Clathrin in gastric acid secretory (parietal) cells: biochemical characterization and subcellular localization

Clathrin in gastric acid secretory (parietal) cells: biochemical characterization and subcellular localization

1  Department of Pharmaceutical Sciences, School of Pharmacy, University of Southern California, Los Angeles 90089-9121; and 2  Department of Molecular and Cell Biology, 3  Lawrence Berkeley Laboratory, and 4  Electron Microscope Lab, University of California, Berkeley, California 94720 Clathrin fro...

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Veröffentlicht in:American Journal of Physiology: Cell Physiology 2000-09, Vol.279 (3), p.C833-C851
Hauptverfasser: Okamoto, Curtis T, Duman, Joseph G, Tyagarajan, Kamala, McDonald, Kent L, Jeng, Young Y, McKinney, Jeana, Forte, Trudy M, Forte, John G
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Blotting, Western
Cells, Cultured
Chemical Fractionation
Chromatography
Clathrin - chemistry
Clathrin - metabolism
Coated Pits, Cell-Membrane - metabolism
Durapatite
Freezing
Gastric Acid - secretion
H(+)-K(+)-Exchanging ATPase - metabolism
Immunologic Techniques
Mass Spectrometry
Microsomes - metabolism
Parietal Cells, Gastric - metabolism
Parietal Cells, Gastric - secretion
Polymers - metabolism
Rabbits
Stomach - metabolism
Subcellular Fractions - metabolism
Tissue Distribution
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Zusammenfassung:1  Department of Pharmaceutical Sciences, School of Pharmacy, University of Southern California, Los Angeles 90089-9121; and 2  Department of Molecular and Cell Biology, 3  Lawrence Berkeley Laboratory, and 4  Electron Microscope Lab, University of California, Berkeley, California 94720 Clathrin from H-K-ATPase-rich membranes derived from the tubulovesicular compartment of rabbit and hog gastric acid secretory (parietal) cells was characterized biochemically, and the subcellular localization of membrane-associated clathrin in parietal cells was characterized by immunofluorescence, electron microscopy, and immunoelectron microscopy. Clathrin from H-K- ATPase-rich membranes was determined to be comprised of conventional clathrin heavy chain and a predominance of clathrin light chain A. Clathrin and adaptors could be induced to polymerize quantitatively in vitro, forming 120-nm-diameter basketlike structures. In digitonin-permeabilized resting parietal cells, the intracellular distribution of immunofluorescently labeled clathrin was suggestive of labeling of the tubulovesicular compartment. Clathrin was also unexpectedly localized to canalicular (apical) membranes, as were -adaptin and dynamin, suggesting that this membrane domain of resting parietal cells is endocytotically active. At the ultrastructural level, clathrin was immunolocalized to canalicular and tubulovesicular membranes. H-K-ATPase was immunolocalized to the same membrane domains as clathrin but did not appear to be enriched at the specific subdomains that were enriched in clathrin. Finally, in immunofluorescently labeled primary cultures of parietal cells, in contrast to the H-K-ATPase, intracellular clathrin was found not to translocate to the apical membrane on secretagogue stimulation. Taken together, these biochemical and morphological data provide a framework for characterizing the role of clathrin in the regulation of membrane trafficking from tubulovesicles and at the canalicular membrane in parietal cells. hydrogen-potassium-adenosinetriphosphatase; apical membrane recycling; tubulovesicles; dynamin; gastric microsomes
ISSN:0363-6143
1522-1563
DOI:10.1152/ajpcell.2000.279.3.c833