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Journal of Virology, July 2000, p. 6433-6441, Vol. 74, No. 14
Experimental Neurobiology and Physiopathology
Unit, INSERM U433,1 and Hôpital
Neurologique,2 Lyon, France
Received 3 December 1999/Accepted 26 April 2000
Human T-cell lymphotropic virus type 1 (HTLV-1) is the causative
agent of a chronic progressive myelopathy called tropical spastic
paraparesis/HTLV-1-associated myelopathy (TSP/HAM). In this disease,
lesions of the central nervous system (CNS) are associated with
perivascular infiltration by lymphocytes. We and others have
hypothesized that these T lymphocytes infiltrating the CNS may play a
prominent role in TSP/HAM. Here, we show that transient contact of
human or rat astrocytes with T lymphocytes chronically infected by
HTLV-1 impairs some of the major functions of brain astrocytes. Uptake
of extracellular glutamate by astrocytes was significantly decreased
after transient contact with infected T cells, while the expression of
the glial transporters GLAST and GLT-1 was decreased. In
two-compartment cultures avoiding direct cell-to-cell contact, similar
results were obtained, suggesting possible involvement of soluble
factors, such as cytokines and the viral protein Tax-1. Recombinant
Tax-1 and tumor necrosis factor alpha (TNF- Human T-cell lymphotropic
virus type 1 (HTLV-1) (49) is the etiological agent of an
inflammatory demyelinating pathology of the central nervous system
(CNS) known as tropical spastic paraparesis/HTLV-1-associated
myelopathy (TSP/HAM) (18, 47). This neurological syndrome is
a chronic progressive encephalomyelopathy characterized by
corticospinal attack (9, 36). To date, the precise
mechanisms causing TSP/HAM remain largely undetermined. Nevertheless,
several studies have emphasized the prime role of the high number of
circulating HTLV-1-infected T lymphocytes (viral load) in the
appearance of TSP/HAM (46, 63). Such high viral load has
been considered a consequence of an inefficient immune response to
HTLV-1 (26). In TSP/HAM patients, marked infiltration of the
CNS by infected T cells is consistently observed (33, 59),
particularly in demyelinating lesions. These T cells harboring provirus
and expressing the viral protein Tax-1 (33, 42, 43) may
cause bystander effects damaging neural cells or affecting their
functions (25). Possible implication of direct infection of
neural cells is not well documented in TSP/HAM, as viral products can
hardly be detected in neural cells (34).
One important notion when considering the effects of the virus on the
CNS is that certain impairments occurring in actually infected cells
may be perpetuated via indirect effects of the virus on neural cells.
Such impairment may persist and propagate via the secretion of soluble
factors, such as cytokines, chemokines, or metalloproteinases (19,
20, 22, 57, 58, 60, 61), and eventually pervade the entire
neuraxis. In the case of TSP/HAM, this view is consistent with (i) the
presence, in the lesions, of cells expressing the viral product Tax-1
(43), which is known to transactivate many cellular genes
including several inflammatory molecules (8), (ii) the
expression of inflammatory cytokines in infiltrated T cells and
astrocytes (57, 65), and (iii) the expression pattern of
metalloproteinases and their inhibitors (20, 23, 60).
Our working hypothesis is that T lymphocytes persistently infected with
HTLV-1 may initiate functional perturbations in astrocytes by
expressing inflammatory molecules and viral proteins, in particular Tax-1. Previous studies in our laboratory have shown that astrocytes secrete inflammatory cytokines after transient contact with T cells
persistently infected with HTLV-1, whether or not they produce virus
(19). Such activated astrocytes may prolong and amplify the
deleterious effects produced by invading T cells, given the crucial
roles of astrocytes in brain homeostasis (production of energetic
metabolites for neurons and oligodendrocytes, neurotransmitter catabolism, and ionic homeostasis [24]). One of the
major roles of astrocytes is the control of the CNS excitability
(13) by regulating the extracellular concentration of
neurotransmitters, especially the major excitatory (glutamate) and
inhibitory ( We have previously shown that transient exposure of human or rat
astrocytes to cell lines of T lymphocytes chronically infected with
HTLV-1 induces GS expression in these astrocytes (1). This
altered catabolism of glutamate in astrocytes is mediated by the viral
transactivator Tax-1 and has suggested that the deleterious effects of
HTLV-1 infection may be caused by a compromised management of glutamate
by astrocytes. In this study, we investigated glutamate uptake by
astrocytes, since this step is crucial in the clearance of glutamate
from the extracellular space and, subsequently, in the provision of
metabolic precursors to neurons and oligodendrocytes. We show that
glutamate accumulation and expression of mRNAs encoding glial glutamate
transporters are significantly reduced in astrocyte culture after
transient contact with HTLV-1-infected T lymphocytes. These effects
result at least partly from paracrine effects of the viral protein
Tax-1 via tumor necrosis factor alpha (TNF- Unless otherwise noted, all reagents were obtained from Sigma
(L'Isle d'Abeau, France).
Cell cultures.
Primary cultures of astrocytes were obtained
by mechanical disaggregation of microdissected cortices from 1-day-old
rat pups or of sensory motor cortices from the human fetus (embryonic
day 116). The dissociated cells were diluted to a density of 2 × 105 cells/ml in Dulbecco's modified Eagle essential medium
(DMEM) Glutamax (Life Technologies, Cergy Pontoise, France) containing 25 mM glucose, supplemented with 20% heat-inactivated fetal calf serum
(FCS) and gentamicin (1 µg/ml). Cells were seeded in 35-mm-diameter culture dishes precoated with poly-L-lysine (3 µg/ml in
0.1 M borate buffer [pH 8.4]) as described by Yavin and Yavin
(66). Cultures were incubated at 37°C in a moist 5%
CO2-95% air atmosphere. The medium was changed 2 days
after plating (DMEM Glutamax, 25 mM glucose, 10% FCS) and every 3 days
thereafter until confluence. At that point, the FCS concentration was
progressively decreased to 2% over 1 week. Using this procedure, we
obtained 3-week-old cultures in which more than 95% of cells were of
astrocytic phenotype. This was systematically determined by detection
of glial fibrillary acidic protein (GFAP; a specific astrocytic marker)
using immunocytochemistry (data not shown).
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Human T-Cell Lymphotropic Virus Type 1-Infected T
Lymphocytes Impair Catabolism and Uptake of Glutamate by Astrocytes via
Tax-1 and Tumor Necrosis Factor Alpha
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) decreased glutamate
uptake by astrocytes. Tax-1 probably acts by inducing TNF-, as the
effect of Tax-1 was abolished by anti-TNF- antibody. The expression
of glutamate-catabolizing enzymes in astrocytes was increased for
glutamine synthetase and decreased for glutamate dehydrogenase, the
magnitudes of these effects being correlated with the level of Tax-1
transcripts. In conclusion, Tax-1 and cytokines produced by
HTLV-1-infected T cells impair the ability of astrocytes to manage the
steady-state level of glutamate, which in turn may affect neuronal and
oligodendrocytic functions and survival.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-aminobutyric acid) amino acids. Astrocytes scavenge
glutamate from the synaptic cleft and terminate its action via
high-affinity sodium-dependent glutamate transporters specific to glia.
These are the excitatory amino acid transporters 1 and 2 (EAAT1 and
EAAT2 in humans, the rat counterparts being GLAST and GLT-1,
respectively) (6, 29). Glutamate taken up by astrocytes is
converted to glutamine by glutamine synthetase (GS; EC 6.3.1.2), and
also passes into the astrocytic tricarboxylic (TCA) cycle
(39) by conversion into -ketoglutarate by glutamate
dehydrogenase (GDH; EC.1.4.1.3). If glutamate management is impaired
within astrocytes, this will compromise the functional integrity of the
CNS in general and that of neurons and oligodendrocytes in particular,
as these cells depend on metabolic precursors provided by astrocytes
(48) and are highly sensitive to excessive concentrations of
extracellular glutamate (7, 37, 54).
). Such bystander effects
of Tax-1-producing cells emphasize the importance of the interaction
between astrocytes and HTLV-1-infected T cells in the physiopathology
of TSP/HAM.
MATERIALS AND METHODS
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Abstract
Introduction
Materials and Methods
Results
Discussion
References
Transient coculture of astrocytes and T lymphocytes.
Transient contact of astrocytes (previously FCS deprived) with
HTLV-1-infected T lymphocytes was performed by replacing the medium in
the astrocyte culture with C91PL or C8166/45 cell suspensions (astrocyte/T-cell ratio, 10:1), which had been gamma irradiated (136 Gy) to prevent further proliferation. After 20 h, the T cells were
removed by several washes with fresh medium, and the astrocytes were
cultured for up to 30 days postcontact in DMEM Glutamax-25 mM
glucose-2% FCS, changed twice a week. Using rat astrocyte cultures, the complete elimination of T cells from astrocyte culture after transient contact (day 4) was verified by the absence of human glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and TNF- (by reverse transcription-PCR [RT-PCR]) and of CD4+ T
lymphocytes (by fluorescence-activated cell sorting). Transient contact
with the C91PL cell suspension led to astrocyte infection; the
proportions of infected cells were around 2% for primary rat astrocytes, 20% for human Dev cells, and 90% for human fetal primary astrocytes. To test the effect of soluble factors produced by chronically infected T cells, such as Tax-1 and cytokines, the C91PL
and C8166/45 T-cell lines were seeded in cell culture inserts (0.4-µm
pore size; Becton Dickinson, La Pont de Claix, France) and placed for
96 h over astrocyte cultures, thus avoiding effects due to
cell-cell contact. This procedure thus allows only soluble factors to
diffuse from the inserts. The use of virus-producing T cells (C91PL) in
the inserts never led to infection of astrocytes (no p24 and Tax-1 as
assessed by immunofluorescence).
Glutamate uptake. The uptake protocol was adapted from that used by Drejer and coworkers (12). The assay buffer was prepared from phenol-free DMEM containing 5 mM glucose, but without glutamate and glutamine (Life Technologies). L-[3H]glutamate (L-3,4-[3H]glutamic acid; 22,000 Ci/mol; NEN, DuPont) was added to the assay buffer (1 µCi/well, i.e., 46 nmol), and the final glutamate concentrations were obtained with unlabeled L-glutamate. The preassay buffer was prepared similarly but without [3H]glutamate. The assay and preassay buffers were prewarmed in a cell incubator (37°C, atmosphere with 5% CO2 and 95% air).
The astrocyte cultures were rinsed with 1 ml of the phenol-free DMEM without glutamate and glutamine and then preincubated at least for 30 min in a cell culture incubator. Uptake assays were performed at 37°C in a water bath in two steps of 5-min incubation (1 ml/well), first with preassay buffer then with assay buffer containing [3H]glutamate. Within these 10 min, the kinetics of glutamate uptake is linear, as reported by others (30). The uptake medium was rapidly removed, cell plates were kept on ice, and the wells were rinsed with 2 ml of ice-cold preassay buffer containing excess (1 mM) glutamate to avoid reverse transport. The cells were immediately lysed with radioimmunoprecipitation assay buffer (150 mM NaCl, 1% Triton X-100, 0.1% sodium dodecyl sulfate, 10 mM Tris-HCl [pH 7.2], 1 mM EDTA, 1% sodium deoxycholate, 1% aprotinin; 500 µl/well) and 100-µl aliquots were analyzed for incorporated radioactivity by scintillation spectrometry (2 ml of UltimaGold; Packard, Groningen, The Netherlands) at an efficiency of about 60% (Packard Tri-Carb TR1600 LS analyzer). Glutamate uptake was expressed with respect to the DNA rather than protein content, as preliminary data showed that infection by HTLV-1 resulted in a significant increase in protein levels compared to control cells (13% ± 0.11%, mean ± standard error of the mean [SEM], n = 48, P < 0.01). As there was no cell loss, we examined the DNA amount which is related to the number of cells. The amount of DNA per culture well was not altered (35.8 ± 0.3 versus 37.4 ± 0.3 µg, mean ± SEM, n = 48, corresponding to 4.5% ± 0.8% increase; quantification using the DNA-binding fluorochrome Hoechst 33258). Briefly, 10-µl aliquots of the cell suspension were added to the Hoechst 33258 assay solution (100 mM Tris base, 2 M NaCl, 10 mM EDTA, 0.1 µg of H33258/ml [pH 7.4]) in 96-well black microplates (Black Cliniplate; Labsystems). The fluorescence was read using a Titertek Fluoroskan II fluorometer (360-nm excitation and 460-nm emission), and the DNA amount was expressed in nanograms per milliliter (DNA standard curve established with fish sperm DNA [Boehringer]). We checked the correlation between DNA contents and cell numbers using cell suspensions of various densities. Glutamate concentrations ranging from 1 to 500 µM were used to determine the Km and Vmax for glutamate uptake using a hyperbolic model (Origin 5.0; Microcal, Northampton, Mass.). The specificity of glutamate transport was assessed using 1 mM competitive inhibitor, DL-threo-hydroxyaspartic acid (
-THA), an
excitatory amino acid analogue known to have a high apparent affinity
for all glial transporters (15). Nonspecific glutamate
transport was evaluated at 4°C, conditions under which active
transport of glutamate is abolished.
Effect of Tax-1 and TNF- on glutamate transport.
The
plasmids containing one sequence encoding Tax-1-glutathione
S-transferase (GST) or GST alone (courtesy of P. Jalinot, Lyon, France) were used to synthesize the corresponding proteins (5). The specific binding of GST with glutathione is used to purify subsequently Tax-1-GST or GST. Recombinant Tax-1-GST was diluted in fresh medium (DMEM Glutamax, 5 mM glucose, 2% FCS) for
treatment; an equal volume of sterile water was added to the same
medium as a control. Treatments with the protein GST alone served as
another control ensuring the specificity of the effect of the
recombinant Tax-1-GST protein. Rat recombinant TNF- (Diaclone Research) was used under the same conditions. Cotreatments, with or
without specific antibodies, were made under the same conditions. In
treated astrocyte cultures, supernatants were collected at different
days posttreatment and assayed for TNF- using human- or rat-specific
kits (CytoScreen ultrasensitive enzyme-linked immunosorbent assay kit;
BioSource International, Camarillo, Calif.). In Tax-1-treated cultures,
the samples were collected at 24 h posttreatment.
DNA-RNA purification and RT-PCR analysis. Total RNAs from astrocyte cultures (control or treated, at different days posttreatment) were prepared by solubilization and extraction with RNAzol (Bioprobe, Montreuil/Bois, France) using a protocol adapted from that of Chomczynski and Sacchi (10). The concentration and purity of the extracted RNA were determined spectrophotometrically (Beckman DU-640 instrument). RNA integrity was checked by electrophoresis on denaturating agarose gels, subsequently stained by ethidium bromide.
The primers were designed using the Wisconsin Package version 9.1 (Genetics Computer Group, Madison, Wis.) supporting SRS (Sequence Retrieval System) Indexes version 4.08 (EBI, Hinxton, United Kingdom). The specificity of the primers and internal probes was verified using the GenBank database (European Molecular Biology Laboratory, Heidelberg, Germany). Computer services were available at GIS INFOBIOGEN servers (MESR/AFM, Villejuif, France). The primers designed by Kinoshita and coworkers were used for Tax-1 amplification (31). Table 1 summarizes the selected PCR primers and specific internal probes for GS, GDH, GLAST, GLT-1, TNF-, GFAP, cyclophilin A (CyP-A), and Tax-1.
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.
The PCR products were quantified by Southern blotting (separation by
1.8% agarose gel electrophoresis and electroblotting on positively charged nylon membranes; ICN) and hybridization with specific [-32P]ATP-5'-end-labeled internal oligonucleotide
probes (Table 1). After exposure to an NEN-Reflection autoradiographic
film, the specific labeled bands were cut out and counted on a liquid
scintillation analyzer. Slot blot (Bio-Rad) analysis confirmed the
reliability of our Southern blot procedure. Tax-1 mRNA was detected
using the same RT-PCR procedure (35 cycles). Genomic DNA contamination was assessed by the same PCR procedure but without RT. In rat astrocyte
cultures, the absence of residual C91PL T lymphocytes was checked by
PCR using human-specific GAPDH primers (day 4 postcontact). RT-PCR on
HTLV-1-infected human cells were run on DNase-treated total RNA as
previously described (1). For correlation analyses between
transcripts encoding Tax-1, GS, and GDH, the samples were amplified in
one PCR session, and the amounts of mRNAs were evaluated using the same
three radiolabeled probes for all experiments.
Immunocytochemistry and TNF- assays.
HTLV-1-specific
proteins were detected by indirect immunofluorescence using a
polyclonal rabbit antiserum raised against the viral transactivator
Tax-1 (NIH 467). Human and rat astrocytes were cultured in Labtek
chambers (Nalge Nunc, Naperville, Ill.) and then fixed with acetone (10 min at 
20°C) on various days postcontact. The primary antibody
incubation was in phosphate-buffered saline for 45 min at 37°C.
Fluorescein isothiocyanate-labeled anti-rabbit immunoglobulin
antibodies (Biosys) were used as second antibodies (30 min at room
temperature). TNF- was assayed in the collected culture supernatants
(stored at 20°C) using EIA kits specific for rat TNF-
(CytoScreen ultrasensitive, 0.7 pg/ml; BioSource International) or
human TNF- (CytoScreen).
Data analysis. Results are expressed as the mean ± SEM. Student's t test was used to compare the results obtained by treated versus naive cultures.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Experimental design.
The effects on astrocyte cultures of
transient coculture with HTLV-1-infected T cells were investigated
using persistently infected producer (C91PL) or nonproducer (C8166/45)
T-cell lines. In most of the study, rat astrocytes were used because of
the difficulty of obtaining normal human material; nevertheless, the relevance of the data obtained in rat cells was confirmed using a human
cell line, Dev, exhibiting the astrocytic phenotype and human primary
astrocytes obtained from fetal cortex (one experiment). Infected T
cells and astrocytes were cocultured for 20 h. These T cells were
carefully eliminated, as verified by the absence of human-specific
GAPDH and TNF- by RT-PCR and of CD4+ T cells by
fluorescence-activated cell sorting. No cell loss occurred in the
cultures tested, as shown by cell counting and quantitation of protein
or DNA. At various intervals postcontact, we studied glutamate uptake
and expression of mRNAs encoding glutamate transporters (GLT-1 and
GLAST), GS, and GDH. The influence of soluble factors was evaluated
using two-compartment culture in which infected T cells were placed in
inserts, thereby avoiding cell-to-cell contact. To identify the
signaling molecules mediating the observed effects, astrocyte cultures
were treated by recombinant Tax-1 and TNF-, with or without their
specific antibodies.
Glutamate transport after transient contact with HTLV-1-infected T
cells.
Glutamate uptake was estimated by the concentration of
radiolabeled glutamate accumulating within astrocytes, once transported from culture medium. We first determined the optimal conditions for
glutamate uptake in naive astrocyte cultures obtained from rat cortex
(n = 4). The uptake velocity was linear for at least 20 min for extracellular glutamate concentrations of 100 to 200 µM. The
glutamate concentration in the culture medium under investigation can
be considered constant, as less than 3% of radiolabeled glutamate was
cleared from the extracellular space. Thereafter, we determined the
kinetic properties of tritiated L-glutamate uptake with
respect to the extracellular concentration of glutamate at 10 min by
measuring the rate of radiolabeled glutamate accumulation in
astrocytes. Curve fitting and subsequent statistical analyses showed
that glutamate transport was compatible with a hyperbolic model
characterized by a Km of 72 ± 16 µM and
a Vmax of 121 ± 12 nmol of
glutamate/min/ng of DNA (mean ± SEM, n = 3, P < 0.05) (Fig. 1A). Hill plot analysis using linear regression gave Hill coefficients of 0.9 to 1, which is
consistent with a single-site transport system. The specificity of
glutamate transport was verified by evaluating (i) the passive diffusion of glutamate (accumulation at 4°C) into the cellular compartment (1.8% ± 0.1% of the mean value obtained at 37°C,
n = 3, extracellular glutamate concentration of 100 µM) and (ii) the degree of inhibition of glutamate transport by the
competitive inhibitor, -THA (1 mM at 37°C; 97.1% ± 0.1%
inhibition, n = 6, P < 0.005). These results are
in agreement with those published for cultured astrocytes obtained from
rat cortices (see review by Robinson and Dowd [51]).
Thereafter, glutamate uptake was measured with extracellular
concentration of 100 µM glutamate unless otherwise specified. In
addition, in situ autoradiography of tritiated D-aspartate
uptake indicated that all cultured astrocytes had the capacity to
uptake glutamate (not shown). We also determined the affinity and
maximal velocity of glutamate uptake in human Dev cell cultures
containing around 20% of cells of astrocytic phenotype
(Km = 14.6 ± 2.7 µM and
Vmax = 5.1 ± 0.2 nmol
glutamate/min/ng of DNA; n = 3).
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Involvement of soluble factors released by HTLV-1-infected T lymphocytes. As HTLV-1-infected T lymphocytes are known to continuously express the viral protein Tax-1 and cytokines (35, 56), we examined the paracrine effect of soluble factors released by HTLV-1-infected T cells. Primary astrocyte cultures established from rat or human fetal cortex were cocultivated in two separate compartments with the C8166/45 T-cell line. We have previously verified the high level of Tax-1 expression by immunocytochemistry and RT-PCR in this cell line. These T lymphocytes were seeded in inserts and placed over the astrocyte monolayer for 96 h without direct T-cell astrocyte contact. Such transient exposure decreased glutamate uptake by 37.4% ± 2.3% (n = 3, P < 0.05) in rat astrocyte cultures (Fig. 1B). The relevance of this result obtained in rat was verified in human astrocyte cultures with insert containing C91PL T lymphocytes: glutamate uptake was decreased by 44.1% ± 2.0% (n = 3, P < 0.001) (Fig. 1B). These data indicate that HTLV-1-infected T lymphocytes, whether or not they produce virus, are able to alter glutamate uptake in astrocytes via soluble factors.
The possible implication of Tax-1 was assessed using hybridoma B cells secreting antibodies against Tax-1. In these experiments, human Dev cells were directly exposed to HTLV-1-infected T cells (C91PL), while hybridoma cells were seeded in culture inserts (106 cells) above the Dev cell monolayer. As shown in Fig. 2A, coculture with anti-Tax-1 hybridoma completely reversed the effect of infected T cells on glutamate uptake in Dev cells. Note that glutamate uptake in human Dev cells was more dramatically decreased for extracellular concentrations of glutamate smaller than 100 µM.
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Tax-1 protein decreases glutamate uptake by astrocytes via
TNF-.
The potent transactivator protein Tax-1 may be one of the
soluble factors (3, 5, 11) responsible for the effect of HTLV-1-infected T lymphocytes on glutamate uptake by astrocytes. To
determine the effect of extracellular Tax-1 on glutamate transport, rat
astrocytes were treated with the recombinant protein Tax-1-GST (5). The control was the immediate rinsing with the medium containing recombinant Tax-1 (25 nM, i.e., 1.5 µg of Tax-1-GST/ml, 0-h treatment), which showed no difference in glutamate uptake compared
to naive astrocytes (96% ± 7% of control value, n = 3) (Fig. 2B). Glutamate uptake was decreased by treatment with 25 and 50 nM Tax-1 (2, 4, 8, 16, and 24 h) but not with the protein GST alone (113% ± 7% of control value, n = 4). The
maximal reduction (63% ± 4% of control value, n = 9, P < 0.01) (Fig. 2B) in glutamate transport was obtained
after 4 h of treatment with 50 nM Tax-1 (3 µg of Tax-1-GST/ml).
The specificity of this effect was confirmed using anti-Tax-1
antibodies (NIH 467, diluted 1/100), which completely neutralized the
effect of Tax-1 protein (106% ± 6% of control value, n = 3) (Fig. 2B) at its optimal concentration (Tax-1-GST at 3 µg/ml, 4 h). The specificity of the blockade by anti-Tax-1 antibody was checked using irrelevant antibodies (63% ± 6% of control value, n = 3, P < 0.01).
secreted by astrocytes, as Tax-1 has been shown to induce cultured
astrocytes to secrete inflammatory cytokines, including TNF-
(11, 40). Treatment of rat astrocytes with 50 nM Tax-1 (3 µg of Tax-1-GST/ml, 4 h) induced a secretion of TNF- in
these astrocytes (2.6 ± 0.2 pg/ml, n = 3),
whereas TNF- was not secreted with the protein GST alone
(n = 6). Treatment (for 4 h) of rat astrocytes
with exogenous rat recombinant TNF- (10 ng/ml; Diaclone Research)
reduced glutamate uptake by 35% ± 5% (n = 3, P < 0.01; range, 20 to 55%) (Fig. 2B). The specificity of the effect
was shown using anti-TNF- antibodies, which prevented the decrease (101% ± 8% of control value, n = 3). Finally, Tax-1
seems to decrease glutamate uptake in astrocytes via TNF-, as
anti-TNF- antibodies virtually suppressed (103% ± 5% of control
value, n = 3) the effect of Tax-1 on glutamate
transport (Tax-1-GST [3 µg/ml] and anti-TNF- antibody
[1/100], 4 h) (Fig. 2B).
The metabolic fate of glutamate taken up by astrocytes largely depends
on the catabolic enzymes, GS and GDH (see the introduction). Therefore,
the effect of HTLV-1-infected T cells (C91PL) on the expression of GS
and GDH was investigated by RT-PCR in rat astrocytes transiently
exposed to HTLV-1-infected T cells at a period when glutamate uptake
was reduced (n = 3). GS and GDH mRNAs were upregulated and downregulated, respectively (Table
2). The magnitudes of these opposite
changes were inversely correlated. These changes were also correlated
with the level of Tax-1 transcripts expressed by cultured cells (note
that 2 to 5% of astrocytes were expressing Tax-1 immunoreactivity, as
shown below).
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Prolonged expression of Tax-1 and TNF-.
As we observed a
long-term decrease in glutamate uptake induced by infected T cells
(79.4% ± 4.1% of control value, n = 4, day 22, P < 0.05), we examined the expression of Tax-1 and
TNF- in primary astrocytes and the Dev cell line over the month
following contact with the T-cell line C91PL. mRNA encoding Tax-1 (Fig. 3A) and Tax-1 protein were detected as
early as 2 days postcontact and were persistently expressed throughout
the period of observation, but without production of viral particles
(55a). We found that 2 to 5% of rat astrocytes and about
20% of human Dev cells showed Tax-1 immunoreactivity during long-term
cultures. Such persistent expression of Tax-1 was closely associated
with a sustained secretion of the proinflammatory cytokine TNF-.
Within the first week following transient contact with the
HTLV-1-infected T-cell line C91PL, TNF- (Fig. 3B) was secreted in
the culture supernatants from the human Dev cell line (460 pg/ml) and
human primary astrocytes (628 pg/ml), and TNF- mRNA was detected in
Dev cells until 30 days postcontact (Fig. 3A). In rat primary
astrocytes, TNF- secretion was observed within the first week
postcontact (71 pg/ml), and TNF- transcripts were detected at least
until 22 days postcontact. Stimulation of rat astrocyte cultures by
HTLV-1-infected T lymphocytes also expressing Tax-1 (C8166/45, placed
for 96 h in cell culture inserts over the astrocyte monolayer)
induced sustained secretion of TNF- by astrocytes at least for 3 weeks postcontact (8 pg/ml) (Fig. 3B). Control cultures of rat and
human astrocytes with noninfected CD4+ T lymphocytes (CEM
cell line) did not result in TNF- secretion. These data indicate
that TNF- secretion is associated with the presence of
Tax-1-expressing cells, regardless of their lymphocytic or astrocytic
phenotype.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Examination of TSP/HAM patients has consistently revealed invasion of the CNS by T cells harboring provirus and expressing the viral protein Tax-1 (42, 43). These data have led to a consensus on the importance of CNS infiltration by HTLV-1-infected T cells in the physiopathology of TSP/HAM, although many subsequent events remain unaddressed. In this study, we used transient coculture of astrocytes with HTLV-1-infected T lymphocytes to mimic CNS invasion by infected T lymphocytes and examined the functional consequence on astrocytes. Indeed, an effective operation of astrocytes is critical in brain homeostasis and neural cell survival. These glial cells are essential managers of a variety of metabolic pathways involved in energy storage, ionic equilibrium, and the control of extracellular concentrations of various neurotransmitters. In particular, the main excitatory amino acid glutamate is specifically taken up and then catabolized by astrocytes. Our data show that glutamate management is significantly impaired in astrocytes following transient contact with infected T cells, whether or not they produce virus. Such astrocyte impairments triggered by HTLV-1 may have deleterious effects on neighboring cells by affecting their electrical activity and energy metabolism (55). In human astrocytes, the effects were even greater than in rat cells, confirming the clinical relevance of our model.
Activation of astrocytes by infected T lymphocytes.
Transient
contact of cultured astrocytes with infected T cells did not affect the
amount of DNA or the number of cells. There was even an increase in the
expression of astrocyte-specific proteins, such as GFAP and GS,
indicating that the presence of HTLV-1-infected T cells did not promote
a general shutoff, but rather induced factors targeting specific
astrocytic functions. Marked activation of astrocytes was observed
after transient contact with HTLV-1-infected T lymphocytes
(19). This activation was characterized by the sustained
expression of the proinflammatory cytokine TNF- and upregulation of
the gliofilament protein GFAP. These changes in astrocytes produced by
infected T lymphocytes are typical of astrocytes engaging a variety of
regulatory processes in response to several types of insults
(4).
Glutamate uptake by astrocytes. Glutamate uptake by astrocytes is crucial in the regulation of its extracellular concentration and intracellular metabolism (glutamine synthesis, ammonia detoxification, and energy/cell respiration). Glutamate accumulation was consistently reduced in astrocyte cultures treated with HTLV-1-infected T lymphocytes. This decrease was due to a change in the net transport activity rather than to an accelerated turnover of glutamate catabolism (e.g., by increased GS activity), as a similar decrease was observed using tritiated D-aspartate, which is not metabolized by GS and GDH.
Glutamate is mainly transported into astrocytes via two high-affinity, sodium-dependent transporters (6, 28), GLAST/EAAT1 and GLT-1/EAAT2. Analysis of the expression of their messengers shows a significant decrease in both, occurring as early as 3 days after contact with HTLV-1-producing T lymphocytes. The decreased glutamate transport probably results from the downregulation of genomic expression of glial glutamate transporters, as glutamate uptake was found to correlate with the expression of the transporters' messengers (16, 52). At a more functional level, such decreased glutamate uptake by astrocytes should increase the extracellular level of glutamate, which in turn may perturb neuronal transmission (e.g., a decreased signal-to-noise ratio or temporal detuning) or even exert an excitotoxic effect. Another retrovirus, feline immunodeficiency virus, has also been shown to decrease glutamate uptake in cultured astrocytes. In this model, the effect was interpreted as a result of direct infection of astrocytes (67), whereas with HTLV-1, the decreased glutamate uptake was observed even after contact with a noninfectious HTLV-1-infected T-cell line.Implication of soluble factors.
The possible involvement of
soluble factors in the effects of HTLV-1-infected T cells was verified
using transient cocultures with astrocytes and HTLV-1-infected T
lymphocytes in two distinct compartments, which resulted in a reduction
of glutamate uptake similar to that observed with single compartment
coculture (direct cell-to-cell contact). This raised the possibility
that infected T lymphocytes may impair glutamate uptake and catabolism
by bystander effects via soluble factors, such as the viral protein
Tax-1 and cytokines. In our model, we clearly showed that human as well as rat astrocytes secrete TNF- after transient contact with
infectious or noninfectious HTLV-1-infected T-cell lines (C91PL or
C8166/45), both expressing Tax-1. The addition of recombinant Tax-1
protein to the culture medium was also able to induce TNF-
secretion. Involvement of Tax-1 and TNF- in the effects of HTLV-1
infection on glutamate uptake was further substantiated by the
decreased glutamate uptake after application of recombinant Tax-1 or
TNF-. Coincubation with both Tax-1 and anti-TNF- antibody
abolished the effect of Tax-1 on glutamate transport, providing
evidence that TNF- acts as the mediator of the Tax-1-induced
decrease in glutamate uptake. These findings are in agreement with the induction of TNF- expression by Tax-1 (11) and the
decreased glutamate uptake induced by TNF- in astrocytes
(14). Thus, we can assume that the signaling cascade leading
to the decreased uptake of glutamate in astrocytes successively
involves two paracrine mediators, Tax-1 and TNF-.
in the physiopathology of TSP/HAM is also
suggested by the presence of this cytokine in astrocytes and T
lymphocytes within CNS lesions of TSP/HAM patients (57). The
molecular events downstream of TNF- are not precisely known for its
effects on glutamate uptake. But TNF- may affect other molecular or
cellular processes, such as migration and activation of lymphocytes, be
toxic for oligodendrocytes, and alter the expression of other cytokines
(2, 45). The present work underscores the importance of
examining nonclassical effects of TNF- (17), other than
its well-documented ability to enhance inflammatory processes.
Glutamate catabolism and energy metabolism.
Effective
inactivation of glutamate uptaken by astrocytes is achieved by the
glial enzymes GS and GDH. Therefore, the functional outcome of the
decreased glutamate accumulation induced by HTLV-1-infected T
lymphocytes must be considered by taking into account the ability of
astrocytes to metabolize glutamate via GS and GDH. In this regard, we
show that transient contact with HTLV-1-infected T cells expressing
Tax-1 (C91PL and C8166/45) led to imbalanced expression of
glutamate-glutamine cycle enzymes in rat (this study) and human
(1) astrocytes (increase for GS and decrease for GDH). We
have previously shown that Tax-1 protein transactivates the GS gene
promoter (1). In the present study, we further show that the
magnitude of these opposite changes correlates with the level of viral
Tax-1 mRNA, demonstrating the critical role of Tax-1-expressing T
lymphocytes and astrocytes in the effects observed. The Tax-1-induced
imbalance between GS and GDH is expected to preferentially drive
glutamate catabolism toward the formation of glutamine, rather than
toward the TCA cycle. Decreased GDH expression may result in
insufficient energetic stores in astrocytes, as the mitochondrial
enzyme GDH primarily catabolizes the metabolic pool of glutamate to
generate -ketoglutarate, which passes into the TCA cycle
(48). Such effect on the energy store may be enhanced by the
decreased intracellular pool of glutamate following its impaired
uptake. Thus, astrocytes represent an important target for
HTLV-1-infected T lymphocytes infiltrating the CNS, possibly depleting
energy precursors for the surrounding cells, in particular neurons and
oligodendrocytes, which need to be continuously fed with essential
metabolites (lactate and -ketoglutarate) released by astrocytes
(24).
Functional significance. The present study demonstrates that HTLV-1-infected T cells impair the uptake and metabolism of glutamate by astrocytes. Although the in vivo significance of our results must be evaluated cautiously, these data suggest that Tax-1 initiates a divergent and high-gain transduction cascade which may pervade the entire CNS. Indeed, at each step of this cascade, the input signal can affect several targets which, in turn, can amplify the output signal. The magnitude of the resulting bystander effects is probably enhanced by factors secreted by infected T cells, but also by astrocytes (cytokines, chemokines, integrins, and metalloproteinases and their endogenous inhibitors). These factors probably affect the number of infected/activated T cells infiltrating the CNS and the extent of migration of these cells through the CNS parenchyma (61, 62, 64). Once in the CNS, Tax-expressing T lymphocytes may persist and expand within the CNS, as Tax is able to prevent T cells from undergoing apoptosis (44) that may be stimulated by neighboring astrocytes (32). In conclusion, our results demonstrate a great susceptibility of astrocytes vis-à-vis HTLV-1-infected T cells, which significantly alters the metabolism of an important excitatory amino acid, glutamate. Clinically, current knowledge on glutamate neurotransmission and metabolism suggests that astrocytic glutamate metabolism may be an effective therapeutic target in TSP/HAM.
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ACKNOWLEDGMENTS |
|---|
This work was financially supported by French research associations for multiple sclerosis (ARSEP and LFSEP), ANRS, Sidaction, and INSERM. R.S. was a recipient of fellowships from ARSEP and LFSEP.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: INSERM U433, Faculté de Médecine Laënnec, F69372 Lyon cedex 08, France. Phone: (33) 4 7877 8759. Fax: (33) 4 7877 8616. E-mail: giraudon{at}lyon151.inserm.fr.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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