L11: Posttranacriptiona Regulation Of Eukaryotic Gene Expression Flashcards
Post transcriptional control of eukaryotic gene expression
Regulation of transcription initiation: principal mechanism controlling gene expression
Mechanisms operate after RNA pol has bound promoter and RNA synthesis has begun. Some are co-transcriptional
Multiple control points
mRNAs never occur as free RNA molecules
Always have associated proteins
Ribonucleoprotein (RNP) complexes. Contain other RNAs. Involved in transcript processing steps. Components of RNP complexes change as mRNA is processed, leaves nucleus and when in cytoplasm
Mature mRNA/ transcript= mature mRNP
mRNA with 5’ cap, poly(A) tail & introns removed
Ready to leave nucleus
If still in nucleus= nuclear mRNPs
If in cytoplasm= cytoplasmic mRNPs
If not processed correctly = degraded by nuclear exosomes (need cap, tail and associated proteins to be deemed ok)
RNA pol II carboxy-terminal domain (CTD)
mRNA capping
10x longer than rest of pol II when extended
Docking site for numerous capping proteins
Couples RNA processing with transcriptional elongation
5’ cap: capping proteins (factors) bind when Ser5 residues in repeats are phosphorylated (late in transcription initiation)
5’ cap
After ~25 bases of mRNA synthesised
Phosphatase removes 5’ phosphate
Guanyl transferase adds GMP in reverse linkage (5’ to 5’ linkage)
Methyl transferase adds methyl group to guanosine. Methyl group added to second ribose of some transcripts
Cap-binding complex added
Protects 5’ cap from degradation
Consensus sequence
Sequence representing most frequent residues at positions in sequence (determined from aligning sequences of same gene, gene region or genomic region or protein or protein region)
Important consensus sequences in mRNA 3’ processing
All present in gene sequence encoding mRNA
AAUAAA: poly(A) signal. 10-35 nucleotides upstream of cleavage and poly(A) tail attachment site.
GU rich region beyond cleavage site
CA nucleotide pair at least 30 nucleotides upstream of GU rich region
Poly-A pol (PAP)
Adds ~200 As to cleaved 3’ end -> 3’ end protected from exonucleases
Intron splicing
For short transcripts with few introns: Occurs after 3’ end processing steps
For longer transcripts with multiple introns: occurs before transcription ends
Consensus sequences at 5’ and 3’ spice sites within intron. 5’ = GU & 3’ = AG
Splicing proteins associated with CTD of RNA pol II
Intron splicing
Adenosine at branch point attacks 5’ splice site -> sugar-phosphate backbone cleaved. Cleaved 5’ end of intron covalently linked to adenosine -> lariat structure formed
3’ end of upstream exon reacts with 5’ end of next exon. Sugar phosphate backbones joined. Lariat intron sequence released -> degraded by nuclear RNases
Alternative splicing
75% of human genes produce transcripts that are alternatively spliced
Increases coding potential of eukaryotic genomes. One gene doesn’t necessarily code for only one protein.
Some genes encode transcripts that show constitutive splicing. Same mature transcript made continuously by cells
Some genes encode transcripts that show cell specific and/or time specific alternative splicing
Splicing done by spliceosome. 5’= GU and 3’= AG recognised for each intron
Regulation of Alternative Splicing
Dependent on gene regulatory proteins present
Negative regulation: repressor proteins block access of splicing machinery to particular splice sites on pre-mRNA.
Positive regulation: activator proteins bind specific nucleotide sequences. May be many nucleotides from splice site = splicing enhancers. Activator proteins directs splicing machinery to an otherwise overlooked splice site
mRNA transport from nucleus
Only fully processed RNAs are exported. Incorrectly processed or damaged transcripts are degraded in nucleus (exosomes)
Particular hnRNP proteins must be associated with mRNA before it can be exported. Some dissociate before export through NPC some remain attached to exported mRNA. Entire set of hnRNP protein marks mRNA as being export ready or not. Nuclear export receptor (aka nuclear transport receptor) must be present -> complex of proteins and transcript can exit nucleus
Export through nuclear pore complex (NPC): ~30 different proteins (nucleoporins). H2O filled channel. Protein filaments extend into nucleoplasm & cytoplasm. In nucleoplasm -> form nuclear basket.
In cytoplasm: nuclear export receptor dissociates; reimported to nucleoplasm. Proteins are exchanged. E.g CBC exchanged for translation IF
Mature mRNAs differ in their stability
Stable mature mRNAs persist after transcription of genes is repressed
Half life of prokaryotic mRNA: few mins (good thing. Need to react dynamically to where they are -> change expression patterns)
Half life of most mRNAs from multicellular eukaryotes = many hours (cellular environment more controlled, reliable & constant -> longer lived)
3’ UTRs carry info that control mRNA lifetimes. Binding sites for proteins involved in deadenylation, decapping and degradation -> exonucleolytic decay
