Human herpesvirus 8 interleukin-6 contributes to primary effusion lymphoma cell viability via suppression of proapoptotic cathepsin D, a cointeraction partner of vitamin K epoxide reductase complex subunit 1 variant 2.

[primary effusion lymphoma]

Human herpesvirus 8 (HHV-8 ) interleukin-6 (vIL-6 ) promotes cell proliferation and survival and is proangiogenic , implicating it as a contributor to virus-associated Kaposi 's sarcoma , primary effusion lymphoma (PEL ), and multicentric Castleman 's disease . Although predominantly lytically expressed , vIL-6 is also produced at low , functional levels during latency in PEL cells . Unlike other IL -6 cytokines , vIL-6 is secreted very inefficiently and localizes in the endoplasmic reticulum (ER ). ER-localized vIL-6 supports PEL cell proliferation and survival , mediated in part through its interaction with the largely uncharacterized ER-resident protein vitamin K epoxide reductase complex subunit 1 variant 2 (VKORC 1 v 2 ). Here , we report that the ER-transiting and functionally mitogenic secreted proenzyme (pCatD ) form of cathepsin D (mature CatD ), a proapoptotic lysosomal aspartate protease , is an interaction partner of VKORC 1 v 2 and that vIL-6 promotes this interaction . Depletion of vIL-6 in PEL cells increased levels of the catalytically active , proteolytically cleaved form of CatD , corresponding with decreased PEL cell viability . Ectopic expression of CatD in PEL cells induced apoptosis , suggesting that CatD suppression by vIL-6 is biologically significant . In the context of high -density culture or reactivation of HHV-8 lytic replication in PEL cells , CatD depletion substantially reduced stress-induced apoptosis and increased virus production . In contrast , CatD overexpression , vIL-6 depletion , and peptide-mediated disruption of vIL-6 -VKORC 1 v 2 interaction inhibited replication and cell survival . Combined , our data identify pCatD as an interaction partner of VKORC 1 v 2 , demonstrate a role of vIL-6 in CatD suppression via VKORC 1 v 2 in PEL cells , and identify a biologically significant mechanism of vIL-6 prosurvival and proreplication activities via VKORC 1 v 2 .