Involvement of RelA-Associated Inhibitor in Regulation of Trophoblast Differentiation via Interaction with Transcriptional Factor Specificity Protein-1

Author:

Minekawa Ryoko1,Sakata Masahiro1,Okamoto Yoko1,Hayashi Masami1,Isobe Aki1,Takeda Takashi2,Yamamoto Toshiya3,Koyama Masayasu1,Ohmichi Masahide1,Tasaka Keiichi1,Imai Kenichi4,Okamoto Takashi4,Murata Yuji1

Affiliation:

1. Department of Obstetrics and Gynecology (R.M., M.S., Y.O., M.H., A.I., M.K., M.O., K.T., Y.M.), Osaka University Graduate School of Medicine, Osaka 565-0871, Japan;

2. Department of Gynecology (T.T.), Osaka Medical Center for Cancer and Cardiovascular Diseases, Osaka 594-1101, Japan;

3. Department of Obstetrics and Gynecology (T.Y.), Sakai Municipal Hospital, Sakai 221-1700, Japan;

4. Department of Molecular and Cellular Biology (K.I., T.O.), Nagoya City University Graduate School of Medical Sciences, Nagoya 464-8601, Japan

Abstract

Glucose transporter-1 (GLUT1), one of the key functional indicators of placental differentiation, has an important role in placental glucose transport. We previously showed that the protein levels of GLUT1 and nuclear transcription factor specificity protein-1 (Sp1) in rat choriocarcinoma cells (Rcho-1 cells) decreased during the differentiation of these cells to giant cells. We also showed that Sp1 was involved in the regulation of GLUT1 gene expression during this process. RelA-associated inhibitor (RAI) is an inhibitor of nuclear factor-κB that was identified by a yeast two-hybrid screen and is preferably expressed in human placenta and heart. RAI was also found to interact with Sp1 and exert an inhibitory effect against the DNA-binding activity of Sp1. We first show here that RAI mRNA expression increased as gestation proceeded and that RAI was localized mainly in the syncytiotrophoblast throughout pregnancy. The chloramphenicol acetyltransferase activity assay in Rcho-1 cells revealed that cotransfection of RAI expression vector resulted in decreased activity of the rat GLUT1 promoter but not in that of a mutated rat GLUT1 promoter lacking the Sp1 binding site. Furthermore, the protein level of RAI increased during differentiation. In addition, transfection of RAI expression vector promoted the morphological differentiation of Rcho-1 cells, and RAI knockdown using RAI-specific small interfering RNA reveals inhibitory effects on the morphological differentiation, as assessed by photomicroscopy. Taken together, these findings suggest that RAI may be involved in the regulation of trophoblast differentiation via interaction with Sp1.

Publisher

The Endocrine Society

Subject

Endocrinology

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