Absence of functional insulin receptor substrate-3 (IRS-3) gene in humans

Insulin receptor substrate (IRS) proteins play important roles in insulin action and pancreatic beta-cell function. At least four mammalian IRS molecules have been identified. Although genes and cDNAs encoding human IRS-1, IRS-2, and IRS-4 have been cloned, IRS-3 has been identified only in rodents....

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Bibliographic Details
Published in:Diabetologia 2002-12, Vol.45 (12), p.1697-1702
Main Authors: BJÖRNHOLM, M, HE, A. R, ATTERSAND, A, LAKE, S, LIU, S. C. H, LIENHARD, G. E, TAYLOR, S, ARNER, P, ZIERATH, J. R
Format: Article
Language:English
Subjects:
Adipocytes
Adipocytes - metabolism
Adult
Amino Acid Sequence - genetics
Animals
Bioinformatics
Biological and medical sciences
Body fat
Cloning
Cloning, Molecular
Computational Biology
Diabetes
Diabetes. Impaired glucose tolerance
Endocrine pancreas. Apud cells (diseases)
Endocrinopathies
Etiopathogenesis. Screening. Investigations. Target tissue resistance
Female
Gene Deletion
Gene Library
Genes
Genome, Human
Genomes
Hospitals
Humans
Insulin Receptor Substrate Proteins
Insulin resistance
Kinases
Male
Medical sciences
Metabolism
Mice
Middle Aged
Molecular Sequence Data
Musculoskeletal system
Phosphoproteins - deficiency
Phosphoproteins - genetics
Phosphoproteins - physiology
Phosphorylation
Physiology
Proteins
Rats
Reverse Transcriptase Polymerase Chain Reaction
Signal transduction
Tyrosine - metabolism
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Summary:Insulin receptor substrate (IRS) proteins play important roles in insulin action and pancreatic beta-cell function. At least four mammalian IRS molecules have been identified. Although genes and cDNAs encoding human IRS-1, IRS-2, and IRS-4 have been cloned, IRS-3 has been identified only in rodents. Thus, we have attempted to clone the human IRS-3 gene. Insulin-stimulated rat or human adipocytes were subjected to Western blot analysis to assess IRS-3 tyrosine phosphorylation. Human liver and adipose cDNA libraries were screened in an effort to clone IRS-3 cDNA. A PCR-based approach was designed to amplify IRS-3 cDNA. Reverse transcription PCR was carried out using mRNA from adipose tissue, liver, and skeletal muscle as templates in combination with an in silico screen using mouse IRS-1, IRS-2 and IRS-3 in a tblastn search of the draft public human genome. In human adipocytes we did not detect a M(r) 60 000 phosphoprotein corresponding to IRS-3, whereas in rat adipocytes IRS-3 protein and insulin-stimulated tyrosine phosphorylation was readily observed. None of the molecular approaches provided evidence for a functional IRS-3gene in human tissue. Two deletions in human IRS-3 gene were identified using bioinformatics. The human IRS-3 gene product is predicted to lack a phosphotyrosine binding domain and also the sequence corresponding amino acid 353-407 of murine IRS-3. The contiguous sequence of genomic DNA between these two homologous regions does not have the coding information for human IRS-3. In silico screening of the human IRS-3 genome region, combined with further biological and molecular validation, provides evidence against a functional IRS-3 in humans.
ISSN:0012-186X
1432-0428
DOI:10.1007/s00125-002-0945-z