Divergent roles of growth factors in the GnRH regulation of puberty in mice
Sara A. DiVall, … , Sally Radovick, Andrew Wolfe
Sara A. DiVall, … , Sally Radovick, Andrew Wolfe
Published July 12, 2010
Citation Information: J Clin Invest. 2010;120(8):2900-2909. https://doi.org/10.1172/JCI41069.
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Research Article Endocrinology

Divergent roles of growth factors in the GnRH regulation of puberty in mice

Abstract

Pubertal onset, initiated by pulsatile gonadotropin-releasing hormone (GnRH), only occurs in a favorable, anabolic hormonal milieu. Anabolic factors that may signal nutritional status to the hypothalamus include the growth factors insulin and IGF-1. It is unclear which hypothalamic neuronal subpopulation these factors affect to ultimately regulate GnRH neuron function in puberty and reproduction. We examined the direct role of the GnRH neuron in growth factor regulation of reproduction using the Cre/lox system. Mice with the IR or IGF-1R deleted specifically in GnRH neurons were generated. Male and female mice with the IR deleted in GnRH neurons displayed normal pubertal timing and fertility, but male and female mice with the IGF-1R deleted in GnRH neurons experienced delayed pubertal development with normal fertility. With IGF-1 administration, puberty was advanced in control females, but not in females with the IGF-1R deleted in GnRH neurons, in control males, or in knockout males. These mice exhibited developmental differences in GnRH neuronal morphology but normal number and distribution of neurons. These studies define the role of IGF-1R signaling in the coordination of somatic development with reproductive maturation and provide insight into the mechanisms regulating pubertal timing in anabolic states.

Authors

Sara A. DiVall, Tameeka R. Williams, Sarah E. Carver, Linda Koch, Jens C. Brüning, C. Ronald Kahn, Fredric Wondisford, Sally Radovick, Andrew Wolfe

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Figure 3

Generation of the GnRH-IGFRKO mouse.

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Generation of the GnRH-IGFRKO mouse. (A) The Igf1r gene with exon 3 flan...
(A) The Igf1r gene with exon 3 flanked by loxP sites (large arrows) before (top panel) and after (bottom panel) Cre recombination. Primers used for detection of the truncated Igf1r gene are labeled p4, p5, and p6. (B) PCR analysis of genomic DNA isolated from tissues of a GnRH-IGFRKO mouse. The floxed Igf1r gene is indicated by the 750-bp band, and the excised Igf1r gene is indicated by the 490-bp band. (C) Sections (40 μm) of hypothalami from control littermates or GnRH-IGFRKO mice were incubated with anti-GnRH and anti–IGF-1R antibody with secondary antibodies conjugated to a fluorophore emitting red (GnRH) or green (IGFR) wavelengths. Long arrows indicate neurons that stain for GnRH and IGF-1R. Short arrows indicate neurons that stain for IGF-1R only. Scale bars: 20 μm.