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Core promoter

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recognition site for the basal transcription apparatus ... Inr: centered at position 1; ~25% of promoters. TATA box: centered at -40; ~20% of promoters ... – PowerPoint PPT presentation

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Title: Core promoter


1
Core Promoters Transcription Start Sites
  • Core promoter
  • region of 100 bp flanking the transcription
    start site
  • recognition site for the basal transcription
    apparatus
  • Implicated in gene regulation, not just
    initiation
  • Identified sequence motifs
  • Inr centered at position 1 25 of promoters
  • TATA box centered at -40 20 of promoters
  • DPE centered at 20 8 of promoters
  • DRE DNA replication-related-element 25
  • 6 more motifs defined computationally

2
Transcription Start Sites
  • Full-Length cDNAs
  • Cap-trapped libraries
  • 5 ESTs directed cDNA screening
  • 5 RACE primer extension
  • Whole genome tiling arrays
  • Tissue- and stage-specificity
  • Alternative 5 exons
  • Comparative genomics may help

3
Core Promoter Prediction Example of Ohler et al.
2002
  • Selected 2,000 clusters of 5 ESTs
  • 3 ESTs within 11 bp
  • 1 cap-trapped EST
  • 5-most EST defines position 1
  • Find overrepresented words
  • Search within -60 to 40
  • MEME finds 10 sequence motifs 4 known and 6
    novel
  • Re-train and run McPromoter
  • Evaluate on Adh region and chromosome arm 2R
  • Sensitivity / Specifity 65 / 29 to 19 / 69
    (threshold-dependent)
  • Conclusion Good enough to direct wet lab
    experiments

4
P-elements Target Promoters
  • gt 50,000 mapped insertions
  • Insertions associated with 40 of genes

5
Drosophila Promoter Annotation
P-element insertion sites Promoter
predictions Curated gene models - open boxes
5UTRs
6
DNase I Hypersensitive Sites
  • Sites of Accessible or Open Chromatin
  • Southern Blot Assay Method
  • Partial digestion of chromatin with DNase I
  • Complete digestion with a restriction enzyme
  • Southern blot to identify and locate site(s)
  • DNase digest is partial, so fragments are
    size-fractionated prior to detection
  • Related Methods
  • Restriction enzyme hypersensitivity
  • Chemical modification

7
Additional Methods
  • ENCODE Methods
  • ChIP-chip of proteins at promoters
  • RNA pol II, TBP, etc.
  • Transfection of reporter constructs
  • DNase I hypersensitive sites
  • EST-like sequencing of plasmid libraries
  • Quantitative PCR detection
  • Other Approaches
  • In vitro transcription assays
  • What else?

8
Sample ENCODE Region (Fig.3)
  • Promoter finding methods correlate with each
    other and with 5 exons
  • Functional assays of constructs look good
  • RNA Pol II ChIP-chip can be very effective and
    scales to the genome
  • DNaseI hypersenstitve sites correlate with
    promoters
  • Some genes appear to have promoters at both ends
    antisense?

9
Summary of Methods
  • Transcription Start Sites
  • 5-ESTs, cDNA screening, and 5-RACE are scalable
  • Whole genome tiling array hybridization is a key
  • Core Promoters
  • ChIP-chip with promoter-associated proteins is a
    key
  • Reporter constructs tested in functional assays
    in fly cells?
  • DNase hypersensitve sites
  • Will high-throughput methods be effective and
    scalable?
  • Are hypersenstive sites mostly promoters?
  • Computational Methods
  • Refinements to promoter prediction
  • Comparative sequence analysis
  • Comparative promoter prediction?

10
Promoter Annotation in Drosophila
  • 14,000 protein-coding genes
  • gt10,000 associated with 5 ESTs
  • How many alternative promoters?
  • Release 3 annotation suggests 3 of genes
  • How many non-protein-coding genes?
  • Project Scale 20,000 fly promoters?
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