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Promoters and transcription factors Context Transcription -The conversion of DNA information to RNA information. Happens before splicing Mechanism for transcription is RNA polymerase. Followed by translation - The conversion of RNA information to amino acid sequence RNA polymerase >10 subunits Several types I-III Type II is involved in "gene" transcription. Type I and III transcribe ribosomal and transfer RNA Characteristics of transcription Polymerase does not recognise its promoter directly, only through use of promoters can transcription take place. TBP (TATA box) is a common element in initiation complex but may not bind to a TATA box in all cases TBP binds Several in the minor groove other transcription factors must also bind How transcription elements are discovered Use of a reporter system Procedural, makes the enzyme assay routine Artifacts present, not all factors will be present Chop off the DNA until you get a change in the reporter enzyme levels Mutate a potential site (Single bp changes) Consensus sequences Promoters vs Enhancers Characteristics of each Promoters <200 bp from start Enhancers < 'several kb' May end up closer due to bending Typically more global regulatory elements, tissue or time specific Enhancers several closely packed sites Promoters more dispersed Both consist of < 10 bp elements Example: CAAT Box " " " Sequence is used by alpha globin, adenovirus, fibrinogen, two proteins from rat liver Other sequences around CAAT box probably influence what actually gets bound to the CAAT box A conserved DNA element does not necessarily imply that the same regulatory element is binding. Enhancers " Can be either upstream or downstream. " Could change density of supercoiling. " Provide an entry site for the polymerase. " Anchor the DNA at a place within the cell for access. " Silencers " Insulators Genomic structure " A obvouly recent field " Look at the genome anatomy " Top down look at the problem TRANSFAC " " Database of transcription factors Classifed by a system similar to EC number, but not directly compairable " Open (to non comerical) and updateable " Utilized by a variety of tools Sequence repeats May have different densities Called microsatellite DNA TTAGGG on the ends on chromosome at the telomeres Transposable elements 35% of human genome is TE >50% of corn is TE 1.8% of C. elegans is TE 15% of Drosophila is TE Types of TE's LTR's (Long terminal repeats) Retroviruse elements Short 80-300bp segments SINES And longer 6-8 kb segments LINES Psuedogenes " A snapshot of evolution " New gene functions gained by gene duplication. " The duplicated gene is then free to mutate " processed psudeogenes, no introns or promoter regions, thought to be due to RT Synteny " " " Fancy word for gene order The sequence of a gene may change much faster than the order of the genes May be a very useful confirmation or hint of the function of a gene Operon/clusters " " " " It is normal for a prokaryote to transcribe clusters of genes which are translated toghter as well. May cluster genes working on the same metabolic process togther Eukaryotes there is not the co-transcription and the clustering is not found Gene order is still very conserved ACR " Ancient conserved regions " 20-40% of coding sequences are ACRs " Possibly represent proteins present at the time of prokaryotic/eukaryotic split Horozontal gene transfer " As opposed to vertical transer (inheritance) " Mitochondira/Chloroplasts " Significant in bacteria 12.8% in E. coli