Author
GLADUE, DOUGLAS - University Of Connecticut | |
O'DONNELL, VIVIAN - University Of Connecticut | |
BAKER-BRANSTETTER, RYAN - Oak Ridge Institute For Science And Education (ORISE) | |
Pacheco Tobin, Juan | |
Holinka-Patterson, Lauren | |
Fernandez Sainz, Ignacio | |
LU, ZHIQIANG - Us Deparment Of Homeland Security | |
BROCCHI, E - Lombardy And Emilia Romagna Experimental Zootechnic Institute | |
BAXT, BARRY - Former ARS Employee | |
PICONNE, MARIA - University Of Connecticut | |
Rodriguez, Luis | |
Borca, Manuel |
Submitted to: Journal of Virology
Publication Type: Peer Reviewed Journal Publication Acceptance Date: 8/19/2012 Publication Date: 8/29/2012 Citation: Gladue, D.P., O'Donnell, V., Baker-Branstetter, R., Pacheco Tobin, J., Holinka-Patterson, L.G., Fernandez Sainz, I.J., Lu, Z., Brocchi, E., Baxt, B., Piconne, M.E., Rodriguez, L.L., Borca, M.V. 2012. Foot and mouth disease virus non structural protein 2C interacts with Beclin1 modulating virus replication. Journal of Virology. 86(22):12080-12090. doi:10.1128/JVI.01610-12. Interpretive Summary: Foot-and-mouth disease virus (FMDV) is the causative agent of foot-and-mouth disease. Replication of the virus is a highly multifarious process that occurs in association with host cell membrane in specific areas called replication complex. The largest viral protein found in these in the replication complex, 2C, is thought to have multiple roles during virus replication. However, studies examining the function of FMDV 2C have been rather limited. To better understand the role of 2C in the process of virus replication we used a yeast two-hybrid approach to identify host proteins that interact with 2C. We report here that cellular Beclin1 is a specific host binding partner for 2C. Beclin1 is an important regulator of a cellular metabolic pathway named authophagy, which is required for efficient FMDV replication. We present evidence that confirmed that 2C-Beclin1 interaction initially identified by the yeast two-hybrid approach was further confirmed by co-immunoprecipitation and confocal microscopy to actually occur in FMDV infected cells. Interestingly, the induction of over-expression of Beclin1 strongly reduces virus yield in cell culture. Further work demonstrated that this excess of Beclin1estimulates the enzymatic destruction of virus inside the infected cells, a process that is normally absent during the infection. It is proposed as a hypothesis that during the infection 2C binds to Beclin1 to prevent the enzymatic destruction of the virus. These results suggest that interaction between FMDV 2C and host protein Beclin1 could be essential for virus replication and perhaps a potential target to develop anti-viral strategies. Technical Abstract: Foot-and-mouth disease virus (FMDV), the causative agent of foot-and-mouth disease (FMD), is an Apthovirus within the Picornaviridae family. Replication of the virus occurs in association with replication complexes that are formed by host cell membrane rearrangements. The largest viral protein in the replication complex, 2C, is thought to have multiple roles during virus replication. However, studies examining the function of FMDV 2C have been rather limited. To better understand the role of 2C in the process of virus replication we used a yeast two-hybrid approach to identify host proteins that interact with 2C. We report here that cellular Beclin1 is a specific host binding partner for 2C. Beclin1 is a regulator of the autophagy pathway, a metabolic pathway required for efficient FMDV replication. The 2C-Beclin1 interaction initially identified by the yeast two-hybrid approach was further confirmed by co-immunoprecipitation and confocal microscopy to actually occur in FMDV infected cells. Over-expression of either Beclin1 or Bcl-2, another important autophagy factor, strongly affects virus yield in cell culture. The fusion of lysosomes to autophagosomes containing viral proteins is not seen during FMDV infection, a process that is stimulated by Beclin1; however, in FMDV-infected cells over-expressing Beclin1 this fusion occurs, suggesting that 2C binds to Beclin1 to prevent the fusion of lysosomes to autophagosomes, allowing for virus survival. The critical amino acid residues in 2C that mediate the interaction with Beclin1 were mapped in detail using alanine scanning mutagenesis. Using reverse genetics we demonstrated that modifications to 2C in areas critical for interaction with Beclin1 are also critical for virus growth. These results suggest that interaction between FMDV 2C and host protein Beclin1 could be essential for virus replication. |