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Endocrinology, doi:10.1210/en.2004-0223
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Endocrinology Vol. 146, No. 1 383-391
Copyright © 2005 by The Endocrine Society

Cell-Specific Expression of Glucose-Dependent-Insulinotropic Polypeptide Is Regulated by the Transcription Factor PDX-1

Lisa I. Jepeal, Yoshio Fujitani, Michael O. Boylan, Cherrell N. Wilson, Christopher V. Wright and M. Michael Wolfe

Section of Gastroenterology (L.I.J., M.O.B., C.N.W., M.M.W.), Boston University School of Medicine and Boston Medical Center, Boston, Massachusetts 02118; and Department of Cell and Developmental Biology (Y.F., C.V.W.), Vanderbilt University Medical Center, Nashville, Tennessee 37232

Address all correspondence and requests for reprints to: M. Michael Wolfe, M.D., Section of Gastroenterology, Boston Medical Center, 650 Albany Street, Boston, Massachusetts 02118. E-mail: michael.wolfe{at}bmc.org.

Glucose-dependent insulinotropic polypeptide (GIP) is a potent stimulator of insulin secretion and comprises an important component of the enteroinsular axis. GIP is synthesized in enteroendocrine K-cells located principally in the upper small intestine. The homeobox-containing gene PDX-1 is also expressed in the small intestine and plays a critical role in pancreatic development and in the expression of pancreatic-specific genes. Previous studies determined that the transcription factors GATA-4 and ISL-1 are important for GIP expression. In this study, we demonstrate that PDX-1 is also involved in regulating GIP expression in K-cells. Using immunohistochemistry, we verified the expression of PDX-1 protein in the nucleus of GIP-expressing mouse K-cells and evaluated the expression of PDX-1, serotonin, and GIP in wild-type and PDX-1–/– mice at 18.5 d after conception. Although we demonstrated a 97.8% reduction in the number of GIP-expressing cells in PDX-1–/– mice; there was no statistical difference in the number of serotonin-positive cells. Additionally, PDX-1 transcripts and protein were detected in a GIP-expressing neuroendocrine cell line, STC-1. Electromobility shift assays using STC-1 nuclear extracts demonstrated the specific binding of PDX-1 protein to a specific regulatory region in the GIP promoter. Using chromatin immunoprecipitation analysis, we demonstrated binding of PDX-1 to this same region of the GIP promoter in intact cells. Lastly, overexpression of PDX-1 in transient transfection assays led to a specific increase in the activity of GIP/Luc reporter constructs. The results of these studies indicate that the transcription factor PDX-1 plays a critical role in the cell-specific expression of the GIP gene.




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