A striking similarity in the organization of the E-selectin and beta interferon gene promoters.

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Mol Cell Biol. 1994 October; 14(10): 6464-6475

A striking similarity in the organization of the E-selectin and beta interferon gene promoters.

M Z Whitley, D Thanos, M A Read, T Maniatis and T Collins

Department of Pathology, Brigham and Women's Hospital, Boston, Massachusetts 02115.

ABSTRACT

Transcription of the endothelial leukocyte adhesion molecule1 (E-selectin or ELAM-1) gene is induced by the inflammatorycytokines interleukin-1 beta and tumor necrosis factor alpha(TNF-alpha). In this report, we identify four positive regulatorydomains (PDI to PDIV) in the E-selectin promoter that are requiredfor maximal levels of TNF-alpha induction in endothelial cells.In vitro DNA binding studies reveal that two of the domainscontain novel adjacent binding sites for the transcription factorNF-kappa B (PDIII and PDIV), a third corresponds to a recentlydescribed CRE/ATF site (PDII), and a fourth is a consensus NF-kappaB site (PDI). Mutations that decrease the binding of NF-kappaB to any one of the NF-kappa B binding sites in vitro abolishedcytokine-induced E-selectin gene expression in vivo. Previousstudies demonstrated a similar correlation between ATF bindingto PDII and E-selectin gene expression. Here we show that thehigh-mobility-group protein I(Y) [HMG I(Y)] also binds specificallyto the E-selectin promoter and thereby enhances the bindingof both ATF-2 and NF-kappa B to the E-selectin promoter in vitro.Moreover, mutations that interfere with HMG I(Y) binding decreasethe level of cytokine-induced E-selectin expression. The organizationof the TNF-alpha-inducible element of the E-selectin promoteris remarkably similar to that of the virus-inducible promoterof the human beta interferon gene in that both promoters requireNF-kappa B, ATF-2, and HMG I(Y). We propose that HMG I(Y) functionsas a key architectural component in the assembly of inducibletranscription activation complexes on both promoters.

Mol Cell Biol. 1994 October; 14(10): 6464-6475

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