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Retention and stimulus-dependent recycling of dense core vesicle content in neuroendocrine cells
Author(s) -
Roslyn A. Bauer,
Ruth L. Overlease,
Janet L. Lieber,
Joseph K. Angleson
Publication year - 2004
Publication title -
journal of cell science
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.384
H-Index - 278
eISSN - 1477-9137
pISSN - 0021-9533
DOI - 10.1242/jcs.01093
Subject(s) - exocytosis , vesicle , biology , immunogold labelling , colocalization , microbiology and biotechnology , secretory vesicle , golgi apparatus , prolactin , endosome , stimulation , biophysics , intracellular , biochemistry , secretion , endocrinology , hormone , membrane , antibody , immunology , endoplasmic reticulum
We have used fluorescence imaging of individual exocytic events in combination with immunogold electron microscopy and FM1-43 photoconversion to study the stimulus-dependent recycling of dense core vesicle content in isolated rat pituitary lactotrophs. Secretory stimulation with high external [K(+)] resulted in 100 exocytic sites per cell that were labeled by extracellular antibodies against the peptide hormone prolactin. Morphological analysis demonstrated that the prolactin was retained and internalized in intact dense cores. Vesicles containing non-secreted, internalized prolactin did not colocalize with DiI-LDL that had been chased into lysosomes but did transiently colocalize with internalized transferrin. The recycling vesicles also trafficked through a syntaxin 6-positive compartment but not the TGN38-positive trans-Golgi. Recycling vesicles, which returned to the cell surface in a slow basal manner, could also be stimulated to undergo exocytosis with a high release probability during subsequent exocytic stimulation with external K(+). These studies suggest a functional role for recycling vesicles that retain prolactin.

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