A multiple cytokine- and second messenger-responsive element in the enhancer of the human interleukin-6 gene: similarities with c-fos gene regulation.

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Mol Cell Biol. 1989 December; 9(12): 5537-5547

A multiple cytokine- and second messenger-responsive element in the enhancer of the human interleukin-6 gene: similarities with c-fos gene regulation.

A Ray, P Sassone-Corsi and P B Sehgal

Rockefeller University, New York, New York 10021.

ABSTRACT

Interleukin-6 (IL-6) is a major systemic alarm signal that indicatesthe occurrence of tissue damage. The IL-6 gene is induced invarious cell types by serum, inflammation-associated cytokines,viruses, and second-messenger agonists. There is an overallfunctional similarity between IL-6 and c-fos promoters, sincetransfection of excess amounts of either promoter DNA into intactHeLa cells modulates the function of the heterologous promoterconstruct. Furthermore, the transcription regulatory factorFos transrepresses both the IL-6 and c-fos promoters. The 115-basepair (bp) region from -225 to -111 in the IL-6 5'-flanking region,which shares nucleotide sequence similarity with the c-fos serumresponse (SRE) and adjacent AP-1-like (the CGTCA motif) elements,confers responsiveness to several reagents, including serum,forskolin, and phorbol ester, upon the heterologous herpesvirusthymidine kinase (TK) promoter. In gel shift assays using nuclearextracts from HeLa cells, the 115-bp IL-6 enhancer formed severalcomplexes that (i) were increased when extracts from inducedHeLa cells were used and (ii) were inhibited most efficientlyby the fos E DNA fragment (-700 to -100) and by c-fos oligonucleotidescontaining an intact AP-1-like site (the CGTCA motif). The 23-bpoligonucleotide designated AR1 from within the IL-6 enhancerregion (-173 to -151) contains a CGTCA motif and bound nuclearproteins that also associated with c-fos oligonucleotides containingeither an intact SRE or AP-1-like site. A single copy of AR1inserted upstream of the herpesvirus TK promoter rendered thisheterologous promoter inducible by IL-1 alpha, tumor necrosisfactor, and serum as well as by activators of the protein kinaseA (forskolin) and protein kinase C (phorbol ester) signal transductionpathways. Mutations in the AP-1-like site within AR1 (CGTCA----GTTCA)decreased inducibility of the chimeric IL-6/TK/chloramphenicolacetyltransferase gene by phorbol ester and by forskolin butnot by serum, IL-1 alpha, or tumor necrosis factor. These datanot only show that the AR1 segment from within the IL-6 enhancerbinds nuclear proteins that also bind to c-fos regulatory elementsbut also demonstrate that a single copy of this 23-bp elementis functionally sufficient to confer responsiveness to a varietyof inducers and thus define a multiple-response element.

Mol Cell Biol. 1989 December; 9(12): 5537-5547

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