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Research Article Free access | 10.1172/JCI118229

Expression of VAMP-2-like protein in kidney collecting duct intracellular vesicles. Colocalization with Aquaporin-2 water channels.

S Nielsen, D Marples, H Birn, M Mohtashami, N O Dalby, M Trimble, and M Knepper

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Nielsen, S. in: PubMed | Google Scholar

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Marples, D. in: PubMed | Google Scholar

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Birn, H. in: PubMed | Google Scholar

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Mohtashami, M. in: PubMed | Google Scholar

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Dalby, N. in: PubMed | Google Scholar

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Trimble, M. in: PubMed | Google Scholar

Department of Cell Biology, University of Aarhus, Denmark.

Find articles by Knepper, M. in: PubMed | Google Scholar

Published October 1, 1995 - More info

Published in Volume 96, Issue 4 on October 1, 1995
J Clin Invest. 1995;96(4):1834–1844. https://doi.org/10.1172/JCI118229.
© 1995 The American Society for Clinical Investigation
Published October 1, 1995 - Version history
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Abstract

Body water balance is controlled by vasopressin, which regulates Aquaporin-2 (AQP2) water channels in kidney collecting duct cells by vesicular trafficking between intracellular vesicles and the plasma membrane. To examine the molecular apparatus involved in vesicle trafficking and vasopressin regulation of AQP2 in collecting duct cells, we tested if targeting proteins expressed in the synaptic vesicles, namely vesicle-associated membrane proteins 1 and 2 (VAMP1 and 2), are expressed in kidney collecting duct. Immunoblotting revealed specific labeling of VAMP2 (18-kD band) but not VAMP1 in membrane fractions prepared from kidney inner medulla. Controls using preadsorbed antibody or preimmune serum were negative. Bands of identical molecular size were detected in immunoblots of brain membrane vesicles and purified synaptic vesicles. VAMP2 in kidney membranes was cleaved by tetanus toxin, revealing a tetanus toxin-sensitive VAMP homologue. Similarly, tetanus toxin cleaved VAMP2 in synaptic vesicles. In kidney inner medulla, VAMP2 was predominantly expressed in the membrane fraction enriched for intracellular vesicles, with little or no VAMP2 in the plasma membrane enriched fraction. This was confirmed by immunocytochemistry using semithin cryosections, which showed mainly vesicular labeling in collecting duct principal cells, with no labeling of intercalated cells. VAMP2 immunolabeling colocalized with AQP2 labeling in intracellular vesicles, as determined by immunoelectron microscopy after double immunolabeling of isolated vesicles. Quantitative analysis of 1,310 vesicles revealed a highly significant association of both AQP2 and VAMP2 in the same vesicles (P < 0.0001). Furthermore, the presence of AQP2 in vesicles immunoisolated with anti-VAMP2 antibodies was confirmed by immunoblotting. In conclusion, VAMP2, a component of the neuronal SNARE complex, is expressed in vesicles carrying AQP2, suggesting a role in vasopressin-regulated vesicle trafficking of AQP2 water channels.

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