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TitleA three-helix junction is the interface between two functional domains of prohead RNA in 29 DNA packaging.
Journal, issue, pagesJ Virol, Vol. 86, Issue 21, Page 11625-11632, Year 2012
Publish dateAug 15, 2012
AuthorsWei Zhao / Mitul Saha / Ailong Ke / Marc C Morais / Paul J Jardine / Shelley Grimes /
PubMed AbstractThe double-stranded-DNA bacteriophages employ powerful molecular motors to translocate genomic DNA into preformed capsids during the packaging step in phage assembly. Bacillus subtilis bacteriophage ...The double-stranded-DNA bacteriophages employ powerful molecular motors to translocate genomic DNA into preformed capsids during the packaging step in phage assembly. Bacillus subtilis bacteriophage 29 has an oligomeric prohead RNA (pRNA) that is an essential component of its packaging motor. The crystal structure of the pRNA-prohead binding domain suggested that a three-helix junction constitutes both a flexible region and part of a rigid RNA superhelix. Here we define the functional role of the three-helix junction in motor assembly and DNA packaging. Deletion mutagenesis showed that a U-rich region comprising two sides of the junction plays a role in the stable assembly of pRNA to the prohead. The retention of at least two bulged residues in this region was essential for pRNA binding and thereby subsequent DNA packaging. Additional deletions resulted in the loss of the ability of pRNA to multimerize in solution, consistent with the hypothesis that this region provides the flexibility required for pRNA oligomerization and prohead binding. The third side of the junction is part of a large RNA superhelix that spans the motor. The insertion of bases into this feature resulted in a loss of DNA packaging and an impairment of initiation complex assembly. Additionally, cryo-electron microscopy (cryoEM) analysis of third-side insertion mutants showed an increased flexibility of the helix that binds the ATPase, suggesting that the rigidity of the RNA superhelix is necessary for efficient motor assembly and function. These results highlight the critical role of the three-way junction in bridging the prohead binding and ATPase assembly functions of pRNA.
External linksJ Virol / PubMed:22896620 / PubMed Central
MethodsEM (single particle)
Resolution17.0 - 17.3 Å
Structure data

EMDB-2162:
Structure of bacteriophage phi29 prohead particle with a double insertion mutation (U92,U93) in the pRNA
Method: EM (single particle) / Resolution: 17.3 Å

EMDB-5451:
Bacteriophage phi29 prohead particle with a single insertion mutation (U92) in the pRNA
Method: EM (single particle) / Resolution: 17.0 Å

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