1. The proximal promoter of the human cathepsin G gene conferring myeloid-specific expression includes C/EBP, c-myb and PU.1 binding sites
- Author
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Urban Gullberg, Andreas Lennartsson, Anders Lindmark, and Daniel Garwicz
- Subjects
Cathepsin G ,Recombinant Fusion Proteins ,Molecular Sequence Data ,Cathepsin D ,Cathepsin E ,Cathepsin F ,Biology ,Response Elements ,Transfection ,Cathepsin B ,chemistry.chemical_compound ,Proto-Oncogene Proteins c-myb ,Cathepsin H ,Cathepsin L1 ,Cell Line, Tumor ,Proto-Oncogene Proteins ,Genetics ,Humans ,Myeloid Cells ,Luciferases ,Promoter Regions, Genetic ,Regulation of gene expression ,Binding Sites ,Base Sequence ,Serine Endopeptidases ,General Medicine ,U937 Cells ,Hematology ,Molecular biology ,Cathepsins ,GC Rich Sequence ,DNA-Binding Proteins ,Gene Expression Regulation, Neoplastic ,chemistry ,Mutation ,CCAAT-Enhancer-Binding Proteins ,Mutagenesis, Site-Directed ,Trans-Activators ,Transcription Initiation Site ,K562 Cells - Abstract
Cathepsin G is a hematopoietic serine protease stored in the azurophil granules of neutrophil granulocytes. The mRNA of cathepsin G is transiently expressed during the promyelocyte stage of neutrophil maturation. The protease plays several roles in inflammatory actions of neutrophils, such as bactericidal effects. A human cathepsin G gene fragment of 6 kb directs a promyelocyte-specific expression in transgenic mice, indicating the presence of necessary cis-acting elements. However, neither the precise architecture of the promoter, nor the trans-acting factors responsible for its activation, have been characterized. In the present work, 2.6 kb upstream of the translation start site of the human cathepsin G gene was cloned. When transfected to monoblast-like U937 or to acute promyelocytic leukemia NB4 cells, both expressing endogenous cathepsin G, the initial 360 bp upstream of the translation start were sufficient to direct a strong expression of a luciferase reporter gene. No expression was observed in erythroid K562 control cells. Further deletions revealed three major regulatory regions containing the consensus binding-sites for the transcription factors C/EBP, c-myb and PU.1. Moreover, a GC-rich region, similar to a cis-element in the proteinase 3 promoter, was identified. Direct binding of the trans-factors C/EBPalpha, C/EBPepsilon, c-myb and PU.1 to the promoter was shown by chromatin immunoprecipitation. The functional significance of the cis-elements was verified by site-directed mutagenesis. Mutations of the putative PU.1 site moderately decreased the activity of the promoter in monoblastic U937 cells, but not in promyelocytic NB4 cells. Separate mutations of the putative C/EBP binding site, c-myb-binding site or the GC-rich element resulted in a dramatically reduced transcriptional activity in both cell lines, suggesting cooperation between corresponding trans-factors.
- Published
- 2005