doi: 10.1210/en.2015-1645.
Epub 2015 Dec 15.
Conditional Deletion of Bmal1 in Ovarian Theca Cells Disrupts Ovulation in Female Mice
Affiliations
- PMID: 26671182
- PMCID: PMC5393362
- DOI: 10.1210/en.2015-1645
Item in Clipboard
Conditional Deletion of Bmal1 in Ovarian Theca Cells Disrupts Ovulation in Female Mice
Endocrinology.
2016 Feb.
Abstract
Rhythmic events in female reproductive physiology, including ovulation, are tightly controlled by the circadian timing system. The molecular clock, a feedback loop oscillator of clock gene transcription factors, dictates rhythms of gene expression in the hypothalamo-pituitary-ovarian axis. Circadian disruption due to environmental factors (eg, shift work) or genetic manipulation of the clock has negative impacts on fertility. Although the central pacemaker in the suprachiasmatic nucleus classically regulates the timing of ovulation, we have shown that this rhythm also depends on phasic sensitivity to LH. We hypothesized that this rhythm relies on clock function in a specific cellular compartment of the ovarian follicle. To test this hypothesis we generated mice with deletion of the Bmal1 locus in ovarian granulosa cells (GCs) (Granulosa Cell Bmal1 KO; GCKO) or theca cells (TCs) (Theca Cell Bmal1 KO; TCKO). Reproductive cycles, preovulatory LH secretion, ovarian morphology and behavior were not grossly altered in GCKO or TCKO mice. We detected phasic sensitivity to LH in wild-type littermate control (LC) and GCKO mice but not TCKO mice. This decline in sensitivity to LH is coincident with impaired fertility and altered patterns of LH receptor (Lhcgr) mRNA abundance in the ovary of TCKO mice. These data suggest that the TC is a pacemaker that contributes to the timing and amplitude of ovulation by modulating phasic sensitivity to LH. The TC clock may play a critical role in circadian disruption-mediated reproductive pathology and could be a target for chronobiotic management of infertility due to environmental circadian disruption and/or hormone-dependent reprogramming in women.
Figures
A, Serum levels of LH at ZT12 on proestrus were suppressed by treatment with CET (n = 4; *, P < .05 vs saline [n = 5]). B, Dose-response curve for eLH treatment. All 3 doses (50, 200, or 800 IU; n = 3–4 per treatment) stimulated more oocyte release at ZT18 (*, P < .001). C, Rhythm of ovarian sensitivity to eLH in adult C57BL6/J mice (n = 3–6 per treatment time; *, P < .05 vs ZT3, ZT6, and ZT9). D, Free-running circadian rhythm of sensitivity to LH in C57BL6/J mice (*, P < .05 vs ZT6; n = 3–6 per treatment time). E, A diurnal rhythm of sensitivity to eLH in juvenile eCG-primed mice (**, P < .001 vs ZT0–ZT9 on estrus, n = 3–6 per treatment time). F, A circadian rhythm of responsiveness to eLH in juvenile-eCG-primed mice housed in DD (*, P < .05 vs the nadir at CT6 on estrus, n = 3–4 per treatment time). In F, the time of CET injection (CT5) is not shown due to scaling of the x-axis. In C–F, saline failed to stimulate ovulation. Data are presented as mean ± SEM and fit to a nonlinear regression (see Materials and Methods). The shaded areas in C–F indicate the dark phase.
Targeted deletion of Bmal1 in granulosa (GCKO) and theca/stromal (TCKO) cells of the ovary using the CRE:LOX system. Transgenic GCKO (Cyp19-Cre;Bmal1flx/flx) and TCKO (Cyp17-Cre;Bmal1flx/flx) mice were crossed with TOM-GFP mice to produce TCKO-TOM-GFP and GCKO-TOM-GFP transgenic mice (see Supplemental Methods). As shown in A, CRE-driven eGFP expression in GCKO-TOM-GFP is nearly completely limited to the mural and cumulus GC layer with little to any GFP expression detected in the TC/SC compartment or the ovarian surface epithelium (OSE). B, In TCKO-TOM-GFP mice, CRE-driven GFP is more dispersed and spotty in the interstitial cells and limited the TC layer of larger antral follicles with no signal detected in the GC compartment or surface epithelium. Representative images of whole mount (C) pituitary gland and (D) liver from a GCKO mouse. A small number of cells in these tissues from both transgenic strains were positive for GFP (<5%). Scale bars: 0.25 μm shown in A (A and B), 0.05 mm shown in C (C and D), and 0.25 mm shown in E (E and F). Images are representative of 3–4 mice per genotype (LC, GCKO, and TCKO).
A, Representative reproductive cycle graphs from LC, GCKO, and TCKO transgenic mice. B, Analysis of (top) cycle length and (bottom) percentage of time spent in each day of the cycle reveals no significant difference between LC, GCKO, and TCKO transgenic mice (n = 9 per group). C, Serum LH measured on proestrus from ZT3–ZT18 reveals that both GCKO and TCKO transgenic mice had appreciable surges of serum LH with both rhythms peaking at ZT12 (*, P < .05, n = 3–4 samples per time point). D, Levels of serum P4 at ZT6 and ZT18 on proestrus were not significantly affected by targeted deletion of Bmal1 in either GCKO or TCKO transgenic mice (n = 3 samples per time point except for ZT6 in LC mice [n = 2]). Data are labeled according to genotype and time of serum collection. All data are presented as mean ± SEM.
A, Rhythm of sensitivity to eLH in cycling adult LC (n = 3; both ZT18 and ZT6), GCKO (ZT18 n = 5, ZT6 n = 4), and TCKO (ZT18 n = 5, ZT6 n = 6) mice. Both LC and GCKO transgenic mice displayed strong diurnal rhythms of eLH sensitivity with peak responses to eLH treatment at ZT18 (*, P < .05 vs ZT6) for both. In contrast, adult cycling TCKO mice did not maintain a rhythm of sensitivity to eLH (P > .05 ZT18 vs ZT6). B, Diurnal rhythms of sensitivity to LH in juvenile-eCG-primed LC (n = 4–8 per time of treatment), GCKO (n = 5–6 per time of treatment), and TCKO (n = 4–6 per time of treatment) mice. Both LC (open circles) and GCKO (gray squares) mice displayed diurnal rhythms of responsiveness with significant peaks of responsiveness to eLH treatment at ZT9–ZT12 (*, P < .05 vs troughs at ZT0, ZT3, and ZT18). TCKO mice (black triangles) did not show a significant rhythm in response to phasic eLH. Data are presented as mean ± SEM and in B data are fit to a nonlinear regression (see Materials and Methods). In B, # indicates difference between TCKO and GCKO, and + indicates a significant difference between TCKO and LC mice.
Abundance of clock gene mRNA in ovaries recovered from LC (n = 3), GCKO (n = 3), and TCKO (n = 3) mice on proestrus. LC mice displayed diurnal rhythms of Bmal1, Per1, and Rev-erbα mRNA abundance (P < .05 indicated in top right of each panel). Rhythms of Bmal1 and Rev-erbα mRNA abundance were disrupted in both GCKO and TCKO mice. Although still rhythmic, the absolute level of Per1 mRNA was suppressed in both GCKO and TCKO mice. Although not significant by CircWave analysis, Cry1 mRNA abundance oscillated at low amplitude with a peak near midday in LC mice and was altered in both GCKO and TCKO mice. Clock mRNA displayed a low amplitude rhythm in TCKO mice that was not detected in LC or GCKO mice. Data are presented as mean ± SEM; n = 3 samples per time point except for ZT24 in TCKO mice (n = 2). (#, P < .05 GCKO vs TCKO; *, P < .05 LC vs GCKO or TCKO). Values for target mRNA abundance were calculated using the ΔΔCT method as described in Materials and Methods with β-actin as the reference gene. Data were fit to a nonlinear regression (see Materials and Methods).
Rhythms of Lhcgr and Fshr expression in whole ovary tissue recovered from LC (n = 3), GCKO (n = 3), and TCKO (n = 3) transgenic mice. In both LC and GCKO mice we detected a significant diurnal rhythm of Lhcgr mRNA abundance (P < .05 for both) that was abolished in TCKO transgenic mice. There was a marked increase in Lhcgr expression at ZT24 in TCKO mice (#, P < .05) when compared with the same time point in both LC and GCKO mice. A low amplitude oscillation of Fshr mRNA expression was detected in GCKO transgenic mice with a peak in the morning (ZT1.99). Daily variation of Fshr mRNA abundance was not significant in either LC or TCKO transgenic mice. Data are presented as mean ± SEM. n = 3 ovaries from 3 different mice per time point. #, P < .05 GCKO vs TCKO; *, P < .05 LC vs GCKO or TCKO. Only those rhythms labeled directly with a P value were considered significant by CircWave analyses. Values for target mRNA abundance were calculated using the ΔΔCT method as described in Materials and Methods, with β-actin as the reference gene. Data were fit to a nonlinear regression (see Materials and Methods).
Similar articles
-
Rhythmic expression of circadian clock genes in the preovulatory ovarian follicles of the laying hen.PLoS One. 2017 Jun 12;12(6):e0179019. doi: 10.1371/journal.pone.0179019. eCollection 2017. PLoS One. 2017. PMID: 28604799 Free PMC article.
-
Circadian clock function in the mammalian ovary.J Biol Rhythms. 2015 Feb;30(1):7-19. doi: 10.1177/0748730414554222. Epub 2014 Nov 3. J Biol Rhythms. 2015. PMID: 25367899 Review.
-
Global but not gonadotrope-specific disruption of Bmal1 abolishes the luteinizing hormone surge without affecting ovulation.Endocrinology. 2013 Aug;154(8):2924-35. doi: 10.1210/en.2013-1080. Epub 2013 Jun 4. Endocrinology. 2013. PMID: 23736292
-
[The roles of clock genes in obesity].Nihon Rinsho. 2013 Feb;71(2):244-8. Nihon Rinsho. 2013. PMID: 23631200 Review. Japanese.
-
Alterations of circadian clockworks during differentiation and apoptosis of rat ovarian cells.Chronobiol Int. 2011 Jul;28(6):477-87. doi: 10.3109/07420528.2011.589933. Chronobiol Int. 2011. PMID: 21797776
Cited by
-
Neuroendocrine effects of the duper mutation in Syrian hamsters: a role for Cryptochrome 1.Front Physiol. 2024 Feb 20;15:1351682. doi: 10.3389/fphys.2024.1351682. eCollection 2024. Front Physiol. 2024. PMID: 38444761 Free PMC article.
-
The transcription factor VAX1 in VIP neurons of the suprachiasmatic nucleus impacts circadian rhythm generation, depressive-like behavior, and the reproductive axis in a sex-specific manner in mice.Front Endocrinol (Lausanne). 2023 Dec 22;14:1269672. doi: 10.3389/fendo.2023.1269672. eCollection 2023. Front Endocrinol (Lausanne). 2023. PMID: 38205198 Free PMC article.
-
The stromal microenvironment and ovarian aging: mechanisms and therapeutic opportunities.J Ovarian Res. 2023 Dec 13;16(1):237. doi: 10.1186/s13048-023-01300-4. J Ovarian Res. 2023. PMID: 38093329 Free PMC article. Review.
-
Effects of time-restricted feeding on letrozole-induced mouse model of polycystic ovary syndrome.Sci Rep. 2023 Feb 2;13(1):1943. doi: 10.1038/s41598-023-28260-5. Sci Rep. 2023. PMID: 36732546 Free PMC article.
-
The Circadian Clock, Nutritional Signals and Reproduction: A Close Relationship.Int J Mol Sci. 2023 Jan 12;24(2):1545. doi: 10.3390/ijms24021545. Int J Mol Sci. 2023. PMID: 36675058 Free PMC article. Review.
References
-
- Kennaway DJ. The role of circadian rhythmicity in reproduction. Hum Reprod Update. 2005;11:91–101. - PubMed
-
- Boden MJ, Kennaway DJ. Circadian rhythms and reproduction. Reproduction. 2006;132:379–392. - PubMed
-
- Bronson FH, Vom Saal FS. Control of the preovulatory release of luteinizing hormone by steroids in the mouse. Endocrinology. 1979;104:1247–1255. - PubMed
-
- Goldman BD. The circadian timing system and reproduction in mammals. Steroids. 1999;64:679–685. - PubMed
-
- Legan SJ, Karsch FJ. A daily signal for the LH surge in the rat. Endocrinology. 1975;96:57–62. - PubMed
MeSH terms
Substances
Grants and funding
LinkOut - more resources
Full Text Sources
Other Literature Sources
Molecular Biology Databases
Research Materials
