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Active lytic infection of human primary tonsillar B cells by KSHV and its noncytolytic control by activated CD4+ T cells
Jinjong Myoung, Don Ganem
Jinjong Myoung, Don Ganem
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Research Article

Active lytic infection of human primary tonsillar B cells by KSHV and its noncytolytic control by activated CD4+ T cells

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Abstract

Kaposi sarcoma–associated herpesvirus (KSHV) is a B-lymphotropic virus whose primary site of replication is the oropharynx. KSHV can infect both T and B cells from primary tonsillar explant cultures. However, T cells do not support lytic replication, while B cells spontaneously produce substantial amounts of infectious virus. Here, we provide evidence for a mechanism by which activated T cells may promote or stabilize latency of KSHV infection in B cells. When mixed cultures of B cells and activated T cells were exposed to KSHV, little spontaneous virus production was observed. Removing T cells from the mix or treating the mixed culture with immune suppressants enhanced virus production. Adding back activated T cells to purified infected B cells efficiently suppressed KSHV production, primarily due to CD4+ T cells. This suppressive activity required T cell activation and direct cell-cell contact, but not prior exposure to KSHV antigen. Suppression was not MHC restricted and did not result in killing of the target cell. We therefore propose that oropharyngeal T cells activated by a variety of stimuli can recognize ligands on infected target B cells, leading to signaling events that prevent spontaneous lytic activation and promote latent infection in this compartment.

Authors

Jinjong Myoung, Don Ganem

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Figure 1

Isolated B cells support spontaneous lytic replication of KSHV.

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Isolated B cells support spontaneous lytic replication of KSHV.
PHA-stim...
PHA-stimulated unfractionated tonsillar cells and fractionated T or B cells were infected by rKSHV.219 at MOI 3 for 6 to 12 hours (the length of viral infection did not affect the outcomes). Excess unbound viruses were extensively washed. Infected cultures were left uninduced or induced by valproate (600 μM) and/or CsA (1 μg/ml) for 5 days. Culture supernatants were titrated on 293 cells, and IUs (see Methods) were plotted with background subtracted. Each dot represents IUs in the culture supernatant of each individual tonsillar cell. The mean of data from 6 different tonsils is indicated by the horizontal bar. *P < 0.05; ***P < 0.001 by Student’s t test.

Copyright © 2026 American Society for Clinical Investigation
ISSN: 0021-9738 (print), 1558-8238 (online)

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