Structural insights into the assembly and regulation of distinct viral capsid complexes

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作者
Subir Sarker
María C. Terrón
Yogesh Khandokar
David Aragão
Joshua M. Hardy
Mazdak Radjainia
Manuel Jiménez-Zaragoza
Pedro J. de Pablo
Fasséli Coulibaly
Daniel Luque
Shane R. Raidal
Jade K. Forwood
机构
[1] School of Animal and Veterinary Sciences,NSW Department of Primary Industries and Charles Sturt University
[2] Charles Sturt University,Monash Biomedicine Discovery Institute and Department of Biochemistry and Molecular Biology
[3] Graham Centre for Agricultural Innovation,undefined
[4] Centro Nacional de Microbiología/ISCIII,undefined
[5] ,undefined
[6] School of Biomedical Sciences,undefined
[7] Charles Sturt University,undefined
[8] Australian Synchrotron,undefined
[9] Infection and Immunity Program,undefined
[10] Monash University,undefined
[11] Física de la Materia Condensada,undefined
[12] Universidad Autónoma de Madrid,undefined
[13] Insituto de Física de la Materia Condensada (IFIMAC),undefined
[14] Universidad Autónoma de Madrid,undefined
来源
Nature Communications | / 7卷
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摘要
The assembly and regulation of viral capsid proteins into highly ordered macromolecular complexes is essential for viral replication. Here, we utilize crystal structures of the capsid protein from the smallest and simplest known viruses capable of autonomously replicating in animal cells, circoviruses, to establish structural and mechanistic insights into capsid morphogenesis and regulation. The beak and feather disease virus, like many circoviruses, encode only two genes: a capsid protein and a replication initiation protein. The capsid protein forms distinct macromolecular assemblies during replication and here we elucidate these structures at high resolution, showing that these complexes reverse the exposure of the N-terminal arginine rich domain responsible for DNA binding and nuclear localization. We show that assembly of these complexes is regulated by single-stranded DNA (ssDNA), and provide a structural basis of capsid assembly around single-stranded DNA, highlighting novel binding interfaces distinct from the highly positively charged N-terminal ARM domain.
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