Your search keyword '"Connexin 43 analysis"' showing total 6 results

1. Improved antigen retrieval in freeze-fracture cytochemistry by evaporation of carbon as first replication layer.

Author

Schlörmann W, John M, Steiniger F, Westermann M, and Richter W

Subjects

Animals, Antigens immunology, Caveolin 1 analysis, Caveolin 1 immunology, Connexin 43 analysis, Connexin 43 immunology, Gold Compounds, Mice, NIH 3T3 Cells immunology, NIH 3T3 Cells metabolism, Antigens analysis, Carbon chemistry, Freeze Fracturing methods, Histocytochemistry methods

Abstract

The recently developed freeze-fracture replica immunolabeling technique uses sodium dodecyl sulfate to clean replicas obtained from chemically unfixed, rapidly frozen cells by evaporation of platinum as first and carbon as second replication layer. The detergent dissolves remains of cellular material with the exception of components which are in direct contact to the replica film. Membrane lipids and membrane protein complexes of the protoplasmic and the exoplasmic membrane halves remain attached to the replica film and are accessible for cytochemical localization. We immunolabeled the membrane proteins caveolin-1 and connexin 43 in mouse cell lines as well as the membrane attached protein tetrachloroethene reductive dehalogenase (PceA) in bacterial cells at freeze-fracture replicas generated by different evaporation parameters. The labeling experiments for caveolin-1 and the PceA showed that freeze-fracture replication of cellular membranes accomplished with thin platinum layers as well as replication with carbon as first evaporation layer lead in these cases to an improved antigen retrieval, whereas the labeling efficiency of connexin 43 was not affected by different evaporation conditions.

Published

2007

2. In differentiating prefusion myoblasts connexin43 gap junction coupling is upregulated before myoblast alignment then reduced in post-mitotic cells.

Author

Gorbe A, Becker DL, Dux L, Krenacs L, and Krenacs T

Subjects

Animals, Blotting, Western, Cell Differentiation, Cell Fusion, Cell Membrane chemistry, Cells, Cultured, Cyclin-Dependent Kinase Inhibitor p21 metabolism, Cyclin-Dependent Kinase Inhibitor p27 metabolism, Cytoplasm chemistry, Fluorescent Dyes analysis, Fluorescent Dyes metabolism, Microscopy, Confocal, Mitosis, Myoblasts metabolism, Rats, Up-Regulation, Connexin 43 analysis, Connexin 43 metabolism, Gap Junctions, Myoblasts chemistry, Myoblasts cytology

Abstract

Previously we have shown that during in vivo muscle regeneration differentiating rat primary myoblasts transiently upregulate connexin43 (Cx43) gap junctions and leave cell cycle synchronously. Here, we studied the temporal regulation of Cx expression in relation to functional dye coupling in allogenic primary myoblast cultures using western blotting, immuno-confocal microscopy and dye transfer assays. As in vivo, Cx43 was the only Cx isotype out of Cx26, 32, 37, 40, 43 and 45 found in cultured rat myoblasts by immunostaining. Cultured myoblasts showed similar temporal regulation of Cx43 expression and phenotypic maturation to those regenerating in vivo. Cx43 protein was progressively upregulated in prefusion myoblasts, first by the cytoplasmic assembly in sparse myoblast meshworks and then in cell membrane particles in aligned cells. Dye injection using either Lucifer Yellow alone, Cascade Blue with a non-junction permeant FITC-dextran revealed an extensive gap junction coupling between the sparse interacting myoblasts and a reduced communication between the aligned, but still prefused cells. The aligned myoblasts, uniformly upregulate p21(waf1/cip1) and p27(kip1) cell cycle control proteins. Taken together, in prefusion myoblasts less membrane-bound Cx43 was found to mediate substantially more efficient dye coupling in the growing cell fraction than those in the aligned post-mitotic myoblasts. These and our in vivo results in early muscle differentiation are consistent with the role of Cx43 gap junctions in synchronizing cell cycle control of myoblasts to make them competent for a coordinated syncytial fusion.

Published

2006

3. Transient upregulation of connexin43 gap junctions and synchronized cell cycle control precede myoblast fusion in regenerating skeletal muscle in vivo.

Author

Gorbe A, Becker DL, Dux L, Stelkovics E, Krenacs L, Bagdi E, and Krenacs T

Subjects

Animals, Cell Cycle Proteins analysis, Cyclin-Dependent Kinase Inhibitor p21, Cyclin-Dependent Kinase Inhibitor p27, Desmin analysis, Elapid Venoms pharmacology, Gap Junctions chemistry, Gap Junctions ultrastructure, Immunohistochemistry, Ki-67 Antigen analysis, Microscopy, Electron, Muscle Fibers, Skeletal chemistry, Muscle Fibers, Skeletal physiology, Muscle Fibers, Skeletal ultrastructure, Muscle, Skeletal chemistry, Muscle, Skeletal ultrastructure, Myoblasts chemistry, Rats, Rats, Wistar, Regeneration drug effects, Time Factors, Tumor Suppressor Proteins analysis, Up-Regulation, Cell Cycle physiology, Connexin 43 analysis, Muscle, Skeletal physiology, Myoblasts physiology, Regeneration physiology

Abstract

The spatio-temporal expression of gap junction connexins (Cx) was investigated and correlated with the progression of cell cycle control in regenerating soleus muscle of Wistar rats. Notexin caused a selective myonecrosis followed by the complete recapitulation of muscle differentiation in vivo, including the activation, commitment, proliferation, differentiation and fusion of myogenic cells. In regenerating skeletal muscle, only Cx43 protein, out of Cx-s 26, -32, -37, -40, -43 and -45, was detected in desmin positive cells. Early expression of Cx43 in the proliferating single myogenic progenitors was followed by a progressive upregulation in interacting myoblasts until syncytial fusion, and then by a rapid decline in multinucleate myotubes. The significant upregulation of Cx43 gap junctions in aligned myoblasts preceding fusion was accompanied by the widespread nuclear expression of cyclin-dependent kinase inhibitors p21(waf1/Cip1) and p27(kip1) and the complete loss of Ki67 protein. The synchronized exit of myoblasts from the cell cycle following extensive gap junction formation suggests a role for Cx43 channels in the regulation of cell cycle control. The potential of Cx43 channels to stimulate p21(waf1/Cip1) and p27(kip1) is known. In the muscle, proving the involvement of Cx43 in either a direct or a bystander cell cycle regulation requires functional investigations.

Published

2005

4. Fibroblasts form a body-wide cellular network.

Author

Langevin HM, Cornbrooks CJ, and Taatjes DJ

Subjects

Animals, Biomarkers analysis, Cell Communication, Connective Tissue Cells cytology, Connexin 43 analysis, Dermis chemistry, Fibroblasts chemistry, Fluorescent Antibody Technique, Indirect, Gap Junctions ultrastructure, Humans, Male, Mice, Mice, Inbred C57BL, Microscopy, Confocal, Microscopy, Electron, Transmission, Signal Transduction, Dermis cytology, Fibroblasts cytology

Abstract

"Loose" connective tissue forms a network extending throughout the body including subcutaneous and interstitial connective tissues. The existence of a cellular network of fibroblasts within loose connective tissue may have considerable significance as it may support yet unknown body-wide cellular signaling systems. We used a combination of histochemistry, immunohistochemistry, confocal scanning laser microscopy (confocal microscopy), and electron microscopy to investigate the extent and nature of cell-to-cell connections within mouse subcutaneous connective tissue. We found that fibroblasts formed a reticular web throughout the tissue. With confocal microscopy, 30% of fibroblasts' processes could be followed continuously from one cell to another. Connexin 43 immunoreactivity was present at apparent points of cell-to-cell contact. Electron microscopy revealed that processes from adjacent cells were in close apposition to one another, but gap junctions were not observed. Our findings indicate that soft tissue fibroblasts form an extensively interconnected cellular network, suggesting they may have important and so far unsuspected integrative functions at the level of the whole body.

Published

2004

5. Expression of connexin 43 and ZO-1 in differentiating ameloblasts and odontoblasts from rat molar tooth germs.

Author

João SM and Arana-Chavez VE

Subjects

Ameloblasts cytology, Animals, Animals, Newborn, Cell Differentiation, Fluorescent Antibody Technique, Indirect, Gap Junctions chemistry, Gap Junctions ultrastructure, Membrane Proteins analysis, Microscopy, Confocal, Odontoblasts cytology, Phosphoproteins analysis, Rats, Rats, Wistar, Tight Junctions chemistry, Tight Junctions ultrastructure, Tooth Germ cytology, Zonula Occludens-1 Protein, Ameloblasts chemistry, Connexin 43 analysis, Odontoblasts chemistry, Odontogenesis physiology, Tooth Germ chemistry

Abstract

We studied the distribution of connexin (Cx) 43 and ZO-1 by confocal laser scanning microscopy at early stages of dentinogenesis and amelogenesis. Labeling for Cx43 was observed at early stages of differentiation in both the epithelial cells and differentiating odontoblasts. Immunolabeling was detected at the distal and medial regions of undifferentiated ameloblasts and between cells from stratum intermedium and stellate reticulum. Differentiating odontoblasts exhibited immunoreaction for this antibody at their distal end. Immunoreactivity for ZO-1 was observed at regions that correspond to the proximal and distal junctional complexes of differentiating ameloblasts. Staining for ZO-1 was observed at apical regions of odontoblasts with a punctate appearance. In more advanced stages, expression of Cx43 was more evident on ameloblasts, especially at the junctional complexes. Punctate immunolabeling for Cx43 was observed at the lateral sides of differentiating ameloblasts and between the other cells of the enamel organ. Immunoreaction for ZO-1 in ameloblasts was more evident than at the previous stage. It was also observed at the distal end of differentiated odontoblasts. The present study showed that differentiating ameloblasts and odontoblasts express Cx43 and ZO-1 as early as the start of the differentiation process. In addition, the expression of these junctional proteins increases as differentiation of cells continues.

Published

2003

6. Connexin 43 and the glucose transporter, GLUT1, in the ciliary body of the rat.

Author

Shin BC, Suzuki T, Tanaka S, Kuraoka A, Shibata Y, and Takata K

Subjects

Animals, Cell Membrane chemistry, Ciliary Body ultrastructure, Fluorescent Antibody Technique, Indirect, Glucose Transporter Type 1, Immunoblotting, Male, Microscopy, Fluorescence, Microscopy, Immunoelectron, Rats, Rats, Wistar, Ciliary Body chemistry, Connexin 43 analysis, Monosaccharide Transport Proteins analysis

Abstract

To investigate the relationship between the gap junction protein connexin 43 and the glucose transporter GLUT1, their localization was visualized by double-immunofluorescence microscopy using frozen sections as well as immunogold staining of ultrathin frozen sections. In pigmented epithelial cells, most of the GLUT1 was localized along the plasma membrane facing the blood vessels, whereas in non-pigmented epithelial cells, it was present along the plasma membrane facing the aqueous humor. Connexin 43 was abundant in the ciliary body and localized mainly in the gap junctions connecting the pigmented and non-pigmented epithelial cells. Localization of GLUT1 and connexin 43 in the blood-aqueous barrier suggests that GLUT1, connexin 43, and GLUT1 disposed in this order could be a machinery responsible for the transport of glucose across the blood-aqueous barrier.

Published

1996