GATA4 Is a Key Regulator of Steroidogenesis and Glycolysis in Mouse Leydig Cells

Author:

Schrade Anja12,Kyrönlahti Antti1,Akinrinade Oyediran13,Pihlajoki Marjut12,Häkkinen Merja142,Fischer Simon5,Alastalo Tero-Pekka1,Velagapudi Vidya6,Toppari Jorma7,Wilson David B.28,Heikinheimo Markku142

Affiliation:

1. Children’s Hospital (A.S., A.K., O.A., M.P., T.-P.A., M.H.), University of Helsinki, Helsinki 00014, Finland

2. Departments of Pediatrics (A.S., M.P., D.B.W., M.H.), Washington University in St. Louis, St. Louis, Missouri 63110

3. Institute of Biomedicine (O.A.), University of Helsinki, Helsinki 00014, Finland

4. School of Pharmacy (M.H.), University of Eastern Finland, Kuopio 70211, Finland

5. Institute of Applied Biotechnology (S.F.), University of Applied Sciences Biberach, Biberach 88400, Germany

6. Metabolomics Unit (V.V.), Institute for Molecular Medicine Finland, University of Helsinki 00014, Helsinki, Finland

7. Departments of Physiology and Pediatrics (J.T.), University of Turku, Turku 20520, Finland

8. Department of Developmental Biology (D.B.W.), Washington University in St. Louis, St. Louis, Missouri 63110

Abstract

Transcription factor GATA4 is expressed in somatic cells of the mammalian testis. Gene targeting studies in mice have shown that GATA4 is essential for proper differentiation and function of Sertoli cells. The role of GATA4 in Leydig cell development, however, remains controversial, because targeted mutagenesis experiments in mice have not shown a consistent phenotype, possibly due to context-dependent effects or compensatory responses. We therefore undertook a reductionist approach to study the function of GATA4 in Leydig cells. Using microarray analysis and quantitative RT-PCR, we identified a set of genes that are down-regulated or up-regulated after small interfering RNA (siRNA)-mediated silencing of Gata4 in the murine Leydig tumor cell line mLTC-1. These same genes were dysregulated when primary cultures of Gata4flox/flox adult Leydig cells were subjected to adenovirus-mediated cre-lox recombination in vitro. Among the down-regulated genes were enzymes of the androgen biosynthetic pathway (Cyp11a1, Hsd3b1, Cyp17a1, and Srd5a). Silencing of Gata4 expression in mLTC-1 cells was accompanied by reduced production of sex steroid precursors, as documented by mass spectrometric analysis. Comprehensive metabolomic analysis of GATA4-deficient mLTC-1 cells showed alteration of other metabolic pathways, notably glycolysis. GATA4-depleted mLTC-1 cells had reduced expression of glycolytic genes (Hk1, Gpi1, Pfkp, and Pgam1), lower intracellular levels of ATP, and increased extracellular levels of glucose. Our findings suggest that GATA4 plays a pivotal role in Leydig cell function and provide novel insights into metabolic regulation in this cell type.

Publisher

The Endocrine Society

Subject

Endocrinology

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