Effect of levetiracetam on the gene expression of placental transporters in a murine model.

Abstract

Levetiracetam (LEV) is an antiseizure medication prescribed to women during childbearing age. The impact of LEV on placental transporters is poorly understood. This study aimed to assess the effect of LEV exposure on the messenger RNA (mRNA) expression of placental transporters for hormones and nutrients and to correlate their expression with the drug's serum concentration in pregnant mice. Studies were conducted on gestational days (GD) 13 and 18, following oral treatment with 100mg/kg LEV or the vehicle every 24h after weaning. Serum LEV measurements were performed by High-performance liquid chromatography with a UV detector (HPLC-UV). The weight, height, and width of the fetuses were also analyzed. In addition, the placental expression of transporters xCt, Lat1, Oatp4a1, Fr-α, Rfc, and Snat4 was evaluated through semi-quantitative real-time polymerase chain reaction (qPCR). The Kruskal-Wallis and the Mann-Whitney U tests were used to determine the statistical significance (p<.05). The correlation between serum LEV concentration and placental gene expression was evaluated using the Spearman test. The weight, height, and width were lower in the fetuses exposed to LEV compared with the control group (p<.05). The number of fetuses was lower in the LEV-exposed group than in the control GD 13group (p<.001). No significant differences were detected in the mRNA expression level at GD 13. At GD 18, the expression of Lat1, Oatp4a1, xCT, and Snat4 was higher in the group treated with LEV compared with the control group (p<.05), whereas the expression of Rfc was lower (p<.05). No correlation was identified between serum LEV concentrations and gene expression levels. The repression of the Rfc transcript by LEV at GD 18 suggests that the protein expression would be abolished contributing to the observed intrauterine growth restriction (IUGR). Furthermore, the significant increase in mRNA of xCt, Snat4, Oatp4a1, and Lat1 might be a compensatory mechanism for fetal survival at GD 18.