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BOR - Papers in Press, published online ahead of print November 27, 2002.
Biol Reprod 2002, 10.1095/biolreprod.102.008862
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BIOLOGY OF REPRODUCTION 68, 1631–1640 (2003)
DOI: 10.1095/biolreprod.102.008862
© 2003 by the Society for the Study of Reproduction, Inc.


Testis

Developmental, Stage-Specific, and Hormonally Regulated Expression of Growth Hormone Secretagogue Receptor Messenger RNA in Rat Testis1

M.L. Barreiro3, J.S. Suominen4, F. Gaytán3, L. Pinilla3, L.K. Chopin5, F.F. Casanueva6, C. Diéguez7, E. Aguilar3, J. Toppari4, and M. Tena-Sempere2,3

Department of Cell Biology, Physiology, and Immunology,3 University of Córdoba, 14004 Córdoba, Spain Departments of Physiology and Pediatrics,4 University of Turku, 20520 Turku, Finland Centre for Molecular Biotechnology,5 Queensland University of Technology, Brisbane, Queensland, Australia Departments of Medicine6 Physiology,7 University of Santiago de Compostela, 15705 Santiago de Compostela, Spain

Recent evidence from our research suggested the direct role of ghrelin in the control of testicular function. However, the pattern of expression and hormonal regulation of the gene encoding its cognate receptor (i.e., the growth hormone-secretagogue receptor [GHS-R]) in the male gonad remains to be fully elucidated. In this paper, overall expression of GHS-R mRNA in rat testis was compared with that of the functional receptor form, namely GHS-R type 1a, in different developmental and experimental settings. In addition, cellular distribution of GHS-R within adult testis tissue was assessed. Our analyses demonstrated persistent expression of the GHS-R gene in rat testis throughout postnatal development. In contrast, testicular expression of GHS-R type 1a mRNA remained undetectable before puberty and sharply increased thereafter. In adult testis, GHS-R1a mRNA expression presented a scattered pattern of cellular distribution, including Sertoli and Leydig cells that also showed specific GHS-R1a immunoreactivity. Expression of total GHS-R and specific GHS-R1a mRNAs was detected in isolated seminiferous tubule preparations, with varying levels throughout the defined stages of the spermatogenic cycle. In addition, testicular expression of total GHS-R and GHS-R1a mRNAs was up-regulated by exposure to ghrelin in vitro and after stimulation with FSH in vivo. In conclusion, our data demonstrate that expression of the GHS-R gene in rat testis takes place in a developmental, stage-specific, and hormonally regulated manner. Divergent expression of total GHS-R and type 1a specific mRNAs was detected at certain stages of postnatal development and spermatogenic cycle, thus raising the possibility that, in addition to net changes in GHS-R gene expression, the balance between receptor subtypes may represent a novel mechanism for the tuning of ghrelin sensitivity in rat testis.

1 Supported by grant PM-98-0163 from DGESIC (Ministerio de Ciencia y Tecnología, Spain); project 1FD97-0696-02 (FEDER); and grants from the Academy of Finland and Turku University Central Hospital.

2 Correspondence: Manuel Tena-Sempere, Physiology Section, Department of Cell Biology, Physiology and Immunology, Faculty of Medicine, University of Córdoba, Avda. Menéndez Pidal s/n, 14004 Córdoba, Spain. FAX: 34 957 218288; fi1tesem{at}uco.es




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