than manual counting, however, this difference disappeared in higher framerate movies (>150 fps). In conclusion, our data suggest the Nyquist theorem is unreliable for setting sampling rate for CBF measurement. Instead, sampling rate should be 3–4 times faster than CBF for accurate CBF assessment. Especially if CBF calculation is to be automated.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Quantifying cilia beat frequency using high‐speed video microscopy: Assessing frame rate requirements when imaging different ciliated tissues

Scopulovic

Francis

Pandžić

et al. 2022

Physiological Reports

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“…JAM-C distributed nonclassically in the apical membranes of Müller cells and retinal pigment epithelial (RPE) ( Daniele et al, 2007 ; Economopoulou et al, 2009 ), and JAM-C knockdown inhibits human RPE cell migration but not proliferation and decreases the permeability of monolayer hRPE ( Hou et al, 2012 ). JAM3 is expressed in multiciliated cells (MCCs) in the airway epithelium, and JAM3 lacking causes a delay in BB assembly/positioning during MCC differentiation ( Mateos-Quiros et al, 2021 ).…”

Section: Introductionmentioning

confidence: 99%

The Roles of Junctional Adhesion Molecules (JAMs) in Cell Migration

Wang

Liu

2022

Front. Cell Dev. Biol.

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The review briefly summarizes the role of the family of adhesion molecules, JAMs (junctional adhesion molecules), in various cell migration, covering germ cells, epithelial cells, endothelial cells, several leukocytes, and different cancer cells. These functions affect multiple diseases, including reproductive diseases, inflammation-related diseases, cardiovascular diseases, and cancers. JAMs bind to both similar and dissimilar proteins and take both similar and dissimilar effects on different cells. Concluding relevant results provides a reference to further research.

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Epigenetic regulation of H3K27me3 in laying hens with fatty liver hemorrhagic syndrome induced by high-energy and low-protein diets

Cui,

Ru,

Wang

et al. 2024

BMC Genomics

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Background Fatty liver hemorrhagic syndrome (FLHS) in the modern poultry industry is primarily caused by nutrition. Despite encouraging progress on FLHS, the mechanism through which nutrition influences susceptibility to FLHS is still lacking in terms of epigenetics. Results In this study, we analyzed the genome-wide patterns of trimethylated lysine residue 27 of histone H3 (H3K27me3) enrichment by chromatin immunoprecipitation-sequencing (ChIP-seq), and examined its association with transcriptomes in healthy and FLHS hens. The study results indicated that H3K27me3 levels were increased in the FLHS hens on a genome-wide scale. Additionally, H3K27me3 was found to occupy the entire gene and the distant intergenic region, which may function as silencer-like regulatory elements. The analysis of transcription factor (TF) motifs in hypermethylated peaks has demonstrated that 23 TFs are involved in the regulation of liver metabolism and development. Transcriptomic analysis indicated that differentially expressed genes (DEGs) were enriched in fatty acid metabolism, amino acid, and carbohydrate metabolism. The hub gene identified from PPI network is fatty acid synthase (FASN). Combined ChIP-seq and transcriptome analysis revealed that the increased H3K27me3 and down-regulated genes have significant enrichment in the ECM-receptor interaction, tight junction, cell adhesion molecules, adherens junction, and TGF-beta signaling pathways. Conclusions Overall, the trimethylation modification of H3K27 has been shown to have significant regulatory function in FLHS, mediating the expression of crucial genes associated with the ECM-receptor interaction pathway. This highlights the epigenetic mechanisms of H3K27me3 and provides insights into exploring core regulatory targets and nutritional regulation strategies in FLHS.

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Junctional Adhesion Molecule 3 Expression in the Mouse Airway Epithelium Is Linked to Multiciliated Cells

Cited by 7 publications

References 52 publications

Quantifying cilia beat frequency using high‐speed video microscopy: Assessing frame rate requirements when imaging different ciliated tissues

Quantifying cilia beat frequency using high‐speed video microscopy: Assessing frame rate requirements when imaging different ciliated tissues

The Roles of Junctional Adhesion Molecules (JAMs) in Cell Migration

Epigenetic regulation of H3K27me3 in laying hens with fatty liver hemorrhagic syndrome induced by high-energy and low-protein diets

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