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      Enlargeosome traffic: exocytosis triggered by various signals is followed by endocytosis, membrane shedding or both.

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          Abstract

          Enlargeosomes are cytoplasmic organelles discharged by regulated exocytosis, identified by immunofluorescence of their membrane marker, desmoyokin/Ahnak, but never revealed at the ultrastructural level. Among the numerous enlargeosome-positive cells, the richest and most extensively characterized are those of a PC12 clone, PC12-27, defective of classical neurosecretion. By using ultrastructural immunoperoxidase labeling of formaldehyde-fixed, Triton-X-100-permeabilized PC12-27 cells, we have now identified the enlargeosomes as small vesicles scattered in the proximity of, but never docked to, the plasma membrane. Upon stimulation, these vesicles undergo exocytosis [rapid after the Ca(2+) ionophore, ionomycin, much slower after either the phorbol ester, phorbol myristate acetate (PMA), or ATP, working through a P2Y receptor], with appearance in the plasma membrane of typical desmoyokin/Ahnak (d/A)-positive, Omega-shaped and open profiles evolving into flat patches. Postexocytic removal of the exocytized d/A-positive membrane occurs by two processes: generation of endocytic vesicles, predominant after ionomycin and ATP 100-500 microM; and shedding of membrane-bound cytoplasmic bodies, predominant after PMA and 1 mM ATP, containing little or no trace of endoplasmic reticulum, Golgi, endo/lysosomes and also of a plasma membrane marker. Depending on the stimulation, therefore, the cell-surface expansion by enlargeosome exocytosis is not always recycled but can induce release of specific membranes, possibly important in the pericellular environment.

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          Author and article information

          Journal
          Traffic
          Traffic (Copenhagen, Denmark)
          Wiley
          1398-9219
          1398-9219
          Jun 2007
          : 8
          : 6
          Affiliations
          [1 ] Center of Excellence in Cell Development, Vita-Salute San Raffaele University, DIBIT, via Olgettina 58, 20132 Milan, Italy.
          Article
          TRA566
          10.1111/j.1600-0854.2007.00566.x
          17488290
          5377332d-121e-412a-af33-43d894d591f1
          History

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