4.6 Article

CpG methylation suppresses transcriptional activity of human syncytin-1 in non-placental tissues

Journal

EXPERIMENTAL CELL RESEARCH
Volume 312, Issue 7, Pages 1011-1020

Publisher

ELSEVIER INC
DOI: 10.1016/j.yexcr.2005.12.010

Keywords

syncytin-1; human endogenous retroviruses W; trophoblast cells; cell fusion; placenta; DNA methylation

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Syncytin-1 is a captive envelope glycoprotein encoded by one of human endogenous retroviruses W. It is expressed exclusively in the placental trophoblast where it participates in cell-to-cell fusion during differentiation of syncytiotrophobast. In other tissues, however, syncytin-1 expression must be kept in check because inadvertent cell fusion might be dangerous for tissue organization and integrity. We describe here an inverse correlation between CpG methylation of syncytin-1 51 long terminal repeat and its expression. Hypomethylation of the syncytin-1 51 long terminal repeat in the placenta and in the choriocarcinoma-derived cell line BeWo was detected. However, other analyzed primary cells and cell lines non-expressing syncytin-1 contain proviruses heavily methylated in this sequence. CpG methylation of syncytin-1 is resistant to the effect of the demethylating agent 5-azacytidine. The inhibitory role of CpG methylation is further confirmed by transient transfection of in-vitro-methylated syncytin-1 promoter-driven reporter construct. Altogether, we conclude that CpG methylation plays a principal role in the transcriptional suppression of syncytin-1 in non-placental tissues, and, in contrast, demethylation of the syncytin-1 promoter in trophoblast is a prerequisite for its expression and differentiation of multinucleated syncytiotrophoblast. (c) 2005 Elsevier Inc. All rights reserved.

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