Bovine herpesvirus type 4 (BoHV-4), like other herpesviruses, induces a series of alterations in the host cell that modify the intracellular environment in favor of viral replication, survival and spread. This research examined the impact of BoHV-4 infection on autophagy in BoHV-4 infected Madin Darby bovine kidney (MDBK) cells. Protein extracts of BoHV-4 infected and control MDBK cells were subjected to Western blot. The concentrations of the autophagy and apoptosis-related proteins Beclin 1, p21, PI3 kinase, Akt1/2, mTOR, phospho mTOR, p62 and the light chain three (LC3) were normalized to the actin level and expressed as the densitometric ratio. Western blot analysis of virus-infected cells revealed that autophagic degradation pathway was induced in the late phase of BoHV-4 infection. After 48 h post-infection the protein LC3II, which is essential for autophagy was found to be markedly increased, while infection of MDBK cells with BoHV-4 resulted in a depletion of p62 levels. Becline 1, PI3 kinase, Akt1/2 and p21 expression increased between 24 and 48 h post-infection. Surprisingly, mTOR and its phosphorylated form, which are negative regulators of autophagy, also increased after 24 h post-infection. In conclusion, our findings suggest that BoHV-4 has developed mechanisms for modulation of autophagy that are probably part of a strategy designed to enhance viral replication and to evade the immune system. Additional studies on the relationship between autophagy and BoHV-4 replication and survival, in both lytic and latent replication phases, are needed to understand the role of autophagy in BoHV-4 pathogenesis.

Bovine herpesvirus type 4 infection modulates autophagy in a permissive cell line / Montagnaro, Serena; Ciarcia, Roberto; Pagnini, F; DE MARTINO, Luisa; Puzio, Mv; Granato, Ge; Avino, F; Pagnini, Ugo; Iovane, Giuseppe; Giordano, A.. - In: JOURNAL OF CELLULAR BIOCHEMISTRY. - ISSN 1097-4644. - 114:7(2013), pp. 1529-1535. [10.1002/jcb.24494]

Bovine herpesvirus type 4 infection modulates autophagy in a permissive cell line.

MONTAGNARO, SERENA;CIARCIA, ROBERTO;DE MARTINO, LUISA;PAGNINI, UGO;IOVANE, GIUSEPPE;
2013

Abstract

Bovine herpesvirus type 4 (BoHV-4), like other herpesviruses, induces a series of alterations in the host cell that modify the intracellular environment in favor of viral replication, survival and spread. This research examined the impact of BoHV-4 infection on autophagy in BoHV-4 infected Madin Darby bovine kidney (MDBK) cells. Protein extracts of BoHV-4 infected and control MDBK cells were subjected to Western blot. The concentrations of the autophagy and apoptosis-related proteins Beclin 1, p21, PI3 kinase, Akt1/2, mTOR, phospho mTOR, p62 and the light chain three (LC3) were normalized to the actin level and expressed as the densitometric ratio. Western blot analysis of virus-infected cells revealed that autophagic degradation pathway was induced in the late phase of BoHV-4 infection. After 48 h post-infection the protein LC3II, which is essential for autophagy was found to be markedly increased, while infection of MDBK cells with BoHV-4 resulted in a depletion of p62 levels. Becline 1, PI3 kinase, Akt1/2 and p21 expression increased between 24 and 48 h post-infection. Surprisingly, mTOR and its phosphorylated form, which are negative regulators of autophagy, also increased after 24 h post-infection. In conclusion, our findings suggest that BoHV-4 has developed mechanisms for modulation of autophagy that are probably part of a strategy designed to enhance viral replication and to evade the immune system. Additional studies on the relationship between autophagy and BoHV-4 replication and survival, in both lytic and latent replication phases, are needed to understand the role of autophagy in BoHV-4 pathogenesis.
2013
Bovine herpesvirus type 4 infection modulates autophagy in a permissive cell line / Montagnaro, Serena; Ciarcia, Roberto; Pagnini, F; DE MARTINO, Luisa; Puzio, Mv; Granato, Ge; Avino, F; Pagnini, Ugo; Iovane, Giuseppe; Giordano, A.. - In: JOURNAL OF CELLULAR BIOCHEMISTRY. - ISSN 1097-4644. - 114:7(2013), pp. 1529-1535. [10.1002/jcb.24494]
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11588/561806
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