AI Article Synopsis

  • - The study determined the cryo-EM structure of human rhinovirus B14, revealing that 13-bp RNA duplexes are symmetrically bound around the virus's icosahedral capsid, making up about 12% of its ssRNA genome.
  • - These RNA duplexes create a quasi-dodecahedral cage inside the capsid, interacting with the inner wall through non-covalent forces, particularly with basic amino acids nearby.
  • - Comparing RNA-filled virions to empty capsids showed significant conformational changes in specific residues upon RNA release, suggesting mechanisms involved in rhinovirus assembly and uncoating, which could inform new antiviral strategies.

Article Abstract

The cryo-EM structure of the human rhinovirus B14 determined in this study reveals 13-bp RNA duplexes symmetrically bound to regions around each of the 30 two-fold axes in the icosahedral viral capsid. The RNA duplexes (~12% of the ssRNA genome) define a quasi-dodecahedral cage that line a substantial part of the capsid interior surface. The RNA duplexes establish a complex network of non-covalent interactions with pockets in the capsid inner wall, including coulombic interactions with a cluster of basic amino acid residues that surround each RNA duplex. A direct comparison was made between the cryo-EM structure of RNA-filled virions and that of RNA-free (empty) capsids that resulted from genome release from a small fraction of viruses. The comparison reveals that some specific residues involved in capsid-duplex RNA interactions in the virion undergo remarkable conformational rearrangements upon RNA release from the capsid. RNA release is also associated with the asynchronous opening of channels at the 30 two-fold axes. The results provide further insights into the molecular mechanisms leading to assembly of rhinovirus particles and their genome uncoating during infection. They may also contribute to development of novel antiviral strategies aimed at interfering with viral capsid-genome interactions during the infectious cycle.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11561273PMC
http://dx.doi.org/10.1038/s42003-024-07213-2DOI Listing

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