Multiplicity of expression of Na+,K+-ATPase {alpha}-subunit isoforms in the gill of Atlantic salmon (Salmo salar): cellular localisation and absolute quantification in response to salinity change

The ability to reverse the net direction of gill ion transport in response to a salinity change is critical for euryhaline teleosts and involves a complex cellular and molecular remodelling of the gill epithelium. The present study aimed to clarify the cellular localisation and exact quantitative in...

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Bibliographic Details
Published in:Journal of Experimental Biology
Main Authors: Madsen, Steffen S., Kiilerich, Pia, Tipsmark, Christian K.
Format: Text
Language:English
Published: Company of Biologists 2009
Subjects:
Research Article
Atlantic salmon
Salmo salar
Online Access:http://jeb.biologists.org/cgi/content/short/212/1/78
https://doi.org/10.1242/jeb.024612
Description
Summary:The ability to reverse the net direction of gill ion transport in response to a salinity change is critical for euryhaline teleosts and involves a complex cellular and molecular remodelling of the gill epithelium. The present study aimed to clarify the cellular localisation and exact quantitative inter-relationship of Na+,K+–ATPase α- and β-subunit transcripts in Atlantic salmon gill during salinity change. The combined expression level of all α-isoforms in the gill increased by 100% after freshwater (FW) to seawater (SW) transfer. The α 1a and α 1b isoforms were both in the range 1–6 amol 20 ng–1 total RNA; α 1a decreased and α 1b increased after SW-transfer, their ratio changing from 5:1 in FW to 0.26:1 in SW. The α 1c and α 3 levels were 10- and 100-fold lower, respectively. The β 1 -subunit mRNA level was 0.1–0.3 amol 20 ng–1 total RNA, thus much lower than the sum of α-subunits. Even though increasing 3-fold after SW-transfer, β-subunit availability may still limit functional pump synthesis. The mRNAs of the predominant α 1a and α 1b isoforms were localised by in situ hybridisation in specific gill cells of both FW and SW salmon. Labelling occurred mainly in presumed chloride cells and cells deep in the filament but occasionally also on lamellae. Overall, the salinity-induced variation in labelling pattern and intensity matched the quantification data. In conclusion, the predominant switching of Na+,K+–ATPase α-subunit isoform mRNA during salinity acclimation reflects a marked remodelling of mitochondrion-rich cells (MRCs) in the gill and probably tuning of the pump performance to accomplish a net reversal of gill ion transport in hypo- and hypertonic environments.

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