Fetal and maternal NLRP3 signaling is required for preterm labor and birth
Kenichiro Motomura, … , Adi L. Tarca, Nardhy Gomez-Lopez
Kenichiro Motomura, … , Adi L. Tarca, Nardhy Gomez-Lopez
Published August 22, 2022
Citation Information: JCI Insight. 2022;7(16):e158238. https://doi.org/10.1172/jci.insight.158238.
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Research Article Immunology Reproductive biology

Fetal and maternal NLRP3 signaling is required for preterm labor and birth

Abstract

Preterm birth is the leading cause of neonatal morbidity and mortality worldwide. One of every 4 preterm neonates is born to a mother with intra-amniotic inflammation driven by invading bacteria. However, the molecular mechanisms underlying this hostile immune response remain unclear. Here, we used a translationally relevant model of preterm birth in Nlrp3-deficient and -sufficient pregnant mice to identify what we believe is a previously unknown dual role for the NLRP3 pathway in the fetal and maternal signaling required for the premature onset of the labor cascade leading to fetal injury and neonatal death. Specifically, the NLRP3 sensor molecule and/or inflammasome is essential for triggering intra-amniotic and decidual inflammation, fetal membrane activation, uterine contractility, and cervical dilation. NLRP3 also regulates the functional status of neutrophils and macrophages in the uterus and decidua, without altering their influx, as well as maternal systemic inflammation. Finally, both embryo transfer experimentation and heterozygous mating systems provided mechanistic evidence showing that NLRP3 signaling in both the fetus and the mother is required for the premature activation of the labor cascade. These data provide insights into the mechanisms of fetal-maternal dialog in the syndrome of preterm labor and indicate that targeting the NLRP3 pathway could prevent adverse perinatal outcomes.

Authors

Kenichiro Motomura, Roberto Romero, Jose Galaz, Li Tao, Valeria Garcia-Flores, Yi Xu, Bogdan Done, Marcia Arenas-Hernandez, Derek Miller, Pedro Gutierrez-Contreras, Marcelo Farias-Jofre, Siddhesh Aras, Lawrence I. Grossman, Adi L. Tarca, Nardhy Gomez-Lopez

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Figure 3

Nlrp3 deficiency impairs LPS-induced fetal membrane activation.

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Nlrp3 deficiency impairs LPS-induced fetal membrane activation. (A) Pre...
(A) Pregnant Nlrp3+/+ and Nlrp3–/– mice were intra-amniotically injected with LPS (100 ng/25 μL) or PBS on 16.5 days post coitum (dpc). The fetal membranes were collected on 17.5 dpc. The spatial localization of the murine fetal membranes and a schematic diagram of the common pathway of labor are shown. (B) Heatmap visualization of inflammatory gene expression in the fetal membranes (n = 13–15 per group). (C) Expression of inflammation-associated genes in the fetal membranes (n = 13–15 per group). (D) Immunoblotting of pro-CASP and CASP-1 p20 in the fetal membranes (n = 6 per group). The expression was normalized by ACTB and shown as relative quantification. (E) Concentrations of total IL-1β in the fetal membranes (n = 8–9 per group). Values were adjusted by the total protein concentration in each sample. Data are shown as box-and-whisker plots where midlines indicate medians, boxes indicate interquartile ranges, and whiskers indicate minimum and maximum values. (F) Immunoblotting of mature IL-1β in fetal membrane lysates immunoprecipitated with anti–IL-1β antibody. Eight samples were pooled for each group. (G) Representative immunofluorescence images showing the expression of mature IL-1β in the fetal membranes (n = 3–4 per group). All images were taken at 200× original magnification. Scale bars represent 20 μm. Inset images show isotype control staining from the same case. The P values of the comparisons between PBS- and LPS-injected dams of each genotype were determined by Mann-Whitney U test. *P < 0.05; **P < 0.01; ***P < 0.001; (+) Ctrl., positive control.