Retroviral Capsid Assembly: A Role for the CA Dimer in Initiation

Retroviral Capsid Assembly: A Role for the CA Dimer in Initiation

In maturing retroviral virions, CA protein assembles to form a capsid shell that is essential for infectivity. The structure of the two folded domains [N-terminal domain (NTD) and C-terminal domain (CTD)] of CA is highly conserved among various retroviruses, and the capsid assembly pathway, although...

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Veröffentlicht in:Journal of molecular biology 2009-06, Vol.389 (2), p.438-451
Hauptverfasser: Purdy, John G., Flanagan, John M., Ropson, Ira J., Craven, Rebecca C.
Format: Artikel
Sprache:eng
Schlagworte:
CA protein
Capsid - chemistry
Capsid Proteins - physiology
electrostatic control of assembly
Kinetics
nucleation of capsid assembly
Protein Multimerization
Retroviridae
Retrovirus
retrovirus maturation
Rous sarcoma virus
Rous sarcoma virus - physiology
Static Electricity
Virus Assembly
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container_end_page 451
container_issue 2
container_start_page 438
container_title Journal of molecular biology
container_volume 389
creator Purdy, John G.
Flanagan, John M.
Ropson, Ira J.
Craven, Rebecca C.
description In maturing retroviral virions, CA protein assembles to form a capsid shell that is essential for infectivity. The structure of the two folded domains [N-terminal domain (NTD) and C-terminal domain (CTD)] of CA is highly conserved among various retroviruses, and the capsid assembly pathway, although poorly understood, is thought to be conserved as well. In vitro assembly reactions with purified CA proteins of the Rous sarcoma virus (RSV) were used to define factors that influence the kinetics of capsid assembly and provide insights into underlying mechanisms. CA multimerization was triggered by multivalent anions providing evidence that in vitro assembly is an electrostatically controlled process. In the case of RSV, in vitro assembly was a well-behaved nucleation-driven process that led to the formation of structures with morphologies similar to those found in virions. Isolated RSV dimers, when mixed with monomeric protein, acted as efficient seeds for assembly, eliminating the lag phase characteristic of a monomer-only reaction. This demonstrates for the first time the purification of an intermediate on the assembly pathway. Differences in the intrinsic tryptophan fluorescence of monomeric protein and the assembly-competent dimer fraction suggest the involvement of the NTD in the formation of the functional dimer. Furthermore, in vitro analysis of well-characterized CTD mutants provides evidence for assembly dependence on the second domain and suggests that the establishment of an NTD–CTD interface is a critical step in capsid assembly initiation. Overall, the data provide clear support for a model whereby capsid assembly within the maturing virion is dependent on the formation of a specific nucleating complex that involves a CA dimer and is directed by additional virion constituents.
doi_str_mv 10.1016/j.jmb.2009.04.006
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source MEDLINE; Elsevier ScienceDirect Journals
subjects CA protein
Capsid - chemistry
Capsid Proteins - physiology
electrostatic control of assembly
Kinetics
nucleation of capsid assembly
Protein Multimerization
Retroviridae
Retrovirus
retrovirus maturation
Rous sarcoma virus
Rous sarcoma virus - physiology
Static Electricity
Virus Assembly
title Retroviral Capsid Assembly: A Role for the CA Dimer in Initiation
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