ATG16L1 governs placental infection risk and preterm birth in mice and women
Bin Cao, … , Colin Macones, Indira U. Mysorekar
Bin Cao, … , Colin Macones, Indira U. Mysorekar
Published December 22, 2016
Citation Information: JCI Insight. 2016;1(21):e86654. https://doi.org/10.1172/jci.insight.86654.
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Research Article Microbiology Reproductive biology

ATG16L1 governs placental infection risk and preterm birth in mice and women

Abstract

The placenta is a barrier against maternal-fetal transmission of pathogens. Placental infections can cause several adverse pregnancy outcomes, including preterm birth (PTB). Yet, we have limited knowledge regarding the mechanisms the placenta uses to control infections. Here, we show that autophagy, a cellular recycling pathway important for host defense against pathogens, and the autophagy gene Atg16L1 play a key role in placental defense and are negatively associated with PTB in pregnant women. First, we demonstrate that placentas from women who delivered preterm exhibit reduced autophagy activity and are associated with higher infection indicators. Second, we identify the cellular location of the autophagy activity as being in syncytial trophoblasts. Third, we demonstrate that higher levels of autophagy and ATG16L1 in human trophoblasts were associated with increased resistance to infection. Accordingly, loss of autophagy or ATG16L1 impaired trophoblast antibacterial defenses. Fourth, we show that Atg16l1-deficient mice gave birth prematurely upon an inflammatory stimulus and their placentas were significantly less able to withstand infection. Finally, global induction of autophagy in both mouse placentas and human trophoblasts increased infection resistance. Our study has significant implications for understanding the etiology of placental infections and prematurity and developing strategies to mitigate placental infection–induced PTB.

Authors

Bin Cao, Colin Macones, Indira U. Mysorekar

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Figure 4

ATG16L1 in STBs regulates resistance to infection.

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ATG16L1 in STBs regulates resistance to infection. (A) Western blot dete...
(A) Western blot detection of autophagy proteins ATG16L1, ATG7, BECLIN-1 and LC3 in BeWo CTBs and STBs and quantification of ATG16L1 protein levels in CTBs and STBs. Mean values ± SEM of 3 independent experiments. (B) Western blot detection of ATG16L1 in STBs after exposure to control or ATG16L1-specific siRNA. (C) Quantification of bacterial load in STBs treated with control or ATG16L1-specific siRNA. The graph shows mean values ± SEM of 4 independent experiments. *P < 0.05, **P < 0.01 by Mann-Whitney U test.