MKRN3 inhibits puberty onset via interaction with IGF2BP1 and regulation of hypothalamic plasticity
Lydie Naulé, … , Ana Paula Abreu, Ursula B. Kaiser
Lydie Naulé, … , Ana Paula Abreu, Ursula B. Kaiser
Published April 24, 2023
Citation Information: JCI Insight. 2023;8(8):e164178. https://doi.org/10.1172/jci.insight.164178.
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Research Article Endocrinology Neuroscience

MKRN3 inhibits puberty onset via interaction with IGF2BP1 and regulation of hypothalamic plasticity

Abstract

Makorin ring finger protein 3 (MKRN3) was identified as an inhibitor of puberty initiation with the report of loss-of-function mutations in association with central precocious puberty. Consistent with this inhibitory role, a prepubertal decrease in Mkrn3 expression was observed in the mouse hypothalamus. Here, we investigated the mechanisms of action of MKRN3 in the central regulation of puberty onset. We showed that MKRN3 deletion in hypothalamic neurons derived from human induced pluripotent stem cells was associated with significant changes in expression of genes controlling hypothalamic development and plasticity. Mkrn3 deletion in a mouse model led to early puberty onset in female mice. We found that Mkrn3 deletion increased the number of dendritic spines in the arcuate nucleus but did not alter the morphology of GnRH neurons during postnatal development. In addition, we identified neurokinin B (NKB) as an Mkrn3 target. Using proteomics, we identified insulin-like growth factor 2 mRNA-binding protein 1 (IGF2BP1) as another target of MKRN3. Interactome analysis revealed that IGF2BP1 interacted with MKRN3, along with several members of the polyadenylate-binding protein family. Our data show that one of the mechanisms by which MKRN3 inhibits pubertal initiation is through regulation of prepubertal hypothalamic development and plasticity, as well as through effects on NKB and IGF2BP1.

Authors

Lydie Naulé, Alessandra Mancini, Sidney A. Pereira, Brandon M. Gassaway, John R. Lydeard, Kayleigh Rutherford, John C. Magnotto, Han Kyeol Kim, Joy Liang, Cynara Matos, Steven P. Gygi, Florian T. Merkle, Rona S. Carroll, Ana Paula Abreu, Ursula B. Kaiser

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Figure 3

Mkrn3 deletion in mice is associated with early onset of puberty in female mice and a tendency toward early puberty in male mice.

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Mkrn3 deletion in mice is associated with early onset of puberty in fem...
(A) Relative Mkrn3 mRNA levels in the ARC of Mkrn3WT and Mkrn3KO females across PND10, PND15, PND20, and PND25 (n = 6 per genotype and age). Statistics were performed using 2-way ANOVA, followed by Tukey’s post hoc test. (B) Representative Western blot autoradiographic image of Mkrn3 protein and β-actin in the MBH of Mkrn3WT and Mkrn3KO females at PND10. (C) Representative immunohistochemistry images of Mkrn3 protein in the POA and the arcuate nucleus (ARC) of Mkrn3WT and Mkrn3KO females at PND10. Scale bar = 100 μm. 3V, third ventricle. (DG) Age at vaginal opening (D) and cumulative percentage of female mice exhibiting vaginal opening (E), and age at first estrus (F) and cumulative percentage of female mice with first estrus (G), in Mkrn3WT (n = 8) and Mkrn3KO (n = 10) females. (H) Age at preputial separation and (I) cumulative percentage of male mice exhibiting preputial separation in Mkrn3WT (n = 10) and Mkrn3KO (n = 11) males. Statistics were performed using unpaired 2-tailed t test. (J) Body weight of Mkrn3WT (n = 11) and Mkrn3KO (n = 15) male and Mkrn3WT (n = 8) and Mkrn3KO (n = 10) female mice measured weekly from weaning (PND21) to adulthood (PND84). Statistics were performed using 2-way ANOVA, followed by Tukey’s post hoc test. Data are presented as the mean ± SEM values. *P < 0.05, ***P < 0.0001 of Mkrn3KO compared with Mkrn3WT.