Oligospermic infertility associated with an androgen receptor mutation that disrupts interdomain and coactivator (TIF2) interactions
Farid J. Ghadessy, … , Mark A. Trifiro, Eu Leong Yong
Farid J. Ghadessy, … , Mark A. Trifiro, Eu Leong Yong
Published June 1, 1999
Citation Information: J Clin Invest. 1999;103(11):1517-1525. https://doi.org/10.1172/JCI4289.
View: Text | PDF
Article

Oligospermic infertility associated with an androgen receptor mutation that disrupts interdomain and coactivator (TIF2) interactions

Abstract

Structural changes in the androgen receptor (AR) are one of the causes of defective spermatogenesis. We screened the AR gene of 173 infertile men with impaired spermatogenesis and identified 3 of them, unrelated, who each had a single adenine→guanine transition that changed codon 886 in exon 8 from methionine to valine. This mutation was significantly associated with the severely oligospermic phenotype and was not detected in 400 control AR alleles. Despite the location of this substitution in the ligand-binding domain (LBD) of the AR, neither the genital skin fibroblasts of the subjects nor transfected cell types expressing the mutant receptor had any androgen-binding abnormality. However, the mutant receptor had a consistently (approximately 50%) reduced capacity to transactivate each of 2 different androgen-inducible reporter genes in 3 different cell lines. Deficient transactivation correlated with reduced binding of mutant AR complexes to androgen response elements. Coexpression of AR domain fragments in mammalian and yeast two-hybrid studies suggests that the mutation disrupts interactions of the LBD with another LBD, with the NH2-terminal transactivation domain, and with the transcriptional intermediary factor TIF2. These data suggest that a functional element centered around M886 has a role, not for ligand binding, but for interdomain and coactivator interactions culminating in the formation of a normal transcription complex.

Authors

Farid J. Ghadessy, Joyce Lim, Abdullah A.R. Abdullah, Valerie Panet-Raymond, Chee Keong Choo, Rose Lumbroso, Thein G. Tut, Bruce Gottlieb, Leonard Pinsky, Mark A. Trifiro, Eu Leong Yong

×

Figure 2

Options: View larger image (or click on image) Download as PowerPoint
Dissociation kinetics of ARs in genital skin fibroblasts. Normal (C, ope...
Dissociation kinetics of ARs in genital skin fibroblasts. Normal (C, open circles and bold lines) and mutant (CML, filled circles and normal lines; KLH, filled squares and thin lines) fibroblast monolayers were exposed to 2 nM [3H]MB (top), 3 nM [3H]DHT (middle), or 3 nM [3H]T (bottom) at 37°C (left) or 42°C (right) for 2 hours. The radiolabeled medium was discarded and replaced with one containing 200-fold excess unlabeled androgen; replicate samples were removed at the indicated times and assayed for [3H]androgen that was still receptor bound. Each data point, the mean of 4 replicates, is expressed as a percentage of maximum binding at time 0. Vertical axes are on the same logarithmic scale, except for bottom right panel.