Induction of the mouse serum amyloid A3 gene by cytokines requires both C/EBP family proteins and a novel constitutive nuclear factor.

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Mol Cell Biol. 1994 July; 14(7): 4475-4484

Induction of the mouse serum amyloid A3 gene by cytokines requires both C/EBP family proteins and a novel constitutive nuclear factor.

J H Huang and W S Liao

Department of Biochemistry and Molecular Biology, University of Texas M. D. Anderson Cancer Center, Houston 77030.

ABSTRACT

Serum amyloid A (SAA) is a major acute-phase protein synthesizedand secreted mainly by the liver. In response to acute inflammation,its expression may be induced up to 1,000-fold, primarily asa result of a 200-fold increase in the rate of SAA gene transcription.We have previously demonstrated that a 350-bp promoter fragmentfrom the mouse SAA3 gene was necessary and sufficient to conferliver-specific and cytokine-induced expression. Deletion studiesidentified a distal response element that is responsible forthe cytokine response and has properties of an inducible transcriptionalenhancer. In this study, we further analyzed the distal responseelement and showed that it consists of three functionally distinctelements: the A element constitutes a weak binding site forC/EBP family proteins, the B element also interacts with C/EBPfamily proteins but with a much higher binding affinity, andthe C element interacts with a novel constitutive nuclear factor,SEF-1. Site-specific mutation studies revealed that all threeelements were required for maximum promoter activity. C/EBPalpha, C/EBP beta, and C/EBP delta were capable of interactingwith elements A and B. Under noninduced conditions, C/EBP alphawas the major binding factor; however, upon cytokine stimulationC/EBP beta- and C/EBP delta-binding activities were dramaticallyincreased and became the predominant binding factors. Consistentwith these binding studies were the cotransfection experimentsin which C/EBP beta and C/EBP delta were shown to be potenttransactivators for the SAA3 promoter. Moreover, the transactivationrequired an intact B element despite the presence of other functionalC/EBP-binding sites. Interestingly, although element C did notinteract with C/EBP directly, it was nevertheless required formaximum transactivation by C/EBP delta. Our studies thus demonstratethat both C/EBP family proteins and SEF-1 are required to transactivatethe SAA3 gene.

Mol Cell Biol. 1994 July; 14(7): 4475-4484

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