Lecture 1 DNA damage. Damage Reversal. Base excision repair. Mismatch repair Lecture 2 Nucleotide excision repair: cellular and clinical aspects Nucleotide excision repair: genes and proteins Lecture 3 Replication of damaged DNA. Mutagenesis and carcinogenesis Learning outcomes (Lecture 1a) Understanding: •Different types of DNA damage •Three examples of ways in which cells can reverse damage in situ •Basic mechanism of Base Excision Repair •To gain an understanding of the molecular mechanisms that maintain genome stability •To appreciate the importance of this topic for human health. Course Learning objectives Procarcinogen Inactive Products Ultimate Carcinogen DNA DNA Damage Mutations Chromosome Rearrangements Cell Death Activation of Oncogenes Inactivation of Tumour Suppressor Genes Cancer Pre-cancerous cells Defence Mechanisms DNA Repair Detoxification Cell cycle arrest Other disorders 1.1 DNA Damage UV Ionizing Monofuctional Bifunctional Radiation Chemicals Chemicals Non distorting chemical damage Minor distorting chemical damage Major distorting chemical damage Interstrand cross links Strand breaks - + + + - + + + + - + - + + - - - + - + + + - H3C N N H O H3C N N H O 1 2 3 4 5 6 Cyclobutane pyrimidine dimer (CPD) Major UV photoproducts H3C N NH2 O 1 6 5 4 3 2 N 1 TC (6-4) photoproduct (6-4PP) CH3 7-methylguanine O CH3 O-6-methylguanine CH3 3-methyladenine Methylated purines CH3 1-methyladenine 1 2 3 4 6 5 O CH3 3-methylcytosine 1.2 Aspects of DNA repair 1. Initial damage 2. Repair of damage 3. Genes involved 4. Mechanism of action of gene products 5. Replication of unremoved damage. Cell cycle progression. 6. Biological consequences of damage, repair and failure to repair. 1.3 Damage reversal 1. Photoreactivation PR light No PR light UV Dose Time Friedberg et al, 2005 DNA Repair and Mutagenesis 1.4 Photolyase mechanism Friedberg et al, 2005 DNA Repair and Mutagenesis 1.5 O CH3 O-6-methylguanine CH3 CH3 Thymine O-6-methylguanine Mispairing of O-6-methylguanine with thymine Methylated purines Damage reversal 2. Repair of O6-methylguanine 6 6 1.6 2. Repair of O6-methylguanine Damage reversal Treat E.coli with indicated dose of MNNG, then expose to high dose Adaptation Adapted Control Friedberg et al, 2005 DNA Repair and Mutagenesis 1.7 Dual activities of Ada methyltransferase Friedberg et al, 2005 DNA Repair and Mutagenesis 1.8 Induction of ada gene Ogt gene is not inducible Friedberg et al, 2005 DNA Repair and Mutagenesis 1.9 •Similar mechanism to E. coli, but for O-6-meG alone, like Ogt, not inducible. •K/o mouse constructed, very sensitive to carcinogenesis by methylating agents. •Conversely transgenic mice bearing MGMT gene are more resistant. •Many cancer cell lines are Mex-. MGMT silenced by methylation in about 50% of tumours. •Mex- cells are sensitive to killing and mutagenesis by alkylating agents. •Many cancer therapy drugs are alkylating agents, eg temozolomide. •Patrin2 binds MGMT and depletes it. Currently in clinical trials together with temozolomide. Alkyltransferases in mammalian cells 1.10 Damage reversal 3. Oxidative demethylation (A3) wt alkB Friedberg et al, 2005 DNA Repair and Mutagenesis alkB survival 1.11 Mechanism ar Base Excision Repair 8-hydroxyguanine Deamination of bases 3-d structures of glycosylases Protection from 8-oxoguanine Base Excision-Repair 3-d structures of APendonucleases APE1 ENDO IV Summary (Lecture 1a) •DNA damage can cause distortions of different severity •UV damage is repaired by photoreversal (not in placental mammals) •O6-methylguanine is repaired by a specific methyltransferase •1-methyladenine and 3-methylcytosine are repaired by oxidative demethylation •Spontaneous lesions are removed by Base Excision Repair Learning outcomes (Lecture 1b) Understanding: •Detailed mechanism of mismatch repair in E. coli and eukaryotes •How mismatch repair is important both for cancer protection and cancer therapy Mismatch Repair (A5, A6) •DNA polymerases replicate DNA very faithfully Accurate insertion Associated 3’-5’ exonuclease for proof-reading Error rates c. 10-6 or less •But genomes are big: E. coli 3x106 bp, mammals 3x109 •Errors can be single base mismatches or small insertions or deletions caused by base slippage •Mismatches are repaired by the MMR system which recognises the mismatched bases •But there’s a problem 1.12 Methylation-directed mismatch repair Dam- strains (methylation deficient) are mutators Dam protein Friedberg et al, 2005 DNA Repair and Mutagenesis 1.13 Mismatch recognition and strand discrimination in E. coli MutH, MutL and MutS- strains are mutators CH3 CH3 S2 L2 H 1.14 JCUB 3-D structure of MutS Structural homodimer Functional heterodimer Jiricny, Current Biology, 2000 Jiricny, NRMCB, 2006 Activities of MutS Sliding clamp Crucial Phe in Phe-X-Glu contacts mismatch 1.15 Late steps in MMR in E. coli Friedberg et al, 2005 DNA Repair and Mutagenesis UvrD helicase II unwinds SSB covers exposed ss DNA DNA Ligase 1.16 Eukaryotic homologues of MutH,L,S MutS: Msh2 MMR Msh3 MMR Msh4 Meiosis Msh5 Meiosis Msh6 MMR MutL: Mlh1 MMR Mlh2 ? Mlh3 MMR Pms1 ? Pms2 MMR (= Pms1 in yeast) MutH: No homologues Neither yeast nor Drosophila has methylated DNA Strand discrimination based on nicks/ends in daughter DNA MMR proteins interact with PCNA at replication fork 1.17 G T T GT GT GTC GTAC Mismatch Repair in eukaryotes G C T A GT CA GT CA GTC CAG GTAC CATG Removal and restoration Pms2 Mlh1 G T GTC Pms2 Mlh1 PCNA PCNA Secondary recognition MutLa 1.18 IDL (Insertion-deletion loop) MutSa Preference for single base mismatches and small IDL MutSb Preference for large IDL G T Primary recognition GTC Mismatch Repair in eukaryotes Leading strand: MutLa (Pms2 subunit) cleaves on 5’ side of mismatch. Exo1 degrades 5’ to 3’ Modified from Jiricny, Nature Rev Mol Cell Biol 2006 (A5) MutSa or b binds mismatch MutSa/MutLa translocates to end PCNA Lagging strand: Exo1 degrades 5’ to 3’ 5’ 5’ 3’ 3’ (ExoI) 1.19 Microsatellite instability in tumour tissue from HNPCC (Hereditary non-polyposis colon carcinoma) Lynch Syndrome Aaltonen, et al. Science 260, 812 (1993) Primer 1 CA CA CA CA CA CA CA GT GT GT GT GT GT GT Primer 2 CA CA CA CA CA CA GT GT GT GT GT GT CA Replication Slippage 7 microsatellite repeats 6 repeats 1.20 2-hit tumour suppressor model 1 germ-line mutation Somatic mutation Sporadic colon cancer 1st somatic mutation 2nd somatic mutation Normal allele Mutant allele Most HNPCC result from mutations in hMsh2 or hMlh1 1.21 Extracts of tumour cells are deficient in MMR of dinucleotide loops and single base mismatches HNPCC HNPCC is autosomal dominant MMR proficient MMR deficient MMR proficient MMR proficient MMR deficient Microsatellite instability results from loss of Mismatch Repair 5' T-G-T- G-T-G-T-G-T- G 3' A-C-A-C-A-C-A-C-A-C-A-C-5' misalignment T-G | | 5' T-G T- G-T- G-T- G 3' A-C-A-C-A-C- A-C-A-C-A-C T-G | | 5' T- G T-G-T-G-T- G-T-G-T- G 3' A-C-A-C-A-C-A-C-A-C-A-C 5' T-G-T- G-T-G-T- G-T- G 3' A-C-A-C-A-C-A-C-A-C-A-C 5' T-G-T-G-T- G-T- G-T-G-T- G 3' A-C-A-C-A-C-A- C-A-C-A-C extension reversal (proofreading) mismatch repair 1.22 •Microsatellite instability is a useful diagnostic tool. It’s not the cause of the cancers •Cancers arise from high rate of single-base mismatches during replication •These lead to high frequency of somatic mutations •Why only in colon? Not known O CH3 CH3 CH3 Thymine O-6-methylguanine Mispairing of O-6-methylguanine with thymine 2. Repair of O6-methylguanine Damage reversal 6 6 1.6 •In many tumour cells MGMT is silenced. So alkylating agents are good for therapy. •But often develop resistance. •Select for alkylation-resistance in cells. •MGMT not restored. O6-MeG remains in DNA. Instead cells have lost one of the MMR genes. •Implies MMR somehow sensitises cells to alkylation damage. •Result of futile cycles. O6-MeG:C and O6-MeG:T both recognised as mismatches. •C or T opposite O6-MeG removed by MMR and replaced with C or T. Futile cycles. •Results in cell cycle arrest or apoptosis MMR and resistant tumours 1.23 Loss of MMR protects against MNNG apoptosis 1.24 MMR and cancer MMR deficiency • Increases cancer susceptibility (HNPCC) • Results in resistance to cancer therapy Friedberg et al, 2005 DNA Repair and Mutagenesis Summary (Lecture 1b) •Mismatches are repaired by the Mut(H),L,S system •Mismatches are recognised by MutS and its homologues •Strand discrimination is brought about by methylation in E. coli and nicks/ends in daughter strands in eukaryotes •MMR deficiency leads to HNPCC and is detected by microsatellite instability •Loss of MMR results in resistance to alkylating agents