Literature DB >> 9547304

Microtubules facilitate the stimulated secretion of beta-hexosaminidase in lacrimal acinar cells.

S R da Costa1, F A Yarber, L Zhang, M Sonee, S F Hamm-Alvarez.   

Abstract

Stimulation of lacrimal acini with secretagogues such as carbachol initiates movement and fusion of acinar secretory vesicles with the apical plasma membrane, resulting in release of protein into the nascent tear fluid. Using rabbit lacrimal acini reconstituted in vitro from isolated cells, we have investigated the organization of the apical cytoskeleton and its role in stimulated secretion. Confocal microscopy revealed a microtubule array emanating from the apical region of the acini; the apical region was also enriched in microfilaments and (gamma)-tubulin. Cytokeratin-based intermediate filaments were apically concentrated, and also detected at the cell periphery. Neither confocal microscopy nor biochemical analysis revealed any reorganization of lumenal microfilaments or microtubules which might accompany carbachol-stimulated release of secretory proteins. However, major changes in the acinar microtubule array induced by taxol or nocodazole were correlated with inhibition of carbachol-dependent release of the secreted protein, beta-hexosaminidase. Major changes in lumenal microfilaments induced by jasplakinolide or cytochalasin D did not inhibit the carbachol-dependent release of beta-hexosaminidase; rather, release of beta-hexosaminidase from jasplakinolide- or cytochalasin D-treated carbachol-stimulated acini was markedly increased relative to the release from untreated stimulated acini. Our findings demonstrate that microtubules play a major role in stimulated lacrimal secretion, and suggest a contributory role for microfilaments.

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Year:  1998        PMID: 9547304     DOI: 10.1242/jcs.111.9.1267

Source DB:  PubMed          Journal:  J Cell Sci        ISSN: 0021-9533            Impact factor:   5.285


  18 in total

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Authors:  Silvia R Da Costa; Eunbyul Sou; Jiansong Xie; Francie A Yarber; Curtis T Okamoto; Michael Pidgeon; Michael M Kessels; Austin K Mircheff; Joel E Schechter; Britta Qualmann; Sarah F Hamm-Alvarez
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2.  Use of nucleofection to efficiently transfect primary rabbit lacrimal gland acinar cells.

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4.  Labial Salivary Glands in Infants: Histochemical Analysis of Cytoskeletal and Antimicrobial Proteins.

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Journal:  J Histochem Cytochem       Date:  2016-08       Impact factor: 2.479

5.  Transduced viral IL-10 is exocytosed from lacrimal acinar secretory vesicles in a myosin-dependent manner in response to carbachol.

Authors:  Jiansong Xie; Ronald R Marchelletta; Padmaja B Thomas; Damon T Jacobs; Francie A Yarber; Richard E Cheney; Sarah F Hamm-Alvarez; Melvin D Trousdale
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Journal:  Exp Eye Res       Date:  2005-07-11       Impact factor: 3.467

7.  Actin and non-muscle myosin II facilitate apical exocytosis of tear proteins in rabbit lacrimal acinar epithelial cells.

Authors:  Galina V Jerdeva; Kaijin Wu; Francie A Yarber; Christopher J Rhodes; Daniel Kalman; Joel E Schechter; Sarah F Hamm-Alvarez
Journal:  J Cell Sci       Date:  2005-10-15       Impact factor: 5.285

8.  Dominant-negative PKC-epsilon impairs apical actin remodeling in parallel with inhibition of carbachol-stimulated secretion in rabbit lacrimal acini.

Authors:  Galina V Jerdeva; Francie A Yarber; Melvin D Trousdale; Christopher J Rhodes; Curtis T Okamoto; Darlene A Dartt; Sarah F Hamm-Alvarez
Journal:  Am J Physiol Cell Physiol       Date:  2005-06-01       Impact factor: 4.249

9.  A thermo-responsive protein treatment for dry eyes.

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Journal:  J Control Release       Date:  2014-12-03       Impact factor: 9.776

10.  Biosynthesis, processing, trafficking, and enzymatic activity of mouse neprilysin 2.

Authors:  Kentaro Oh-hashi; Kazumi Ohkubo; Kaoru Shizu; Hibiki Fukuda; Yoko Hirata; Kazutoshi Kiuchi
Journal:  Mol Cell Biochem       Date:  2008-04-19       Impact factor: 3.396

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