DNASE-I HYPERSENSITIVITY SITES AND NUCLEAR-PROTEIN BINDING ON THE FATTY-ACID SYNTHASE GENE - IDENTIFICATION OF AN ELEMENT WITH PROPERTIES SIMILAR TO KNOWN GLUCOSE-RESPONSIVE ELEMENTS

We have shown previously that fatty acid synthase (FAS) gene expression is positively regulated by glucose in rat adipose tissue and liver. In the present study, we have identified in the first intron of the gene a sequence closely related to known glucose-responsive elements such as in the L-pyruvate kinase and S14 genes, including a putative upstream stimulatory factor/major late transcription factor (USF/MLTF) binding site (E-box) (+292 nt to +297 nt), Location of this sequence corresponds to a site of hypersensitivity to DNase I which is present in the liver but not in the spleen, Moreover, using this information from a preliminary report of the present work, others have shown that a +283 nt to +303 nt sequence of the FAS gene can confer glucose responsiveness to a heterologous promoter, The protein binding to this region has been investigated in vitro by a combination of DNase I footprinting and gel-retardation experiments with synthetic oligonucleotides and known nuclear proteins. DNase I footprinting experiments using a +161 nt to +405 nt fragment of the FAS gene demonstrate that a region from +290 nt to +316 nt is protected by nuclear extracts from liver and spleen, This region binds two ubiquitous nuclear factors, USF/MLTF and the CAAT-binding transcription factor/nuclear factor 1 (CTF/NF1). Binding of these factors is similar in nuclear extracts from liver which does or does not express the FAS gene as observed for glucose-reponsive elements in the L-pyruvate kinase and S14 genes, This suggests a posttranslational modification of a factor of the complex after glucose stimulation.