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Journal of Virology, November 2000, p. 10438-10446, Vol. 74, No. 22
Vaccine Research Institute of San Diego, San
Diego, California 92121,1 and Department
of Neuropharmacology, Division of Virology, The Scripps Research
Institute, La Jolla, California 920372
Received 2 June 2000/Accepted 23 August 2000
Borna disease virus (BDV), a nonsegmented, negative-stranded (NNS)
RNA virus, causes central nervous system (CNS) disease in a broad range
of vertebrate species, including felines. Both viral and host factors
contribute to very diverse clinical and pathological manifestations
associated with BDV infection. BDV persistence in the CNS can cause
neurobehavioral and neurodevelopmental abnormalities in the absence of
encephalitis. These BDV-induced CNS disturbances are associated with
altered cytokine and neurotrophin expression, as well as cell damage
that is very restricted to specific brain regions and neuronal
subpopulations. BDV also targets astrocytes, resulting in the
development of prominent astrocytosis. Astrocytes play essential roles
in maintaining CNS homeostasis, and disruption of their normal
activities can contribute to altered brain function. Therefore, we have
examined the effect of BDV infection on the astrocyte's physiology. We
present here evidence that BDV can establish a nonlytic chronic
infection in primary cortical feline astrocytes that is associated with
a severe impairment in the astrocytes' ability to uptake glutamate. In
contrast, the astrocytes' ability to uptake glucose, as well as their
protein synthesis, viability, and rate of proliferation, was not
affected by BDV infection. These findings suggest that, in vivo, BDV
could also affect an important astrocyte function required to
prevent neuronal excitotoxicity. This, in turn, might contribute
to the neuropathogenesis of BDV.
Borna disease (BD)
virus (BDV) causes central nervous system (CNS) disease in a
broad range of vertebrate species (36, 43, 48, 63, 65). BDV
has a nonsegmented, negative-strand (NNS) RNA genome (9,
17). Based on its unique genetic and biological features, BDV is
considered to be the prototypic member of a new virus family,
Bornaviridae, within the order Mononegavirales
(19, 68).
Naturally occurring BDV infections were thought to be mainly restricted
to horses and sheep within certain geographic regions of central
Europe. Current evidence, however, indicates that the natural host
range, geographic distribution, and prevalence of BDV are much broader
than previously considered (36, 43, 63, 65). The genetics,
immune status, and age of the host, as well as viral factors,
contribute to a high degree of heterogeneity in disease symptoms and
pathological manifestations associated with BDV infection. Clinical
manifestations can range from dramatic to subtle or even been
unapparent (32, 36, 43, 63, 65). Nevertheless, all known BDV
isolates are noncytolytic and highly neurotropic (43, 48,
65). Heightened viral gene expression in limbic system structures
and neuronal structural alterations within the hippocampal formation
are the main histopathological hallmarks of BDV infection (32, 34,
35). Immune cell infiltrates are frequently, but not always,
observed in the CNS of BDV-infected animals, and immune-mediated
neuronal damage is thought to be responsible for the clinical symptoms
associated with classic BD (5, 48, 65, 71). BDV affects the
postnatal development of the brain monoaminergic system
(61). However, the cellular and molecular mechanisms whereby
BDV causes CNS disturbances in the absence of encephalitis
remain largely unknown (1, 2, 11, 24, 32, 33, 40, 42,
66).
BDV persistence in the CNS is also characterized by infection of
astrocytes (10, 12, 13) and development of prominent astrocytosis (32, 34, 48, 65). The reactive astrocyte response is a near universal response to brain insults, including viral
infection, and represents a complex process involving profound changes
in the astrocyte gene expression program (28, 57). Astrocytes play essential roles in the maintenance of a CNS
microenvironment compatible with proper neuronal activity (3, 28,
69). Disturbances in astrocyte functions can induce or enhance
neuronal pathology by affecting complex interactions within neuronal
networks (3, 28, 37, 57). Thus, astrocyte glutamate
transporters are essential to maintain low extracellular levels of
glutamate, the major excitatory neurotransmitter in the CNS
(64). Excessive extracellular glutamate levels would
activate neuronal N-methyl-D-aspartic acid
(NMDA) receptors, leading to an increase in calcium influx, which can
result in neurotoxicity and cell death (25, 45, 47, 67).
Both human immunodeficiency virus (HIV) and feline immunodeficiency
virus (FIV) have been shown to affect glutamate uptake by astrocytes,
which is likely to contribute to the neuropathogenesis of these
two lentiviruses (4, 4a, 15, 25, 73, 78). We have
previously documented the preparation of primary feline astrocyte (FeAst) cultures that maintain many of their normal physiological activities, including glutamate and glucose uptake (78). Using this culture system, we have examined whether
BDV persistence in astrocytes leads to an impairment of their normal cell physiology, which in turn could contribute to neuronal damage and
disturbances in CNS functions associated with cases of BDV infection
that proceed in the absence of encephalitis. Here, we present
evidence that BDV can establish a nonlytic chronic infection in primary feline cortical astrocytes that is associated with a severe
and specific impairment in the astrocytes' ability to uptake
glutamate. We discuss the implications of this finding with respect to
the neuropathogenesis of BDV.
Cells and viruses. (i) Enriched astrocyte cultures.
Primary
cultures of cerebral cortical astrocytes were prepared from 2-day-old
offspring of specific-pathogen-free (SPF) cats as described previously
(55, 79) with some modification (6). Briefly,
forebrains were removed aseptically from the skulls; the meninges were
excised under a dissecting microscope, and neocortices were dissected.
The cells were dissociated, without trypsin, by passage through needles
of decreasing gauges (16G1, 19G1, and 25G1) two to three times with a
10-ml syringe. The cells were seeded at a density of 105
cells per cm2 on 12-well tissue culture plates (Costar) in
Dulbecco's modified Eagle's medium (DMEM) (BioWhittaker) containing
10% fetal bovine serum (FBS) and 25 mM glucose and then incubated at
37°C in an atmosphere containing 5% CO2 at 95% humidity.
(ii) Cell lines.
C6 cells (ATCC CCL 107), derived from a rat
glial tumor, were grown in DMEM containing penicillin, streptomycin,
1% glutamine, and 10% heat-inactivated FBS. C6-lacZ cells were
derived from a clone of C6 cells that was stably transfected with a
lacZ gene expression vector which conferred to the cells
high (iii) Virus stock.
The Giessen strain He/80 of BDV was
passaged three times in Lewis rats by intracerebral inoculation. Brain
homogenate from the fourth passage (BDVRp4) was prepared as described
previously (16). Aliquots of BDVRp4 stock were stored at
RNA analysis.
Total RNA was isolated by the TRI reagent
procedure (MRC, Inc., Cincinnati, Ohio). RNA samples were dissolved in
0.5 mM EDTA and stored at Detection of viral proteins. (i) Indirect immunofluorescence
(IIF).
Cells were grown on coverslips and fixed with
acetone-methanol (50:50) for 5 min at room temperature. After several
washes with phosphate-buffered saline (PBS), cells were blocked with PBS-10% normal goat serum for 60 min at room temperature. Double labeling of BDV antigens and the astrocytic marker glial fibrillary acidic protein (GFAP) was done by using a rat serum to BDV and a rabbit
polyclonal serum to GFAP. Binding of primary antibodies was detected
with species-matched secondary antibodies conjugated to either
fluorescein isothiocyanate or rhodamine.
(ii) Immunoblot analysis.
WCE were prepared in 1× sodium
dodecyl sulfate (SDS)-loading buffer (50 mM Tris-HCl [pH 6.5], 100 mM dithiothreitol, 2% SDS, 0.1% BPB, 10% glycerol). Extracts were
analyzed by Western blotting with rabbit polyclonal antibodies to BDV
nucleoprotein (NP [p40]) and phosphoprotein (P [p24]) antigens, as
described previously (20, 31).
Cell proliferation and rate of protein synthesis. (i) Cell
proliferation.
Viable cells were determined by trypan blue
staining. The number of cells for each time point was determined in triplicate.
(ii) Rate of protein synthesis.
Cells were starved for 45 min in medium without cysteine and methionine and containing 1%
dialyzed FBS. 35S-Trans label was added to the cultures (50 µCi/ml). At the indicated postlabeling times, whole-cell lysates were
made by using 1× SDS-gel loading buffer. Incorporation of labeling
into macromolecules was determined by precipitation with
trichloroacetic acid and measurement of 35S label by liquid
scintillation counting.
Glucose uptake assay.
Uptake experiments were conducted
weekly after infection as described previously (78).
Briefly, after the medium was removed, cells were incubated for 3 h in 0.5 ml of serum-free DMEM, containing 5 mM instead of 25 mM
glucose (DMEM5), at 37°C in an atmosphere containing 5%
CO2 at 95% humidity. Afterward, 0.5 ml of fresh DMEM
containing [3H]2-deoxy-D-glucose
(3H-2DG) (final concentration, 48 nM) was added for an
additional 20-min incubation. Uptake was terminated by aspirating the
uptake solution and washing the cells three times with 2 ml of ice-cold PBS. Astrocytes were then lysed by adding 0.5 ml of 10 mM NaOH containing 0.1% Triton X-100, and a 300-µl portion was assayed for
3H by liquid scintillation counting. The protein content
was measured by the method of Bradford (8) in 100 µl of
the remaining lysate. 3H-2DG uptake was expressed in
femtomoles per milligram of protein.
Glutamate uptake assay.
The uptake of
[3H]glutamate (3H-Glu) was determined by the
method described by Volterra et al. (74). Briefly, after
infection and supernatant collection, the medium was replaced by 0.5 ml of fresh medium containing 50 µM glutamate and 18.5 kBq (9.25 pmol)
of 3H-Glu. Uptake was terminated 15 min later by removing
the supernatant and washing the cells three times with 2 ml of ice-cold
PBS containing 5 mM glutamate. Astrocytes were then lysed by 0.5 ml of
10 mM NaOH containing 0.1% Triton X-100, and a 300-µl portion was
assayed for 3H by liquid scintillation counting. The
protein content was measured (8) in 100 µl of the
remaining lysate. Uptake was expressed in femtomoles per milligram of protein.
Statistical analysis and image processing.
A two-factor
(BDV-uninfected versus BDV-infected cultures for 4 to 6 days)
between-group analysis of variance was applied to the mean from
each triplicate for each experiment. Scheffe's contrast procedures
were used to perform post hoc comparisons between the infected
conditions for each day. All agarose gel pictures were taken with a
Stratagene Eagle eye camera. Pictures were scanned with an Agfa
Studiostar scanner, and the composite images were generated with Adobe Photoshop.
Primary FeAst are susceptible to BDV.
We first tested whether
primary FeAst could be infected with our rat-adapted laboratory stock
BDV-He80 strain without requiring adaptation passages in feline cells.
This BDV-He80 viral stock corresponded to the fourth passage in brain
tissue of newborn infected rats. We infected primary FeAst with
BDV-He80 at a multiplicity of infection (MOI) of 0.1 FFU/cell and
analyzed the synthesis of BDV RNA, as well as expression of
viral antigen and production of infectious virus (Fig.
1). Both BDV genomic and subgenomic viral
mRNAs were readily detected by Northern blot hybridization at 48 h
postinfection (p.i.) (Fig. 1A). Levels of BDV genome and mRNA increased
significantly from 48 to 72 h p.i.; thereafter, and until the last
time point analyzed (6 days p.i.), levels of genome RNA remained at the
same level, whereas BDV NP mRNA showed a modest, steady increase (Fig.
1A). No differences were observed between BDV- and mock-infected FeAst
with respect to the levels of the housekeeping cellular mRNA GAPDH
(Fig. 1A). Consistent with our previous findings (78), the
majority of the cells (>90%) were positive for the astrocyte marker
GFAP (Fig. 1B), reflecting a high degree of purity in our astrocyte
primary cultures. About 85% of the cells in the population were
positive for BDV NP antigen at 72 h p.i. as determined by
immunofluorescence (IF) (Fig. 1B and C). The majority of cells that
scored positive in IF for BDV antigen were also GFAP positive. However,
there was a low percentage (ca. 3%) of BDV-positive cells that were
not immunolabeled by the anti-GFAP antibody (Fig. 1C). The cell lineage
of these GFAP-negative cells was not determined in this study. However,
we have previously shown that 2 to 3% of the cells in these primary
astrocyte cultures are microglia, as determined by nonspecific esterase
staining (30). BDV infection of FeAst was productive, since
infectious virus progeny was detected 24 h p.i. (Fig. 1D). Viral
titers increased significantly between 24 and 72 h p.i., followed
by a plateau effect that was maintained until 120 h p.i., the last
time point analyzed (Fig. 1D). Throughout the entire kinetics
experiment, BDV infectivity remained cell associated, and we were
unable to detect at any time cell-free infectious particles in the
tissue culture supernatant (data not shown). We also observed a
correlation between the number of infected cells and production of BDV
infectious progeny (Fig. 1E).
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Borna Disease Virus Persistence Causes Inhibition of Glutamate
Uptake by Feline Primary Cortical Astrocytes
ABSTRACT
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
-galactosidase activity that can be easily detected by in situ
staining for -galactosidase. C6-lacZ cells were grown similarly to
the C6 cells, but with G418 (250 µg/ml) incorporated into the medium
for selection of stably transfected cells.
70°C. The infectious titer (focus-forming units [FFU] per
milliliter) of BDVRp4, as well as those of supernatants and whole-cell
extracts (WCE) from BDV-infected FeAst, was determined by an
immunofocus assay as described previously (16, 39).
Preparation of WCE was done by three cycles of freezing and thawing,
followed by ultrasonication on ice.
70°C. Total RNA (5 µg) from
BDV-infected and mock-infected primary FeAst, as well as from C6 cells,
was analyzed by Northern blot hybridization as described previously
(16, 17). Briefly, RNA was size fractionated by 2.2 M
formaldehyde-agarose gel electrophoresis, transferred by capillarity
with 20× SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate) to
MagnaGraph nylon membrane (MSI, Westboro, Mass.), and UV cross-linked.
Hybridization with 32P-labeled BDVp40 or GAPDH-specific
probes was performed as described previously (16, 17).
Methylene blue (MB) staining of the membrane after transfer and prior
hybridization was used to verify that similar amounts of total RNA were
loaded in all cases.
RESULTS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
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FIG. 1.
(A) Synthesis of BDV RNA in primary FeAst. Primary cat
astrocytes were infected with BDV-He80 at an MOI of 0.1 FFU/cell. At
the indicated times, total RNA from mock- and BDV-infected cells was
analyzed by Northern blot hybridization. BDV genomic and NP mRNAs were
detected with a 32P-labeled NP DNA probe. As a control, the
same blot was also hybridized with a probe for the housekeeping
cellular mRNA GAPDH. MB staining of the membrane after transfer and
prior hybridization was used to verify that similar amounts of total
RNA were loaded in all cases. The positions of the 28S and 18S rRNAs
are indicated. (B) Detection of BDV NP antigen and GFAP expression in
primary FeAst. BDV-infected cells (INF) and mock-infected controls were
fixed at 96 h p.i. and analyzed by indirect immunofluorescence.
Cells were simultaneously labeled with a rabbit antiserum to GFAP
( 
GFAP) and a rat serum to BDV (BDV). (C) The percentage of cells
expressing one or both antigens was determined by counting cells (total
of 250) from five or six different fields. Shown are the average and
standard deviation from two independent experiments. ND, not
determined. (D) Kinetics of BDV multiplication in primary FeAst. Cells
were infected with BDV-He80 at an MOI of 0.1 FFU/cell. At the indicated
times p.i., BDV infectivity in supernatant and in WCE was determined.
Only cell-associated infectivity was detected. Values correspond to the
average and standard deviation of two independent experiments. (E)
Number of BDV-infected cells at different times p.i. FeAst were
infected at an MOI of 0.1 FFU/cell, and at the indicated times after
infection, cells were fixed and examined for expression of BDV NP
antigen by IIF. Values correspond to the average and standard deviation
of two independent experiments.
BDV establishes a nonlytic chronic infection in primary FeAst. Once we verified that primary FeAst were susceptible to BDV, we examined whether BDV could establish a long-term persistent infection in these cells. Primary FeAst were infected with BDV-He80 at an MOI of 0.1 FFU/cell, and 5 days p.i., cells were subcultured at a 1/3 ratio. After 15 days, these cells (FeAst/BDVp1) were subcultured again (1/3 ratio). Subsequent cell passages were done every 20 days, with passage 5 (p5) (100 days p.i.) as the end point of the experiment. As a control, we used mock-infected FeAst cells that were handled in an identical manner to the BDV-infected cells.
Viral genome and subgenomic NP mRNA were readily detected at 80 days p.i. (four cell passages, FeAst/BDVp4) by Northern blot hybridization (Fig. 2A). Likewise, BDV NP and P gene products were detected in FeAst/BDV cells (Fig. 2B). Levels of both BDV genomic and mRNA species in FeAst/BDVp4 were slightly decreased compared to those detected at in BDV-infected FeAst at day 4 p.i., as well as in C6 cells persistently infected with BDV-He80 for 40 days (C6BVp10) (compare Fig. 1A and 2A). IF results showed that most of the cells within the BDV persistently infected FeAst cell population expressed both GFAP and BDV NP antigen (Fig. 2C and Table 1). These results indicated that primary FeAst can sustain long-term BDV replication and transcription. We observed a small, but consistent, percentage of cells that were positive for viral antigen, but negative for GFAP. This subpopulation of GFAP-negative cells did not increase from passages 1 to 5, indicating that they were not being selected under the tissue culture conditions used in our study (Table 1). The percentage of GFAP-negative cells in BDV persistently infected FeAst was similar to that observed in mock-infected control FeAst, suggesting that BDV infection did not affect the expression of this astrocyte marker.
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Infectivity associated with FeAst persistently infected with
BDV.
A characteristic feature of BDV-infected cultured cells is
the extremely low levels, or complete lack, of cell-free virus (CFV).
Likewise, the infectivity detected in FeAst/BDV cultures was cell
associated and remained at similar levels (8 × 103 to
10 × 104 FFU/105 cells) from passages 1 to 5 (100 days of persistence). We did not detect CFV in the tissue
culture supernatant at any time throughout the entire course of the
observation period of the BDV persistently infected FeAst (data not
shown). This finding led us to consider whether BDV-susceptible cells
could become infected when cocultured with BDV persistently infected
FeAst. For this, we cocultured FeAst/BDV and C6-lacZ cells at a 1:1
ratio. The percentage of cells within the population positive for both
LacZ and BDV NP antigen increased from 0 to about 50% between 12 and
72 h after seeding of the cells (Fig.
4). Concomitantly, the majority (>90%) of the cells within the population became BDV NP positive at 72 h
postseeding (Fig. 4).
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BDV affects glutamate uptake in FeAst.
To assess the effects
of BDV infection on astrocyte function, we performed a glutamate uptake
assay. As a baseline, we measured glutamate uptake in mock-infected
cells, which averaged 8,619.07 ± 2,238.11 fmol/mg/15 min, a value
within the same range obtained under similar conditions with human
astrocytes (29). We then determined the ratio of glutamate
uptake between infected and mock-infected control cells that were
identically and simultaneously processed. During the first 10 days
p.i., which we designated as the acute phase of the infection, BDV did
not cause any significant alteration in the 3H-Glu uptake
(Fig. 5A), although the
infected cells showed a tendency toward increased 3H-Glu
uptake during this time. These results were in marked contrast to the
findings with the persistently infected cultures (Fig. 5B). We observed
a very dramatic and sustained effect on the glutamate uptake in
astrocyte cultures persistently infected with BDV. Glutamate uptake was
almost completely inhibited in FeAst/BDVp4 cells, reaching only 2 and
1% at 80 and 91 days p.i., respectively, compared to that in controls.
A strong inhibition of glutamate uptake was still observed at day
96 p.i. (27% of the control value). These results were
statistically significant for all time points to the P < 0.001 level (Fig. 5B).
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DISCUSSION |
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Abstract
Introduction
Materials and Methods
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Discussion
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This study provides, for the first time, evidence that a rat-adapted strain of BDV can establish a nonlytic productive persistent infection in feline cortical astrocytes that is associated with a selective and nearly complete inhibition of the astrocyte's ability to uptake glutamate, an important function required to prevent neuronal excitotoxicity (46).
Diverse mechanisms are likely to contribute to BDV-induced CNS disturbances. Classic BD, both naturally occurring and experimentally induced, is an immune-mediated biphasic behavioral disease that is characterized by a strong immune cell inflammatory response within the CNS (58). In contrast, neonatally infected rats do not have inflammation and are free of clinical signs of classic BD, namely severe neurological disturbances together with high morbidity and mortality. Nonetheless, these rats, referred to as BDV/PTI-NB, exhibit distinct cognitive, neurobehavioral, and specific neurodevelopmental abnormalities (1, 2, 11, 24, 40), which are associated with specific neurochemical alterations (42, 60, 61). The cellular and molecular bases of these BDV-induced CNS disturbances are not well understood. BDV appears to have a specifically enhanced affinity for areas with a high density of aspartate and glutamate receptors in the hippocampal formation, which might contribute to impaired brain function (22). Brains of BDV/PTI-NB rats exhibit a chronic upregulation in the expression levels of several proinflammatory cytokines (66). Altered cytokine expression in the CNS can contribute to the BDV interference with neuroplasticity processes in specific cell populations seen in BDV/PTI-NB rats, thus leading to disturbances in cognitive function (33). Increased cytokine expression by CNS resident cells, mainly microglia and astrocytes, could also modulate astrocyte function, as well as affect the supply of factors required for survival of selective neuronal populations within the cortex and limbic system structures (33).
Astrocytes are the most common cell type in the brain and play a key role in maintaining the appropriate microenvironment in the CNS required for normal neuronal activity (3, 27). One of the most important functions of astrocytes is to regulate the level of extracellular glutamate, a major excitatory neurotransmitter (64). Glutamate accumulates as a consequence of neuronal activity (64). Excessive levels of extracellular glutamate often result in neuron toxicity and death (64). Thus, the astrocyte's function of controlling levels of extracellular glutamate in the brain is essential to maintaining the health of the neuron. Evidence indicates that glutamate-mediated neurotoxicity may play a major role in CNS disorders, including virus-induced diseases (25, 45, 47, 67). Astrocytes are the main cellular target of BDV in the CNS; hence it would be plausible that the disruption of the astrocyte's ability to prevent glutamate-mediated neurotoxicity could contribute to BDV-induced CNS dysfunction in the absence of encephalitis.
BDV dramatically altered glutamate uptake by long-term persistently
infected primary FeAst. This BDV-mediated impairment in glutamate
uptake by astrocytes was not observed during the initial phase of
infection (first 10 days after infection). However, the numbers of
BDV-infected cells and levels of BDV replication were similar in both
cases. This finding suggests that the impairment in glutamate
uptake probably results from a combination of slow progressive changes
in astrocyte cell physiology induced during BDV persistence. A
variety of nonlytic viruses have been shown to be capable of affecting
cell-differentiated functions (21). Therefore, it is
possible that BDV infection can directly interfere with the activity of
the glutamate transporters. The role of a soluble factor secreted by
BDV-infected cells in the inhibition of glutamate uptake was not
examined. Therefore, we cannot formally rule out the possibility that
production of cytokines, or other soluble factors, by the minor
fraction of BDV-infected cells that were GFAP negative could be
responsible for the effect on glutamate uptake by astrocytes. Thus, for
example both interleukin-1 (IL-1) and tumor necrosis factor alpha
(TNF-) have been shown to affect glutamate uptake by astrocytes
(14, 41, 56, 77). Interestingly the expression of these two
cytokines is upregulated in the CNS of PTI-NB rats (66).
Significant changes in temporal expression of IL-1 and TNF have been
reported in BDV/PTI-NB rats (60). This raises the
possibility that, also in vivo, glutamate uptake can be affected at
different levels at early and late stages of BDV infection. Arachidonic
acid and reactive oxygen intermediates, which can be produced by
astrocytes and microglia in response to infection, are also known to
suppress the astrocyte's ability to scavenge glutamate from the
environment (26, 70, 75, 76).
Cell growth and synthesis of macromolecules were not altered in BDV-infected compared to control mock-infected FeAst, indicating that BDV-mediated abrogation of glutamate uptake was not a consequence of a generalized cytotoxicity caused by BDV infection. Recent evidence indicates that glutamate and astrocytes are pivotal components of the coupling of synaptic activity with energy metabolism (38, 54). Glutamate transporters mediate glutamate-induced uptake of glucose in astrocytes. The electrochemical gradient of Na+ that drives the activity of these transporters also triggers the glycolytic processing of glucose, which results in astrocyte release of lactate, the preferred energy substrate of activated neurons (54). Therefore, an impaired astrocyte's ability to uptake glutamate not only can contribute to NMDA-mediated neurotoxicity, but also can compromise the supply of substrate for energy production in neurons. Whether glucose metabolism and lactate production are affected in BDV persistently infected FeAst remains to be determined. On the other hand, the impaired energy metabolism of astrocytes will significantly affect their ability to maintain low levels of extracellular glutamate (23). Glucose uptake was not altered in FeAst persistently infected with either BDV (this report) or FIV (30). These findings illustrate that a noncytolytic virus persistent infection can selectively target and disrupt specific components of interconnected cellular functions.
BDV has been recently implicated in "staggering disease" (SD), a neurological disorder affecting domestic cats in several parts of the world (49, 52, 59, 62). A high percentage (>40%) of cats with SD have been found to be BDV seropositive (49, 52, 59). Both viral antigen and RNA have been detected in brain tissue of diseased cats (51, 53). Moreover, SPF cats inoculated with BDV isolated from a cat with SD developed disease (50). These findings, together with the failure to detect other infectious agents in the CNS of SD cats, suggest a possible causative role of BDV in SD. BDV load in the CNS of SD cats is significantly lower than that observed in BDV infections of other species. More intriguingly, astrocytes, rather than neurons, appear to be the main virus target cell in the feline CNS (18). The mechanisms underlying neuronal damage observed in the brains of cats with SD are unknown, and whether altered astrocyte physiology is a contributing factor remains to be determined. Our findings with BDV-infected primary FeAst make plausible the hypothesis that altered glutamate uptake by astrocytes could contribute to neuronal damage associated with SD in cats.
Previous studies have shown that two lentiviruses, FIV and HIV, can establish a persistent nonlytic infection in astrocytes (7, 72, 78) and lead to a severe impairment, either directly or indirectly, in the glutamate uptake function of astrocytes (4a, 44, 45, 47, 78). The results presented here have shown that BDV, an NNS RNA virus, can also specifically abrogate glutamate uptake by astrocytes. Together, these findings suggest a possible common pathogenic mechanism for causing neuronal damage by viruses that cause a nonlytic persistent infection of astrocytes.
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ACKNOWLEDGMENTS |
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J.-N.B. and C.L. contributed equally to this work.
This work was supported by National Institute of Mental Health AIDS Center grant MH47680 (T.R.P.) and National Institutes of Health grants RR10712 (T.R.P.) and NS12428 (J.C.T.).
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FOOTNOTES |
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* Corresponding author. Mailing address: Imm-6, Division of Virology, Department of Neuropharmacology, The Scripps Research Institute, 10550 N. Torrey Pines Rd., La Jolla, CA 92037. Phone: (858) 784-6462. Fax: (858) 784-9981. E-mail: juanct{at}scripps.edu.
Publication 13322-NP from The Scripps Research Institute.
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Abstract
Introduction
Materials and Methods
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Discussion
References
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