The severe short stature in two siblings with a heterozygous IGF1 mutation is not caused by a dominant negative effect of the putative truncated protein

H A van Duyvenvoorde; J van Doorn; J Koenig; L Gauguin; W Oostdijk; J D Wade; M Karperien; C A L Ruivenkamp; M Losekoot; P A van Setten; M J E Walenkamp; C Noordam; P De Meyts; J M Wit

doi:10.1016/j.ghir.2010.12.004

The severe short stature in two siblings with a heterozygous IGF1 mutation is not caused by a dominant negative effect of the putative truncated protein

Growth Horm IGF Res. 2011 Feb;21(1):44-50. doi: 10.1016/j.ghir.2010.12.004. Epub 2011 Jan 14.

Authors

H A van Duyvenvoorde¹, J van Doorn, J Koenig, L Gauguin, W Oostdijk, J D Wade, M Karperien, C A L Ruivenkamp, M Losekoot, P A van Setten, M J E Walenkamp, C Noordam, P De Meyts, J M Wit

Affiliation

¹ Department of Pediatrics, Leiden University Medical Center, Leiden, The Netherlands. H.A.van_Duyvenvoorde@lumc.nl

PMID: 21237682
DOI: 10.1016/j.ghir.2010.12.004

Abstract

Objective: While in previous studies heterozygosity for an Insulin-Like Growth Factor 1 (IGF1) defect only modestly decreased height and head circumference, we recently reported on two siblings with severe short stature with a maternally transmitted heterozygous duplication of 4 nucleotides, resulting in a frame shift and a premature termination codon in the IGF1 gene. In this paper we describe the structural and functional characteristics of the putative truncated IGF-I protein.

Design: Two children, their mother and maternal grandfather carried the mutation. In addition, two family members who were not affected were included in the study. Mutant (MT) IGF-I was synthesized in oxidized and reduced form using two methods. Neutral gel filtration studies were carried out with wild-type (WT) and synthetic MT IGF-I. Binding analysis of synthetic MT IGF-I to the IGF1R and insulin receptors were performed with EBNA-293 cells, stably transfected with the IGF-I receptor, and IM9 cells. L6 cells were used to examine the mitogenic potency and the potential antagonizing effect of synthetic MT IGF-I by [(3)H]-thymidine incorporation assays.

Results: In the sera of both the carriers and non-carriers the proportion of (125)I-IGF-I that was associated with the 150 kDa complex was somewhat less (varying between ~37 and ~52%) than in normal pooled serum (~53-~63%) and, instead, slightly increased amounts of radioactivity were eluted in the 40-50 kDa fraction (consisting of binary IGF-IGFBP complexes) or remained unbound. Synthetic MT IGF-I did not bind to the IGF-I receptor, nor antagonize the growth-promoting effect of IGF-I. It did bind to IGFBPs, but was barely incorporated into 150 kDa complexes. Because in all cases WT IGF-I immunoreactivity was recovered in one peak, corresponding to the MW of WT IGF-I, i.e. ~7.6 kDa, an interaction of circulating truncated mutant peptide with WT IGF-I is very unlikely.

Conclusions: There is no evidence that the severe short stature associated with heterozygosity for this novel IGF1 mutation in children born from a mother with the same mutation is caused by a dominant negative effect of the truncated protein. We speculate that the growth failure is caused by a combination of partial IGF-I deficiency, placental IGF-I insufficiency, and other genetic factors.

Publication types

Case Reports

MeSH terms

Amino Acid Sequence
Base Sequence
Body Height / genetics
Child
Dwarfism / genetics*
Female
Genes, Dominant
Heterozygote
Humans
Insulin-Like Growth Factor I / chemistry
Insulin-Like Growth Factor I / genetics*
Insulin-Like Growth Factor I / physiology
Male
Molecular Sequence Data
Mutation, Missense* / physiology
Protein Isoforms / genetics
Protein Isoforms / physiology
Siblings

Substances

Protein Isoforms
Insulin-Like Growth Factor I