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Journal of Neuroscience, Vol 15, 1869-1878, Copyright © 1995 by Society for Neuroscience
Antigen presentation by human fetal astrocytes with the cooperative effect of microglia or the microglial-derived cytokine IL-1
KC Williams, NP Dooley, E Ulvestad, A Waage, M Blain, VW Yong and JP Antel
Department of Neurology and Neurosurgery, McGill University, Montreal, Quebec, Canada.
Antigen presentation by endogenous glial cells is postulated to regulate
reactivity of immune cells that gain entry into the CNS. We have previously
observed, using a mixed lymphocyte reaction (MLR) system, that adult
human-derived microglia can function as antigen- presenting cells (APC) for
immediately ex vivo CD4+ T cells in a primary MLR (1 degree MLR) whereas
astrocytes could not. We have now found that fetal human astrocytes can
support CD4+ T cell proliferation in the presence of exogenous human
recombinant (r) IL-2, and that astrocytes can support the continued
proliferation of CD4+ T cells previously sensitized to sister astrocyte
cultures in a secondary MLR. Additionally, adult human microglia, seeded
into the nonpriming astrocyte: CD4+ T cell cocultures at non-T
cell-stimulatory concentrations of 1000-5000 microglial cells per well,
could reverse the inability of astrocytes to present antigen in the primary
MLR. To examine the cellular basis for the inability of human astrocytes to
function as APCs in the primary MLR, astrocyte- and microglial-enriched
populations were established from human embryonic and adult brain,
respectively, and analyzed for their ability to synthesize cytokines
potentially relevant as accessory signals in the MLR. Microglia had
transcript as determined by the reverse transcriptase-polymerase chain
reaction (RT-PCR) and protein as determined by bioassay for IL-1 alpha,
IL-6, and TNF alpha. Human fetal astrocytes had transcript for IL-6 but not
for IL-1 alpha or TNF alpha under basal culture conditions and following
IFN gamma stimulation. The addition of human rIL-1 from 1-50 U/ml could
reverse the inability of astrocytes to present antigen in the primary MLR.
These studies demonstrate that although in vitro highly enriched cultures
of astrocytes absent of microglia cannot present antigen to immediately ex
vivo blood-derived CD4+ T cells in the MLR, in situ, with the cooperative
help of microglia-derived cytokines or accessory surface molecules,
astrocytes may function as central nervous system APCs.
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