EVALUATION OF THE ROLE OF AP1-LIKE PROTEINS IN THE ENHANCED APOLIPOPROTEIN-E GENE-TRANSCRIPTION ACCOMPANYING PHORBOL ESTER-INDUCED MACROPHAGE DIFFERENTIATION

Differentiation of THP1 monocytes to a macrophage phenotype is accompanied by increased apolipoprotein E gene transcription. Using transfection analysis with 5' deletion mutations of the 5' control region of the apo E gene in THP1 cells, we show that the -651 to +86 chloramphenicol acetyltransferase (CAT) construct is efficiently expressed in the monocyte; as has been reported for other cell types. Further, we found that an 176 bp region between -623 to -447 was required for the induction of apolipoprotein E gene transcription during 12-O-tetradecanoylphorbol-13-acetate-induced differentiation of monocytes to macrophages. Gel-retardation patterns of the apolipoprotein E promoter region using nuclear extracts from differentiated or undifferentiated THP1 cells revealed altered binding of Ap1-like nuclear factor/s to the -620 to -583 bp region after macrophage differentiation. Mutation of an Ap1 element at position -602 abolished specific binding of Ap1-like proteins to the -620 to -583 bp fragment of the apo E gene and significantly reduced expression of a -623 to +86 apo E-CAT construct during differentiation. These data indicate that differentiation-related expression of the apolipoprotein E gene following phorbol ester stimulation is transduced by gene elements between -623 and -447. Furthermore, the data indicate that transcriptional activation of the apo E gene during macrophage differentiation is associated with induction of Ap1-like proteins which bind to the Ap1 response element present at -602 in the apolipoprotein E gene and importantly contribute to enhanced gene expression.