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MMG /BIOC 352. The Replisome: DNA Replication in E. coli and Eukaryotes. Spring 2006. Scott W. Morrical. Contact Information. Scott W. Morrical Given B407 656-8260 [email protected]. Lecture Outline:. Overview of DNA Replication Bacterial systems ( E. coli) - PowerPoint PPT Presentation
MMG /BIOC 352
Spring 2006
The Replisome: DNA Replication in E. coli
and Eukaryotes
Scott W. Morrical
Lecture Outline:Overview of DNA Replication Bacterial systems (E. coli) Eukaryotic systems (yeast/human)
The E. coli Replisome Components & sub-assemblies Replisome structure/function Coordination of leading/lagging strand synthesis
The Eukaryotic Replisome Polymerase switching
Okazaki Maturation
Initiation Mechanisms E. coli oriC paradigm Eukaryotic model
Termination Mechanisms Tus-Ter
Fidelity Mechanisms Proofreading Mismatch repair
Processivity Mechanisms:
Structure/Function of Sliding Clamps E. coli -clamp Eukaryotic PCNA
Structure/Function of AAA+ Clamp Loaders E. coli -complex Eukaryotic RFC
Other AAA+ ATPase Machines
Reference list for this topic:
Ref 1: Johnson, A., and O’Donnell, M. (2005) Cellular DNA replicases: components and
dynamics at the replication fork. Annu. Rev. Biochem. 74, 283-315.
Ref 2: Davey, M.J., Jeruzalmi, D., Kuriyan, J., and O’Donnell, M. (2002) Motors and Switches: AAA+ machines within the replisome. Nat. Rev. Mol. Cell Biol. 3,
826-835.
Ref 3: Kong, X.P., Onrust, R., O’Donnell. M. and Kuriyan, J. (1992) Three-dimensional structure of the beta subunit of E. coli DNA polymerase III holoenzyme: asliding clamp. Cell 69, 425-437.
Ref 4: Krishna. T.S., Kong, X.P., Gary, S., Burgers, P.M., and Kuriyan, J. (1994) Crystal structure of eukaryotic DNA polymerase processivity factor PCNA.
Ref 5: Jeruzalmi, D., O’Donnell, M., and Kuriyan, J. (2001) Crystal structure of theprocessivity clamp loader gamma complex of E. coli DNA polymerase III. Cell
106,429-421.
Ref. 6: Bowman, G.D., O’Donnell, M., and Kuriyan, J. (2004) Structural analysis of a eukaryotic sliding DNA clamp-clamp loader complex.
References (cont’d):
Ref 7: Mendez, A., and Stillman, B. (2003) Perpetuating the double helix: molecularmachines at eukaryotic DNA replication origins. Bioessays 25, 1158-1167.
Ref 8: Neylon, C., Kralicek, A.V., Hill, T.M., and Dixon, N.E. (2005) Replication termination
in Escherichia coli: structure and antihelicase activity of the Tus-Ter complex. Micr. Mol. Biol. Rev. 69, 501-526
Further Reading:
Mammalian DNA mismatch repair.Buermeyer et al. (1999) Annu. Rev. Genet. 33, 533-564.
Role of DNA mismatch repair defects in the pathogenesis of human cancer.Peltomaki (2003) J. Clinical Oncology 21, 1174-1179.
DNA Chemistry
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A:T or G:CBasepair
3’-end5’-end
Backbone
Phosphate2’-deoxy-
ribose
5’-end3’-end
Chemical Inheritance-- DNA Replication
DNA Replication Fork • processive
• 5’ to 3’
• semi-conservative
• semi-discontinuous
• high-fidelity
E. Coli Chromosome1 unique origin of bi-directional replication
10 polar termination sites
Replication Progression of E. coli Chromosome
oriC
ter sequences
oriC
oriC
thetastructure
Replication of Eukaryotic Chromosomes
Many different origins on each chromosome firing simultaneously or in a programmed sequence.
DNA Replication Fork Major Protein Components:• DNA polymerase holoenzyme(s)
-- polymerase
-- proofreading exonuclease
-- sliding clamp
-- clamp loader complex
• DNA helicase(s)
• Primase
• ssDNA binding protein
• Other accessory factors needed for correct assembly, processive movement, and fidelity.
Major Components of E. coli Replisome:
PolIII-- DNA polymerase III holoenzyme (Pol III)
DnaG primase
DnaB helicase
SSB-- ssDNA-binding protein
Plus accessory proteins, loading factors
Replisome Mol.Component Wt.[stoichiometry] Gene (kDa) Function
Pol III holoenzyme 791.5 Dimeric, ATP-dependent, processive polymerase/clamp loader Pol III star 629.1 Dimeric polymerase/clamp loader Core 166.0 Monomeric polymerase/exonuclease [2] dnaE 129.9 5’ --> 3’ DNA polymerase [2] dnaQ 27.5 3’ --> 5’ exonuclease [2] holE 8.6 Stimulates exonuclease / complex 297.1 ATP-dependent clamp loader / [1/2] dnaX 47.5/71.1 ATPase, organizes Pol III star and binds DnaB [1] holA 38.7 Binds clamp ’ [1] holB 36.9 Stator, stimulates ATPase in ATP site 1 [1] holC 16.6 Binds SSB [1] holD 15.2 Connects to clamp loader [2 dimers] dnaN 40.6 Homodimeric processivity sliding clamp
Primase [1] dnaG 65.6 Generates primers for Pol III holoenzyme
DnaB helicase [6] dnaB 52.4 Unwinds duplex DNA 5’ --> 3’ ahead of the replication fork
SSB [4] ssb 18.8 Melts 2o structure in ssDNA, binds clamp loader through
E. coli Replisome Stoichiometries
E. coli 2 Sliding Clamp
E. coli Complex-- ATP-dependent clamp loading activity
Clamp Loading Reaction
Structural Organization ofPol III Holoenzyme
DNA Flow in the E. coli Replisome
Replisome Dynamics
Replisome in Motion (zoom out)
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Replisome in Motion (zoom in)
Functional Conservation of Replicase Sub-assemblies
Eukaryotic Replisome Components
S. cerevisiae (kDa) H. sapiens (kDa) Function and remarks [S. pombe name]
RFCa RFC (277.7)a RFC (314.9)a Pentameric clamp loadera
RFC1 (94.9) p140 (128.2) Binds ATP; phosphorylated RFC2 (39.7) p37 (39.2) Binds ATP RFC3 (38.2) p36 (40.6) Binds ATP RFC4 (36.1) p40 (39.7) Binds ATP RFC5 (39.9) p38 (38.5) Binds ATP or ADP
PCNAa PCNA (28.9) a PCNA (28.7) 87 kDa a Homotrimeric sliding clamp a
Pol a Pol (220.2) a Pol (238.7) a Replicative DNA polymerase a
Pol3 (124.6) p125 (123.6) DNA polymerase, 3'-5' exo, binds PCNA; subunit A [S.p. Pol3]
Pol31 (55.3) p50 (51.3) Structural subunit; subunit B [S.p. Cdc1] Pol32 (40.3) p66 (51.4) Binds PCNA; subunit C [S.p. Cdc27];
binds Pol large subunit — p12 (12.4) Structural, stimulates processivity;
subunit D [S.p. Cdm1]
Pol a Pol (378.7) a Pol (350.3) a Replicative DNA polymerase a
Pol2 (255.7) p261 (261.5) DNA polymerase, 3'-5' exo [S.p. Pol2/cdc20] Dpb2 (78.3) p59 (59.5) Binds polymerase subunit [S.p. Dpb2] Dpb3 (22.7) p17 (17.0) Binds Dpb4 Dpb4 (22.0) p12 (12.3) Present in ISW2/yCHRAC chromatin
remodeling complex [S.p. Dpb4]
Pol a Pol (355.6) a Pol (340.6) a DNA polymerase/primase a
Pol1 (166.8) p180 (165.9) DNA polymerase Pol12 (78.8) p68 (66.0) Structural subunit Pri2 (62.3) p55 (58.8) Interacts tightly with p48 Pri1 (47.7) p48 (49.9) RNA primase catalytic subunit
aInformation concerns a protein complex.
Eukaryotic Replisome Components (cont’d)
S. cerevisiae (kDa) H. sapiens (kDa) Function and remarks [S. pombe name]
MCM a MCM (605.6) a MCM (535) a Putative 3'-5' replicative helicase a
Mcm2 (98.8) Mcm2 (91.5) Phosphorylated by Dbf4-dependent kinase Mcm3 (107.5) Mcm3 (91.0) Ubiquitinated, acetylated Mcm4 (105.0) Mcm4 (96.6) Helicase with MCM6,7; phosphorylated by CDK;
aka Cdc54 Mcm5 (86.4) Mcm5 (82.3) Aka Cdc46; Bob1 is a mutant form Mcm6 (113.0) Mcm6 (92.3) Helicase with MCM4,7 Mcm7 (94.9) Mcm7 (81.3) Helicase with MCM4,6; ubiquitinated
RPA a RPA (114) a RPA (100.5) a Single-stranded DNA-binding protein a
RPA70 (70.3) RPA70 (70.3) Binds DNA, stimulates Pol RPA30 (29.9) RPA30 (29) Binds RPA70 and 14, phosphorylated RPA14 (13.8) RPA14 (13.5) Binds RPA30
a Information concerns a protein complex.
Model for Eukaryotic Replisome(Based on E. coli and T4 Phage Models)
Polymerase Switching During Eukaryotic Lagging Strand Synthesis& Okazaki Maturation via RNaseH1 and Fen1/RTH1
Okazaki Maturation Involving Helicase Strand Displacement& Flap Endonuclease Activity of Fen1/RTH1
E. coli: RNA primers removed by 5’ --> 3’ exo activity of DNA polymerase I (Pol I). Simultaneous fill-in with DNA (nick translation rxn) leaves nick that is sealed by ligase.
DNA Replication:
Initiation, Termination, &Fidelity Mechanisms
Scott Morrical
Initiation of E. coli DNA Replication at oriC-- roles of DnaA Initiator Protein and DnaC Helicase Loader
DnaA-- initiator protein
oriC-- replicator sequence
Factors Required for Activation of Eukaryotic Origins
Shameless Speculation About Helicase LoadingMechanisms at Eukaryotic Origins
Replication Termination:Direction-specific Termination of DNA Replication
by E. coli Tus Protein Bound to a Ter Sequence
E. Coli Chromosome1 unique origin of bi-directional replication
10 polar termination sites
Replication Fork Arrest by Correctly Oriented Tus-TerComplex
Alternative Models for the Direction-Specificity of Fork Arrest by Tus-Ter
Replication Fidelity Mechanisms:Spont. Error Frequency
Pol 10-4
Pol + exo 10-7
Pol + exo + MMC 10-9 to 10-10
Single base mismatches-- misincorporation by DNA polymerase,missed by proofreading exonuclease.
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Insertion-deletion loops (IDLs)-- caused by polymerase slippage onrepetitive template, gives rise to Microsatallite Instability (MSI).
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E. coliMethyl-DirectedMismatch RepairSystem
Eukaryotic Homologs of MutS and MutL
Mlh1-Pms1
Heterodimers of Eukaryotic MutS & MutL Homologs
Msh2 Msh3
Mlh1-Mlh2
Msh2 Msh3
Mlh1-Mlh3
Msh2 Msh3
Mlh1-Pms1
Msh2 Msh6
Rad1-Rad10
Msh2 Msh3 Msh4 Msh5
Mlh1-Mlh3
Non-homologoustail removal inrecombinationintermediates
Insertion/deletionloop (IDL)
removal
Repair ofbase-base mismatches
Promotion ofmeiotic crossovers
MutS
MutS
MutL
MutL
*Note: This is yeast nomenclature.Mlh1 paralogs have different namesin yeast and humans.
1 b2-4 b
Sliding Processivity Clampsof DNA Polymerases:
X-ray Structure of-subunit of E. coli DNA Polymerase III
BACKGROUND:
1. Biochemical studies established that beta is essential for processive DNA synthesis by Pol III.
2. Beta exists as a stable dimer in solution.
3. Beta dimer has no intrinsic affinity for DNA, yet in the presence of gamma complex + ATP, beta dimer forms and extremely stable complex with circular, but not with linear, primed DNA molecules.
4. Proposal by O’Donnell & coworkers: 2 is topologically linked, not thermodynamically bound to DNA, and forms a sliding clamp that tethers Pol III.
3’
3’5’
5’
2 Pol III core
Kong, Onrust, O’Donnell, & Kuriyan (1992) “Three-dimensional structure of the betasubunit of E. coli DNA polymerase III holoenzyme: a sliding DNA clamp”. Cell 69, 425-37.
2.5Å resolution
Non-crystallographic 2-foldrotational axis of symmetryperpendicular to face of ring and passing through center of hole.
• Highly symmetrical; almost hexagonal symmetry.
• Protomers interact head-to-tail in 2 interfaces on opposite sides of the ring.
Space-filling Model of Beta Dimer with B-form DNAModeled In
O.D. ≈ 80 Å, I.D. ≈ 35 Å-- easily accommodates B- or A-form (RNA/DNA hybrid) duplex (~25 Å O.D.) without steric repulsions.
Thickness ≈ 34 Å, equal to ~1 full helical repeat of B-form dsDNA.
Connectivity of Beta Subunit
Green (N-terminus)
light blue
purple
red
yellow (C-terminus)
• Dimer interfaces are between domains colored green/blue and red/yellow.
• Domains are numbered 1,2,3 and 1’, 2’, 3’ in the two monomers.
Unexpected Features of the 2 Structure:
1. Internal symmetry.
-- each monomer consists of 3 structural domains of identical chain topology and very similar 3-D structure.
-- this was surprising because there are no internal regions of a.a. sequence homology.
2. Each domain is roughly 2-fold symmetric in architecture, with an outer layer of 2 -sheets providing a scaffold that supports 2 -helices.
Unexpected Features of the 2 Structure (cont’d):
3. Replication of this motif around a circle (2 subunits x 3 domains/subunit) results in a rigid molecule with 12 -helices lining the inner surface of the ring, and with 6 “seamless” interlocking -sheets forming the outer surface.
4. Symmetry of domains gives rise to highly symmetrical and roughly hexagonal star shape of the dimer.
60o rotation about dimer axis superimposes domains.
-- different a.a. sequences, but 80% structurally analogous at C’s.
-- hence the approximately hexagonal symmetry.
Simple Principle Underlying 2 Architecture:
• The 2 outer strands of -sheets in one domain form hydrogen-bonding interactions with corresponding strands in 2 adjacent domains, continued around the circle.
• No distinctions apparent between such -sheet extensions across internal domain boundaries as opposed to intermolecular contacts (i.e. the 2 dimer interfaces also form continuous antiparallel -sheets).
• These interactions lead to a completely closed circle with 6 “seamless” -sheets on the outer surface.
Spatial Arrangement of -helices Within 2 DimerWith Respect To B-form DNA
(assuming duplex is perpendicular to plane of ring)
1. Each of the 12 -helices has similar tilt w.r.t. the axis of the ring, due to their symmetrical arrangement.
Spatial Arrangement of -helices Within 2 DimerWith Respect To B-form DNA (Cont’d)(assuming duplex is perpendicular to plane of ring)
2. The axis of each -helix is almost exactly perpendicular to the local direction of the sugar-phosphate backbone.
--> the helices span the major & minor grooves.
--> effectively prevents entry of the protein into either groove, which should facilitate rapid motion along the duplex
Spatial Arrangement of -helices Within 2 DimerWith Respect To B-form DNA (Cont’d)(assuming duplex is perpendicular to plane of ring)
3. If one a-helix spans the major groove, the one directly across the ring spans the minor groove.
--> damps out variation in interaction energy with sugar-phosphate backbone as the protein moves across the grooves of DNA.
Electrostatic Potential of 2 Dimer
2 contains 38 Asp, 58 Glu, 24 Lys, 50 Arg, and 14 His residues
--> net charge of -15 to -22
• Highly asymmetric electrostatic field:
-- outer edge and both faces strongly negatively charged, but asymmetric from face-to-face.
-- asymmetry may correctly orient 2 w.r.t. primer terminus, complex, and Pol III core.
Electrostatic Potential of 2 Dimer (Cont’d)
2 contains 38 Asp, 58 Glu, 24 Lys, 50 Arg, and 14 His residues
--> net charge of -15 to -22
• Inner surface of hole highly positively-charged:
-- favorable interaction with DNA backbone --> “float on electrostatic cloud”.
-- ??? stabilize dimer around DNA, since electrostatic interactions in dimer interface might not withstand repulsive interactions with DNA ???
Contributions to Stability of Dimer Interface*** Highly Electrostatic ***
1. Continuation, across molecular boundary, of hydrogen-bonded -sheet structure.
--> ≥ 4 strong hydrogen bonds at each of 2 interfaces. (Indistinguishable from continuation of -sheet across interdomain boundaries.)
2. Small hydrophobic core (in white):
Phe-106|Ile-278
Ile-272|Leu-273
packagainst
Contributions to Stability of Dimer Interface (Cont’d)*** Highly Electrostatic ***
3. Electrostatics: potential intermolecular ion pairs:
Lys-74 … Arg-96 … Arg-103 … Arg-105
Glu-298 … Glu-300 … Glu-301 … Glu-303 … Glu-304
4. Charge complementarity at each interface: All positively-charged residues from one monomer, all negatively charged from the other.
5. Relatively little surface area is buried upon dimerization, ~8%.
Conservation of Structure inSliding Processivity Clamps
of DNA Polymerases
dimer trimer
Chain Topology of PCNA Monomer
Domain 2
Domain 1
T4 Gp45 Yeast PCNA
Superposition of Domain 1 FromT4 Gp45 (red) and Yeast PCNA (yellow)
Electrostatic Surface Potentials
Gp45
PCNA
All Ring Holes Accommodate B-form dsDNAor RNA/DNA Hybrid Without Steric Hindrance
ArchaealClamp
EukaryoticClamp
BacterialClamp
P. furiosusPCNA
S. cerevisiaePCNA
E. coliBeta
Main Chain Hydrogen Bonds Between Strandsat PCNA Subunit Interface
P. furiosus yeast human
