Abstract
Transfection of the insulin-producing rat islet tumor cell line RIN-5AH with a full length cDNA of the rat hepatic growth hormone (GH) receptor (GH-R1-638) augments the GH-responsive insulin synthesis in these cells. Using this functional system we analyzed the effect of COOH-terminal truncation of the GH receptor. Two mutated cDNAs encoding truncated GH receptors, GH-R1-294 and GH-R1-454, respectively, were generated by site-directed mutagenesis and transfected into the RIN cells. Both receptor mutants were expressed on the cell surface and displayed normal GH binding affinity. Whereas GH-R1-638 had a molecular mass of about 110 kDa, GH-R1-294 and GH-R1-454 showed molecular masses of 49 and 80 kDa, respectively. Cells expressing GH-R1-454 internalized GH to a similar extent as cells transfected with the full length receptor and the parent cell line, but GH-R1-294-expressing cells showed a markedly reduced capability of GH internalization. In contrast to cells transfected with GH-R1-638, none of the cell lines expressing truncated GH receptors exhibited any increase of the GH-stimulated insulin production. We conclude that domains within the COOH-terminal half of the cytoplasmic part of the GH receptor are required for transduction of the signal for GH-stimulated insulin synthesis, whereas cytoplasmic domains proximal to the transmembrane region are involved in receptor-mediated GH internalization.
| Original language | English |
|---|---|
| Journal | The Journal of Biological Chemistry |
| Volume | 266 |
| Issue number | 26 |
| Pages (from-to) | 17441-5 |
| Number of pages | 5 |
| ISSN | 0021-9258 |
| Publication status | Published - 15 Sept 1991 |
Keywords
- Animals
- Cytoplasm
- Growth Hormone
- Insulinoma
- Kinetics
- Mutagenesis, Site-Directed
- Precipitin Tests
- Rats
- Receptors, Somatotropin
- Transfection
- Tumor Cells, Cultured