Literature DB >> 26384646

The pregnant mouse uterus exhibits a functional kisspeptin/KISS1R signaling system on the day of embryo implantation.

Mehri Fayazi^1,2,3, Michele Calder^4,5,6, Moshmi Bhattacharya^7,8,9, George A Vilos¹⁰, Stephen Power¹¹, Andy V Babwah^12,13,14,15.

Abstract

BACKGROUND: Expression of kisspeptin (protein) and Kiss1r (mRNA) was recently documented in the mouse uterus on D4 of pregnancy (the day of embryo implantation) suggesting that the uterine-based kisspeptin (KP)/kisspeptin receptor (KISS1R) signaling system regulates embryo implantation. Despite this important suggestion, it was never demonstrated that the uterus actually exhibits a functional KP/KISS1R signaling system on D4 of pregnancy. Thus, the goal of this study was to determine whether a functional KP/KISS1R signaling system exists in the mouse uterus on D4 of pregnancy.
FINDINGS: Since kisspeptin/KISS1R signaling triggers the phosphorylation of the mitogen-activated protein kinases p38 and ERK1/2, through immunohistochemical analyses, we determined whether exogenously administered kisspeptin could trigger p38 and ERK1/2 phosphorylation in the uterus on D4 of pregnancy. The results clearly demonstrated that kisspeptin could and that its effects were mediated via KISS1R. Additionally, the robust kisspeptin-triggered response was observed in the pregnant uterus only. Finally, it was demonstrated that on D4 of pregnancy the Kiss1 null uterus expresses functional KISS1R molecules capable of mediating the effects of kisspeptin.
CONCLUSIONS: These results lead us to conclude that on D4 of pregnancy, the mouse uterus expresses a functional KP/KISS1R signaling system strengthening the possibility that this signaling system regulates embryo implantation. These findings strengthen the rationale for determining whether such a functional system exists in the uterus of the human female and if so, what role it might play in human pregnancy.

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Year: 2015 PMID： 26384646 PMCID： PMC4575475 DOI： 10.1186/s12958-015-0105-1

Source DB: PubMed Journal: Reprod Biol Endocrinol ISSN： 1477-7827 Impact factor: 5.211

Introduction

It is now well-established that hypothalamic kisspeptins (KPs), signaling via their cognate receptor KISS1R, are potent triggers of gonadotropin-releasing hormone (GnRH) secretion and mice bearing a deletion of the gene encoding KISS1R in the GnRH neuron display hypogonadotropic hypogonadism and infertility [1, 2]. Therefore, the hypothalamic-based KP/KISS1R signaling system is considered a major regulator of reproduction [3]. The KP/KISS1R signaling system is also expressed in the female reproductive tract and roles have been proposed in positively regulating follicular development, ovulation, embryo implantation and endometrial decidualization [4-7]. Therefore, the peripheral KP/KISS1R signaling system is considered a major regulator of reproduction [8]. We have previously reported that KP (protein) and Kiss1r (mRNA) are highly expressed in the mouse uterus on the day of implantation (that is, D4 after mating with the day of mating designated D0) suggesting a role for this signaling system in regulating embryo implantation [4]. To test this idea further, we turned our attention to mice bearing a global deletion of Kiss1. These mice are infertile and it was assumed that their infertility was due to a lack of hypothalamic KP/KISS1R signaling and the resulting reduction in gonadotropins, estradiol and progesterone [9]. However, despite the add-back of these hormones embryos failed to implant in the Kiss1 null uterus leading us to suggest that it was a lack of uterine and not hypothalamic KP/KISS1R signaling that triggered implantation failure. Despite this important suggestion, we did not actually demonstrate the presence of a functional KP/KISS1R signaling system in the uterus on D4 of pregnancy. Such demonstration would have greatly strengthened our suggestion. Thus, the goal of this study was to determine whether on D4 of pregnancy, the day of embryo implantation, a functional KP/KISS1R signaling system exists in the mouse uterus. It was previously reported that in various cell types, the KP/KISS1R signaling triggers mitogen-activated protein kinase (MAPK) phosphorylation. Specifically, it was demonstrated that KP treatment of KISS1R-expressing cells triggers the phosphorylation of the MAPKs p38 and ERK1/2 [10-12] but not SAPK/JNK [10]. We therefore investigated whether exogenously administered KP could trigger the phosphorylation of MAPKs in the uterus.

Findings

In the following studies 8–12 week old 129S1/SvImJ female mice were used. WT females and estradiol- and gonadotropin-primed Kiss1 null females (as previously described [4]) were mated to WT males (D0) and on the morning of D4 of pregnancy, females which displayed a copulatory plug (evidence of successful mating) were injected with either phosphate-buffered saline (PBS, 100 μl) or KP54 (100 nmol/kg, 100 μl, Tocris Bioscience, Minneapolis, MN, USA) intraperitoneally and 30 min later were rapidly sacrificed. In addition to the use of these pregnant mice, age-matched WT unmated but cycling females were also treated with PBS or KP54 in an identical manner. All experiments were repeated 6 independent times. Immediately after drug or saline treatment, uteri were removed and simultaneously processed for immunohistochemistry using standard techniques [4] and 5 μm-thick slices were simultaneously immunostained to detect phosphorylated p38, ERK1/2 and SAPK/JNK. Care was taken to expose the experimental and control tissue to identical experimental conditions. Phosphorylated p38, pERK1/2 and SAPK/JNK were assayed using the following rabbit monoclonal antibodies: phospho-p38 (D3F9), phospho-p44/42 (ERK1/2) (D13.14.4E) and phospho-SAPK/JNK (81E11) (Cell Signaling, Boston, MA, USA). Antigen-bound primary antibodies were detected with the ImmunoCruz rabbit ABC Staining System sc-2018 (Santa Cruz Biotechnology, Inc. Dallas, TX, USA). Both the primary and secondary detection systems were used according to the manufacturers’ guidelines without any adaptations.

KP triggers p38 phosphorylation in the uterine luminal and glandular epithelia on D4 of pregnancy

Results showed that, compared to PBS-treated pregnant mice (Fig. 1a and b), uteri from KP54-treated pregnant mice exhibited (approximately 5-10-fold) higher levels of phosphorylated p38 in all cells of both the luminal and glandular epithelia (Fig. 1c, d and e). These findings were recapitulated when uteri were removed from untreated pregnant mice and then treated with either PBS or KP54 in vitro in the absence of any effects that KP54 might have triggered in vivo at the level of the hypothalamus, pituitary and ovaries (data not shown).

Fig. 1

KP54 administration to female WT mice on D4 of pregnancy triggers p38 and ERK1/2 phosphorylation but not SAPK/JNK. Phosphorylated p38 expression in the D4 pregnant uterus following PBS-treatment (a); part of the uterus shown in (a) is magnified to better reveal details on the endometrial glands (b). Posphorylated p38 (p-p38) expression in the D4 pregnant uterus following KP54-treatment (c); parts of the uterus shown in (c) are magnified to better reveal details on the endometrial glands and luminal epithelium (d and e). Phosphorylated p38 expression in the non-pregnant uterus following PBS- (f) or KP54 (g) treatment. Phosphorylated ERK1/2 (pERK1/2) expression in the D4 pregnant uterus following PBS-treatment (h) or KP54-treatment (i); part of the uterus shown in (i) is magnified to better reveal details on the luminal epithelium (j). Phosphorylated SAPK/JNK (pSAPK/pJNK) expression in the D4 pregnant uterus following PBS-treatment (k) or KP54-treatment (l). AM: anti-mesometrial pole; LM: longitudinal muscle of the myometrium; CM: circular muscle of the myometrium; E: endometrium; LE: luminal epithelium; GE: glandular epithelium; M: mesometrial pole; UL: uterine lumen

KP barely triggers p38 phosphorylation in the non-pregnant uterus

When these studies were conducted in non-pregnant mice, relative to PBS-treated mice (Fig. 1f), uteri from KP54-treated mice (Fig. 1g) failed to show a strong increase in phosphorylated p38 in any cell type. However, careful examination of several uteri did suggest there was a very weak (approximately 1.2-fold greater) but almost undetectable response in the uterine epithelium. This suggest that KISS1R is weakly expressed in the non-pregnant uterus and/or poorly coupled to p38 phosphorylation. The weak expression suggests the possibility that basal kisspeptin signaling might also play a role in the non-pregnant uterus or that basal expression keeps the uterus in a primed-stated such that it allows for a more rapid upregulation of signaling when it is required during pregnancy.

KP triggers ERK1/2 phosphorylation in the uterine luminal epithelium on D4 of pregnancy

When compared to PBS-treated pregnant mice (Fig. 1h), uteri from KP54-treated pregnant mice exhibited visibly higher levels of phosphorylated ERK1/2 in a subset of cells within the luminal epithelium only (Fig. 1i and j). When this study was conducted in non-pregnant mice, relative to PBS-treated mice, uteri from KP54 treated mice failed to show a visible increase in phosphorylated ERK1/2 in any cell type (data not shown) again supporting the idea that KISS1R is very weakly expressed in the non-pregnant uterus and/or uncoupled to ERK1/2 phosphorylation.

KP fails to trigger SAPK/JNK phosphorylation in the uterus

Consistent with data obtained in KISS1R-expressing Chinese hamster ovary cells [10], relative to PBS-treated pregnant mice (Fig. 1k), uteri from KP54-treated pregnant mice (Fig. 1l) failed to show an increase in phosphorylated SAPK/JNK in any cell type. Failure to detect evidence of SAPK/JNK phosphorylation was not due to a loss in antibody quality since an aliquot of this antibody detected phosphorylated SAPK/JNK in UV-treated human embryonic kidney 293 cells (data not shown).

KP triggers p38 phosphorylation in a KISS1R-specific manner in the uterus on D4 of pregnancy

It was reported that in addition to KISS1R, KP can signal via the NPFF1/GPR147 and NPFF2/GPR74 receptors [13]. Therefore, to determine whether the KP-triggered phosphorylation of p38 and ERK1/2 was KISS1R-specific the following experiment was conducted. Eight to 12 week old WT females were mated to WT males and on the morning of D4 of pregnancy, females were injected intraperitoneally with either PBS (100 μl) or the KISS1R antagonist P234 (100 nmol/kg, 100 μl, Tocris Bioscience, Minneapolis, MN, USA) [14]. Thirty minutes later a group of PBS-treated females was injected with either PBS (100 μl) or KP54 (100 nmol/kg, 100 μl) while the P234-treated group was injected with KP54 (100 nmol/kg, 100 μl). Thirty minutes later, mice were sacrificed and uteri were processed to assay for phosphorylated p38. As expected, based on earlier findings (Fig. 1a-e) results revealed that relative to PBS-treated pregnant mice (Fig. 2a and b), KP-triggered a robust increase in phosphorylated p38 levels in both the luminal and glandular epithelia of pregnant uteri (Fig. 2c and d), however, this KP-triggered increase was completely blocked when mice were pretreated with P234 (Fig. 2e and f). Interestingly, in P234 pretreated mice, phosphorylated p38 levels were visibly lower (by approximately 2-fold) than that of PBS only treated mice (Fig. 2e and f vs. 2a and b) suggesting that on the day of implantation, endogenous KP phosphorylates uterine p38. Based on preliminary data (n = 2), similar observations were made with pERK1/2 levels at the luminal epithelium and again, consistent with earlier experiments, KP54 had no effect on JNK/SAPK phosphorylated levels both in the presence and absence of P234 pre-treatment (n = 2) (data not shown).

Fig. 2

KP signals specifically via KISS1R in the uterus on D4 of pregnancy in WT mice. Phosphorylated p38 expression in the D4 pregnant uterus following 30 min PBS pre-treatment followed by 30 min PBS post-treatment (a); part of the uterus shown in (a) is magnified to better reveal details on the endometrial glands (b). Phosphorylated p38 expression in the D4 pregnant uterus following 30 min PBS pre-treatment followed by 30 min KP54 post-treatment (c); part of the uterus shown in (c) is magnified to better reveal details on the endometrial glands (d). Phosphorylated p38 expression in the D4 pregnant uterus following 30 min P234 pre-treatment followed by 30 min KP54 post-treatment (e); part of the uterus shown in (e) is magnified to better reveal details on the endometrial glands (f). AM: anti-mesometrial pole; LM: longitudinal muscle of the myometrium; CM: circular muscle of the myometrium; E: endometrium; LE: luminal epithelium; GE: glandular epithelium; M: mesometrial pole; UL: uterine lumen

The Kiss1−/− uterus remains responsive to KP

In a previous study we failed to rescue the implantation defect through the add-back of KP to pregnant Kiss1−/− females [4]. We speculated that this could have been due to the inefficient delivery of the drug (which was administered subcutaneously) to the uterus [15]. Another possibility was that although Kiss1r mRNA was still expressed in the Kiss1−/− uterus, this expression did not result in the formation of functional receptor molecules thus precluding the ability of KP to signal and rescue the implantation defect. To test the latter possibility, Kiss1−/− uteri on D4 of pregnancy were assayed for phosphorylated p38 following KP54 treatment. Results showed that relative to PBS-treated pregnant mice (Fig. 3a), uteri from KP54-treated pregnant mice exhibited higher levels of phosphorylated p38 in all cells of both the luminal and glandular epithelia (Fig. 3b). Based on preliminary data (n = 2), similar observations were made with pERK1/2 levels at the luminal epithelium and again, consistent with earlier experiments, KP54 had no effect on JNK/SAPK phosphorylated levels (n = 2) (data not shown). Together, these results confirm the presence of functional KISS1R molecules coupled to p38 and ERK1/2 phosphorylation on D4 of pregnancy in the Kiss1−/− uterus suggesting that failure of exogenous KP to rescue the implantation defect, as reported by Calder et al. [4] was not due to the lack of functional KISS1R molecules in the uterus.

Fig. 3

KP54 administration to female Kiss1 −/− mice on D4 of pregnancy triggers p38 phosphorylation. Phosphorylated p38 expression in the D4 pregnant uterus following PBS-treatment (a) or KP54-treatment (b). AM: anti-mesometrial pole; LM: longitudinal muscle of the myometrium; CM: circular muscle of the myometrium; E: endometrium; LE: luminal epithelium; GE: glandular epithelium; M: mesometrial pole; UL: uterine lumen

Conclusions

The goal of this study was to determine whether on D4 of pregnancy, the day of embryo implantation, a functional KP/KISS1R signaling system exists in the mouse uterus. Our data clearly reveal that one exists and this major finding further strengthens the possibility that this signaling system regulates uterine functions in early pregnancy. Because expression, as determined by phosphorylated p38 and ERK1/2 levels was localized to the uterine epithelia, it is possible that KP/KISS1R signaling regulates embryo implantation. For example, through p38 it might regulate the availability (production and/or secretion) of glandular products essential for implantation, or through both p38 and ERK1/2 might regulate embryo implantation at the uterine epithelium. It is also possible that through paracrine signaling, epithelial KP/KISS1R signaling prepares stromal cells for decidualization in the event of successful implantation [7, 16].

16 in total

Review 1. Role of uterine stromal-epithelial crosstalk in embryo implantation.

Authors: Alison M Hantak; Indrani C Bagchi; Milan K Bagchi
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2. Dependence of fertility on kisspeptin-Gpr54 signaling at the GnRH neuron.

Authors: Milen Kirilov; Jenny Clarkson; Xinhuai Liu; Juan Roa; Pauline Campos; Rob Porteous; Günther Schütz; Allan E Herbison
Journal: Nat Commun Date: 2013 Impact factor: 14.919

3. The metastasis suppressor gene KiSS-1 encodes kisspeptins, the natural ligands of the orphan G protein-coupled receptor GPR54.

Authors: M Kotani; M Detheux; A Vandenbogaerde; D Communi; J M Vanderwinden; E Le Poul; S Brézillon; R Tyldesley; N Suarez-Huerta; F Vandeput; C Blanpain; S N Schiffmann; G Vassart; M Parmentier
Journal: J Biol Chem Date: 2001-07-16 Impact factor: 5.157

4. LC-MS/MS quantification of a neuropeptide fragment kisspeptin-10 (NSC 741805) and characterization of its decomposition product and pharmacokinetics in rats.

Authors: Zhongfa Liu; Chen Ren; William Jones; Ping Chen; Stephanie B Seminara; Yee-Ming Chan; Nicola F Smith; Joseph M Covey; Jeffrey Wang; Kenneth K Chan
Journal: J Chromatogr B Analyt Technol Biomed Life Sci Date: 2013-03-04 Impact factor: 3.205

5. GPR54 regulates ERK1/2 activity and hypothalamic gene expression in a Gα(q/11) and β-arrestin-dependent manner.

Authors: Jacob M Szereszewski; Macarena Pampillo; Maryse R Ahow; Stefan Offermanns; Moshmi Bhattacharya; Andy V Babwah
Journal: PLoS One Date: 2010-09-23 Impact factor: 3.240

6. Disrupted kisspeptin signaling in GnRH neurons leads to hypogonadotrophic hypogonadism.

Authors: Horacio J Novaira; Momodou L Sonko; Gloria Hoffman; Yongbum Koo; Chemyong Ko; Andrew Wolfe; Sally Radovick
Journal: Mol Endocrinol Date: 2014-01-01

7. Kiss1-/- mice exhibit more variable hypogonadism than Gpr54-/- mice.

Authors: Risto Lapatto; J Carl Pallais; Dongsheng Zhang; Yee-Ming Chan; Amy Mahan; Felecia Cerrato; Wei Wei Le; Gloria E Hoffman; Stephanie B Seminara
Journal: Endocrinology Date: 2007-06-26 Impact factor: 4.736

8. Discovery of potent kisspeptin antagonists delineate physiological mechanisms of gonadotropin regulation.

Authors: Antonia K Roseweir; Alexander S Kauffman; Jeremy T Smith; Kathryn A Guerriero; Kevin Morgan; Justyna Pielecka-Fortuna; Rafael Pineda; Michelle L Gottsch; Manuel Tena-Sempere; Suzanne M Moenter; Ei Terasawa; Iain J Clarke; Robert A Steiner; Robert P Millar
Journal: J Neurosci Date: 2009-03-25 Impact factor: 6.167

9. Endogenous mammalian RF-amide peptides, including PrRP, kisspeptin and 26RFa, modulate nociception and morphine analgesia via NPFF receptors.

Authors: Khadija Elhabazi; Jean-Paul Humbert; Isabelle Bertin; Martine Schmitt; Frédéric Bihel; Jean-Jacques Bourguignon; Bernard Bucher; Jérôme A J Becker; Tania Sorg; Hamid Meziane; Benoit Petit-Demoulière; Brigitte Ilien; Frédéric Simonin
Journal: Neuropharmacology Date: 2013-08-02 Impact factor: 5.250

10. Expression and function of kisspeptin during mouse decidualization.

Authors: Peng Zhang; Min Tang; Ting Zhong; Yan Lin; Teng Zong; Chengxue Zhong; BaoPing Zhang; Min Ren; HaiBin Kuang
Journal: PLoS One Date: 2014-05-15 Impact factor: 3.240

9 in total

Review 1. The Role of Kisspeptin in the Pathogenesis of Pregnancy Complications: A Narrative Review.

Authors: Magdalena Szydełko-Gorzkowicz; Elżbieta Poniedziałek-Czajkowska; Radzisław Mierzyński; Maciej Sotowski; Bożena Leszczyńska-Gorzelak
Journal: Int J Mol Sci Date: 2022-06-14 Impact factor: 6.208

Review 2. From inhibition of trophoblast cell invasion to proapoptosis: what are the potential roles of kisspeptins in preeclampsia?

Authors: Viviane C L Gomes; Jenny L Sones
Journal: Am J Physiol Regul Integr Comp Physiol Date: 2021-05-19 Impact factor: 3.210

3. Uterine Gα_q/11 signaling, in a progesterone-dependent manner, critically regulates the acquisition of uterine receptivity in the female mouse.

Authors: Vanessa de Oliveira; Jennifer Schaefer; Michele Calder; John P Lydon; Francesco J DeMayo; Moshmi Bhattacharya; Sally Radovick; Andy V Babwah
Journal: FASEB J Date: 2019-05-15 Impact factor: 5.834

4. Kisspeptin treatment improves fetal-placental development and blocks placental oxidative damage caused by maternal hypothyroidism in an experimental rat model.

Authors: Bianca Reis Santos; Jeane Martinha Dos Anjos Cordeiro; Luciano Cardoso Santos; Erikles Macedo Barbosa; Letícia Dias Mendonça; Emilly Oliveira Santos; Isabella Oliveira de Macedo; Mário Sergio Lima de Lavor; Raphael Escorsim Szawka; Rogeria Serakides; Juneo Freitas Silva
Journal: Front Endocrinol (Lausanne) Date: 2022-07-28 Impact factor: 6.055

Review 5. Kisspeptins and Glucose Homeostasis in Pregnancy: Implications for Gestational Diabetes Mellitus-a Review Article.

Authors: Ezekiel Musa; Mushi Matjila; Naomi S Levitt
Journal: Reprod Sci Date: 2021-01-04 Impact factor: 3.060

6. Beyond the brain-Peripheral kisspeptin signaling is essential for promoting endometrial gland development and function.

Authors: Silvia León; Daniela Fernandois; Alexandra Sull; Judith Sull; Michele Calder; Kanako Hayashi; Moshmi Bhattacharya; Stephen Power; George A Vilos; Angelos G Vilos; Manuel Tena-Sempere; Andy V Babwah
Journal: Sci Rep Date: 2016-07-01 Impact factor: 4.379

7. Kisspeptin: A Potential Factor for Unexplained Infertility and Impaired Embryo Implantation.

Authors: Aaida Mumtaz; Aqsa Khalid; Zehra Jamil; Syeda Sadia Fatima; Sara Arif; Rehana Rehman
Journal: Int J Fertil Steril Date: 2017-02-16

8. Potential roles for the kisspeptin/kisspeptin receptor system in implantation and placentation.

Authors: Kai-Lun Hu; Hsun-Ming Chang; Hong-Cui Zhao; Yang Yu; Rong Li; Jie Qiao
Journal: Hum Reprod Update Date: 2019-05-01 Impact factor: 15.610

9. Peripheral action of kisspeptin at reproductive tissues-role in ovarian function and embryo implantation and relevance to assisted reproductive technology in livestock: a review.

Authors: Michael J D'Occhio; Giuseppe Campanile; Pietro S Baruselli
Journal: Biol Reprod Date: 2020-12-01 Impact factor: 4.285

9 in total