The morphometric changes in the gills of the estuarine crab Chasmagnathus granulatus under hyper- and hyporegulation conditions are not caused by proliferation of specialised cells

Chasmagnathus granulatus is a hyper-hyporegulating crab that inhabits changing habitats of salinity in Brazil, Uruguay and Argentina. Since the gills are the main sites for active ion transport in crabs, the adaptive changes in the gill epithelium occurring under different conditions of salinity wer...

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Detalles Bibliográficos
Autores principales: Genovese, G., Luquet, C.M., Paz, D.A., Rosa, G.A., Pellerano, G.N.
Formato: JOUR
Materias:
Crustacea
Ion-regulation
Salinity
ion
sea water
silver nitrate
acclimatization
animal cell
animal tissue
article
cell labeling
cell proliferation
cell size
controlled study
crab
epithelium
gill
immunohistochemistry
ion transport
morphology
morphometrics
nonhuman
priority journal
respiratory function
salinity
technique
thickness
Adaptation, Physiological
Animals
Brachyura
Cell Division
Coloring Agents
Epithelial Cells
Fresh Water
Gills
Ion Transport
Liver
Pancreas
Sodium Chloride
Animalia
Chasmagnathus granulata
Decapoda (Crustacea)
Acceso en línea:http://hdl.handle.net/20.500.12110/paper_00218782_v197_n2_p239_Genovese
Aporte de:
Biblioteca Digital - Facultad de Ciencias Exactas y Naturales (UBA) de Universidad de Buenos Aires
Descripción
Sumario:Chasmagnathus granulatus is a hyper-hyporegulating crab that inhabits changing habitats of salinity in Brazil, Uruguay and Argentina. Since the gills are the main sites for active ion transport in crabs, the adaptive changes in the gill epithelium occurring under different conditions of salinity were studied by means of morphological and morphometric analysis, and immunohistochemical identification of cell proliferation (BrdU technique). In anterior (1-3) gills the epithelium thickness from crabs acclimatised to 12, 34 and 44 g/l ranged from 1.27 to 2.46 μm, with no significant change during acclimatisation, thus denoting a respiratory function. Medial (4-5) gill epithelium was slightly thicker in extreme salinities, but these differences were not statistically significant. In contrast, epithelial thickness of the posterior (6-8) gills increased significantly up to 8.10 μm (dorsal zone of gill 8) both in hyper- and hyposaline media compared with seawater. The dark areas measured in gill 8 treated with AgNO3 revealed putative ion transporting tissue, especially at 12 and 44 g/l, corresponding to the zones of higher epithelial thickness. Hence these areas seem to participate both in hyper- and hyporegulation. Proliferating cells labelled with BrdU almost never occurred in the gills/salinity combinations studied during the initial 48 h of transfer from seawater to hyperconcentrated or diluted media, thus suggesting an increase in cell size rather than cell proliferation.

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