INTRODUCTIONCell migration is a key aspect of many developmental processes, yet there are relatively few whole-vertebrate embryo culture systems that allow for intravital, high-resolution optical imaging of cell movements, cell-cell interactions, and cell-matrix interactions. Here, we present a protocol for 4D (3D + time), high-resolution confocal imaging of fluorescently labeled cells within living avian embryos. We discuss the culture chamber assembly and interface with a commercially available microscope-stage culture-dish heating system. To demonstrate how the system works, we describe the protocol in use with chick embryos while following individual fluorescently labeled neural crest cells, a major migratory cell population that sorts into complex patterns of discrete streams. By combining the embryo culture directly on glass with confocal 4D time-lapse imaging, we demonstrate that individual neural crest cell migratory behaviors and cell-cell interactions may be visualized for short periods of time (<6 h). This technique can be adapted to study other migratory cell populations or developmental events in whole avian embryos.
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PLoS Pathog
January 2025
Department of Cell Biology and Molecular Genetics, University of Maryland, College Park, Maryland United States of America.
Autophagy plays a crucial role in the host response to Mycobacterium tuberculosis (Mtb) infection, yet the dynamics and regulation of autophagy induction on Mtb-containing vacuoles (MCVs) remain only partially understood. We employed time-lapse confocal microscopy to investigate the recruitment of LC3B (LC3), a key autophagy marker, to MCVs at the single cell level with our newly developed workflow for single cell and single MCV tracking and fluorescence quantification. We show that approximately 70% of MCVs exhibited LC3 recruitment but that was lost in about 40% of those MCVs.
View Article and Find Full Text PDFNat Commun
December 2024
Eunice Kennedy Shriver National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, MD, USA.
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View Article and Find Full Text PDFReprod Biol
December 2024
Department of Animal Reproduction, Anatomy and Genomics, Faculty of Animal Science, University of Agriculture in Krakow, Mickiewicza 24/28, 30-059 Krakow, Poland.
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View Article and Find Full Text PDFBiochem Cell Biol
October 2024
Institut universitaire de Cardiologie et de Pneumologie de Québec-Université Laval, Québec, QC, Canada.
DFAT cells represent an attractive source of stem cells in tissue engineering and in the potential treatment of several clinical conditions. Our objective was to determine whether DFAT cells originate from mature adipocytes and address whether contamination from the stromal vascular fraction (SVF) could be as a source for these cells. A murine adiponectin-creERT;mT/mG model was used with the excision of the cassette induced by tamoxifen injection for the cells expressing adiponectin (adipoq).
View Article and Find Full Text PDFChem Sci
October 2024
Leibniz-Forschungsinstitut für Molekulare Pharmakologie FMP Campus Berlin-Buch 13125 Berlin Germany
The diversity of physiological roles of the endocannabinoid system has turned it into an attractive yet elusive therapeutic target. However, chemical probes with various functionalities could pave the way for a better understanding of the endocannabinoid system at the cellular level. Notably, inverse agonists of CBR - a key receptor of the endocannabinoid system - lagged behind despite the evidence regarding the therapeutic potential of its antagonism.
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