Novel Glial Cells Missing-2 (GCM2) variants in parathyroid disorders

Novel Glial Cells Missing-2 (GCM2) variants in parathyroid disorders

Objective The aim of this study was to analyze variants of the gene glial cells missing-2 (GCM2), encoding a parathyroid cell-specific transcription factor, in familial hypoparathyroidism and in familial isolated hyperparathyroidism (FIHP) without and with parathyroid carcinoma. Design We characteri...

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Veröffentlicht in:European journal of endocrinology 2022-03, Vol.186 (3), p.351-366
Hauptverfasser: Canaff, Lucie, Guarnieri, Vito, Kim, Yoojung, Wong, Betty Y L, Nolin-Lapalme, Alexis, Cole, David E C, Minisola, Salvatore, Eller-Vainicher, Cristina, Cetani, Filomena, Repaci, Andrea, Turchetti, Daniela, Corbetta, Sabrina, Scillitani, Alfredo, Goltzman, David
Format: Artikel
Sprache:eng
Schlagworte:
Adult
Aged
Aged, 80 and over
Animals
Binding Sites
Calcium - blood
Calcium - urine
Clinical Study
DNA - blood
DNA - metabolism
Female
Humans
Hyperparathyroidism - genetics
Hyperparathyroidism - metabolism
Hyperparathyroidism - pathology
Hypoparathyroidism - blood
Hypoparathyroidism - genetics
Infant
Male
Mice
Middle Aged
Mutation
Nuclear Proteins - chemistry
Nuclear Proteins - genetics
Nuclear Proteins - metabolism
Parathyroid Glands - pathology
Parathyroid Glands - surgery
Parathyroid Hormone - blood
Parathyroid Hormone - genetics
Parathyroid Neoplasms - genetics
Parathyroid Neoplasms - metabolism
Parathyroid Neoplasms - pathology
Pedigree
Promoter Regions, Genetic
Sequence Analysis, DNA
Transcription Factors - chemistry
Transcription Factors - genetics
Transcription Factors - metabolism
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Zusammenfassung:Objective The aim of this study was to analyze variants of the gene glial cells missing-2 (GCM2), encoding a parathyroid cell-specific transcription factor, in familial hypoparathyroidism and in familial isolated hyperparathyroidism (FIHP) without and with parathyroid carcinoma. Design We characterized 2 families with hypoparathyroidism and 19 with FIHP in which we examined the mechanism of action of GCM2 variants. Methods Leukocyte DNA of hypoparathyroid individuals was Sanger sequenced for CASR, PTH, GNA11 and GCM2 mutations. DNA of hyperparathyroid individuals underwent MEN1, CDKN1B, CDC73, CASR, RET and GCM2 sequencing. The actions of identified GCM2 variants were evaluated by in vitro functional analyses. Results A novel homozygous p.R67C GCM2 mutation which failed to stimulate transcriptional activity in a luciferase assay was identified in affected members of two hypoparathyroid families. Oligonucleotide pull-down assay and in silico structural modeling indicated that this mutant had lost the ability to bind the consensus GCM recognition sequence of DNA. Two novel (p.I383M and p.T386S) and one previously reported (p.Y394S) heterozygous GCM2 variants that lie within a C-terminal conserved inhibitory domain were identified in three affected individuals of the hyperparathyroid families. One family member, heterozygous for p.I138M, had parathyroid carcinoma (PC), and a heterozygous p.V382M variant was found in another patient affected by sporadic PC. These variants exerted significantly enhanced in vitrotranscriptional activity, including increased stimulation of the PTH promoter. Conclusions We provide evidence that two novel GCM2 R67C inactivating mutations with an inability to bind DNA are causative of hypoparathyroidism. Additionally, we provide evidence that two novel GCM2 variants increased transactivation of the PTH promoter in vitro and are associated with FIHP. Furthermore, our studies suggest that activating GCM2 variants may contribute to facilitating more aggressive parathyroid disease.
ISSN:0804-4643
1479-683X
DOI:10.1530/EJE-21-0433