Upregulation of bcl-2 by the Epstein-Barr virus latent membrane protein LMP1: a B-cell-specific response that is delayed relative to NF-kappa B activation and to induction of cell surface markers.

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J Virol. 1994 September; 68(9): 5602-5612

Upregulation of bcl-2 by the Epstein-Barr virus latent membrane protein LMP1: a B-cell-specific response that is delayed relative to NF-kappa B activation and to induction of cell surface markers.

M Rowe, M Peng-Pilon, D S Huen, R Hardy, D Croom-Carter, E Lundgren and A B Rickinson

Institute of Cancer Studies, University of Birmingham Medical School, United Kingdom.

ABSTRACT

An ability of the Epstein-Barr virus latent membrane proteinLMP1 to enhance the survival of infected B cells through upregulationof the bcl-2 oncogene was first suggested by experiments involvinggene transfection and the selection of stable LMP1+ clones (S.Henderson, M. Rowe, C. Gregory, F. Wang, E. Kieff, and A. Rickinson,Cell 65:1107-1115, 1991). However, it was not possible to ascertainwhether Bcl-2 upregulation was a specific consequence of LMP1expression or an artifact of the selection procedure wherebyrare Bcl-2+ cells already present in the starting populationmight best be able to tolerate the potentially toxic effectsof LMP1. We therefore reexamined this issue by using two differentexperimental approaches that allowed LMP1-induced effects tobe monitored immediately following expression of the viral proteinand in the absence of selective pressures; activation of theNF-kappa B transcription factor and upregulation of the celladhesion molecule ICAM-1 were used as early indices of LMP1function. In the first approach, stable clones of two B-celllines carrying an LMP1 gene under the control of an induciblemetallothionein promoter were induced to express LMP1 in allcells. Activation of NK-kappa B and upregulation of ICAM-1 occurredwithin 24 h and were followed at 48 to 72 h by upregulationof Bcl-2. In the second approach, we tested the generality ofthis phenomenon by transiently expressing LMP1 from a strongconstitutively active promoter in a range of different celltypes. All six B-cell lines tested showed NF-kappa B activationin response to LMP1 expression, and this was followed in fiveof six lines by expression of ICAM-1 and Bcl-2. In the sameexperiments, all three non-B-cell lines showed NF-kappa B activationand ICAM-1 upregulation but never any effect upon Bcl-2. Wetherefore conclude that Bcl-2 upregulation is part of the panoplyof cellular changes induced by LMP1 but that the effect is celltype specific. Our data also suggest that whilst NF-kappa Bmay be an essential component of LMP1 signal transduction, othercell-specific factors may be required to effect some functionsof the viral protein.

J Virol. 1994 September; 68(9): 5602-5612

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