Identification of a conserved lipopolysaccharide-plus-interleukin-4-responsive element located at the promoter of germ line epsilon transcripts.

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Mol Cell Biol. 1991 November; 11(11): 5551-5561

Identification of a conserved lipopolysaccharide-plus-interleukin-4-responsive element located at the promoter of germ line epsilon transcripts.

P Rothman, S C Li, B Gorham, L Glimcher, F Alt and M Boothby

Howard Hughes Medical Institute, Columbia University College of Physicians and Surgeons, New York, New York 10032.

ABSTRACT

Treatment of splenic B lymphocytes and certain B-lineage celllines with the mitogen lipopolysaccharide (LPS) and the lymphokineinterleukin-4 (IL-4) induces expression of germ line immunoglobulinC epsilon transcripts and class switching to the C epsilon gene.We show that LPS-plus-IL-4 induction of germ line epsilon transcripts(termed I epsilon transcripts) occurs at the transcriptionallevel in an Abelson murine leukemia virus-transformed pre-B-cellline. A 1.1-kb region of DNA surrounding the I epsilon promoterendows inducible transcription to a heterologous reporter genestably transfected into these cells; such inducible expressiondepends on combined treatment with LPS and IL-4. Analyses ofconstructs transiently introduced into a B-cell lymphoma linedemonstrated that LPS-plus-IL-4-inducible expression can beconferred by a 179-bp segment of DNA spanning the I epsilontranscriptional initiation site. Mutational analyses demonstratedthat this expression depended on DNA sequences within a conservedregion directly upstream from the I epsilon transcriptionalinitiation region. One nuclear protein that is constitutivelyexpressed in normal B cells binds to the downstream end of theconserved sequence; its binding specificity correlates withthe functional effect of several mutations. Two additional proteins,which are induced by IL-4 treatment of splenic B cells, bindto the transcription initiation sites of I epsilon. These proteinsare indistinguishable in binding assays from proteins previouslyshown to bind an enhancer region of the class II major histocompatibilitycomplex gene A alpha.

Mol Cell Biol. 1991 November; 11(11): 5551-5561

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