EMDB-16229: Cryo-EM structure of the bacterial replication origin opening bas...

Basic information

Entry

Database: EMDB / ID: EMD-16229

• Title: Cryo-EM structure of the bacterial replication origin opening basal unwinding system

Sample

• Complex: Basal unwinding complex
  • Protein or peptide: Chromosomal replication initiator protein DnaA
  • DNA: DNA (5'-D(P*AP*CP*TP*TP*AP*TP*CP*CP*AP*CP*AP*AP*AP*TP*CP*CP*AP*CP*AP*GP*GP*CP*CP*C)-3')
  • DNA: DNA (41-MER)
• Ligand: MAGNESIUM ION
• Ligand: ADENOSINE-5'-TRIPHOSPHATE

• Keywords: DnaA / cryo-EM / BUS complex / replication initiation / REPLICATION

Function / homology

Function:

regulation of DNA replication / DNA replication origin binding / DNA replication initiation / ATP hydrolysis activity / ATP binding / cytoplasm

Domain/homology:

DnaA N-terminal domain / DnaA N-terminal domain / DnaA, N-terminal domain superfamily / Chromosomal replication control, initiator DnaA / Chromosomal replication initiator, DnaA C-terminal / Chromosomal replication control, initiator DnaA, conserved site / Bacterial dnaA protein helix-turn-helix / DnaA protein signature. / Bacterial dnaA protein helix-turn-helix domain / Chromosomal replication control, initiator DnaA-like / Chromosomal replication initiator protein DnaA / Bacterial DnaA ATPAse domain / Trp repressor/replication initiator / ATPases associated with a variety of cellular activities / AAA+ ATPase domain / P-loop containing nucleoside triphosphate hydrolase

Component:

Chromosomal replication initiator protein DnaA

• Biological species: Bacillus subtilis (bacteria) / DNA molecule (others)
• Method: single particle reconstruction / cryo EM / Resolution: 3.2 Å
• Authors: Pelliciari S / Bodet-Lefevre S / Murray H / Ilangovan A

Funding support

United Kingdom, 1 items

Organization	Grant number	Country
Wellcome Trust	204985/Z/16/Z	United Kingdom

• Citation: Journal: Nat Commun / Year: 2023; Title: The bacterial replication origin BUS promotes nucleobase capture.; Authors: Simone Pelliciari / Salomé Bodet-Lefèvre / Stepan Fenyk / Daniel Stevens / Charles Winterhalter / Frederic D Schramm / Sara Pintar / Daniel R Burnham / George Merces / Tomas T Richardson / Yumiko Tashiro / Julia Hubbard / Hasan Yardimci / Aravindan Ilangovan / Heath Murray / ; Abstract: Genome duplication is essential for the proliferation of cellular life and this process is generally initiated by dedicated replication proteins at chromosome origins. In bacteria, DNA replication is initiated by the ubiquitous DnaA protein, which assembles into an oligomeric complex at the chromosome origin (oriC) that engages both double-stranded DNA (dsDNA) and single-stranded DNA (ssDNA) to promote DNA duplex opening. However, the mechanism of DnaA specifically opening a replication origin was unknown. Here we show that Bacillus subtilis DnaA assembles into a continuous oligomer at the site of DNA melting, extending from a dsDNA anchor to engage a single DNA strand. Within this complex, two nucleobases of each ssDNA binding motif (DnaA-trio) are captured within a dinucleotide binding pocket created by adjacent DnaA proteins. These results provide a molecular basis for DnaA specifically engaging the conserved sequence elements within the bacterial chromosome origin basal unwinding system (BUS).

History

Deposition	Nov 28, 2022	-
Header (metadata) release	Feb 14, 2024	-
Map release	Feb 14, 2024	-
Update	Feb 14, 2024	-
Current status	Feb 14, 2024	Processing site: PDBe / Status: Released

Map

• File: Download / File: emd_16229.map.gz / Format: CCP4 / Size: 125 MB / Type: IMAGE STORED AS FLOATING POINT NUMBER (4 BYTES)
• Voxel size: X=Y=Z: 1.072 Å

Density

Contour Level	By AUTHOR: 0.12
Minimum - Maximum	-0.36148095 - 1.4240421
Average (Standard dev.)	0.0008227174 (±0.0343295)

• Symmetry: Space group: 1

Details

EMDB XML:

Map geometry	Axis order X Y Z Origin 0 0 0 Dimensions 320 320 320 Spacing 320 320 320
Cell	A=B=C: 343.04 Å α=β=γ: 90.0 °

Supplemental data

Half map: #2

• File: emd_16229_half_map_1.map

Half map: #1

• File: emd_16229_half_map_2.map

Sample components

Entire : Basal unwinding complex

• Entire: Name: Basal unwinding complex

Components

• Complex: Basal unwinding complex
  • Protein or peptide: Chromosomal replication initiator protein DnaA
  • DNA: DNA (5'-D(P*AP*CP*TP*TP*AP*TP*CP*CP*AP*CP*AP*AP*AP*TP*CP*CP*AP*CP*AP*GP*GP*CP*CP*C)-3')
  • DNA: DNA (41-MER)
• Ligand: MAGNESIUM ION
• Ligand: ADENOSINE-5'-TRIPHOSPHATE

Supramolecule #1: Basal unwinding complex

• Supramolecule: Name: Basal unwinding complex / type: complex / ID: 1 / Parent: 0 / Macromolecule list: #1-#3 / Details: Nucleoprotein complex
• Source (natural): Organism: Bacillus subtilis (bacteria)

Macromolecule #1: Chromosomal replication initiator protein DnaA

• Macromolecule: Name: Chromosomal replication initiator protein DnaA / type: protein_or_peptide / ID: 1 / Number of copies: 7 / Enantiomer: LEVO
• Source (natural): Organism: Bacillus subtilis (bacteria)
• Molecular weight: Theoretical: 50.92998 KDa
• Recombinant expression: Organism: Escherichia coli (E. coli)

Sequence

String:

MENILDLWNQ ALAQIEKKLS KPSFETWMKS TKAHSLQGDT LTITAPNEFA RDWLESRYLH LIADTIYELT GEELSIKFVI PQNQDVEDF MPKPQVKKAV KEDTSDFPQN MLNPKYTFDT FVIGSGNRFA HAASLAVAEA PAKAYNPLFI YGGVGLGKTH L MHAIGHYV IDHNPSAKVV YLSSEKFTNE FINSIRDNKA VDFRNRYRNV DVLLIDDIQF LAGKEQTQEE FFHTFNTLHE ES KQIVISS DRPPKEIPTL EDRLRSRFEW GLITDITPPD LETRIAILRK KAKAEGLDIP NEVMLYIANQ IDSNIRELEG ALI RVVAYS SLINKDINAD LAAEALKDII PSSKPKVITI KEIQRVVGQQ FNIKLEDFKA KKRTKSVAFP RQIAMYLSRE MTDS SLPKI GEEFGGRDHT TVIHAHEKIS KLLADDEQLQ QHVKEIKEQL K

UniProtKB: Chromosomal replication initiator protein DnaA

Macromolecule #2: DNA (5'-D(P*AP*CP*TP*TP*AP*TP*CP*CP*AP*CP*AP*AP*AP*TP*CP*CP*AP*CP...

• Macromolecule: Name: DNA (5'-D(P*AP*CP*TP*TP*AP*TP*CP*CP*AP*CP*AP*AP*AP*TP*CP*CP*AP*CP*AP*GP*GP*CP*CP*C)-3'); type: dna / ID: 2 / Number of copies: 1 / Classification: DNA
• Source (natural): Organism: DNA molecule (others)
• Molecular weight: Theoretical: 7.227697 KDa

Sequence

String:

(DA)(DC)(DT)(DT)(DA)(DT)(DC)(DC)(DA)(DC) (DA)(DA)(DA)(DT)(DC)(DC)(DA)(DC)(DA)(DG) (DG)(DC)(DC)(DC)

Macromolecule #3: DNA (41-MER)

• Macromolecule: Name: DNA (41-MER) / type: dna / ID: 3 / Number of copies: 1 / Classification: DNA
• Source (natural): Organism: DNA molecule (others)
• Molecular weight: Theoretical: 12.855272 KDa

Sequence

String:

(DT)(DA)(DG)(DT)(DA)(DG)(DA)(DA)(DG)(DT) (DA)(DA)(DT)(DA)(DG)(DT)(DA)(DG)(DG)(DG) (DC)(DC)(DT)(DG)(DT)(DG)(DG)(DA)(DT) (DT)(DT)(DG)(DT)(DG)(DG)(DA)(DT)(DA)(DA) (DG) (DT)

Macromolecule #4: MAGNESIUM ION

• Macromolecule: Name: MAGNESIUM ION / type: ligand / ID: 4 / Number of copies: 7 / Formula: MG
• Molecular weight: Theoretical: 24.305 Da

Macromolecule #5: ADENOSINE-5'-TRIPHOSPHATE

• Macromolecule: Name: ADENOSINE-5'-TRIPHOSPHATE / type: ligand / ID: 5 / Number of copies: 7 / Formula: ATP
• Molecular weight: Theoretical: 507.181 Da

Chemical component information

ChemComp-ATP:
ADENOSINE-5'-TRIPHOSPHATE / ATP, energy-carrying molecule*YM

Experimental details

Structure determination

• Method: cryo EM
• Processing: single particle reconstruction
• Aggregation state: particle

Sample preparation

• Buffer: pH: 7.5
• Vitrification: Cryogen name: ETHANE

Electron microscopy

• Microscope: FEI TITAN KRIOS
• Image recording: Film or detector model: GATAN K3 BIOQUANTUM (6k x 4k) / Average electron dose: 48.3 e/Ų
• Electron beam: Acceleration voltage: 300 kV / Electron source: FIELD EMISSION GUN
• Electron optics: Illumination mode: SPOT SCAN / Imaging mode: BRIGHT FIELD / Nominal defocus max: 3.0 µm / Nominal defocus min: 0.7000000000000001 µm
• Experimental equipment: Model: Titan Krios / Image courtesy: FEI Company

Image processing

• Startup model: Type of model: OTHER / Details: Abinitio
• Final reconstruction: Resolution.type: BY AUTHOR / Resolution: 3.2 Å / Resolution method: FSC 0.143 CUT-OFF / Number images used: 1192718
• Initial angle assignment: Type: MAXIMUM LIKELIHOOD
• Final angle assignment: Type: MAXIMUM LIKELIHOOD