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The Journal of Neuroscience, June 1, 2003, 23(11):4775-4784
Previous Article | Next Article
Morphine Withdrawal Increases Glutamate Uptake and Surface Expression of Glutamate Transporter GLT1 at Hippocampal Synapses
Nan-Jie Xu,1 Lan Bao,2 Hua-Ping Fan,1 Guo-Bin Bao,1 Lu Pu,1 Ying-Jin Lu,2 Chun-Fu Wu,3 Xu Zhang,2 andGang Pei1 1 Laboratory of Molecular Cell Biology, Institute of Biochemistry and Cell Biology, 2 Laboratory of Sensory System, Institute of Neuroscience, Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences, Shanghai 200031, China, and 3 Department of Pharmacology, Shenyang Pharmaceutical University, Shenyang 110015, China
Abstract
Top
Abstract
Introduction
Opiate abuse causes adaptive changes in several processes of synaptic transmission in which the glutamatergic system appears a critical element involved in opiate tolerance and dependence, but the underlying mechanisms remain unclear. In the present study, we found that glutamate uptake in hippocampal synaptosomes was significantly increased (by 70% in chronic morphine-treated rats) during the morphine withdrawal period, likely attributable to an increase in the number of functional glutamate transporters. Immunoblot analysis showed that expression of GLT1 (glutamate transporter subtype 1) was identified to be upregulated in synaptosomes but not in total tissues, suggesting a redistribution of glutamate transporter expression. Moreover, the increase in glutamate uptake was reproduced in cultured neurons during morphine withdrawal, and the increase of uptake in neurons could be blocked by dihydrokainate, a specific inhibitor of GLT1. Cell surface biotinylation and immunoblot analysis showed that morphine withdrawal produced an increase in GLT1 expression rather than EAAC1 (excitatory amino acids carrier 1), a neuronal subtype, at the cultured neuronal cell surface, whereas no significant change was observed in that of cultured astrocytes. Electron microscopy also revealed that GLT1 expression was markedly increased in the nerve terminals of hippocampus and associated with the plasma membrane in vivo. These results suggest that GLT1 in hippocampal neurons can be induced to translocate to the nerve terminals and express on the cell surface during morphine withdrawal. The translocation of GLT1 at synapses during morphine withdrawal provides a neuronal mechanism for modulation of excitatory neurotransmission during opiate abuse.
Key words: morphine; rat; hippocampus; glutamate transporter; GLT1; opiate withdrawal
Introduction
Opiate abuse causes long-lasting neural changes in the brain that underpin the behavioral abnormalities associated with cognitive deficits, tolerance, and dependence (Nestler and Aghajanian, 1997; Robbins and Everitt, 1999
Several findings show that glutamate uptake may be involved in memory formation from vertebrate to invertebrate (Ng et al., 1997
In the present study, we showed that glutamate uptake capacity in hippocampus synaptosomes was significantly increased during morphine withdrawal, and this was because of an upregulation of the number of glutamate transporters in the membrane. Furthermore, the increase in capacity was at least in part correlated to the translocation of neuron-expressed glutamate transporter GLT1 to nerve terminals and the induced surface expression of GLT1 at synapses. These results suggest that the glutamate transport mediated by neuronal glutamate transporter GLT1 may be inducible and significant in the altered excitatory neurotransmission during opiate abuse.
Materials and Methods
Preparations of rat brain tissue. Male Sprague Dawley rats (200–220 gm) were obtained from the Laboratory Animal Center, Chinese Academy of Sciences (Shanghai, China). Rats were housed in groups and maintained on a 12 hr light/dark cycle with food and water available ad libitum. All treatments were strictly in accordance with the National Institutes of Health Guide for the Care and Use of Laboratory Animals. Animals were treated with morphine (10 mg/kg, s.c., twice per day at 12 hr intervals) or saline for 10 d (Trujillo and Akil, 19910.5 mg/ml that was determined by Bradford methods (Bradford, 1976
Primary cell culture. Primary hippocampal cultures were prepared from 1 d postnatal Sprague Dawley rats using methods similar to those described previously (Mennerick et al., 1998
Glutamate uptake assay. Glutamate uptake of synaptosomes was initiated by adding 3H-glutamate (10 nM, 45.0 Ci/mmol; Amersham Biosciences, Buckinghamshire, UK) and 30 µM unlabeled glutamate in a final volume of 500 µl of KRH medium (Ullensvang et al., 1997
Biotinylation. Biotinylation of cell surface proteins was performed as described previously (Davis et al., 1998
Western blot analysis. The samples (0.5 mg/ml, 20 µl) from brain tissue or cultured cells of control and chronic morphine-treated groups were loaded, then subjected to 10% SDS-PAGE, and electroblotted onto nitrocellulose membrane using a minigel and mini transblot apparatus (Bio-Rad, Hercules, CA). The membranes were blocked in blocking buffer (20 mM Tris-HCl, pH 7.5, 137 mM NaCl, 0.1% Tween 20, and 15% nonfat milk) at room temperature for 1 hr. Then the membranes were incubated with antibodies of goat anti-GLAST (1.3 µg/ml; C-19 amino acids; Santa Cruz Biotechnology, Santa Cruz, CA) or goat anti-GLT1 (0.4 µg/ml; N-19 amino acids; Santa Cruz Biotechnology), or rabbit anti-EAAC1 (1:1000; provided by Dr. Jian Fei, Institute of Biochemistry and Cell Biology, Shanghai, China) or actin (1:10,000; Santa Cruz Biotechnology), respectively, overnight at 4°C. The blots were washed and incubated with horseradish peroxidase-conjugated anti-rabbit or anti-goat secondary antibody for 1 hr at room temperature (Sigma, St. Louis, MO). Finally, the blots were visualized with enhanced chemiluminescence (Amersham Biosciences). For the quantification of the Western blot data, the developed films were scanned, the immunoreactive bands were digitized, and the densitometry was performed using Scion Image for Windows (Scion, Frederick, MD). The signal for each lane was calculated by summing the area x intensity of immunoreactivity (gray level of immunoreactive band–background level) of the discrete monomer and multimer bands produced by GLT1 and EAAC1 and normalized with internal control bands (actin).
In situ hybridization. The oligonucleotide probes for GLT1, 5'-CAG CCC GCC ACA TAC TGC TCC CAG GAT GAC ACC AAA CA-3', were synthesized by Invitrogen on the basis of the rat GLT1 (GenBank accession number U15098 [GenBank] ). In situ hybridization was performed according to a previous method (Zhang et al., 1994b). The oligonucleotide was labeled at the 3' end with [
- 35S]dATP (NEN, Boston, MA) using terminal transferase enzyme (Amersham Biosciences). Six rats per group were deeply anesthetized with sodium pentobarbital (60 mg/kg, i.p.) and killed. The brains were removed, and the sections (14 µm) of hippocampus were cut in a cryostat. Slide-mounted sections were hybridized overnight at 42°C in a probe concentration of 40 ng/µl in hybridization buffer containing 40% deionized formamide, 3x SSC, 10% dextran sulfate, 5x Denhardt's solution, and 75–100 µg/ml salmon sperm DNA. Then the sections were washed in 1x SSC at 55°C for 30 min. After the washes, the sections were dehydrated and placed in a phosphate screen for 4–5 d, dipped in Hypercoat LM-1 emulsions (Amersham Biosciences), and exposed for periods of 3–5 weeks. After development in Kodak D19, the sections were counterstained with 1% toluidine blue, dehydrated and coverslipped, and photographed under bright-field illumination.
For quantitative analysis of the data, at least three rats were used in each group. GLT1 mRNA-positive neurons were identified as the cells (20–30 µm in diameter) that contained the number of silver grains threefold greater than the background in the pyramidal cell layer of CA1 and CA3 or granule cell layer of dentate gyrus (DG) region in bright-field micrographs. The GLT1 mRNA expression levels in neurons were determined by both the hybridization signals in the neurons and the percentage of positive neurons. A total of
Immunohistochemistry. The brains of rats were prepared for electron microscopy as described previously (Zhang et al., 1995
To determine the percentage of the GLT1-positive nerve terminals in the regions, the data from sections with the identical area of CA1, CA3, and DG in each group were selected, and immunolabeled nerve terminals that form synapses were counted in three sections from different rats in each group. For gold–silver particle quantification, the numbers of gold–silver particles in the nerve terminals and the membrane-associated gold–silver particles per synapse were calculated, respectively. Gold–silver particle associated with membrane was defined as actual contact with the plasma membrane; gold–silver particle in close proximity to the plasma membrane was considered to be intracellular. Synapses without gold–silver grains were eliminated.
Statistical analysis. The results were presented as mean ± SEM. Statistics differences were determined by Student's t test for two-group comparisons or ANOVA followed by Duncan's multiple range test for multiple comparisons among more than two groups.
Results
Increase in glutamate uptake in hippocampus during morphine withdrawal
To test the potential changes in the glutamate uptake machinery during opiate abuse, rats were injected with morphine (10 mg/kg, s.c.) twice per day for 10 d, a procedure known to produce significant morphine tolerance and dependence (Trujillo and Akil, 1991
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Figure 1. Increase of glutamate uptake in hippocampal synaptosomes during withdrawal in chronicmorphine-treatedrats. The results were presented as mean±SEM of four to six rats per group, each tested by triplicate reconstitutions. *p < 0.05 and **p < 0.01 compared with the saline group. A, B, Effect of chronic morphine treatment (Mor) and saline treatment (Sal) on different brain regions. After subcutaneous injection of morphine (10 mg/kg) twice per day at 12 hr intervals for 10 d, the glutamate uptake in the synaptosomal particles of hippocampus (Hip) was increased significantly, whereas that of other regions such as prefrontal cortex (PC), cerebellum (Cer), and brainstem (BS) were decreased. C, Glutamate uptake in synaptosomal particles of hippocampus was increased time dependently after 1,5,10 dmorphine exposure.D, The glutamate uptake was increased to the highest level 12 hr after the termination of morphine treatment and then decreased gradually 24, 36, and 48 hr later. E, Reexposure of the animals to morphine (10 mg/kg) at the 12 hr time point restored the increased glutamate uptake to the normal level 1 hr later, and the increase was initiated again by additional treatment of naloxone (Nal) (1 mg/kg).
To distinguish between increases in affinity and the number of functional transporters, Km and Vmax were determined. Morphine withdrawal increased the Vmax from 332 ± 17.8 to 586 ± 62.3 pmol · mg-1 · min-1 but did not induce any significant changes in Km values, which were 20.8 ± 3.21 and 22.4 ± 6.36 µM for the control and morphine-treated groups, respectively (Fig. 2A). This indicated that the change in glutamate uptake was likely attributable to the increased number of functional transporters.
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Figure 2. Saturation analysis for glutamate uptake during morphine withdrawal by incubating the synaptosomal fractions in different glutamate concentrations. A, Glutamate uptake capacity was increased in synaptosomes during morphine withdrawal. The experiment was replicated for three times, and data were presented as mean±SEM of replicate samples in total (n = 6). B, Data as shown in Eadie-Hofstee transformations indicate an increase in Vmax of glutamate uptake. Sal, Saline treatment; Mor, morphine treatment.
Differential regulation of the expression of glutamate transporter subtypes in hippocampus
To further pinpoint the subtype of glutamate transporters, antibodies of anti-GLAST, anti-GLT1 (N terminal), and anti-EAAC1 were used to detect the amount of protein expressed in hippocampus. As shown in Figure 3A, the antibodies of anti-GLAST and anti-GLT1 each produced bands at
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Figure 3. Immunoblot characterization of glutamate transporters antibodies. A, Protein samples from the hippocampus of adult rat were analyzed by immunoblot analysis using anti-GLAST (left) and anti-GLT1 (right), respectively. Both of the antibodies recognized bands at
Then we examined the changes of the protein level of glutamate transporter subtypes in the hippocampal synaptosomes 12 hr after cessation of morphine. Among three subtypes, the amount of expressed GLT1 was significantly increased in synaptosomal particles in the morphine group compared with that of the saline group, whereas no significant change in GLAST or EAAC1 was observed under the same conditions (Fig. 4). Moreover, no change of GLT1 expression was seen in total lysates of tissue sample during morphine withdrawal, suggesting that the increase of GLT1 expression in synaptosomes might not be attributable to an upregulation of GLT1 in total content.
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Figure 4. Differential regulation of glutamate transporter subtypes in hippocampus after morphine withdrawal. A, During morphine withdrawal, the synaptosomal protein levels of GLT1 (n = 6) were significantly increased in hippocampus compared with the saline control group rather than that of GLAST (n = 5) and EAAC1 (n = 5). The monomer bands at
Upregulation of glutamate uptake and surface expression of GLT1 in cultured neurons
Two isoforms of GLT1, GLT1a and GLT1b, varying in the C terminus are identified in brain so far (Chen et al., 2002As shown in Figure 5, an increase of glutamate uptake was observed in the neurons 1 hr after morphine withdrawal, and this increase was dose dependent and time dependent on chronic morphine treatment (Fig. 5A,B). We also tested the changes in glutamate uptake in cultured neurons 0–2 hr after morphine (10 nM) washout, and the glutamate uptake in the 1 hr time point was the highest (data not shown). In the astrocytes, however, no significant change could be observed in the morphine-treated group (Fig. 5A,B). The glutamate uptake in the astrocytes could be blocked by L-trans-pyrrolidine-2, 4-dicarboxyic acid (PDC) (Tocris Cookson, Bristol, UK), a nonselective glutamate transporter blocker, but not by dihydrokainate (DHK) (Tocris Cookson), a specific inhibitor of GLT1 (Fig. 5C). This is consistent with previous studies that glutamate uptake in astrocytes is primarily mediated by GLAST subtype (Swanson et al., 1997
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Figure 5. Effect of morphine withdrawal on glutamate uptake in chronic morphine-treated hippocampal neurons and astrocytes. A, B, After morphine withdrawal, the increase in glutamate uptake in cultured neurons was morphine dose (A) and time (B) dependent, whereas no significant change was seen in cultured astrocytes. The glutamate uptake in the morphinetreated group was presented as percentage of that of control group. C, Glutamate uptake in cultured astrocytes could be blocked by PDC but not by DHK treatment and was not significantly altered during morphine withdrawal after 7 d morphine (10 nM) treatment. D, Glutamate uptake in cultured neurons was increased after morphine withdrawal and could be blocked by either PDC or DHK treatment. Glutamate, 10 µM. The control rates in the cultured astrocytes and neurons were 1070 ± 93 and 748 ± 48 pmol · mg -1 · min -1 protein, respectively. The data were presented as mean ± SEM of three independent experiments performed in duplicate. Sal, Saline treatment; Mor, morphine treatment.
The question asked then was whether the increase in glutamate uptake in cultured neurons was related to an expression of GLT1 on the cell surface. As an essential control, the possible changes of EAAC1 expression during morphine withdrawal should also be examined considering its expression in the neurons. On the other hand, it is proved that glutamate uptake in astrocytes is mediated by GLAST but not GLT1 (Swanson et al., 1997
The effects of morphine withdrawal are apparent on the Western blots after surface biotinylation shown in Figures 6 and 7. The blots were probed with anti-actin antibody and with antibodies to transporter. Morphine withdrawal produced no significant change in biotinylated (cell surface) or total cell GLT1 expression in cultured astrocytes (Fig. 6). We also tested the effect of morphine on undifferentiated astrocytes without dibutyryl cAMP treatment, in which GLT1 protein is shown to be undetectable (Swanson et al., 1997
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Figure 6. Analysis of GLT1 expression in cultured astrocytes during morphine withdrawal. A, After 7 d morphine treatment, the culture medium containing morphine was withdrawn. The astrocytes were preincubated with 0.01M PBS for 1 hr and were then biotinylated. Westernblots were probed with antibodies to GLT1 and actin. The actin bands provided an index of intracellular proteins. B, Quantitation of immunoblot of GLT1 bands was pooled from three independent experiments. GLT1 immunoreactivity values were normalized to actin in the lysate fraction. The data were expressed as a percentage of the saline-treated group for each fraction (mean ± SEM). There was no significant change in total cell or cell surface GLT1 expression. Sal, Saline treatment; Mor, morphine treatment.
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Figure 7. Analysis of GLT1 and EAAC1 expression in cultured neurons during morphine withdrawal. After 7 d morphine treatment, the culture medium containing morphine was withdrawn. The cultured neurons were preincubated with 0.01 M PBS for 1 hr and were then biotinylated. A, Western blots were probed with antibodies to GLT1 and actin. B, The membranes were then striped and reprobed to EAAC1 and actin. The actin bands provided an index of intracellular proteins. The immunoblot of GLT1 and EAAC1 bands was pooled from three independent experiments. Sal, Saline treatment; Mor, morphine treatment.
Translocation and surface expression of GLT1 at nerve terminals in vivo during morphine withdrawal
A previous study with Northern blot has shown that the total mRNA of GLT1 is upregulated in several brain regions such as striatum and thalamus but not in hippocampus during morphine withdrawal (Ozawa et al., 2001
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Figure 8. Analysis of GLT1 mRNA in hippocampal neurons during morphine withdrawal, as revealed by in situ hybridization. Dark-field micrographs showed GLT1 mRNA distribution in hippocampal CA3 regions in the saline control group (A) and in the morphine group (B). Brightfield micrographs in the insets of A and B presented the positive pyramidal neurons containing GLT1 mRNA (arrows). Asterisks in the dark field of saline group (A) and morphine group (B) indicated the region of these neurons (arrows) located. Scale bars: A, B, 100 µm; insets in A, B, 20 µm.C, The percentage of GLT1-positive neurons in the pyramidal cell layer of CA1 and CA3 or granule cell layer of DG region was quantified, respectively, and no significant change was observed. The results were pooled from the sections (n = 4–6) of three animals in each group. D, The number of silver grains contained in GLT1-positive neurons in CA3 regions was not significantly changed during morphine withdrawal (n = 124 in control group; n = 118 in morphine-treated group). Sal, Saline treatment; Mor, morphine treatment.
The present immunoblot studies demonstrated that GLT1 protein expression was upregulated in the synaptosomal particles and on the cell surface of cultured neurons during morphine withdrawal. However, the possibility still existed that the isolated synaptosomes may be contaminated by astrocytes, and the cell surface expression of GLT1 in cultured neurons was possibly caused by some aspects of the culture procedure in vitro. Then we used both preembedding immunoperoxidase and immunonanogoldsilver labeling to localize GLT1 in vivo and examined the labeling by using electron microscopy. In CA1 and CA3 regions of hippocampus of controlrat, the intensive immunolabeling of GLT1 was primarily seen in astrocytes and their processes (Fig. 9B,C). GLT1 labeling was also seen in the cytoplasm of a few nerve terminals but only occasionally associated with the cell surface of the nerve terminals (Fig. 9C,G,H). Twelve hours after morphine treatment, the intensity of GLT1 labeling in the nerve terminals was increased markedly (Fig. 9D–F). It is striking that gold–silver labeling of GLT1 was often seen on the cell surface of nerve terminals and could associate with the presynaptic membrane (Fig. 9F,H). The quantification of the GLT1 immunolabeling showed that the number of GLT1-positive nerve terminals was increased from
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Figure 9. Translocation and surface expression of GLT1 at hippocampal nerve terminals after morphine withdrawal as revealed by electron microscopy. The morphological results of the CA3 region of the hippocampus were presented as representatives in A–F. A, The ultrastructure without immunolabeling of hippocampal CA3 regions, in which synapses were formed by axonal terminals (a) and dendrites (d). A process of astrocyte was indicated with an asterisk. B, A GLT1-positive astrocyte (asterisks) was present to be juxtaposed to a synapse in the CA3 region of the saline group.C, Anaxonal terminal (a) containing gold–silver particles for GLT1 labeling was seen adjacent to a GLT1-positive astrocyte process (arrowheads) in the saline group. The gold–silver particles (arrows) in the axonal terminal were in the cytoplasm.D, AGLT1-positive axonal terminal(a) made synaptic contact with an unlabeled dendrite(d) in the morphine-treated group.E, Near a GLT1-positive as trocyte(asterisks), an unlabeled axonal terminal (a) formed a synapse with a GLT1-positive dendrite (d) in the morphinetreated group. F, A hippocampal axonal terminal (a) containing GLT1 labeling was shown close to a GLT1-positive astrocyte (arrowheads). Arrow points to gold–silver particle located in the plasma membrane of a dendrite. Double arrowheads point to the labeling in the presynaptic membrane. Scalebars:(inA) A,B,D,E, 1 µm; (in C) C,F, 0.5 µm. G, Quantitative analysis showed that the number of GLT1-positive nerve terminals was increased in both CA1 and CA3 region but not in DG region. The data were pooled from three sections of different rats in each group. The total numbers of terminals counted in CA1, CA3, and DG regions: 496, 519, and 381 in the saline group; 428, 494, and 326 in the morphine group. H, The number of gold–silver particles in nerve terminals that form synapses (Terminal) as well as associated with the plasma membrane per GLT1-positive synapse(Membrane) were quantified in the saline (n=28) and morphine-treated (n=110) groups, respectively. Both particle numbers were significantly increased in the morphine-treated group compared with the control group. *p < 0.05 and **p < 0.01 compared with the saline group. Sal, Saline treatment; Mor, morphine treatment.
Discussion
It is known that opiate abuse exerts extensive adaptive changes in brain functions, including many aspects of neurotransmission, such as transmitter release during morphine withdrawal (Manzoni and Williams, 1999Among the subtypes of glutamate transporters identified, GLT1 is by far the major transporter of the forebrain because, in GLT1 knock-out mice, <6% glutamate transporter activity remains in synaptosomes compared with wild-type animals (Tanaka et al., 1997
It has been shown that GLT1 in neurons is not typically associated with the plasma membrane (Chen et al., 2002
The cellular mechanisms of morphine withdrawal-induced surface expression of GLT1 in neurons remain to be investigated. It is possible that GLT1 could be regulated via protein kinasemediated phosphorylation because GLT1 possesses quite a few putative PKC and PKA phosphorylation sites in its intracellular loops (Kanner, 1993
In summary, the present study revealed an increase of glutamate uptake in hippocampal synaptosomes and provided in vivo evidence showing upregulation and surface expression of glutamate transporters at nerve terminals during morphine withdrawal. The observed accumulation of glutamate transporters at the nerve terminals leads to several functional considerations. It is known that opiate withdrawal causes a significant increase in extracellular glutamate concentration in many brain regions (Aghajanian et al., 1994
Footnotes
Received Nov. 15, 2002; revised Mar. 12, 2003; accepted Mar. 17, 2003.This work was supported by Ministry of Science and Technology Grants G19990 [GenBank] 53907 and G20000 [GenBank] 77800, Chinese Academy of Sciences Grants KSCX2-2, KSCX1-SW-11, and KSCX2-SW-204, the National Natural Science Foundation of China Grants 39840160 and 30024003, Shanghai Science and Technology Committee Grant 018014015, and the K. C. Wong Education Foundation of Hong Kong. We thank Drs. Shi-Gang He and Lin-Yin Feng for their helpful suggestions, Dr.Jian Fei for providing EAAC1 antibodies, and Ya-Lan Wu, Peng Xia, Zhu Wang, Jian-Ping Mao, Wei-Qi Xu, Hai-Jiang Cai, Ji-Song Guan, and Guo-Dong Li for their technical assistance and helpful discussions.
Correspondence should be addressed to either of the following: Dr. Gang Pei, Institute of Biochemistry and Cell Biology, Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences, 320 Yue-Yang Road, Shanghai 200031, China, E-mail: gpei{at}sibs.ac.cn; or Dr. Xu Zhang, Institute of Neuroscience, Shanghai Institutes for Biological Sciences, 320 Yue-Yang Road, Shanghai 200031, China, E-mail: xuzhang{at}ion.ac.cn.
Copyright © 2003 Society for Neuroscience 0270-6474/03/234775-10$15.00/0
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