Congenital hypogonadotropic hypogonadism due to GnRH receptor mutations in three brothers reveal sites affecting conformation and coupling

Journal Article

2012

Permanent link to this Item
http://hdl.handle.net/11427/16221
 http://dx.doi.org/10.1371/journal.pone.0038456
Files
Tello_Congenital_Hypogonadotropic_Hypogonadism_2012.pdf (1.62 MB)
Authors
Tello, Javier A
Newton, Claire L
Bouligand, Jerome
Guiochon-Mantel, Anne
Millar, Robert P
Young, Jacques
Journal Title

PLoS One

Link to Journal
http://journals.plos.org/plosone
Journal ISSN
Volume Title
Publisher

Public Library of Science

Publisher

University of Cape Town

Department
MRC/UCT Receptor Biology Research Group
Faculty
Faculty of Health Sciences
License

http://creativecommons.org/licenses/by/4.0

Series
Abstract
Congenital hypogonadotropic hypogonadism (CHH) is characterized by low gonadotropins and failure to progress normally through puberty. Mutations in the gene encoding the GnRH receptor ( GNRHR1 ) result in CHH when present as compound heterozygous or homozygous inactivating mutations. This study identifies and characterizes the properties of two novel GNRHR1 mutations in a family in which three brothers display normosmic CHH while their sister was unaffected. Molecular analysis in the proband and the affected brothers revealed two novel non-synonymous missense GNRHR1 mutations, present in a compound heterozygous state, whereas their unaffected parents possessed only one inactivating mutation, demonstrating the autosomal recessive transmission in this kindred and excluding X-linked inheritance equivocally suggested by the initial pedigree analysis. The first mutation at c.845 C>G introduces an Arg substitution for the conserved Pro 282 in transmembrane domain (TMD) 6. The Pro282Arg mutant is unable to bind radiolabeled GnRH analogue. As this conserved residue is important in receptor conformation, it is likely that the mutation perturbs the binding pocket and affects trafficking to the cell surface. The second mutation at c.968 A>G introduces a Cys substitution for Tyr 323 in the functionally crucial N/DPxxY motif in TMD 7. The Tyr323Cys mutant has an increased GnRH binding affinity but reduced receptor expression at the plasma membrane and impaired G protein-coupling. Inositol phosphate accumulation assays demonstrated absent and impaired Gα q/11 signal transduction by Pro282Arg and Tyr323Cys mutants, respectively. Pretreatment with the membrane permeant GnRHR antagonist NBI-42902, which rescues cell surface expression of many GNRHR1 mutants, significantly increased the levels of radioligand binding and intracellular signaling of the Tyr323Cys mutant but not Pro282Arg. Immunocytochemistry confirmed that both mutants are present on the cell membrane albeit at low levels. Together these molecular deficiencies of the two novel GNRHR1 mutations lead to the CHH phenotype when present as a compound heterozygote.
Description
Keywords
Substitution mutation
Intracellular receptors
Cell binding
Cell membranes
Mutation detection
Phosphates
Cell binding assay
Mutation

Reference:

Tello, J. A., Newton, C. L., Bouligand, J., Guiochon-Mantel, A., Millar, R. P., & Young, J. (2012). Congenital hypogonadotropic hypogonadism due to GnRH receptor mutations in three brothers reveal sites affecting conformation and coupling. PloS one, 7(6), e38456. doi:10.1371/journal.pone.0038456

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