Characterization of Gastric Na⁺/I^- Symporter of the Rat

Authors: Kotani T.^{1, 3}; Ogata Y.³; Yamamoto I.³; Aratake Y.³; Kawano J-I.²; Suganuma T.²; Ohtaki S.^{1, 3}

Source: Clinical Immunology and Immunopathology, Volume 89, Number 3, December 1998 , pp. 271-278(8)

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Abstract:

Characterization of gastric Na⁺/I^- symporter (NIS) of the rat was carried out. Sequencing of the open reading frame of gastric NIS mRNA showed only three nucleotide changes when compared with FRTL-5 NIS cDNA, and two of these changes led to amino acid changes. The results of Northern blot analysis showed that abundant NIS mRNA was expressed in the stomach when compared with other organs. Western blot analysis using gastric mucosa and FRTL-5 lysates detected the difference in molecular weight between FRTL-5 and gastric mucosa lysates, suggesting abnormal posttranslational modification of gastric NIS protein. Immunohistochemically, gastric NIS protein was located in the cornification layer of the stratified squamous epithelium of the pars proventricularis and in parietal cells and on the apical border of surface epithelial cells of the pars glandularis. Gastric NIS protein was present in tubulovesicular structures and lysosomes in parietal cells by immunoelectron microscopy. Gastric NIS protein exists to trap I^- from the gastric lumen, except in parietal cells. Results indicated that a very large amount of gastric NIS mRNA is expressed to be translated, whereas only a small amount of immature gastric NIS protein is detected. This may indicate that immature gastric NIS protein rapidly degrades to peptides. Copyright 1998 Academic Press.

Language: English

Document Type: Research article

Affiliations: 1: Department of Laboratory Medicine 2: Department of Laboratory Medicine, Second Department of Anatomy, Miyazaki Medical College 3: Laboratory for Clinical Investigation, Miyazaki Medical College Hospital, Kiyotake, Miyazaki, 889-1692, Japan

Publication date: 1998-12-01