Multivalent interactions essential for lentiviral integrase function

Author:

Ballandras-Colas Allison,Chivukula Vidya,Gruszka Dominika T.,Shan Zelin,Singh Parmit K.,Pye Valerie E.,McLean Rebecca K.,Bedwell Gregory J.,Li Wen,Nans Andrea,Cook Nicola J.,Fadel Hind J.,Poeschla Eric M.,Griffiths David J.,Vargas JavierORCID,Taylor Ian A.,Lyumkis Dmitry,Yardimci Hasan,Engelman Alan N.,Cherepanov PeterORCID

Abstract

AbstractA multimer of retroviral integrase (IN) synapses viral DNA ends within a stable intasome nucleoprotein complex for integration into a host cell genome. Reconstitution of the intasome from the maedi-visna virus (MVV), an ovine lentivirus, revealed a large assembly containing sixteen IN subunits (1). Herein, we report cryo-EM structures of the lentiviral intasome prior to engagement of target DNA and following strand transfer, refined at 3.4 and 3.5 Å resolution, respectively. The structures elucidate details of the protein-protein and protein-DNA interfaces involved in lentiviral intasome formation. We show that the homomeric interfaces involved in IN hexadecamer formation and the α-helical configuration of the linker connecting the C-terminal and catalytic core domains are critical for MVV IN strand transfer activity in vitro and for virus infectivity. Single-molecule microscopy in conjunction with photobleaching revealed that the MVV intasome can bind a variable number, up to sixteen molecules, of the lentivirus-specific host factor LEDGF/p75. Concordantly, ablation of endogenous LEDGF/p75 resulted in gross redistribution of MVV integration sites in human and ovine cells. Our data confirm the importance of the expanded architecture observed in cryo-EM studies of lentiviral intasomes and suggest that this organization underlies multivalent interactions with chromatin for integration targeting to active genes.

Publisher

Cold Spring Harbor Laboratory

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