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Inhibition of TGF-β3 restores the invasive capability of extravillous trophoblasts in preeclamptic pregnancies
Isabella Caniggia, … , Martin Post, Stephen J. Lye
Isabella Caniggia, … , Martin Post, Stephen J. Lye
Published June 15, 1999
Citation Information: J Clin Invest. 1999;103(12):1641-1650. https://doi.org/10.1172/JCI6380.
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Article

Inhibition of TGF-β3 restores the invasive capability of extravillous trophoblasts in preeclamptic pregnancies

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Abstract

Preeclampsia, the major cause of maternal morbidity and mortality in developed countries, is associated with abnormalities of placenta function due to shallow invasion of the maternal decidua by trophoblasts. Data suggest that TGF-β may play a role in inhibiting trophoblast outgrowth or invasion, or both. We report that placental TGF-β3 expression is high in early pregnancy but falls at around 9 weeks’ gestation. This pattern is inversely correlated with trophoblast outgrowth and fibronectin synthesis, markers of early trophoblast differentiation toward an invasive phenotype. We demonstrate that TGF-β3 is overexpressed in preeclamptic placentae. In contrast to control placentae, explants from preeclamptic pregnancies fail to exhibit spontaneous invasion in vitro. Significantly, antisense-induced inhibition of TGF-β3 expression, and inhibition of TGF-β3 activity with antibodies, induces the formation of columns of trophoblast cells, which migrate out of the explant into the underlying Matrigel. To our knowledge, this is the first demonstration that the hypoinvasive placental phenotype characteristic of preeclampsia can be essentially normalized in vitro by biochemical manipulation. We speculate that a failure to downregulate expression of TGF-β3 at around 9 weeks’ gestation results in shallow trophoblast invasion and predisposes the pregnancy to preeclampsia.

Authors

Isabella Caniggia, Sorina Grisaru-Gravnosky, Maciej Kuliszewsky, Martin Post, Stephen J. Lye

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Figure 2

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Trophoblast differentiative capability of villous explants is gestationa...
Trophoblast differentiative capability of villous explants is gestational age dependent. Villous explants from first-trimester gestation (5–13 weeks) were cultured for 6 days. Differentiation was monitored by measuring morphological and biochemical markers of trophoblast differentiation. (a) EVT cell outgrowth and migration were expressed as the ratio of EVT outgrowths per villous tip, where the nominator, EVT outgrowths, represents the number of EVT columns sprouting from the villous tips plus the number of islands of EVT invading into the Matrigel. The denominator represents the total number of villous tips in a single explant culture. (b) At day 5, explants were metabolically labeled with [35S]methionine for 18 hours. Fibronectin was isolated from conditioned medium using gelatin-Sepharose beads on the protein extract separated by SDS PAGE. Radiolabeled bands were quantified with the use of a PhosphorImager. Data represent the mean ± SEM of 6–10 different experiments performed in triplicate. *P < 0.05, by ANOVA, compared with 5–7 weeks’ gestation. #P < 0.05, by ANOVA, compared with 8 weeks’ gestation.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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