Your search keyword '"Stefan Bagheri-Fam"' showing total 47 results

1. Corrigendum: A role for TRPC3 in mammalian testis development

Author

Zhenhua Ming, Stefan Bagheri-Fam, Emily R. Frost, Janelle M. Ryan, Brittany Vining, and Vincent R. Harley

Subjects

SOX9, testis, sertoli cells, DSD, TRPC3, TRP, Biology (General), QH301-705.5

Published

2024

2. Y chromosome damage underlies testicular abnormalities in ATR-X syndrome

Author

Nayla Y. León, Thanh Nha Uyen Le, Andrew Garvie, Lee H. Wong, Stefan Bagheri-Fam, and Vincent R. Harley

Subjects

Genetics, Human Genetics, Science

Abstract

Summary: ATR-X (alpha thalassemia, mental retardation, X-linked) syndrome features genital and testicular abnormalities including atypical genitalia and small testes with few seminiferous tubules. Our mouse model recapitulated the testicular defects when Atrx was deleted in Sertoli cells (ScAtrxKO) which displayed G2/M arrest and apoptosis. Here, we investigated the mechanisms underlying these defects. In control mice, Sertoli cells contain a single novel “GATA4 PML nuclear body (NB)” that contained the transcription factor GATA4, ATRX, DAXX, HP1α, and PH3 and co-localized with the Y chromosome short arm (Yp). ScAtrxKO mice contain single giant GATA4 PML-NBs with frequent DNA double-strand breaks (DSBs) in G2/M-arrested apoptotic Sertoli cells. HP1α and PH3 were absent from giant GATA4 PML-NBs indicating a failure in heterochromatin formation and chromosome condensation. Our data suggest that ATRX protects a Yp region from DNA damage, thereby preventing Sertoli cell death. We discuss Y chromosome damage/decondensation as a mechanism for testicular failure.

Published

2024

3. A role for TRPC3 in mammalian testis development

Author

Zhenhua Ming, Stefan Bagheri-Fam, Emily R. Frost, Janelle M. Ryan, Brittany Vining, and Vincent R. Harley

Subjects

SOX9, testis, sertoli cells, DSD, TRPC3, TRP, Biology (General), QH301-705.5

Abstract

SOX9 is a key transcription factor for testis determination and development. Mutations in and around the SOX9 gene contribute to Differences/Disorders of Sex Development (DSD). However, a substantial proportion of DSD patients lack a definitive genetic diagnosis. SOX9 target genes are potentially DSD-causative genes, yet only a limited subset of these genes has been investigated during testis development. We hypothesize that SOX9 target genes play an integral role in testis development and could potentially be causative genes in DSD. In this study, we describe a novel testicular target gene of SOX9, Trpc3. Trpc3 exhibits high expression levels in the SOX9-expressing male Sertoli cells compared to female granulosa cells in mouse fetal gonads between embryonic day 11.5 (E11.5) and E13.5. In XY Sox9 knockout gonads, Trpc3 expression is markedly downregulated. Moreover, culture of E11.5 XY mouse gonads with TRPC3 inhibitor Pyr3 resulted in decreased germ cell numbers caused by reduced germ cell proliferation. Trpc3 is also expressed in endothelial cells and Pyr3-treated E11.5 XY mouse gonads showed a loss of the coelomic blood vessel due to increased apoptosis of endothelial cells. In the human testicular cell line NT2/D1, TRPC3 promotes cell proliferation and controls cell morphology, as observed by xCELLigence and HoloMonitor real-time analysis. In summary, our study suggests that SOX9 positively regulates Trpc3 in mouse testes and TRPC3 may mediate SOX9 function during Sertoli, germ and endothelial cell development.

Published

2024

4. Dataset of differentially expressed genes in mouse P12 testes in response to the loss of ATRX in Sertoli cells

Author

Stefan Bagheri-Fam, Dimuthu Alankarage, Emily R. Frost, and Vincent R. Harley

Subjects

ATRX, Sertoli cells, Microarray, Testis development, Spermatogenesis, Androgen receptor, Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

This dataset represents genes that are dysregulated in the postnatal day 12 (P12) mouse testis when ATRX is specifically inactivated in Sertoli cells (ScAtrxKO mice). The differentially expressed genes included in the dataset may play important roles in the testicular phenotypes observed in the ScAtrxKO mice, which were first reported in our previous work [1]. In fetal ScAtrxKO mice, Sertoli cells undergo apoptosis due to cell cycle defects, resulting in smaller testes with reduced tubule volume [1]. Adult ScAtrxKO mice show a wide range of spermatogenesis defects probably due to a failure of the dysfunctional ATRX protein to interact with the androgen receptor (AR) [1]. ATRX, a chromatin remodeling protein, is widely expressed in the human testis including Sertoli cells [2,3]. In XY individuals, the loss of ATRX leads to ATR-X (alpha thalassemia, mental retardation, X-linked) syndrome associated with a wide range of genital abnormalities such as hypospadias, ambiguous genitalia, and small testes with reduced tubule volume [4–8]. Our dataset contributes towards understanding the mechanism underlying ATRX regulation of testis development and spermatogenesis.

Published

2022

5. The gene encoding the ketogenic enzyme HMGCS2 displays a unique expression during gonad development in mice.

Author

Stefan Bagheri-Fam, Huijun Chen, Sean Wilson, Katie Ayers, James Hughes, Frederique Sloan-Bena, Pierre Calvel, Gorjana Robevska, Beatriz Puisac, Kamila Kusz-Zamelczyk, Stefania Gimelli, Anna Spik, Jadwiga Jaruzelska, Alina Warenik-Szymankiewicz, Sultana Faradz, Serge Nef, Juan Pié, Paul Thomas, Andrew Sinclair, and Dagmar Wilhelm

Subjects

Medicine, Science

Abstract

Disorders/differences of sex development (DSD) cause profound psychological and reproductive consequences for the affected individuals, however, most are still unexplained at the molecular level. Here, we present a novel gene, 3-hydroxy-3-methylglutaryl coenzyme A synthase 2 (HMGCS2), encoding a metabolic enzyme in the liver important for energy production from fatty acids, that shows an unusual expression pattern in developing fetal mouse gonads. Shortly after gonadal sex determination it is up-regulated in the developing testes following a very similar spatial and temporal pattern as the male-determining gene Sry in Sertoli cells before switching to ovarian enriched expression. To test if Hmgcs2 is important for gonad development in mammals, we pursued two lines of investigations. Firstly, we generated Hmgcs2-null mice using CRISPR/Cas9 and found that these mice had gonads that developed normally even on a sensitized background. Secondly, we screened 46,XY DSD patients with gonadal dysgenesis and identified two unrelated patients with a deletion and a deleterious missense variant in HMGCS2 respectively. However, both variants were heterozygous, suggesting that HMGCS2 might not be the causative gene. Analysis of a larger number of patients in the future might shed more light into the possible association of HMGCS2 with human gonadal development.

Published

2020

6. Dataset of differentially expressed genes from SOX9 over-expressing NT2/D1 cells

Author

Louisa Ludbrook, Dimuthu Alankarage, Stefan Bagheri-Fam, and Vincent Harley

Subjects

SOX9, NT2/D1 cells, Microarray, Sex determination, Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

The data presents the genes that are differentially up-regulated or down-regulated in response to SOX9 in a human Sertoli-like cell line, NT2/D1. The dataset includes genes that may be implicated in gonad development and are further explored in our associated article, “SOX9 Regulates Expression of the Male Fertility Gene Ets Variant Factor 5 (ETV5) during Mammalian Sex Development” (D. lankarage, R. Lavery, T. Svingen, S. Kelly, L.M. Ludbrook, S. Bagheri-Fam, et al., 2016) [1]. The necessity of SOX9 for male sex development is evident in instances where SOX9 is lost, as in 46, XY DSD where patients are sex reversed or in mouse knock-out models, where mice lacking Sox9 are sex reversed. Despite the crucial nature of this transcriptional activator, downstream target genes of SOX9 remain largely undiscovered. Here, we have utilized NT2/D1 cells to transiently over-express SOX9 and performed microarray analysis of the RNA. Microarray data are available in the ArrayExpress database (www.ebi.ac.uk/arrayexpress) under accession number E-MTAB-3378.

Published

2016

7. Dynamic expression patterns of Irx3 and Irx5 during germline nest breakdown and primordial follicle formation promote follicle survival in mouse ovaries.

Author

Anqi Fu, Sydney M Oberholtzer, Stefan Bagheri-Fam, Raphael H Rastetter, Claire Holdreith, Valeria L Caceres, Steven V John, Sarah A Shaw, Kathleen J Krentz, Xiaoyun Zhang, Chi-Chung Hui, Dagmar Wilhelm, and Joan S Jorgensen

Subjects

Genetics, QH426-470

Abstract

Women and other mammalian females are born with a finite supply of oocytes that determine their reproductive lifespan. During fetal development, individual oocytes are enclosed by a protective layer of granulosa cells to form primordial follicles that will grow, mature, and eventually release the oocyte for potential fertilization. Despite the knowledge that follicles are dysfunctional and will die without granulosa cell-oocyte interactions, the mechanisms by which these cells establish communication is unknown. We previously identified that two members of the Iroquois homeobox transcription factor gene family, Irx3 and Irx5, are expressed within developing ovaries but not testes. Deletion of both factors (Irx3-Irx5EGFP/Irx3-Irx5EGFP) disrupted granulosa cell-oocyte contact during early follicle development leading to oocyte death. Thus, we hypothesized that Irx3 and Irx5 are required to develop cell-cell communication networks to maintain follicle integrity and female fertility. A series of Irx3 and Irx5 mutant mouse models were generated to assess roles for each factor. While both Irx3 and Irx5 single mutant females were subfertile, their breeding outcomes and ovary histology indicated distinct causes. Careful analysis of Irx3- and Irx5-reporter mice linked the cause of this disparity to dynamic spatio-temporal changes in their expression patterns. Both factors marked the progenitor pre-granulosa cell population in fetal ovaries. At the critical phase of germline nest breakdown and primordial follicle formation however, Irx3 and Irx5 transitioned to oocyte- and granulosa cell-specific expression respectively. Further investigation into the cause of follicle death in Irx3-Irx5EGFP/Irx3-Irx5EGFP ovaries uncovered specific defects in both granulosa cells and oocytes. Granulosa cell defects included poor contributions to basement membrane deposition and mis-localization of gap junction proteins. Granulosa cells and oocytes both presented fewer cell projections resulting in compromised cell-cell communication. Altogether, we conclude that Irx3 and Irx5 first work together to define the pregranulosa cell population of germline nests. During primordial follicle formation, they transition to oocyte- and granulosa cell-specific expression patterns where they cooperate in neighboring cells to build the foundation for follicle integrity. This foundation is left as their legacy of the essential oocyte-granulosa cell communication network that ensures and ultimately optimizes the integrity of the ovarian reserve and therefore, the female reproductive lifespan.

Published

2018

8. Genome-wide ENU mutagenesis in combination with high density SNP analysis and exome sequencing provides rapid identification of novel mouse models of developmental disease.

Author

Georgina Caruana, Peter G Farlie, Adam H Hart, Stefan Bagheri-Fam, Megan J Wallace, Michael S Dobbie, Christopher T Gordon, Kerry A Miller, Belinda Whittle, Helen E Abud, Ruth M Arkell, Timothy J Cole, Vincent R Harley, Ian M Smyth, and John F Bertram

Subjects

Medicine, Science

Abstract

Mice harbouring gene mutations that cause phenotypic abnormalities during organogenesis are invaluable tools for linking gene function to normal development and human disorders. To generate mouse models harbouring novel alleles that are involved in organogenesis we conducted a phenotype-driven, genome-wide mutagenesis screen in mice using the mutagen N-ethyl-N-nitrosourea (ENU).ENU was injected into male C57BL/6 mice and the mutations transmitted through the germ-line. ENU-induced mutations were bred to homozygosity and G3 embryos screened at embryonic day (E) 13.5 and E18.5 for abnormalities in limb and craniofacial structures, skin, blood, vasculature, lungs, gut, kidneys, ureters and gonads. From 52 pedigrees screened 15 were detected with anomalies in one or more of the structures/organs screened. Using single nucleotide polymorphism (SNP)-based linkage analysis in conjunction with candidate gene or next-generation sequencing (NGS) we identified novel recessive alleles for Fras1, Ift140 and Lig1.In this study we have generated mouse models in which the anomalies closely mimic those seen in human disorders. The association between novel mutant alleles and phenotypes will lead to a better understanding of gene function in normal development and establish how their dysfunction causes human anomalies and disease.

Published

2013

9. Failure of SOX9 regulation in 46XY disorders of sex development with SRY, SOX9 and SF1 mutations.

Author

Kevin C Knower, Sabine Kelly, Louisa M Ludbrook, Stefan Bagheri-Fam, Helena Sim, Pascal Bernard, Ryohei Sekido, Robin Lovell-Badge, and Vincent R Harley

Subjects

Medicine, Science

Abstract

BackgroundIn human embryogenesis, loss of SRY (sex determining region on Y), SOX9 (SRY-related HMG box 9) or SF1 (steroidogenic factor 1) function causes disorders of sex development (DSD). A defining event of vertebrate sex determination is male-specific upregulation and maintenance of SOX9 expression in gonadal pre-Sertoli cells, which is preceded by transient SRY expression in mammals. In mice, Sox9 regulation is under the transcriptional control of SRY, SF1 and SOX9 via a conserved testis-specific enhancer of Sox9 (TES). Regulation of SOX9 in human sex determination is however poorly understood.Methodology/principal findingsWe show that a human embryonal carcinoma cell line (NT2/D1) can model events in presumptive Sertoli cells that initiate human sex determination. SRY associates with transcriptionally active chromatin in NT2/D1 cells and over-expression increases endogenous SOX9 expression. SRY and SF1 co-operate to activate the human SOX9 homologous TES (hTES), a process dependent on phosphorylated SF1. SOX9 also activates hTES, augmented by SF1, suggesting a mechanism for maintenance of SOX9 expression by auto-regulation. Analysis of mutant SRY, SF1 and SOX9 proteins encoded by thirteen separate 46,XY DSD gonadal dysgenesis individuals reveals a reduced ability to activate hTES.Conclusions/significanceWe demonstrate how three human sex-determining factors are likely to function during gonadal development around SOX9 as a hub gene, with different genetic causes of 46,XY DSD due a common failure to upregulate SOX9 transcription.

Published

2011

10. Somatic FGFR2 is Required for Germ Cell Maintenance in the Mouse Ovary

Author

Anthony D Bird, Emily R Frost, Stefan Bagheri-Fam, Brittany M Croft, Janelle M Ryan, Liang Zhao, Peter Koopman, and Vincent R Harley

Subjects

Endocrinology

Abstract

During sex determination in the mouse, fibroblast growth factor 9 signals through the fibroblast growth factor receptor 2c isoform (FGFR2c) to trigger Sertoli cell and testis development from 11.5 days post coitum (dpc). In the XX gonad, the FOXL2 and WNT4/RSPO1 pathways drive granulosa cell and ovarian development. The function of FGFR2 in the developing ovary, and whether FGFR2 is required in the testis after sex determination, is not clear. In fetal mouse gonads from 12.5 dpc, FGFR2 shows sexually dimorphic expression. In XX gonads, FGFR2c is coexpressed with FOXL2 in pregranulosa cells, whereas XY gonads show FGFR2b expression in germ cells. Deletion of Fgfr2c in XX mice led to a marked decrease/absence of germ cells by 13.5 dpc in the ovary. This indicates that FGFR2c in the somatic pregranulosa cells is required for the maintenance of germ cells. Surprisingly, on the Fgfr2c-/- background, the germ cell phenotype could be rescued by ablation of Foxl2, suggesting a novel mechanism whereby FGFR2 and FOXL2 act antagonistically during germ cell development. Consistent with low/absent FGFR2 expression in the Sertoli cells of 12.5 and 13.5 dpc XY gonads, XY AMH:Cre; Fgfr2flox/flox mice showed normal testis morphology and structures during fetal development and in adulthood. Thus, FGFR2 is not essential for maintaining Sertoli cell fate after sex determination. Combined, these data show that FGFR2 is not necessary for Sertoli cell function after sex determination but does play an important role in the ovary.

Published

2023

11. FGF9 variant in 46,XY DSD patient suggests a role for dimerization in sex determination

Author

Brittany Croft, Anthony D. Bird, Makoto Ono, Stefanie Eggers, Stefan Bagheri‐Fam, Janelle M. Ryan, Alejandra P. Reyes, Jocelyn van den Bergen, Anne Baxendale, Elizabeth M. Thompson, Andrew J. Kueh, Peter Stanton, Tim Thomas, Andrew H. Sinclair, and Vincent R. Harley

Subjects

Genetics, Genetics (clinical)

Abstract

46,XY gonadal dysgenesis (GD) is a Disorder/Difference of Sex Development (DSD) that can present with phenotypes ranging from ambiguous genitalia to complete male-to-female sex reversal. Around 50% of 46,XY DSD cases receive a molecular diagnosis. In mice, Fibroblast growth factor 9 (FGF9) is an important component of the male sex-determining pathway. Two FGF9 variants reported to date disrupt testis development in mice, but not in humans. Here, we describe a female patient with 46,XY GD harbouring the rare FGF9 variant (missense mutation), NM_002010.2:c.583G A;p.(Asp195Asn) (D195N). By biochemical and cell-based approaches, the D195N variant disrupts FGF9 protein homodimerisation and FGF9-heparin-binding, and reduces both Sertoli cell proliferation and Wnt4 repression. XY Fgf9

Published

2022

12. SOX9 in organogenesis: shared and unique transcriptional functions

Author

Zhenhua Ming, Brittany Vining, Stefan Bagheri-Fam, and Vincent Harley

Subjects

Pharmacology, Male, Cellular and Molecular Neuroscience, Organogenesis, Mutation, Campomelic Dysplasia, Disorders of Sex Development, Molecular Medicine, Humans, SOX9 Transcription Factor, Cell Biology, Molecular Biology, Chromatin

Abstract

The transcription factor SOX9 is essential for the development of multiple organs including bone, testis, heart, lung, pancreas, intestine and nervous system. Mutations in the human SOX9 gene led to campomelic dysplasia, a haploinsufficiency disorder with several skeletal malformations frequently accompanied by 46, XY sex reversal. The mechanisms underlying the diverse SOX9 functions during organ development including its post-translational modifications, the availability of binding partners, and tissue-specific accessibility to target gene chromatin. Here we summarize the expression, activities, and downstream target genes of SOX9 in molecular genetic pathways essential for organ development, maintenance, and function. We also provide an insight into understanding the mechanisms that regulate the versatile roles of SOX9 in different organs.

Published

2022

13. Ovotesticular disorders of sex development in FGF9 mouse models of human synostosis syndromes

Author

Stefan Bagheri-Fam, Brittany Croft, Lingyun Tang, Zhenhua Ming, Peter Koopman, Vincent R. Harley, Liang Zhao, Anthony Daniel Bird, Keiichi Akita, Masayo Harada, and Zhugang Wang

Subjects

Fibroblast Growth Factor 9, Male, medicine.medical_specialty, Male sex determination, Mutation, Missense, SOX9, Biology, 010402 general chemistry, 01 natural sciences, Mice, 03 medical and health sciences, FGF9, Internal medicine, Genetics, medicine, Animals, Humans, Disorders of sex development, Receptor, Fibroblast Growth Factor, Type 2, Gonads, Molecular Biology, Genetics (clinical), 030304 developmental biology, Phenocopy, 0303 health sciences, Sexual Development, Gene Expression Regulation, Developmental, SOX9 Transcription Factor, General Medicine, Sex Determination Processes, Sex reversal, medicine.disease, Phenotype, Ovotesticular Disorders of Sex Development, 0104 chemical sciences, Disease Models, Animal, stomatognathic diseases, Endocrinology, Synostosis, Female, Development of the gonads

Abstract

In mice, male sex determination depends on FGF9 signalling via FGFR2c in the bipotential gonads to maintain the expression of the key testis gene SOX9. In humans, however, while FGFR2 mutations have been linked to 46,XY disorders of sex development (DSD), the role of FGF9 is unresolved. The only reported pathogenic mutations in human FGF9, FGF9S99N and FGF9R62G, are dominant and result in craniosynostosis (fusion of cranial sutures) or multiple synostoses (fusion of limb joints). Whether these synostosis-causing FGF9 mutations impact upon gonadal development and DSD etiology has not been explored. We therefore examined embryonic gonads in the well-characterized Fgf9 missense mouse mutants, Fgf9S99N and Fgf9N143T, which phenocopy the skeletal defects of FGF9S99N and FGF9R62G variants, respectively. XY Fgf9S99N/S99N and XY Fgf9N143T/N143T fetal mouse gonads showed severely disorganized testis cords and partial XY sex reversal at 12.5 days post coitum (dpc), suggesting loss of FGF9 function. By 15.5 dpc, testis development in both mutants had partly recovered. Mitotic analysis in vivo and in vitro suggested that the testicular phenotypes in these mutants arise in part through reduced proliferation of the gonadal supporting cells. These data raise the possibility that human FGF9 mutations causative for dominant skeletal conditions can also lead to loss of FGF9 function in the developing testis, at least in mice. Our data suggest that, in humans, testis development is largely tolerant of deleterious FGF9 mutations which lead to skeletal defects, thus offering an explanation as to why XY DSDs are rare in patients with pathogenic FGF9 variants.

Published

2020

14. Functional Analysis of Mmd2 and Related PAQR Genes During Sex Determination in Mice

Author

Liang, Zhao, Ella, Thomson, Ee T, Ng, Enya, Longmuss, Terje, Svingen, Stefan, Bagheri-Fam, Alexander, Quinn, Vincent R, Harley, Leonard C, Harrison, Emanuele, Pelosi, and Peter, Koopman

Abstract

Sex determination in eutherian mammals is controlled by the Y-linked gene Sry, which drives the formation of testes in male embryos. Despite extensive study, the genetic steps linking Sry action and male sex determination remain largely unknown. Here, we focused on Mmd2, a gene that encodes a member of the progestin and adipoQ receptor (PAQR) family. Mmd2 is expressed during the sex-determining period in XY but not XX gonads, suggesting a specific role in testis development.We used CRISPR to generate mouse strains deficient in Mmd2 and its 2 closely related PAQR family members, Mmd and Paqr8, which are also expressed during testis development. Following characterization of Mmd2 expression in the developing testis, we studied sex determination in embryos from single knockout as well as Mmd2;Mmd and Mmd2;Paqr8 double knockout lines using quantitative RT-PCR and immunofluorescence.Analysis of knockout mice deficient in Sox9 and Nr5a1 revealed that Mmd2 operates downstream of these known sex-determining genes. However, fetal testis development progressed normally in Mmd2-null embryos. To determine if other genes might have compensated for the loss of Mmd2, we analyzed Paqr8 and Mmd-null embryos and confirmed that in both knockout lines, sex determination occurred normally. Finally, we generated Mmd2;Mmd and Mmd2;Paqr8 double-null embryos and again observed normal testis development.These results may reflect functional redundancy among PAQR factors, or their dispensability in gonadal development. Our findings highlight the difficulties involved in identifying genes with a functional role in sex determination and gonadal development through expression screening and loss-of-function analyses of individual candidate genes and may help to explain the paucity of genes in which variations have been found to cause human disorders/differences of sex development.

Published

2021

15. Functional analysis of Mmd2 and related PAQR genes during sex determination in mice

Author

Alexander E. Quinn, Ee Ting Ng, Leonard C. Harrison, Thomson E, Vincent R. Harley, Emanuele Pelosi, Enya Longmuss, Liang Zhao, Peter Koopman, Terje Svingen, and Stefan Bagheri-Fam

Subjects

Genetics, Mmd2, Candidate gene, Male sex determination, SOX9, Sex determination, Biology, Sertoli cell, Testis determining factor, medicine.anatomical_structure, CRISPR, Testis, Knockout mouse, medicine, Gene, Paqr8, Mmd

Abstract

Sex determination in eutherian mammals is controlled by the Y-linked gene Sry, which drives the formation of testes in male embryos. Despite extensive study, the genetic steps linking Sry action and male sex determination remain largely unknown. Here, we focused on Mmd2, a gene that encodes a member of the progestin and adipoQ receptor (PAQR) family. We show that Mmd2 is expressed during the sex-determining period in XY but not XX gonads, specifically in the Sertoli cell lineage which orchestrates early testis development. Analysis of knockout mice deficient in Sox9 and Sf1 revealed that Mmd2 operates downstream of these known sex-determining genes. However, when we used CRISPR to ablate Mmd2 in the mouse, fetal testis development appeared to progress normally. To determine if other genes might have compensated for the loss of Mmd2, we identified the closely related PAQR family members Paqr8 and Mmd as also being expressed during testis development. We used CRISPR to generate mouse strains deficient in Paqr8 and Mmd, but both knockout lines appeared phenotypically normal and fertile. Finally, we generated Mmd2;Mmd and Mmd2;Paqr8 double-null embryos and again observed normal testis development. These results may reflect functional redundancy among these factors. Our findings highlight the difficulties involved in identifying genes with a functional role in sex determination and gonadal development through expression screening and loss-of-function analyses of individual candidate genes, and may help to explain the paucity of genes in which variations have been found to cause human disorders/differences of sex development.

Published

2021

16. Heterozygous deletion of Sox9 in mouse mimics the gonadal sex reversal phenotype associated with campomelic dysplasia in humans

Author

Stefan Bagheri-Fam, Alexander N. Combes, Cheuk Kwan Ling, and Dagmar Wilhelm

Subjects

Male, endocrine system, Heterozygote, Sex Differentiation, Disorders of Sex Development, SOX9, Biology, Steroidogenic Factor 1, Andrology, 03 medical and health sciences, Mice, Genetics, medicine, Animals, Humans, Disorders of sex development, Allele, Gonads, Molecular Biology, Genetics (clinical), 030304 developmental biology, Mice, Knockout, 0303 health sciences, Sexual differentiation, 030305 genetics & heredity, Campomelic Dysplasia, Gene Expression Regulation, Developmental, SOX9 Transcription Factor, General Medicine, Sex reversal, medicine.disease, Campomelic dysplasia, Mice, Inbred C57BL, Disease Models, Animal, Phenotype, embryonic structures, Knockout mouse, Female, Haploinsufficiency

Abstract

Heterozygous mutations in the human SOX9 gene cause the skeletal malformation syndrome campomelic dysplasia which in 75% of 46, XY individuals is associated with male-to-female sex reversal. Although studies in homozygous Sox9 knockout mouse models confirmed that SOX9 is critical for testis development, mice heterozygous for the Sox9-null allele were reported to develop normal testes. This led to the belief that the SOX9 dosage requirement for testis differentiation is different between humans, which often require both alleles, and mice, in which one allele is sufficient. However, in prior studies, gonadal phenotypes in heterozygous Sox9 XY mice were assessed only by either gross morphology, histological staining or analyzed on a mixed genetic background. In this study, we conditionally inactivated Sox9 in somatic cells of developing gonads using the Nr5a1-Cre mouse line on a pure C57BL/6 genetic background. Section and whole-mount immunofluorescence for testicular and ovarian markers showed that XY Sox9 heterozygous gonads developed as ovotestes. Quantitative droplet digital PCR confirmed a 50% reduction of Sox9 mRNA as well as partial sex reversal shown by an upregulation of ovarian genes. Our data show that haploinsufficiency of Sox9 can perturb testis development in mice, suggesting that mice may provide a more accurate model of human disorders/differences of sex development than previously thought.

Published

2020

17. Long-range upstream and downstream enhancers control distinct subsets of the complex spatiotemporal Sox9 expression pattern

Author

Stefan Bagheri-Fam, Barrionuevo, Francisco, Dohrmann, Ulrike, Gunther, Thomas, Schule, Roland, Kemler, Rolf, Mallo, Moises, Kanzler, Benoit, and Scherer, Gerd

Subjects

DNA binding proteins -- Research, Gene expression -- Research, Genetically modified mice -- Research, Biological sciences

Abstract

Factors which influence the expression of Sox9, a transcription factor in transgenic mice are studied.

Published

2006

18. Genes and Gene Defects Affecting Gonadal Development and Sex Determination

Author

Stefan Bagheri-Fam and Dagmar Wilhelm

Subjects

0303 health sciences, Male Phenotype, Secondary sex characteristic, 030305 genetics & heredity, Embryogenesis, Biology, medicine.disease, Andrology, 03 medical and health sciences, 5. Gender equality, medicine, Sex organ, Disorders of sex development, Development of the gonads, Gene, 030304 developmental biology, Hormone

Abstract

Sex in mammals is determined genetically with the acquisition of either the XX (female) or XY (male) chromosomes at the time of fertilization. The chromosomal sex will determine if, during embryogenesis, ovaries or testes form from the bipotential gonadal anlage, the genital ridges. Hormones produced by testes and ovaries will then drive most, if not all, secondary sexual characteristics, resulting in the female or male phenotype. Each of these sequential steps is promoted by specific genes and mutations in these genes can lead to disorders of sex development (DSDs).

Published

2019

19. SOX9 regulates expression of the male fertility gene Ets variant factor 5 ( ETV5 ) during mammalian sex development

Author

R. Lavery, Sabine Kelly, Louisa Mabel Ludbrook, Terje Svingen, Peter Koopman, Vincent R. Harley, Dimuthu Alankarage, and Stefan Bagheri-Fam

Subjects

Male, 0301 basic medicine, endocrine system, Cell type, animal structures, Somatic cell, SOX9, Biology, Biochemistry, ETV1, Cell Line, Gene Knockout Techniques, Mice, 03 medical and health sciences, stomatognathic system, FGF9, medicine, Animals, Sertoli Cells, Gene Expression Regulation, Developmental, SOX9 Transcription Factor, Cell Biology, Sex reversal, musculoskeletal system, Sertoli cell, Molecular biology, Up-Regulation, DNA-Binding Proteins, Fertility, 030104 developmental biology, Testis determining factor, medicine.anatomical_structure, embryonic structures, Transcription Factors

Abstract

In humans, dysregulation of the sex determining gene SRY-box 9 (SOX9) leads to disorders of sex development (DSD). In mice, knock-out of Sox9 prior to sex determination leads to XY sex reversal, while Sox9 inactivation after sex determination leads to spermatogenesis defects. SOX9 specifies the differentiation and function of Sertoli cells from somatic cell precursors, which then orchestrate the development and maintenance of other testicular cell types, largely through unknown mechanisms. Here, we describe a novel testicular target gene of SOX9, Ets variant factor 5 (ETV5), a transcription factor responsible for maintaining the spermatogonial stem cell niche. Etv5 was highly expressed in wild-type XY but not XX mouse fetal gonads, with ETV5 protein localized in the Sertoli cells, interstitial cells and germ cells of the testis. In XY Sox9 knock-out gonads, Etv5 expression was strongly down-regulated. Similarly, knock-down of SOX9 in the human Sertoli-like cell line NT2/D1 caused a decrease in ETV5 gene expression. Transcriptomic analysis of NT2/D1 cells over-expressing SOX9 showed that ETV5 expression was increased in response to SOX9. Moreover, chromatin immunoprecipitation of these cells, as well as of embryonic mouse gonads, showed direct binding of SOX9 to ETV5 regulatory regions. We demonstrate that SOX9 was able to activate ETV5 expression via a conserved SOX site in the 5' regulatory region, mutation of which led to loss of activation. In conclusion, we present a novel target gene of SOX9 in the testis, and suggest that SOX9 regulation of ETV5 contributes to the control of male fertility.

Published

2016

20. The gene encoding the ketogenic enzyme HMGCS2 displays a unique expression during gonad development in mice

Author

Beatriz Puisac, Alina Warenik-Szymankiewicz, Stefania Gimelli, Dagmar Wilhelm, Sean M. Wilson, Juan Pié, Serge Nef, Paul Q. Thomas, Katie L. Ayers, Anna Spik, Pierre Calvel, Kamila Kusz-Zamelczyk, Stefan Bagheri-Fam, Frédérique Sloan-Béna, Sultana M.H. Faradz, Huijun Chen, Jadwiga Jaruzelska, Gorjana Robevska, James N. Hughes, Andrew H. Sinclair, University of Melbourne, University of Queensland [Brisbane], Murdoch Children’s Research Institute [Melbourne, Australia], University of Adelaide, Geneva University Hospital (HUG), University of Geneva [Switzerland], Génétique Animale et Biologie Intégrative (GABI), Université Paris-Saclay-AgroParisTech-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), University of Zaragoza - Universidad de Zaragoza [Zaragoza], ISS Aragon, Polish Academy of Sciences (PAN), Geneva University Hospitals and Geneva University, Poznan University of Medical Sciences [Poland] (PUMS), Universitas Diponegoro, Australian Research Council FT110100327, Australian Research Council DP170100045, National Health & Medical Research Council program grant APP1074258, Riset Unggulan Univeritas Diponegoro [PNBP] 316-01/UN7.5.1/PG/2015, Swiss National Science Foundation (SNSF) European Commission IZ73Z0_152347/1, Gobierno de Aragon B32_17R, and European Social Fund (ESF) European Commission

Subjects

Hydroxymethylglutaryl-CoA Synthase, Male, Embryology, [SDV]Life Sciences [q-bio], Disorders of Sex Development, Gene Expression, Gonadal dysgenesis, Gonadal Dysgenesis, medicine.disease_cause, Epithelium, Mice, Animal Cells, Testis, Medicine and Health Sciences, ddc:576.5, Testes, Disorders of sex development, Regulation of gene expression, Genetics, 0303 health sciences, Mutation, Multidisciplinary, 030305 genetics & heredity, Gene Expression Regulation, Developmental, Cell Differentiation, Ovaries, Testis determining factor, Medicine, Female, Anatomy, Cellular Types, Gonadal Dysgenesis/genetics/pathology, Genital Anatomy, Research Article, Heterozygote, endocrine system, Adolescent, Science, Mutation, Missense, Missense/genetics, Testis/growth & development/pathology, SOX9, Biology, Ovary/growth & development/pathology, 03 medical and health sciences, Disorders of Sex Development/genetics/pathology, medicine, Animals, Humans, Gonads, Gene, 030304 developmental biology, [SDV.GEN]Life Sciences [q-bio]/Genetics, Sertoli Cells, Hydroxymethylglutaryl-CoA Synthase/genetics, Ovary, Embryos, Reproductive System, Biology and Life Sciences, Epithelial Cells, Cell Biology, medicine.disease, Sex-Determining Region Y Protein, Campomelic dysplasia, Biological Tissue, Germ Cells, Developmental/genetics, Gene Expression Regulation, Sex-Determining Region Y Protein/genetics, Gonads/growth & development/pathology, Sertoli Cells/metabolism, Developmental Biology

Abstract

International audience; Disorders/differences of sex development (DSD) cause profound psychological and reproductive consequences for the affected individuals, however, most are still unexplained at the molecular level. Here, we present a novel gene, 3-hydroxy-3-methylglutaryl coenzyme A synthase 2 (HMGCS2), encoding a metabolic enzyme in the liver important for energy production from fatty acids, that shows an unusual expression pattern in developing fetal mouse gonads. Shortly after gonadal sex determination it is up-regulated in the developing testes following a very similar spatial and temporal pattern as the male-determining gene Sry in Sertoli cells before switching to ovarian enriched expression. To test if Hmgcs2 is important for gonad development in mammals, we pursued two lines of investigations. Firstly, we generated Hmgcs2-null mice using CRISPR/Cas9 and found that these mice had gonads that developed normally even on a sensitized background. Secondly, we screened 46,XY DSD patients with gonadal dysgenesis and identified two unrelated patients with a deletion and a deleterious missense variant in HMGCS2 respectively. However, both variants were heterozygous, suggesting that HMGCS2 might not be the causative gene. Analysis of a larger number of patients in the future might shed more light into the possible association of HMGCS2 with human gonadal development.

Published

2020

21. Dynamic expression patterns of Irx3 and Irx5 during germline nest breakdown and primordial follicle formation promote follicle survival in mouse ovaries

Author

Stefan Bagheri-Fam, Kathleen J. Krentz, Dagmar Wilhelm, Chi-chung Hui, Claire Holdreith, Valeria L. Caceres, Anqi Fu, Steven V. John, Xiaoyun Zhang, Joan S. Jorgensen, Raphael H. Rastetter, Sarah A. Shaw, and Sydney M. Oberholtzer

Subjects

0301 basic medicine, Cancer Research, Embryology, Immunofluorescence, Cell Communication, QH426-470, Germline, Connexins, Epithelium, Basement Membrane, Mice, Animal Cells, Medicine and Health Sciences, Genetics (clinical), education.field_of_study, Gene Expression Regulation, Developmental, Animal Models, Cell biology, Extracellular Matrix, Ovaries, medicine.anatomical_structure, Experimental Organism Systems, OVA, Female, Folliculogenesis, Cellular Types, Anatomy, Cellular Structures and Organelles, Research Article, Cell Physiology, Granulosa cell, Population, Mice, Nude, Ovary, Mouse Models, Biology, Research and Analysis Methods, 03 medical and health sciences, Follicle, Model Organisms, Genetics, medicine, Animals, education, Immunoassays, Molecular Biology, Ecology, Evolution, Behavior and Systematics, Homeodomain Proteins, Granulosa Cells, Bone morphogenetic protein 15, Embryos, Reproductive System, Biology and Life Sciences, Epithelial Cells, Cell Biology, Oocyte, 030104 developmental biology, Germ Cells, Biological Tissue, Oocytes, Immunologic Techniques, Lutein Cells, Transcription Factors, Developmental Biology

Abstract

Women and other mammalian females are born with a finite supply of oocytes that determine their reproductive lifespan. During fetal development, individual oocytes are enclosed by a protective layer of granulosa cells to form primordial follicles that will grow, mature, and eventually release the oocyte for potential fertilization. Despite the knowledge that follicles are dysfunctional and will die without granulosa cell-oocyte interactions, the mechanisms by which these cells establish communication is unknown. We previously identified that two members of the Iroquois homeobox transcription factor gene family, Irx3 and Irx5, are expressed within developing ovaries but not testes. Deletion of both factors (Irx3-Irx5EGFP/Irx3-Irx5EGFP) disrupted granulosa cell-oocyte contact during early follicle development leading to oocyte death. Thus, we hypothesized that Irx3 and Irx5 are required to develop cell-cell communication networks to maintain follicle integrity and female fertility. A series of Irx3 and Irx5 mutant mouse models were generated to assess roles for each factor. While both Irx3 and Irx5 single mutant females were subfertile, their breeding outcomes and ovary histology indicated distinct causes. Careful analysis of Irx3- and Irx5-reporter mice linked the cause of this disparity to dynamic spatio-temporal changes in their expression patterns. Both factors marked the progenitor pre-granulosa cell population in fetal ovaries. At the critical phase of germline nest breakdown and primordial follicle formation however, Irx3 and Irx5 transitioned to oocyte- and granulosa cell-specific expression respectively. Further investigation into the cause of follicle death in Irx3-Irx5EGFP/Irx3-Irx5EGFP ovaries uncovered specific defects in both granulosa cells and oocytes. Granulosa cell defects included poor contributions to basement membrane deposition and mis-localization of gap junction proteins. Granulosa cells and oocytes both presented fewer cell projections resulting in compromised cell-cell communication. Altogether, we conclude that Irx3 and Irx5 first work together to define the pregranulosa cell population of germline nests. During primordial follicle formation, they transition to oocyte- and granulosa cell-specific expression patterns where they cooperate in neighboring cells to build the foundation for follicle integrity. This foundation is left as their legacy of the essential oocyte-granulosa cell communication network that ensures and ultimately optimizes the integrity of the ovarian reserve and therefore, the female reproductive lifespan., Author summary Fertility is a concern in women’s health, especially when the reported average age of mothers is rising (2016, CDC DB232). Of concern in aging mothers is ovarian follicle health, which requires active communication between its cell components that include a single egg and its surrounding granulosa support cells. The process used to establish cell-cell communication within follicles is unknown but begins during fetal development. We discovered that two related genes, Irx3 and Irx5, direct network construction. If Irx3 and Irx5 are eliminated in mice, oocyte-granulosa cell contact is lost, and all follicles die within short order. Analysis of additional Irx3 and Irx5 mutant mice highlighted that each factor is important for establishing follicle integrity. During fetal development, they work together in the same cell to establish the identity of future granulosa support cells. Then, as the follicles form, they continue to work cooperatively, but in different cells. While Irx5 expression remains in granulosa cells, Irx3 expression transitions to the oocyte and together, they promote cell patterns and interacting zones to synchronize the follicle as an interactive unit. Although the work of Irx3 and Irx5 is finished in the perinatal ovary, their impact lasts a lifetime as it establishes long-term follicle integrity and therefore, fertility.

Published

2018

22. Testis Determination Requires a Specific FGFR2 Isoform to Repress FOXL2

Author

Veraragavan P. Eswarakumar, Stefan Bagheri-Fam, Dagmar Wilhelm, Vincent R. Harley, Meiyun Yong, Peter Koopman, Anthony Daniel Bird, Janelle Ryan, and Liang Zhao

Subjects

Forkhead Box Protein L2, 0301 basic medicine, Male, medicine.medical_specialty, endocrine system, Gonad, Female sex determination, Male sex determination, Down-Regulation, Embryonic Development, Mice, Transgenic, Biology, Mice, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, Wnt4 Protein, Internal medicine, Testis, WNT4, medicine, Animals, Protein Isoforms, Humans, Receptor, Fibroblast Growth Factor, Type 2, Research Articles, Ovary, Wnt signaling pathway, Gene Expression Regulation, Developmental, Sex Determination Processes, Sex reversal, Embryo, Mammalian, Spermatozoa, Cell biology, Mice, Inbred C57BL, 030104 developmental biology, Forkhead box L2, medicine.anatomical_structure, Testis determining factor, embryonic structures, Female, 030217 neurology & neurosurgery

Abstract

Male sex determination in mammals relies on sex determining region Y-mediated upregulation of sex determining region-box 9 (SOX9) expression in XY gonads, whereas Wnt family member (WNT)/R-spondin 1 signaling and forkhead box L2 (FOXL2) drive female sex determination in XX gonads. Fibroblast growth factor (FGF) 9 signaling ensures sustained SOX9 expression through repression of one of the ovarian pathways (WNT signaling), whereas the significance of FGF-mediated repression of the FOXL2 pathway has not been studied. Previously, we demonstrated that FGFR2 is the receptor for FGF9 in the XY gonad. Whether a specific isoform (FGFR2b or FGFR2c) is required was puzzling. Here, we show that FGFR2c is required for male sex determination. Initially, in developing mouse embryos at 12.5 to 13.5 days postcoitum (dpc), XY Fgfr2c-/- gonads appear as ovotestes, with SOX9 and FOXL2 expression predominantly localized to the posterior and anterior gonadal poles, respectively. However, by 15.5 dpc, XY Fgfr2c-/- gonads show complete male-to-female sex reversal, evident by the lack of SOX9 and ectopic expression of FOXL2 throughout the gonads. Furthermore, ablation of the Foxl2 gene leads to partial or complete rescue of gonadal sex reversal in XY Fgfr2c-/- mice. Together with previous findings, our data suggest that testis determination involves FGFR2c-mediated repression of both the WNT4- and FOXL2-driven ovarian-determining pathways.

Published

2017

23. Male Sexual Differentiation

Author

Catherine H. Sterling, Dagmar Wilhelm, and Stefan Bagheri-Fam

Subjects

Sexual differentiation, Physiology, Biology

Published

2017

24. Altered SOX9 genital tubercle enhancer region in hypospadias

Author

Sabina Benko, Robb U. de Iongh, Christopher T. Gordon, Rajini Sreenivasan, Stanislas Lyonnet, Stefan Bagheri-Fam, and Vincent R. Harley

Subjects

0301 basic medicine, Male, endocrine system, medicine.medical_specialty, Genotype, Endocrinology, Diabetes and Metabolism, Clinical Biochemistry, Preputial gland, Clitoris, Mice, Transgenic, SOX9, Biology, Regulatory Sequences, Nucleic Acid, Biochemistry, Cell Line, 03 medical and health sciences, Mice, Endocrinology, Internal medicine, medicine, Animals, Humans, Disorders of sex development, Genital tubercle, Enhancer, Molecular Biology, Mice, Knockout, Hypospadias, SOX9 Transcription Factor, Cell Biology, Genitalia, Female, medicine.disease, Campomelic dysplasia, Mice, Inbred C57BL, 030104 developmental biology, medicine.anatomical_structure, embryonic structures, Mutation, Molecular Medicine, Female

Abstract

Human mutations in the SOX9 gene or its regulatory region can disrupt testicular development, leading to disorders of sex development (DSDs). Our previous work involving the genomic analysis of isolated DSD patients revealed a 78kb minimal sex determining region (RevSex) far upstream of SOX9 that was duplicated in 46,XX and deleted in 46,XY DSDs. It was postulated that RevSex contains a gonadal enhancer. However, the most highly conserved sub-region within RevSex, called SR4, was neither responsive to sex determining factors in vitro nor active in the gonads of transgenic mice, suggesting that SR4 may not be functioning as a testicular enhancer. Interestingly, SR4 transgenic mice showed reporter activity in the genital tubercle, the primordium of the penis and clitoris, a previously unreported domain of Sox9 expression. SOX9 protein was detected in the genital tubercle, notably in the urethral plate epithelium, preputial glands, ventral surface ectoderm and corpus cavernosa. SR4 may therefore function as a Sox9 genital tubercle enhancer, mutations of which could possibly lead to hypospadias, a birth defect seen in the DSD patients in the RevSex study. SR4 activity and the observed SOX9 expression pattern suggest that SR4 may function as a Sox9 genital tubercle enhancer. However, conditional ablation of Sox9 in the genital tubercle using Shh-Cre/+;Sox9flox/flox mice revealed no genital tubercle abnormalities, possibly due to compensation by similar Sox factors. To conclude, we have identified a novel regulatory enhancer driving Sox9 expression during external genitalia development.

Published

2016

25. Sox9 gene regulation and the loss of the XY/XX sex-determining mechanism in the mole vole Ellobius lutescens

Author

Rajini Sreenivasan, Pascal Bernard, Ryohei Sekido, Kevin Christopher Knower, Stefan Bagheri-Fam, Walter Just, Vincent R. Harley, and Robin Lovell-Badge

Subjects

Male, endocrine system, Gonad, Genetic Vectors, Molecular Sequence Data, Y chromosome, Conserved sequence, Evolution, Molecular, Mice, Y Chromosome, Testis, Genetics, medicine, Animals, Humans, Cloning, Molecular, Enhancer, Conserved Sequence, Sequence Deletion, Regulation of gene expression, Binding Sites, Base Sequence, Models, Genetic, biology, Arvicolinae, Genetic Variation, SOX9 Transcription Factor, Sequence Analysis, DNA, Sex Determination Processes, biology.organism_classification, Ellobius, HEK293 Cells, Testis determining factor, medicine.anatomical_structure, Gene Expression Regulation, Mutagenesis, Site-Directed, Ellobius tancrei, Female, Sequence Alignment

Abstract

In most mammals, the Y chromosomal Sry gene initiates testis formation within the bipotential gonad, resulting in male development. SRY is a transcription factor and together with SF1 it directly up-regulates the expression of the pivotal sex-determining gene Sox9 via a 1.3-kb cis-regulatory element (TESCO) which contains an evolutionarily conserved region (ECR) of 180 bp. Remarkably, several rodent species appear to determine sex in the absence of Sry and a Y chromosome, including the mole voles Ellobius lutescens and Ellobius tancrei, whereas Ellobius fuscocapillus of the same genus retained Sry. The sex-determining mechanisms in the Sry-negative species remain elusive. We have cloned and sequenced 1.1 kb of E. lutescens TESCO which shares 75% sequence identity with mouse TESCO indicating that testicular Sox9 expression in E. lutescens might still be regulated via TESCO. We have also cloned and sequenced the ECRs of E. tancrei and E. fuscocapillus. While the three Ellobius ECRs are highly similar (94-97% sequence identity), they all display a 14-bp deletion (Δ14) removing a highly conserved SOX/TCF site. Introducing Δ14 into mouse TESCO increased both basal activity and SF1-mediated activation of TESCO in HEK293T cells. We propose a model whereby Δ14 may have triggered up-regulation of Sox9 in XX gonads leading to destabilization of the XY/XX sex-determining mechanism in Ellobius. E. lutescens/E. tancrei and E. fuscocapillus could have independently stabilized their sex determination mechanisms by Sry-independent and Sry-dependent approaches, respectively.

Published

2012

26. Abstracts: Poster Presentations

Author

Daniel Peter Czech, Stefan Bagheri-Fam, Andrew H. Sinclair, Francis Poulet, Peter Koopman, Brigitte Boizet-Bonhoure, Vincent R. Harley, Anthony Argentaro, and Helena Sim

Subjects

0303 health sciences, Calmodulin, biology, Chemistry, Complex formation, Medicine (miscellaneous), 030209 endocrinology & metabolism, Cell biology, 03 medical and health sciences, 0302 clinical medicine, Testis determining factor, biology.protein, Ovarian cell, Ectopic expression, 030304 developmental biology

Published

2011

27. Antagonistic regulation ofCyp26b1by transcription factors SOX9/SF1 and FOXL2 during gonadal development in mice

Author

Terje Svingen, Josephine Bowles, Emanuele Pelosi, David Schlessinger, Kenichi Kashimada, Stefan Bagheri-Fam, Chun-Wei Feng, Peter Koopman, and Vincent R. Harley

Subjects

Forkhead Box Protein L2, Male, Steroidogenic factor 1, endocrine system, medicine.medical_specialty, SOX9, Biology, Biochemistry, Research Communications, Mice, Cytochrome P-450 Enzyme System, Internal medicine, Testis, Gene expression, Genetics, medicine, Animals, Molecular Biology, Regulation of gene expression, Gene Expression Regulation, Developmental, Forkhead Transcription Factors, SOX9 Transcription Factor, Retinoic Acid 4-Hydroxylase, Sex Determination Processes, Up-Regulation, Cell biology, DNA-Binding Proteins, Forkhead box L2, medicine.anatomical_structure, Endocrinology, RNA Splicing Factors, Germ line development, Transcription Factor Gene, Germ cell, Transcription Factors, Biotechnology

Abstract

Sex determination in fetal germ cells depends on a balance between exposure to retinoic acid (RA) and the degradation of RA achieved by the testis-specific expression of the catabolic cytochrome P450 enzyme, CYP26B1. Therefore, identification of factors regulating the expression of the Cyp26b1 gene is an important goal in reproductive biology. We used in situ hybridization to demonstrate that Cyp26b1 and transcription factor genes steroidogenic factor-1 (Sf1) and Sry-related HMG box 9 (Sox9) are coexpressed in Sertoli cells, whereas Cyp26b1 and Sf1 are coexpressed in Leydig cells in mouse fetal testes. In the mouse gonadal somatic cell line TM3, transfection of constructs expressing SOX9 and SF1 activated Cyp26b1 expression, independently of the positive regulator RA. In embryonic gonads deficient in SOX9 or SF1, Cyp26b1 expression was decreased relative to wild-type (WT) controls, as measured by quantitative RT-PCR (qRT-PCR). Furthermore, qRT-PCR showed that Cyp26b1 up-regulation by SOX9/SF1 was attenuated by the ovarian transcription factor Forkhead box L2 (FOXL2) in TM3 cells, whereas in Foxl2-null mice, Cyp26b1 expression in XX gonads was increased ∼20-fold relative to WT controls. These data support the hypothesis that SOX9 and SF1 ensure the male fate of germ cells by up-regulating Cyp26b1 and that FOXL2 acts to antagonize Cyp26b1 expression in ovaries.—Kashimada, K., Svingen, T., Feng, C.-W., Pelosi, E., Bagheri-Fam, S., Harley, V. R., Schlessinger, D., Bowles, J., Koopman, P. Antagonistic regulation of Cyp26b1 by transcription factors SOX9/SF1 and FOXL2 during gonadal development in mice.

Published

2011

28. Protein tyrosine kinase 2 beta (PTK2B), but not focal adhesion kinase (FAK), is expressed in a sexually dimorphic pattern in developing mouse gonads

Author

Peter J. McClive, Terje Svingen, Annemiek Beverdam, Andrew H. Sinclair, Stefan Bagheri-Fam, Vincent R. Harley, and Peter Koopman

Subjects

Male, Cell signaling, Sex Differentiation, PTK2, Biology, Focal adhesion, Mice, Testis, Animals, Gonads, In Situ Hybridization, Sertoli Cells, PTK2B, Reverse Transcriptase Polymerase Chain Reaction, Days post coitum, SOX9 Transcription Factor, Immunohistochemistry, Molecular biology, Cell biology, Intracellular signal transduction, Focal Adhesion Kinase 2, Focal Adhesion Kinase 1, Female, Tyrosine kinase, Developmental Biology, Proto-oncogene tyrosine-protein kinase Src

Abstract

Sexual reproduction is essential for the propagation and the maintenance of fitness of our species, and is dependent on the correct development of the bipotential genital ridges into testes and ovaries. Although several transcription factors, secreted signaling molecules, and their receptors have been found to be important for testis determination and early gonad development, comparatively little research has been carried out into intracellular signal transduction pathways activated during these processes. Focal adhesion kinase (FAK) and protein tyrosine kinase 2 beta (PTK2B) form one group of cytosolic tyrosine kinases that are known to be important for processes such as cell proliferation, differentiation, and motility. Here, we describe the temporal and spatial expression patterns of Fak and Ptk2b mRNA and protein during sex determination and early gonadogenesis in mouse embryos. Ptk2b mRNA and PTK2B protein were expressed in testes from 11.5 days post coitum onward, predominantly in developing Sertoli cells, in a SOX9-dependent manner. Fak mRNA and FAK protein were expressed in gonads of both sexes at all stages examined. Our data suggest cell type- and stage-specific roles for PTK2B during early testis development. Developmental Dynamics 239:2735–2741, 2010. © 2010 Wiley-Liss, Inc.

Published

2010

29. Conserved regulatory modules in the Sox9 testis-specific enhancer predict roles for SOX, TCF/LEF, Forkhead, DMRT, and GATA proteins in vertebrate sex determination

Author

Andrew H. Sinclair, Vincent R. Harley, Stefan Bagheri-Fam, and Peter Koopman

Subjects

Male, endocrine system, animal structures, Oryzias, Molecular Sequence Data, Biology, Biochemistry, Conserved sequence, Evolution, Molecular, Mice, stomatognathic system, Sequence Homology, Nucleic Acid, biology.animal, Testis, Animals, Enhancer, Gene, Conserved Sequence, Phylogeny, Genetics, Comparative genomics, Binding Sites, Genome, Base Sequence, Vertebrate, SOX9 Transcription Factor, Sequence Analysis, DNA, Cell Biology, Sex Determination Processes, biology.organism_classification, Enhancer Elements, Genetic, Testis determining factor, Organ Specificity, Regulatory sequence, Vertebrates, embryonic structures, Sequence Alignment, Transcription Factors

Abstract

While the primary sex determining switch varies between vertebrate species, a key downstream event in testicular development, namely the male-specific up-regulation of Sox9, is conserved. To date, only two sex determining switch genes have been identified, Sry in mammals and the Dmrt1-related gene Dmy (Dmrt1bY) in the medaka fish Oryzias latipes. In mice, Sox9 expression is evidently up-regulated by SRY and maintained by SOX9 both of which directly activate the core 1.3 kb testis-specific enhancer of Sox9 (TESCO). How Sox9 expression is up-regulated and maintained in species without Sry (i.e. non-mammalian species) is not understood. In this study, we have undertaken an in-depth comparative genomics approach and show that TESCO contains an evolutionarily conserved region (ECR) of 180 bp which is present in marsupials, monotremes, birds, reptiles and amphibians. The ECR contains highly conserved modules that predict regulatory roles for SOX, TCF/LEF, Forkhead, DMRT, and GATA proteins in vertebrate sex determination/differentiation. Our data suggest that tetrapods share common aspects of Sox9 regulation in the testis, despite having different sex determining switch mechanisms. They also suggest that Sox9 autoregulation is an ancient mechanism shared by all tetrapods, raising the possibility that in mammals, SRY evolved by mimicking this regulation. The validation of ECR regulatory sequences conserved from human to frogs will provide new insights into vertebrate sex determination.

Published

2010

30. Mutations of the SRY-Responsive Enhancer of SOX9 Are Uncommon in XY Gonadal Dysgenesis

Author

Ina Georg, Kevin Christopher Knower, Gerd Scherer, Vincent R. Harley, Stefan Bagheri-Fam, and Peter Wieacker

Subjects

Genetics, Embryology, Mutation, Endocrinology, Diabetes and Metabolism, Point mutation, Gonadal dysgenesis, SOX9, Sex reversal, Biology, medicine.disease_cause, medicine.disease, XY gonadal dysgenesis, Campomelic dysplasia, Testis determining factor, medicine, Developmental Biology

Abstract

During mouse sex determination, SRY upregulates the core testis-specific enhancer of Sox9, TESCO. Mutations in human SRY are found in one third of cases with XY pure gonadal dysgenesis (XY GD; Swyer syndrome), while two thirds remain unexplained. Heterozygous SOX9 mutations can cause XY GD in association with the skeletal malformation syndrome campomelic dysplasia. We hypothesized that human TESCO mutations could cause isolated XY GD. Sixty-six XY GD cases with an intact SRY were analyzed for TESCO point mutations or deletions. No mutations were identified. We conclude that TESCO mutations are not a common cause of XY GD.

Published

2010

31. Male-specific expression ofAldh1a1in mouse and chicken fetal testes: Implications for retinoid balance in gonad development

Author

Peter Koopman, Craig A. Smith, Vincent R. Harley, Josephine Bowles, Stefan Bagheri-Fam, D. Knight, Kelly N. Roeszler, Andrew H. Sinclair, and Chun-Wei Feng

Subjects

Male, medicine.medical_specialty, Sex Differentiation, medicine.drug_class, Somatic cell, Retinoic acid, Mice, Transgenic, Tretinoin, Chick Embryo, SOX9, Biology, Aldehyde Dehydrogenase 1 Family, Mice, Retinoids, chemistry.chemical_compound, Pregnancy, Internal medicine, Testis, Gene expression, medicine, Animals, Retinoid, Genes, sry, DNA Primers, Base Sequence, Gene Expression Regulation, Developmental, Retinal Dehydrogenase, SOX9 Transcription Factor, Aldehyde Dehydrogenase, Cell biology, Isoenzymes, ALDH1A1, Endocrinology, Testis determining factor, chemistry, biology.protein, Female, Development of the gonads, Developmental Biology

Abstract

Balanced production and degradation of retinoids is important in regulating development of several organ systems in the vertebrate embryo. Among these, it is known that retinoic acid (RA), and the retinoid-catabolyzing enzyme CYP26B1 together regulate the sex-specific behavior of germ cells in developing mouse gonads. We report here that the gene encoding a cytosolic class-1 aldehyde dehydrogenase, ALDH1A1, a weak catalyst of RA production, is strongly expressed in a male-specific manner in somatic cells of the developing mouse testis, beginning shortly after Sry expression is first detectable. This expression pattern is conserved in the developing male gonad of the chicken and is dependent on the testis-specific transcription factor SOX9. Our data suggest that low levels of RA may be required for early developmental events in the testis, or that Aldh1a1 expression in the fetus may prefigure a later requirement for ALDH1A1 in regulating spermatogenesis postnatally. Developmental Dynamics 238:2073-2080, 2009. (C) 2009 Wiley-Liss, Inc.

Published

2009

32. Sox9-dependent expression of Gstm6 in Sertoli cells during testis development in mice

Author

Mathew Robson, Stefan Bagheri-Fam, Mahdi Banan Khojasteh, Peter J. McClive, Pascal Bernard, Andrew H. Sinclair, Terje Svingen, Mahboubeh Salehi, Annemiek Beverdam, Peter Koopman, and Vincent R. Harley

Subjects

Male, Genetically modified mouse, endocrine system, Embryology, Somatic cell, Mice, Transgenic, SOX9, Biology, Mice, Endocrinology, Testis, medicine, Animals, Reproductive system, In Situ Hybridization, Glutathione Transferase, Regulation of gene expression, Sertoli Cells, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, Ovary, Gene Expression Regulation, Developmental, Obstetrics and Gynecology, SOX9 Transcription Factor, Cell Biology, Sertoli cell, Molecular biology, Cell biology, Mice, Inbred C57BL, Testis determining factor, medicine.anatomical_structure, Reproductive Medicine, Female, Development of the gonads

Abstract

GlutathioneS-transferases (GSTs) are an important family of multifunctional enzymes that play a role in the protection of tissues by the detoxification of hazardous and carcinogenic compounds. We found previously thatGstm6is upregulated in the somatic cells of male mouse fetal gonads relative to female gonads. In this study, we describe the spatial and temporal expression pattern ofGstm6during mouse development. We show thatGstm6is predominantly expressed in the reproductive system, at significantly higher levels in XY gonads compared with XX gonads from 11.5 dpc onwards, and remains expressed in the testes in adult mice. Its expression is associated with the Sertoli cell lineage, and is dependent on the expression of the male sex-determining geneSox9. Our data suggest thatGstm6plays a male-specific role in gonad development or function, possibly by modulating the exposure of somatic tissue and/or germ cells to endogenous or exogenous toxicants.

Published

2009

33. Loss of Fgfr2 leads to partial XY sex reversal

Author

Irumini Uthpala Anushini Jayakody, Stefan Bagheri-Fam, Vincent R. Harley, Helena Sim, Pascal Bernard, Makoto Mark Taketo, and Gerd Scherer

Subjects

Male, Male sex determination, Disorders of Sex Development, XY sex reversal, FGF9, Mice, 0302 clinical medicine, Testis, Disorders of sex development, Mice, Knockout, 0303 health sciences, High Mobility Group Proteins, SOX9 Transcription Factor, Sex reversal, Coelomic epithelium, Cell biology, Testis determining factor, medicine.anatomical_structure, embryonic structures, PGDS, Female, SOX9, Fibroblast Growth Factor 9, Disorders of sexual development, endocrine system, medicine.medical_specialty, Gonad, Biology, 03 medical and health sciences, Internal medicine, medicine, Animals, Receptor, Fibroblast Growth Factor, Type 2, Gonads, Molecular Biology, 030304 developmental biology, Sertoli Cells, Ovotestis, Cell Biology, Sex determination, Sex Determination Processes, medicine.disease, stomatognathic diseases, Endocrinology, FGFR2, FGF signalling, 030217 neurology & neurosurgery, Transcription Factors, Developmental Biology

Abstract

In mammals, sex is determined in the bipotential embryonic gonad by a balanced network of gene actions which when altered causes disorders of sexual development (DSD, formerly known as intersex). In the XY gonad, presumptive Sertoli cells begin to differentiate when SRY up-regulates SOX9, which in turn activates FGF9 and PGDS to maintain its own expression. This study identifies a new and essential component of FGF signaling in sex determination. Fgfr2 mutant XY mice on a mixed 129/C57BL6 genetic background had either normal testes, or developed ovotestes, with predominantly testicular tissue. However, backcrossing to C57BL6 mice resulted in a wide range of gonadal phenotypes, from hypoplastic testes to ovotestes with predominantly ovarian tissue, similar to Fgf9 knockout mice. Since typical male-specific FGF9-binding to the coelomic epithelium was abolished in Fgfr2 mutant XY gonads, these results suggest that FGFR2 acts as the receptor for FGF9. Pgds and SOX9 remained expressed within the testicular portions of Fgfr2 mutant ovotestes, suggesting that the Prostaglandin pathway acts independently of FGFR2 to maintain SOX9 expression. We could further demonstrate that double-heterozygous Fgfr2/Sox9 knockout mice developed ovotestes, demonstrating that both Fgfr2 and Sox9 can act as modifier intersex genes in the heterozygous state. In summary, we provide evidence that FGFR2 is important for male sex determination in mice, thereby rendering human FGFR2 a candidate gene for unsolved DSD cases such as 10q26 deletions.

Published

2008

34. Homozygous Inactivation of Sox9 Causes Complete XY Sex Reversal in Mice1

Author

Francisco J. Barrionuevo, Christoph Englert, Makoto Mark Taketo, Gerd Scherer, Stefan Bagheri-Fam, Ralf Kist, and Jürgen Klattig

Subjects

endocrine system, medicine.medical_specialty, animal structures, Gonad, Cre recombinase, Cell Biology, General Medicine, SOX9, Sex reversal, Biology, Sertoli cell, Cell biology, medicine.anatomical_structure, Endocrinology, Testis determining factor, stomatognathic system, Reproductive Medicine, Internal medicine, embryonic structures, WNT4, Primary sex determination, medicine

Abstract

In the presence of the Y-chromosomal gene Sry, the bipotential mouse gonads develop as testes rather than as ovaries. The autosomal gene Sox9, a likely and possibly direct Sry target, can induce testis development in the absence of Sry. Sox9 is thus sufficient but not necessarily essential for testis induction. Mutational inactivation of one allele of SOX9/Sox9 causes sex reversal in humans but not in mice. Because Sox9 –/– embryos die around Embryonic Day 11.5 (E11.5) at the onset of testicular morphogenesis, differentiation of the mutant XY gonad can be analyzed only ex vivo in organ culture. We have therefore conditionally inactivated both Sox9 alleles in the gonadal anlagen using the CRE/loxP recombination system, whereby CRE recombinase is under control of the cytokeratin 19 promoter. Analysis of resulting Sox9 –/– XY gonads up to E15.5 reveals immediate, complete sex reversal, as shown by expression of the early ovary-specific markers Wnt4 and Foxl2 and by lack of testis cord and Leydig cell formation. Sry expression in mutant XY gonads indicates that downregulation of Wnt4 and Foxl2 is dependent on Sox9 rather than on Sry. Our results provide in vivo proof that, in contrast to the situation in humans, complete XY sex reversal in mice requires inactivation of both Sox9 alleles and that Sox9 is essential for testogenesis in mice. developmental biology, gene regulation, ovary, Sertoli cells, testis

Published

2006

35. Testis determination requires the function of a specific FGFR2 isoform

Author

Daniel Bird, Li Li, Raymond Lai, Vincent R. Harley, Dagmar Wilhelm, Janelle Ryan, Jacob V.P. Eswarakumar, Stefan Bagheri-Fam, and Meiyun Yong

Subjects

Gene isoform, Embryology, Biology, Developmental biology, Function (biology), Developmental Biology, Cell biology

Published

2017

36. Comparative Genomics of the SOX9 Region in Human and Fugu rubripes: Conservation of Short Regulatory Sequence Elements within Large Intergenic Regions

Author

Dietmar Pfeifer, Conchita Ferraz, Stefan Bagheri-Fam, Jacques Demaille, and Gerd Scherer

Subjects

Yeast artificial chromosome, endocrine system, animal structures, 5' Flanking Region, Sequence analysis, Molecular Sequence Data, Regulatory Sequences, Nucleic Acid, Biology, Mice, Intergenic region, stomatognathic system, Sequence Homology, Nucleic Acid, Genetics, Animals, Humans, Amino Acid Sequence, Enhancer, Gene, Conserved Sequence, Comparative genomics, Base Sequence, Sequence Homology, Amino Acid, High Mobility Group Proteins, Chromosome Mapping, SOX9 Transcription Factor, DNA, Genomics, Sequence Analysis, DNA, musculoskeletal system, Takifugu, Chromosome 17 (human), Regulatory sequence, embryonic structures, DNA, Intergenic, Sequence Alignment, Chromosomes, Human, Pair 17, Transcription Factors

Abstract

Campomelic dysplasia (CD), a human skeletal malformation syndrome with XY sex reversal, is caused by heterozygous mutations in and around the gene SOX9. SOX9 has an extended 5' control region, as indicated by CD translocation breakpoints scattered over 1 Mb proximal to SOX9 and by expression data from mice transgenic for human SOX9-spanning yeast artificial chromosomes. To identify long-range regulatory elements within the SOX9 5' control region, we compared approximately 3.7 Mb and 195 kb of sequence around human and Fugu rubripes SOX9, respectively. We identified only seven and five protein-coding genes in the human and F. rubripes sequences, respectively. Four of the F. rubripes genes have been mapped in humans; all reside on chromosome 17 but show extensive intrachromosomal gene shuffling compared with the gene order in F. rubripes. In both species, very large intergenic distances separate SOX9 from its directly flanking genes: 2 Mb and 500 kb on either side of SOX9 in humans, and 68 and 97 kb on either side of SOX9 in F. rubripes. Comparative sequence analysis of the intergenic regions revealed five conserved elements, E1-E5, up to 290 kb 5' to human SOX9 and up to 18 kb 5' to F. rubripes SOX9, and three such elements, E6-E8, 3' to SOX9. Where available, mouse sequences confirm conservation of the elements. From the yeast artificial chromosome transgenic data, elements E3-E5 are candidate enhancers for SOX9 expression in limb and vertebral column, and 8 of 10 CD translocation breakpoints separate these elements from SOX9.

Published

2001

37. SOX9 Regulates MicroRNA miR-202-5p/3p Expression During Mouse Testis Differentiation1

Author

Dagmar Wilhelm, Elanor N. Wainwright, Joan S. Jorgensen, Kathryn S. McClelland, Tara Davidson, Peter Koopman, Selene L. Fernandez-Valverde, Vincent R. Harley, Youngha Kim, Stefan Bagheri-Fam, Ryan J. Taft, Terje Svingen, and Vy Truong

Subjects

Regulation of gene expression, endocrine system, Gonad, Sexual differentiation, urogenital system, Cellular differentiation, Male sex determination, Cell Biology, General Medicine, SOX9, Biology, Molecular biology, medicine.anatomical_structure, Testis determining factor, Reproductive Medicine, medicine, Ectopic expression

Abstract

MicroRNAs are important regulators of developmental gene expression, but their contribution to fetal gonad development is not well understood. We have identified the evolutionarily conserved gonadal microRNAs miR-202-5p and miR-202-3p as having a potential role in regulating mouse embryonic gonad differentiation. These microRNAs are expressed in a sexually dimorphic pattern as the primordial XY gonad differentiates into a testis, with strong expression in Sertoli cells. In vivo, ectopic expression of pri-miR-202 in XX gonads did not result in molecular changes to the ovarian determination pathway. Expression of the primary transcript of miR-202-5p/3p remained low in XY gonads in a conditional Sox9-null mouse model, suggesting that pri-miR-202 transcription is downstream of SOX9, a transcription factor that is both necessary and sufficient for male sex determination. We identified the pri-miR-202 promoter that is sufficient to drive expression in XY but not XX fetal gonads ex vivo. Mutation of SOX9 and SF1 binding sites reduced ex vivo transactivation of the pri-miR-202 promoter, demonstrating that pri-miR-202 may be a direct transcriptional target of SOX9/SF1 during testis differentiation. Our findings indicate that expression of the conserved gonad microRNA, miR-202-5p/3p, is downstream of the testis-determining factor SOX9, suggesting an early role in testis development.

Published

2013

38. SOX9 regulates microRNA miR-202-5p/3p expression during mouse testis differentiation

Author

Elanor N, Wainwright, Joan S, Jorgensen, Youngha, Kim, Vy, Truong, Stefan, Bagheri-Fam, Tara, Davidson, Terje, Svingen, Selene L, Fernandez-Valverde, Kathryn S, McClelland, Ryan J, Taft, Vincent R, Harley, Peter, Koopman, and Dagmar, Wilhelm

Subjects

Male, Mice, Knockout, Sertoli Cells, Sex Differentiation, Transcription, Genetic, Organogenesis, Gene Expression Regulation, Developmental, Cell Differentiation, SOX9 Transcription Factor, Mice, MicroRNAs, Testis, Animals, Promoter Regions, Genetic

Abstract

MicroRNAs are important regulators of developmental gene expression, but their contribution to fetal gonad development is not well understood. We have identified the evolutionarily conserved gonadal microRNAs miR-202-5p and miR-202-3p as having a potential role in regulating mouse embryonic gonad differentiation. These microRNAs are expressed in a sexually dimorphic pattern as the primordial XY gonad differentiates into a testis, with strong expression in Sertoli cells. In vivo, ectopic expression of pri-miR-202 in XX gonads did not result in molecular changes to the ovarian determination pathway. Expression of the primary transcript of miR-202-5p/3p remained low in XY gonads in a conditional Sox9-null mouse model, suggesting that pri-miR-202 transcription is downstream of SOX9, a transcription factor that is both necessary and sufficient for male sex determination. We identified the pri-miR-202 promoter that is sufficient to drive expression in XY but not XX fetal gonads ex vivo. Mutation of SOX9 and SF1 binding sites reduced ex vivo transactivation of the pri-miR-202 promoter, demonstrating that pri-miR-202 may be a direct transcriptional target of SOX9/SF1 during testis differentiation. Our findings indicate that expression of the conserved gonad microRNA, miR-202-5p/3p, is downstream of the testis-determining factor SOX9, suggesting an early role in testis development.

Published

2013

39. Genome-wide ENU mutagenesis in combination with high density SNP analysis and exome sequencing provides rapid identification of novel mouse models of developmental disease

Author

Helen E. Abud, John F. Bertram, Ian M. Smyth, Christopher T. Gordon, Tim J Cole, Adam H. Hart, Megan J. Wallace, Belinda Whittle, Georgina Caruana, Peter G. Farlie, Kerry A. Miller, Vincent R. Harley, Ruth M. Arkell, Stefan Bagheri-Fam, and Michael S. Dobbie

Subjects

Male, Embryology, Genetic Screens, Knowledge management, Anatomy and Physiology, Mouse, Organogenesis, Left-Right Determination Factors, Respiratory System, lcsh:Medicine, Disease, Genome, DNA Ligase ATP, Mice, Phenomics, Exome, lcsh:Science, Exome sequencing, Skin, Extracellular Matrix Proteins, Multidisciplinary, Homozygote, High-Throughput Nucleotide Sequencing, Anemia, Animal Models, Hematology, Developmental Nephrology, Phenotype, Nephrology, Medicine, Female, SNP array, Research Article, DNA Ligases, Genotype, Clinical Research Design, High density, Biology, Polymorphism, Single Nucleotide, Congenital Abnormalities, Model Organisms, Genetic Mutation, Genetics, Animals, Animal Models of Disease, Alleles, Germ-Line Mutation, Government, business.industry, lcsh:R, Reproductive System, Biotechnology, Mice, Inbred C57BL, Disease Models, Animal, Mutagenesis, Ethylnitrosourea, Genetics of Disease, lcsh:Q, business, Organism Development, Developmental Biology, Genome-Wide Association Study, Mutagens

Abstract

Background Mice harbouring gene mutations that cause phenotypic abnormalities during organogenesis are invaluable tools for linking gene function to normal development and human disorders. To generate mouse models harbouring novel alleles that are involved in organogenesis we conducted a phenotype-driven, genome-wide mutagenesis screen in mice using the mutagen N-ethyl-N-nitrosourea (ENU). Methodology/Principal Findings ENU was injected into male C57BL/6 mice and the mutations transmitted through the germ-line. ENU-induced mutations were bred to homozygosity and G3 embryos screened at embryonic day (E) 13.5 and E18.5 for abnormalities in limb and craniofacial structures, skin, blood, vasculature, lungs, gut, kidneys, ureters and gonads. From 52 pedigrees screened 15 were detected with anomalies in one or more of the structures/organs screened. Using single nucleotide polymorphism (SNP)-based linkage analysis in conjunction with candidate gene or next-generation sequencing (NGS) we identified novel recessive alleles for Fras1, Ift140 and Lig1. Conclusions/Significance In this study we have generated mouse models in which the anomalies closely mimic those seen in human disorders. The association between novel mutant alleles and phenotypes will lead to a better understanding of gene function in normal development and establish how their dysfunction causes human anomalies and disease.

Published

2013

40. Excess DAX1 leads to XY ovotesticular disorder of sex development (DSD) in mice by inhibiting steroidogenic factor-1 (SF1) activation of the testis enhancer of SRY-box-9 (Sox9)

Author

Louisa M. Ludbrook, Ryohei Sekido, Robin Lovell-Badge, Pascal Bernard, Vincent R. Harley, Janelle Ryan, Dagmar Wilhelm, and Stefan Bagheri-Fam

Subjects

Steroidogenic factor 1, Male, endocrine system, medicine.medical_specialty, Genotype, Granulosa cell, Disorders of Sex Development, Mice, Transgenic, SOX9, Biology, Gonadal Dysgenesis, Steroidogenic Factor 1, Mice, Endocrinology, Fetus, Internal medicine, Testis, medicine, Animals, Cells, Cultured, DAX-1 Orphan Nuclear Receptor, RNA-Binding Proteins, SOX9 Transcription Factor, Sex reversal, medicine.disease, Sertoli cell, Sex-Determining Region Y Protein, Campomelic dysplasia, DNA-Binding Proteins, Mice, Inbred C57BL, Cytoskeletal Proteins, Testis determining factor, medicine.anatomical_structure, Models, Animal, Female, DAX1

Abstract

Human DAX1 duplications cause dosage-sensitive sex reversal (DSS) whereby chromosomally XY individuals can develop as females due to gonadal dysgenesis. However, the mechanism of DSS-adrenal hypoplasia congenita on X, gene 1 (DAX1) action in the fetal testis is unknown. We show that in fetal testes from XY Dax1-overexpressing transgenic mice, the expression of the key testis-promoting gene sex-determining region on Y (SRY)-box-9 (Sox9) is reduced. Moreover, in XY Sox9 heterozygotes, in which testis development is usually normal, Dax1 overexpression results in ovotestes, suggesting a DAX1-SOX9 antagonism. The ovarian portion of the XY ovotestes was characterized by expression of the granulosa cell marker, Forkhead box-L2, with complete loss of the Sertoli cell markers, SOX9 and anti-Müllerian hormone, and the Leydig cell marker CYP17A1. However, the expression of SRY and steroidogenic factor-1 (SF1), two key transcriptional regulators of Sox9, was retained in the ovarian portion of the XY ovotestes. Using reporter mice, Dax1 overexpression reduced activation of TES, the testis enhancer of Sox9, indicating that DAX1 might repress Sox9 expression via TES. In cultured cells, increasing levels of DAX1 antagonized SF1-, SF1/SRY-, and SF1/SOX9-mediated activation of TES, due to reduced binding of SF1 to TES, providing a likely mechanism for DSS.

Published

2012

41. Defective survival of proliferating Sertoli cells and androgen receptor function in a mouse model of the ATR-X syndrome

Author

Terje Svingen, Andrew H. Sinclair, Peter Koopman, Vincent R. Harley, Alexander N. Combes, Anthony Argentaro, and Stefan Bagheri-Fam

Subjects

Male, X-linked Nuclear Protein, Apoptosis, Testicle, Biology, medicine.disease_cause, Mice, alpha-Thalassemia, Testis, Genetics, medicine, Animals, Immunoprecipitation, Promoter Regions, Genetic, Molecular Biology, Transcription factor, Genetics (clinical), ATRX, Cells, Cultured, Cell Proliferation, Regulation of gene expression, Homeodomain Proteins, Mice, Knockout, Mutation, Sertoli Cells, Cell Cycle, DNA Helicases, Nuclear Proteins, General Medicine, Sequence Analysis, DNA, Cell cycle, Sertoli cell, Chromatin Assembly and Disassembly, Androgen receptor, Mice, Inbred C57BL, Disease Models, Animal, medicine.anatomical_structure, Gene Expression Regulation, Receptors, Androgen, Cancer research, Mental Retardation, X-Linked, Female, Transcription Factors

Abstract

X-linked ATR-X (alpha thalassemia, mental retardation, X-linked) syndrome in males is characterized by mental retardation, facial dysmorphism, alpha thalassemia and urogenital abnormalities, including small testes. It is unclear how mutations in the chromatin-remodeling protein ATRX cause these highly specific clinical features, since ATRX is widely expressed during organ development. To investigate the mechanisms underlying the testicular defects observed in ATR-X syndrome, we generated ScAtrxKO (Sertoli cell Atrx knockout) mice with Atrx specifically inactivated in the supporting cell lineage (Sertoli cells) of the mouse testis. ScAtrxKO mice developed small testes and discontinuous tubules, due to prolonged G2/M phase and apoptosis of proliferating Sertoli cells during fetal life. Apoptosis might be a consequence of the cell cycle defect. We also found that the onset of spermatogenesis was delayed in postnatal mice, with a range of spermatogenesis defects evident in adult ScAtrxKO mice. ATRX and the androgen receptor (AR) physically interact in the testis and in the Sertoli cell line TM4 and co-operatively activate the promoter of Rhox5, an important direct AR target. We also demonstrate that ATRX directly binds to the Rhox5 promoter in TM4 cells. Finally, gene expression of Rhox5 and of another AR-dependent gene, Spinlw1, was reduced in ScAtrxKO testes. These data suggest that ATRX can directly enhance the expression of androgen-dependent genes through physical interaction with AR. Recruitment of ATRX by DNA sequence-specific transcription factors could be a general mechanism by which ATRX achieves tissue-specific transcriptional regulation which could explain the highly specific clinical features of ATR-X syndrome when ATRX is mutated.

Published

2011

42. Inhibition of SRY-Calmodulin Complex Formation Induces Ectopic Expression of Ovarian Cell Markers in Developing XY Gonads

Author

Francis Poulat, Daniel Peter Czech, Peter Koopman, Anthony Argentaro, Andrew H. Sinclair, Vincent R. Harley, Helena Sim, Stefan Bagheri-Fam, Brigitte Boizet-Bonhoure, Institut de génétique humaine (IGH), and Université de Montpellier (UM)-Centre National de la Recherche Scientifique (CNRS)

Subjects

Forkhead Box Protein L2, Male, Mice, 0302 clinical medicine, Endocrinology, Chlorocebus aethiops, Testis, ComputingMilieux_MISCELLANEOUS, Spermatic Cord, 0303 health sciences, Sexual differentiation in humans, Forkhead Transcription Factors, SOX9 Transcription Factor, Recombinant Proteins, Forkhead box L2, medicine.anatomical_structure, Testis determining factor, COS Cells, geographic locations, Transcriptional Activation, endocrine system, medicine.medical_specialty, animal structures, Gonad, Active Transport, Cell Nucleus, SOX9, Biology, Y chromosome, 03 medical and health sciences, Organ Culture Techniques, Calmodulin, Internal medicine, parasitic diseases, medicine, Animals, Spermatogenesis, Transcription factor, 030304 developmental biology, Cell Nucleus, [SDV.GEN]Life Sciences [q-bio]/Genetics, social sciences, Sex Determination Processes, Embryo, Mammalian, Antigens, Differentiation, Sex-Determining Region Y Protein, Calmodulin-Binding Proteins, Ectopic expression, Thrombospondins, 030217 neurology & neurosurgery

Abstract

The transcription factor sex-determining region of the Y chromosome (SRY) plays a key role in human sex determination, because mutations in SRY cause disorders of sex development in XY individuals. During gonadal development, Sry in pre-Sertoli cells activates Sox9 gene transcription, committing the fate of the bipotential gonad to become a testis rather than an ovary. The high-mobility group domain of human SRY contains two independent nuclear localization signals, one bound by calmodulin (CaM) and the other by importin-β. Although XY females carry SRY mutations in these nuclear localization signals that affect SRY nuclear import in transfected cells, it is not known whether these transport mechanisms are essential for gonadal development and sex determination. Here, we show that mouse Sry protein binds CaM and that a CaM antagonist reduces CaM binding, nuclear accumulation, and transcriptional activity of Sry in transfected cells. CaM antagonist treatment of cultured, sexually indifferent XY mouse fetal gonads led to reduced expression of the Sry target gene Sox9, defects in testicular cord formation, and ectopic expression of the ovarian markers Rspondin1 and forkhead box L2. These results indicate the importance of CaM for SRY nuclear import, transcriptional activity, testis differentiation, and sex determination.

Published

2011

43. Sox9 is required for invagination of the otic placode in mice

Author

Stefan Bagheri-Fam, Makoto Mark Taketo, Gerd Scherer, Francisco J. Barrionuevo, Annette Neubüser, Angela Naumann, and Volker Speth

Subjects

endocrine system, medicine.medical_specialty, animal structures, Xenopus, Ectoderm, SOX9, Biology, Mice, stomatognathic system, Internal medicine, Otic placode, medicine, Animals, Inner ear, Mouse inner ear development, Molecular Biology, SOXE Transcription Factors, Neural tube, High Mobility Group Proteins, Receptor, EphA4, Embryo, SOX9 Transcription Factor, Cell Biology, biology.organism_classification, Embryo, Mammalian, Cell biology, DNA-Binding Proteins, medicine.anatomical_structure, Endocrinology, Invagination, Ear, Inner, embryonic structures, sense organs, Otic Placodes, Spiral Ganglion, Sox9, Developmental Biology, Transcription Factors

Abstract

The HMG-domain-containing transcription factor Sox9 is an important regulator of chondrogenesis, testis formation and development of several other organs. Sox9 is expressed in the otic placodes, the primordia of the inner ear, and studies in Xenopus have provided evidence that Sox9 is required for otic specification. Here we report novel and different functions of Sox9 during mouse inner ear development. We show that in mice with a Foxg1 Cre -mediated conditional inactivation of Sox9 in the otic ectoderm, otic placodes form and express markers of otic specification. However, mutant placodes do not attach to the neural tube, fail to invaginate, and subsequently degenerate by apoptosis, resulting in a complete loss of otic structures. Transmission-electron microscopic analysis suggests that cell–cell contacts in the Sox9 mutant placodes are abnormal, although E-cadherin, N-cadherin, and beta-catenin protein expression are unchanged. In contrast, expression of Epha4 was downregulated in mutant placodes. In embryos with a Keratin-19 Cre -mediated mosaic inactivation of Sox9 , Sox9-negative and Sox9-positive cells in the otic ectoderm sort out from one another. In these embryos only Sox9-positive cells invaginate and form one or several micro-vesicles, whereas Sox9-negative cells stay behind and die. Our findings demonstrate that, in contrast to Xenopus , Sox9 is not required for the initial specification of the otic placode in the mouse, but instead controls adhesive properties and invagination of placodal cells in a cell-autonomous manner.

Published

2007

44. Homozygous inactivation of Sox9 causes complete XY sex reversal in mice

Author

Francisco, Barrionuevo, Stefan, Bagheri-Fam, Jürgen, Klattig, Ralf, Kist, Makoto M, Taketo, Christoph, Englert, and Gerd, Scherer

Subjects

Male, Gene Expression Profiling, Homozygote, Disorders of Sex Development, High Mobility Group Proteins, Embryonic Development, Fluorescent Antibody Technique, Mice, Transgenic, SOX9 Transcription Factor, Mice, Inbred C57BL, Wnt Proteins, Mice, Wnt4 Protein, Proto-Oncogene Proteins, Mutation, Testis, Animals, Female, Gene Silencing, Gonads, Mullerian Ducts, Transcription Factors

Abstract

In the presence of the Y-chromosomal gene Sry, the bipotential mouse gonads develop as testes rather than as ovaries. The autosomal gene Sox9, a likely and possibly direct Sry target, can induce testis development in the absence of Sry. Sox9 is thus sufficient but not necessarily essential for testis induction. Mutational inactivation of one allele of SOX9/Sox9 causes sex reversal in humans but not in mice. Because Sox9(-/-) embryos die around Embryonic Day 11.5 (E11.5) at the onset of testicular morphogenesis, differentiation of the mutant XY gonad can be analyzed only ex vivo in organ culture. We have therefore conditionally inactivated both Sox9 alleles in the gonadal anlagen using the CRE/loxP recombination system, whereby CRE recombinase is under control of the cytokeratin 19 promoter. Analysis of resulting Sox9(-/-) XY gonads up to E15.5 reveals immediate, complete sex reversal, as shown by expression of the early ovary-specific markers Wnt4 and Foxl2 and by lack of testis cord and Leydig cell formation. Sry expression in mutant XY gonads indicates that downregulation of Wnt4 and Foxl2 is dependent on Sox9 rather than on Sry. Our results provide in vivo proof that, in contrast to the situation in humans, complete XY sex reversal in mice requires inactivation of both Sox9 alleles and that Sox9 is essential for testogenesis in mice.

Published

2005

45. SOX13 is up-regulated in the developing mouse neuroepithelium and identifies a sub-population of differentiating neurons

Author

Vincent R. Harley, Yi Wang, and Stefan Bagheri-Fam

Subjects

Central Nervous System, Population, Central nervous system, Cell Cycle Proteins, Biology, Autoantigens, Mice, Developmental Neuroscience, Cell Movement, medicine, Animals, Progenitor cell, education, Mitosis, Transcription factor, Cell Nucleus, Neurons, education.field_of_study, Stem Cells, Neurogenesis, High Mobility Group Proteins, Brain, Gene Expression Regulation, Developmental, Cell Differentiation, Epithelial Cells, Up-Regulation, Neuroepithelial cell, Mice, Inbred C57BL, medicine.anatomical_structure, Testis determining factor, Spinal Cord, Neuroscience, Developmental Biology, Transcription Factors

Abstract

In mammals, most of the twenty SOX (SRY HMG box) transcription factors are expressed during embryogenesis and play an important role in cell fate determination. We show here that SOX13 is expressed in the developing mouse brain and spinal cord from E12.5 to E15.5, where it is largely confined to the differentiating zone rather than to the proliferating zone. In particular, we found that SOX13 expression was activated in a subset of neural progenitors as they exit the cycle of mitosis, migrate away from the ventricular zone, and start to differentiate into neurons. The SOX13 protein always localized to the nuclei of the differentiating neuronal cells, consistent with a role for SOX13 as a transcription factor during neurogenesis. Our data suggest a role for SOX13 in the specification and/or differentiation of a specific subset of neurons in the developing central nervous system.

Published

2004

46. Failure of SOX9 Regulation in 46XY Disorders of Sex Development with SRY, SOX9 and SF1 Mutations

Author

Robin Lovell-Badge, Kevin Christopher Knower, Stefan Bagheri-Fam, Helena Yin Yee Sim, Pascal Bernard, Louisa M. Ludbrook, Sabine Kelly, Vincent R. Harley, and Ryohei Sekido

Subjects

Male, Steroidogenic factor 1, Steroidogenic Factor 1, medicine.disease_cause, Biochemistry, Molecular cell biology, 0302 clinical medicine, Testis, Morphogenesis, Transcriptional regulation, Disorders of sex development, SOX9 Transcription Factor, Genetics, 0303 health sciences, Mutation, Sexual Differentiation, Multidisciplinary, Sexual differentiation in humans, musculoskeletal system, Up-Regulation, Enhancer Elements, Genetic, Testis determining factor, Organ Specificity, embryonic structures, Medicine, Research Article, endocrine system, animal structures, Science, DNA transcription, SOX9, Biology, Cell Line, 03 medical and health sciences, stomatognathic system, Genetic Mutation, medicine, Humans, Gene Networks, 030304 developmental biology, Disorder of Sex Development, 46,XY, Cofactors, Sex Determination, medicine.disease, Sex-Determining Region Y Protein, Genetics of Disease, Trans-Activators, Mutant Proteins, Gene expression, Gene Function, 030217 neurology & neurosurgery, Developmental Biology

Abstract

BackgroundIn human embryogenesis, loss of SRY (sex determining region on Y), SOX9 (SRY-related HMG box 9) or SF1 (steroidogenic factor 1) function causes disorders of sex development (DSD). A defining event of vertebrate sex determination is male-specific upregulation and maintenance of SOX9 expression in gonadal pre-Sertoli cells, which is preceded by transient SRY expression in mammals. In mice, Sox9 regulation is under the transcriptional control of SRY, SF1 and SOX9 via a conserved testis-specific enhancer of Sox9 (TES). Regulation of SOX9 in human sex determination is however poorly understood.Methodology/principal findingsWe show that a human embryonal carcinoma cell line (NT2/D1) can model events in presumptive Sertoli cells that initiate human sex determination. SRY associates with transcriptionally active chromatin in NT2/D1 cells and over-expression increases endogenous SOX9 expression. SRY and SF1 co-operate to activate the human SOX9 homologous TES (hTES), a process dependent on phosphorylated SF1. SOX9 also activates hTES, augmented by SF1, suggesting a mechanism for maintenance of SOX9 expression by auto-regulation. Analysis of mutant SRY, SF1 and SOX9 proteins encoded by thirteen separate 46,XY DSD gonadal dysgenesis individuals reveals a reduced ability to activate hTES.Conclusions/significanceWe demonstrate how three human sex-determining factors are likely to function during gonadal development around SOX9 as a hub gene, with different genetic causes of 46,XY DSD due a common failure to upregulate SOX9 transcription.

Published

2011

47. Long-range upstream and downstream enhancers control distinct subsets of the complex spatiotemporal Sox9 expression pattern

Author

Francisco J. Barrionuevo, Rolf Kemler, Stefan Bagheri-Fam, Gerd Scherer, Ulrike Dohrmann, Roland Schüle, Benoît Kanzler, Moisés Mallo, and Thomas Günther

Subjects

animal structures, Molecular Sequence Data, Notochord, Biology, Conserved sequence, Mice, Neural crest, Cranial neural crest, Campomelic dysplasia, Inner ear, medicine, Animals, Humans, Transgenic mice, Cis-regulatory elements, Gut, Intestinal Mucosa, Enhancer, Promoter Regions, Genetic, Node, Molecular Biology, Conserved Sequence, beta Catenin, Regulation of gene expression, Reporter gene, Binding Sites, Neuroectoderm, Base Sequence, High Mobility Group Proteins, Brain, Gene Expression Regulation, Developmental, SOX9 Transcription Factor, Cell Biology, Molecular biology, medicine.anatomical_structure, Enhancer Elements, Genetic, Ear, Inner, embryonic structures, SOX9, Transcription Factors, Developmental Biology

Abstract

SOX9 is an evolutionary conserved transcription factor that is expressed in a variety of tissues, with essential functions in cartilage, testis, heart, glial cell, inner ear and neural crest development. By comparing human and pufferfish genomic sequences, we previously identified eight highly conserved sequence elements between 290 kb 5′ and 450 kb 3′ to human SOX9. In this study, we assayed the regulatory potential of elements E1 to E7 in transgenic mice using a lacZ reporter gene driven by a 529 bp minimal mouse Sox9 promoter. We found that three of these elements and the Sox9 promoter control distinct subsets of the tissue-specific expression pattern of Sox9. E3, located 251 kb 5′ to SOX9, directs lacZ expression to cranial neural crest cells and to the inner ear. E1 is located 28 kb 5′ to SOX9 and controls expression in the node, notochord, gut, bronchial epithelium and pancreas. Transgene expression in the neuroectoderm is mediated by E7, located 95 kb 3′ to SOX9, which regulates expression in the telencephalon and midbrain, and by the Sox9 minimal promoter which controls expression in the ventral spinal cord and hindbrain. We show that E3-directed reporter gene expression in neural crest cells of the first but not of the second and third pharyngeal arch is dependent on beta-catenin, revealing a complex regulation of Sox9 in cranial neural crest cells. Moreover, we identify and discuss highly conserved transcription factor binding sites within enhancer E3 that are in good agreement with current models for neural crest and inner ear development. Finally, we identify enhancer E1 as a cis-regulatory element conserved between vertebrates and invertebrates, indicating that some cis-regulatory sequences that control developmental genes in vertebrates might be phylogenetically ancient.