Regulation of taurine transporter expression by NO in cultured human retinal pigment epithelial cells

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

Regulation of taurine transporter expression by NO in cultured human retinal pigment epithelial cells

Christy C. Bridges¹, M. Shamsul Ola¹, Puttur D. Prasad², Amira El-Sherbeny¹, Vadivel Ganapathy²^,³, and Sylvia B. Smith¹^,⁴

Departments of ¹ Cellular Biology and Anatomy, ² Obstetrics and Gynecology, ³ Biochemistry and Molecular Biology, and ⁴ Ophthalmology, Medical College of Georgia, Augusta, Georgia 30912

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Taurine is actively transported at the retinal pigment epithelial (RPE) apical membrane in an Na⁺- and Cl-dependent manner. Diabetes may alter the function of the taurinetransporter. Because nitric oxide (NO) is a molecule implicatedin the pathogenesis of diabetes, we asked whether NO would alterthe activity of the taurine transporter in cultured ARPE-19 cells.The activity of the transporter was stimulated in the presenceof the NO donor 3-morpholinosydnonimine. The stimulatory effectsof 3-morpholinosydnonimine were not observed during the initial16-h treatment; however, stimulation of taurine uptake was elevateddramatically above control values with 20- and 24-h treatments.Kinetic analysis revealed that the stimulation was associatedwith an increase in the maximal velocity of the transporter withno significant change in the substrate affinity. The NO-inducedincrease in taurine uptake was inhibited by actinomycin D andcycloheximide. RT-PCR analysis and nuclear run-on assays providedevidence for upregulation of the transporter gene. This studyprovides the first evidence of an increase in taurine transportergene expression in human RPE cells cultured under conditions ofelevated levels ofNO.

cell culture

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

TAURINE, a $beta$ -aminosulfonic acid, is the most abundant free amino acid in the retina (38). A high concentration of taurineis essential for maintenance of the structural and functionalintegrity of the retina (20, 34). The precise physiologicalrole of taurine in the retina has yet to be established, althoughit has been suggested to function in calcium modulation (23,29, 34) and osmoregulation (7, 46, 50). Taurine isan unusual biological molecule. It is an amino acid that is notrequired for protein synthesis, it accumulates in excitable tissues,and its turnover rate is low (7-10 days). The only known metabolicrole of taurine is in the synthesis of taurine-conjugated bileacids. Taurine is a zwitterion at physiological pH and, hence,carries no net charge. Because the intracellular concentrationof taurine in tissues such as retina, heart, and placenta is 20-40mM, taurine has been proposed to function as an osmolyte (39).This proposed role is intriguing, because retinal cell edema isassociated with pathologies such as ischemia and reperfusion duringdiabetic retinopathy, macular edema, and neurodegeneration (15,24). Taurine has been proposed also to function as an antioxidant.Taurine, in concert with zinc, protects rod outer segment membranesfrom ion and/or water entry occurring as a consequence of membranelipid peroxidation (37). Recently, Keyes and Zimmerman (28)showed that taurine, in combination with retinol, protects lipidsfrom oxidative damage and may play a key role in protecting retinalpigment epithelial (RPE) lipids during exposure to cycliclight.

In the retina, the concentration of taurine is highest in photoreceptor and RPE cells (27, 35, 55). These observationshave prompted numerous investigations of transport mechanismsfor taurine. Functional studies suggest that a transporter fortaurine is present on the apical membrane of RPE (32, 33)and in cultured human RPE cells (30). Recently cDNAs for thehuman taurine transporter have been cloned, and sequence homologyplaces it within the gene family of Na⁺- and Cl-dependent neurotransmitter transporters (25, 41). The humantaurine transporter cDNA encodes a protein of 619 amino acidswith 12 putative transmembrane domains. The taurine transporterin various cell types, including RPE cells, is regulated by signaltransduction pathways (3, 13, 26, 40), hypertonicity(50, 51), and extracellular taurine levels (19, 26).

Recently, the effect of diabetes on taurine transporter activity was investigated. In vitro studies by Stevens et al. (47)reported that high glucose levels rapidly and specifically decreasedthe activity and mRNA levels of the transporter in cultured RPEcells. In contrast, in vivo studies of RPE from diabetic ratsshowed that uptake of taurine was elevated, rather than decreased,suggesting that diabetes stimulates the activity of the taurinetransporter (53). A molecule implicated in the pathogenic complicationsof diabetes, including diabetic retinopathy, is nitric oxide (NO)(14, 42, 48). Circulating levels of NO are elevated in diabetesmellitus (2, 29). Yilmaz and co-workers (58) reported afivefold elevation of NO in the vitreous of patients with proliferativediabetic retinopathy compared with nondiabetic control patients.NO is produced by different isoforms of NO synthases (NOS) (57).In the retina, constitutive NOS and inducible NOS (iNOS) are present,the former in amacrine and ganglion cells and the latter in RPEand Müller cells (16, 45, 57). The cytokine-inducible formof NOS has been demonstrated also in RPE cells. There is evidencethat NOS activity is increased in retinas of diabetic rats (8).Given that NO levels are increased in diabetic retinopathy (42,58) and that the diabetic condition may affect taurine transport(47, 53), we were interested in determining the effects ofNO on taurine transport in vitro. In the present study, we usedthe well-differentiated RPE cell line ARPE-19 (9, 10) toassess the effects of various NO donors on the activity and expressionof the human taurine transporter. We demonstrate that exposureof cells to the NO donor 3-morpholinosydnonimine (SIN-1) leadsto a dramatic increase in taurine transport activity. We furtherdemonstrate that exposure of these cells to SIN-1 upregulatestaurine transporter geneexpression.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Materials. [1,2-³H]taurine, [2,3-³H]alanine, [2,3,4,5-³H]arginine, and [ $alpha$ -³²P]uridine triphosphate were purchased from Amersham Pharmacia(Piscataway, NJ); [3,4-³H]glutamine and [2,3-³H]glutamate from NEN Research Products (Boston, MA); and [³H(N)]carnitine and [4,5-³H]leucine from Moravek Biochemicals (Brea, CA). TRIzol reagentand cell culture supplies were purchased from Life Technologies(Gaithersburg, MD); Ultrahyb hybridization solution from Ambion(Austin, TX); restriction enzymes and pGEM-T vector from Promega(Madison, WI); SIN-1, sodium nitroprusside (SNP), and methyleneblue from Research Biochemicals International (Natick, MA); actinomycinD, cycloheximide, ascorbic acid, glutathione, $beta$ -alanine, trypanblue solution, lipopolysaccharide (LPS, Escherichia coli), and8-bromoguanosine 3',5'-cyclic monophosphate (8-BrcGMP) from SigmaChemical (St. Louis, MO); and recombinant human interferon- $gamma$ (IFN- $gamma$ )from Biosource International (Camarillo, CA). Human RPE (ARPE-19)cells were purchased from American Type Culture Collection (Manassas,VA). Tissue-Tek OCT embedding compound was obtained from MilesLaboratories (Elkhart, IN); the polyclonal antibody against rattaurine transporter as well as the immunogenic control peptidefrom Alpha Diagnostic International (San Antonio, TX); and themonoclonal anti-nitrotyrosine antibody from Upstate Biologicals(Lake Placid,NY).

Animals. Three-week-old albino (ICR) mice were obtained from Harlan Sprague Dawley (Indianapolis, IN). Animals were maintained on a12:12-h light-dark cycle and were fed the standard Purina mousechow diet. Care and use of the animals adhered to the principlesset forth in The Guiding Principles in the Care and Use of Animals(DHEW Publication No. 80-23).

Cell culture. ARPE-19 cells were cultured in 75-cm² flasks with Dulbecco's modified Eagle's medium-nutrient mixture F-12 (DMEM-F-12) supplementedwith 10% fetal bovine serum, 100 U/ml penicillin, and 100 µg/mlstreptomycin. Cultures were passaged by dissociation in 0.05%(wt/vol) trypsin and seeded in 24-well culture plates. In oneset of experiments assessing the effects of NO donors in conjunctionwith elevated glucose levels, cells were exposed for 24 h to DMEM-F-12containing 17 mM glucose or to DMEM-F-12 containing 45 mMglucose.

Uptake measurements in ARPE-19 cells. For uptake experiments, the culture medium was removed from ARPE-19 cells and the cells were subsequently washed twice withuptake buffer. The composition of the uptake buffer was 25 mMHEPES-Tris, 140 mM NaCl, 5.4 mM KCl, 1.8 mM CaCl₂, 0.8 mM MgSO₄,and 5 mM glucose, pH 7.5. For experiments dealing with the influenceof Na⁺ and Cl on the transport process, the uptake buffers consisted of 20mM HEPES-Tris (pH 7.5) containing 140 mM NaCl, sodium gluconate,or N-methyl-D-glucamine chloride. Uptake was initiated by additionof 250 µl of uptake buffer containing radiolabeled substrates.Uptake measurements were done with a 15-min incubation at 37°C.At the end of the incubation, uptake was terminated by removalof the medium by aspiration followed by three washes with ice-colduptake buffer without the radiolabeled substrates. The cells werethen solubilized in 0.5 ml of 1% sodium dodecyl sulfate (SDS)in 0.2 N NaOH and transferred to scintillation vials for quantitationofradioactivity.

NO donors. To determine the effects of NO on the activity of taurine transporter in ARPE-19 cells, confluent cultures were incubatedin the absence or presence of NO donors SIN-1 or SNP, and theuptake of [³H]taurine was measured. The majority of experiments were donewith SIN-1, the more potent of the two NO donors in stimulatingthe taurine transporter. In one set of experiments, cells wereincubated simultaneously with the cytokines LPS (20 ng/ml) andIFN- $gamma$ (1 µg/ml), and the uptake of [³H]taurine was measured. The recovery of the stimulation of taurineuptake was assessed by incubating ARPE-19 cells with 1 mM SIN-1for 24 h, removing the uptake buffer, and replacing the bufferwith culture medium. Cells were then maintained in the mediumfor 0, 2, 4, 6, and 24 h before assessment of the recovery ofstimulated uptake of [³H]taurine. To test the specificity of NO donors in stimulatingthe activity of the taurine transporter, ARPE-19 cells were incubatedwith 1 mM SIN-1 for 24 h at 37°C, and then uptake of [³H]taurine and the radiolabeled compounds glutamate, glutamine,alanine, arginine, carnitine, and leucine was measured for 15min. The capacity of antioxidants and NO scavengers to block theSIN-1-induced stimulation of taurine uptake by the taurine transporterwas examined by incubating ARPE-19 cells in uptake buffer containingSIN-1 only vs. SIN-1 in the presence of ascorbate (10 mM), glutathione(10 mM), or methylene blue (1 mM). Cells were treated also withascorbate (10 mM), glutathione (10 mM), or methylene blue (1 mM)independently to assess whether these agents had any effect oftheir own on taurine uptake by cultured ARPE-19 cells. Cells weretreated also for 16 h with 8-BrcGMP (100 µM), a cell-permeablecGMP analog, and the uptake of [³H]taurine was measured. To determine whether cells incubated withSIN-1 were positive for nitrotyrosine, ARPE-19 cells were culturedto confluency on chamber slides. They were incubated for 2 h inthe presence or absence of SIN-1. Cells were fixed in 4% paraformaldehydefor 10 min and permeabilized with acetone for 5 min. Slides wereincubated overnight with the polyclonal antibody against nitrotyrosine(1:100) at 4°C. The sections were subsequently incubated overnightat 4°C with FITC-conjugated anti-mouse IgG (1:100). Sections wereexamined by epifluorescence using a Zeiss Axioplan 2 microscopeequipped with a Spot camera and Spot software (version 2.2).

Data analysis. Each uptake experiment was performed in duplicate or triplicate and was repeated two to four times. Data analysis (analysisof variance) was performed using the NCSS statistical softwarepackage (P < 0.05 was considered significant). Kinetic analysiswas done using the computer program Fig.P (version 6.0, Biosoft,Cambridge, UK). Data are presented as means ±SE.

Semiquantitative RT-PCR analysis of the steady-state levels of mRNAs for taurine transporter and glyceraldehyde-3-phosphate dehydrogenase. Confluent cultures of ARPE-19 cells were treated with or without 1 mM SIN-1 for 24 h at 37°C, and poly(A)⁺ mRNA was then prepared from these cells using the TRIzol reagent.RT-PCR was carried out using primer pairs specific for human taurinetransporter and human glyceraldehyde-3-phosphate dehydrogenase(GAPDH). The primers specific for human taurine transporter were5'-GCTAGCTGCATAGTAGTC-3' (sense) and 5'-TGGAACACACCTCACTGC-3'(antisense) and corresponded to nucleotide positions 872-889 and1751-1769, respectively, of the human taurine transporter cDNA(41). The primers specific for human GAPDH were 5'-AAGGCTGAGAACGGGAAGCTTGTCATCAAT-3'(sense) and 5'-TTCCCGTTCAGCTCAGGGATGACCTTGCCC-3' (antisense),corresponding to nucleotide positions 241-270 and 711-740 in humanGAPDH cDNA (49). Each of these RT-PCR products was subclonedin pGEM-T vector and sequenced to establish its identity. Forsemiquantitative RT-PCR, PCR following reverse transcription wascarried out with various numbers of cycles (range 9-30). The productswere size fractionated on an agarose gel and subjected to Southernhybridization with probes specific for the taurine transporteror GAPDH. These probes were generated by labeling the respectivesubcloned RT-PCR products with [³²P]dCTP. The intensity of the hybridization signal was quantifiedusing the STORM PhosphorImaging System (Molecular Dynamics, Sunnyvale,CA). The relationship between the intensity of the signal andthe PCR cycle number was then analyzed to determine the linearrange for the PCR product formation. The intensities of the signalswithin the linear range were used for dataanalysis.

Nuclear run-on transcription assay. To monitor SIN-1-induced changes in the transcription rate of the taurine transporter gene, the nuclear run-on assay was performedas described elsewhere (18) with modifications. ARPE-19 cellswere incubated for 24 h with or without 1 mM SIN-1. Nuclei wereisolated by homogenization with 10 strokes in a Dounce homogenizerin 2 ml of lysis buffer [10 mM Tris · HCl, pH 7.4, 3 mM CaCl₂,2 mM MgCl₂, and 1% (vol/vol) NP-40] followed by centrifugationat 500 g for 5 min at 4°C. Pelleted nuclei were frozen immediatelyin liquid nitrogen in 200 µl of freezing buffer [50 mM Tris ·HCl, pH 8.3, 40% (vol/vol) glycerol, 5 mM MgCl₂, and 0.1 mM EDTA]until the assay was performed. The in vitro labeling of nascentRNA was performed in 200 µl of 2× reaction buffer {10 mM Tris· HCl, pH 8.0, 5 mM MgCl₂, 0.3 M KCl, 10 mM dithiothreitol, 1mM each ATP, GTP, and CTP, and 10 µl of [ $alpha$ -³²P]UTP (10 mCi/ml)}. The mixture was incubated for 30 min at 30°C.RNA was isolated using the TRIzol reagent according to the manufacturer'sinstructions. RNA was suspended in 50 µl of 10 mM N-tris(hydroxymethyl)methyl-2-aminoethanesulfonicacid, pH 7.4, 10 mM EDTA, and 0.2% (wt/vol) SDS, heated for 5min at 90°C, and added directly to the hybridization solution.To prepare membranes for hybridization with radiolabeled RNA,20 µg of plasmid DNA, containing the human taurine transportercDNA in pGEM-T vector, were linearized with the restriction enzymeSalI. DNA was denatured by addition of 0.4 M NaOH for 30 min atroom temperature and then neutralized by addition of 6× saline-sodiumcitrate (SSC) and placement on ice. The slot-blot apparatus wasprepared, and 5 µg of plasmid DNA were applied to each slot underlow vacuum. Each slot was rinsed with 500 µl of 6× SSC. Membranestrips were prehybridized for 2 h at 68°C in Ultrahyb hybridizationbuffer. Membranes were hybridized overnight at 68°C using 1 mlof the same buffer containing radiolabeled RNA. After hybridization,membranes were washed twice for 5 min each in 2× SSC and 0.1%SDS at 68°C and twice for 15 min each in 0.1% SSC and 0.1% SDSat 68°C and exposed to X-rayfilm.

Laser scanning confocal microscopic analysis of taurine transporter in cultured ARPE-19 cells and in intact RPE. Immunohistochemical methods were used to localize taurine transporter in cultured human ARPE-19 cells and in RPE of intactmouse eyes. Eyes from 3-wk-old albino mice were enucleated andfrozen immediately in Tissue-Tek OCT, and 10-µm-thick cryosectionswere prepared. The cells were fixed with ice-cold methanol, andthe cryosections were fixed with ice-cold acetone. Cells and cryosectionswere blocked with 10% normal goat serum. Samples were incubatedwith an affinity-purified polyclonal antibody against rat taurinetransporter. The rabbit anti-taurine transporter antibody (AlphaDiagnostics) was prepared using a 20-mer peptide (designated Tau-11)near the carboxy-terminal cytoplasmic region of rat TAUT-1 (43).The immunogenic peptide used in production of the antibody shows100% homology to rat and mouse and 90% to human and canine taurinetransporter. The antibody has been shown to cross-react with mouse,human, rat, and cat tissues. Cells were incubated with the primaryantibody for 3 h at room temperature at a dilution of 1:100; tissuecryosections were incubated for 3 h at room temperature at a dilutionof 1:50 and incubated overnight at 4°C. To demonstrate the specificityof the antibody, the primary antibody was neutralized with anexcess of the antigenic peptide before use for incubation withtissue sections. Additional negative controls included using bufferonly and 0.1% normal rabbit serum in place of the primary antibody.After they were rinsed, all samples were incubated overnight at4°C with an FITC-conjugated AffiniPure goat anti-rabbit IgG ata dilution of 1:100. Cells and cryosections were optically sectioned(z-series) using a Nikon Diaphot 200 Laser Scanning Confocal ImagingSystem (Molecular Dynamics). Images were analyzed using the ImageDisplay 3.2 software package (Silicon Graphics, Mountain View,CA).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The present study focused on the role of NO in the regulation of the human taurine transporter in cultured human ARPE-19 cells.Before testing the activity of the transporter in ARPE-19 cells,we sought to establish its presence using immunohistochemicalmethods. ARPE-19 cells were cultured to confluency on plasticchamber supports. The cells were incubated with a commerciallyavailable, affinity-purified antibody against the taurine transporter.As shown in Fig. 1, laser scanning confocal optical sections ofcells demonstrated intense labeling with the antibody. In Fig.1A, cells were sectioned optically in the vertical plane, allowingthe distribution of the protein to be viewed from the sides ofthe cells. There appeared to be protein distributed throughoutthe cell cytoplasm. In Fig. 1B, cells were scanned in a horizontalplane, allowing the cells to be viewed from above. There was anabundance of bright fluorescence across the apical surface ofthe cells. These data supported the use of ARPE-19 cells for studyof taurine uptake activity. Incubation of cells with the antibodythat had been incubated with an excess of immunogenic controlpeptide resulted in no positive staining (Fig. 1C). Although itis necessary to use cultured cells to study the activity of thetaurine transporter, we considered it essential also to confirmthe presence of the taurine transporter in RPE cells in an intactmammalian retina, inasmuch as there have been no immunohistochemicalstudies documenting the presence of the transporter in RPE. Tothis end, we used cryosections of mouse retina (Fig. 2). A hematoxylin-and-eosin-stainedcryosection of the outer retina (Fig. 2A) is provided for comparisonto the photomicrograph of the immunolabeled section (Fig. 2B).The outer portion of the retina, including the outer nuclear layerof photoreceptor cell nuclei, and the inner segments of thesecells are labeled. The RPE is the single layer of epithelial cellsbetween choroid and outer segments. Figure 2B shows a cryosectionof mouse retina incubated with the antibody against the taurinetransporter. The taurine transporter was detected abundantly inRPE and was present throughout much of the RPE cell cytoplasm.The taurine transporter was expressed also in the photoreceptorcell inner segments, in which the endoplasmic reticulum, Golgiapparatus, and other organelles are located (Fig. 2B). Labelingwas present in other regions of the retina, including the retinalganglion cell layer and outer plexiform layer (data not shown).

View larger version (24K):
[in this window]
[in a new window]

Fig. 1. Laser scanning confocal microscopic immunolocalization of taurine transporter in cultured human ARPE-19 cells and mouse retina. ARPE-19 cells were grown to confluency on laminin-coated chamber slides and processed for immunohistochemistry using a primary antibody against taurine transporter followed by an FITC-labeled secondary antibody. A: optical section of cells taken in a vertical plane (x,z). Bright band of fluorescence is indicative of positive detection of the antibody in cultured cells. Top and bottom arrows at left of A point to apical and basal surfaces of cells. B: optical section of cells taken in a horizontal plane (x,y) shows taurine transporter on apical retinal pigment epithelial (RPE) surface. C: horizontal section of cells incubated with peptide that had been preincubated with antibody against taurine transporter (negative control) shows no positive staining. Original magnifications ×600.

View larger version (93K):
[in this window]
[in a new window]

Fig. 2. Laser scanning confocal microscopic immunolocalization of taurine transporter in intact mouse retinal tissue. Eyes of ICR albino mice were frozen in OCT embedding medium, and cryosections were prepared and subjected to immunohistochemical detection of taurine transporter using a commercially available antibody. A: hematoxylin-and-eosin-stained cryosection of outer portion of normal mouse retina showing outer layers of the retina. B: immunolocalization of taurine transporter. Arrow points to intense labeling of the RPE; arrowhead points to labeling of inner segments (IS). Magnification ×400. ONL, outer nuclear layer; OS, outer segments; CH, choroid.

Stimulation of human taurine transporter by NO donors. Figure 3A shows the effect of the NO donors SIN-1 and SNP on the uptake of 80 nM [³H]taurine by the taurine transporter in human ARPE-19 cells. BothNO donors, at 1 mM and when incubated with cells for 24 h, stimulatedthe uptake process. SIN-1 was a more potent stimulator of taurineuptake than SNP. Exposure of ARPE-19 cells to SIN-1 led to a 3.5-foldstimulation of taurine uptake. Exposure of cells to 1 mM SNP undersimilar conditions resulted in an ~2.5-fold stimulation of taurineuptake. Figure 3B shows the dose-response relationship for SIN-1.SIN-1 was ineffective up to 100 µM. The stimulation was seen onlyat 1 mM. The effect was observed with freshly prepared SIN-1.Incubation of cells with "spent" SIN-1 (i.e., SIN-1 that had beenprepared 48 h before incubation) showed a markedly reduced stimulatoryeffect (data not shown).

View larger version (13K):
[in this window]
[in a new window]

Fig. 3. Effects of NO donors on uptake of taurine in cultured ARPE-19 cells. A: uptake of [³H]taurine (80 nM) in the absence (control) or presence of 1 mM 3-morpholinosydnonimine (SIN-1) or sodium nitroprusside (SNP) for 24 h. B: dose-response relationship for effect of SIN-1 on uptake of 80 nM [³H]taurine (treatment time 24 h). Values are means ± SE for 4 determinations from 2 independent experiments.

To determine whether incubation of cells with NO donors affected Na⁺ or Cl dependency of the taurine transporter, cells were incubated for24 h with or without SIN-1, and the uptake of [³H]taurine was measured in the presence of NaCl in the absenceof Na⁺ but in the presence of Cl (N-methyl-D-glucose chloride) or in the presence of Na⁺ but the absence of Cl (sodium gluconate). The inhibition of taurine uptake by $beta$ -alanine,a known competitive inhibitor of taurine uptake (54), was alsoassessed in cells exposed to SIN-1. As shown in Table 1, taurineuptake was observed only in the presence of NaCl. In the absenceof Na⁺ or Cl, the uptake was reduced to 5% of the control. SIN-1 stimulatedthe uptake only in the presence of NaCl but did not stimulatetaurine uptake in the absence of Na⁺ or Cl. $beta$ -Alanine inhibited taurine uptake in the presence and absenceof SIN-1. These data suggest that NO did not affect the Na⁺/Cl dependency of the taurine transporter, nor did it alter the inhibitoryeffect of $beta$ -alanine on taurine uptake. We also analyzed the Na⁺- and Cl-activation kinetics of taurine uptake in control cells and incells treated with SIN-1 (data not shown). The activation of taurineuptake with increasing concentrations of Na⁺ (the concentration of Cl was kept constant at 140 mM) exhibited a sigmoidal relationshipin control and SIN-1-treated cells. In both cases, the Hill coefficientwas 2 (1.7 ± 0.6 and 2.2 ± 0.1 in control and SIN-1-treated cells,respectively). The activation of taurine uptake with increasingconcentrations of Cl (the concentration of Na⁺ was kept constant at 140 mM) exhibited a hyperbolic relationshipin control and SIN-1-treated cells. In both cases, the Hill coefficientwas 1 (0.96 ± 0.10 and 0.93 ± 0.07 in control and SIN-1-treatedcells, respectively). Thus the Na⁺-Cl-taurine stoichiometry remained 2:1:1 in control cells and incells treated with SIN-1.

View this table:
[in this window]
[in a new window]

Table 1. Influence of SIN-1 on Na⁺ and Cl dependency of taurine uptake

To determine whether stimulation of taurine uptake by SIN-1 was influenced by exposure of cells to high glucose, ARPE-19 cellswere incubated for 24 h in medium containing high (45 mM) or normal(17 mM) glucose present in the DMEM-F-12 culture medium (9,10). For each glucose concentration, cells were incubated withor without 1 mM SIN-1. Uptake of [³H]taurine (80 nM) in cells grown in high or low glucose withoutSIN-1 was 1.89 ± 0.08 and 1.80 ± 0.06 pmol · mg protein¹ · 15 min¹, respectively. Uptake of [³H]taurine in cells grown in high or low glucose in the presenceof SIN-1 was 3.59 ± 0.11 and 3.53 ± 0.10 pmol · mg protein¹ · 15 min¹, respectively. These data suggest that exposure of cells for24 h to high levels of glucose does not alter the SIN-1-inducedstimulation of taurine uptake by ARPE-19 cells. To determine whetherinduction of iNOS activity with cytokines can replicate the resultsachieved by the addition of the NO donor molecules, RPE cellswere incubated for 48 h with the cytokines LPS (20 ng/ml) andIFN- $gamma$ (1 µg/ml). It has been shown in cultured RPE cells thatincubation with these cytokines induces the synthesis of iNOSand production of NO (45). Uptake of [³H]taurine (80 nM) in cells grown in the presence of both of thesecytokines was 2.50 ± 0.11 pmol · mg protein¹ · 15 min¹, which was ~50% greater than uptake in control cells (1.73 ±0.06 pmol · mg protein¹ · 15 min¹). These data suggest that exposure of RPE cells to cytokinesknown to induce NOS can stimulate taurine uptake in a manner similarto exposure directly to NOdonors.

Time course of stimulation of taurine uptake by SIN-1. After determining that SIN-1 stimulated the uptake of taurine in ARPE-19 cells after 24 h of incubation, we performed a time-coursestudy. Figure 4 shows the data for exposure of cells for variouslengths of time to 1 mM SIN-1. During the initial 16 h of exposureto SIN-1, the uptake of taurine was similar to that of cells notexposed to the NO donor; however, by 18 h the uptake of taurinein SIN-1-treated cells increased and was dramatically elevatedabove control values by 20 and 24 h.

View larger version (9K):
[in this window]
[in a new window]

Fig. 4. Time course of stimulation of taurine uptake by SIN-1. ARPE-19 cells were exposed to 1 mM SIN-1 for various lengths of time, and uptake of [³H]taurine (80 nM) was determined. Parallel experiments were carried out with cells cultured similarly, but in the absence of SIN-1. Results are given as percentage of taurine uptake measured in corresponding control cells not treated with SIN-1. Values are means ± SE for 4 determinations from 2 independent experiments.

Inhibition of NO-induced stimulation of taurine transporter by antioxidants and NO scavengers. To determine whether the stimulation of taurine uptake by SIN-1 could be inhibited by antioxidants and NO scavengers, ARPE-19cells were incubated for 24 h with or without 1 mM SIN-1 in thepresence or absence of antioxidants, ascorbate (10 mM) or glutathione(10 mM), or with the NO scavenger methylene blue (1 mM). The uptakeof [³H]taurine (80 nM) was then measured for 15 min in these cells.As shown in Fig. 5, uptake of taurine was threefold higher incells treated with SIN-1 alone than in cells treated similarlybut in the absence of SIN-1. When cells were incubated simultaneouslywith SIN-1 and ascorbate or SIN-1 and glutathione, the SIN-1 stimulationof taurine uptake was markedly attenuated. Similarly, methyleneblue also attenuated the stimulatory effect of SIN-1 on taurineuptake. These antioxidants and NO scavengers by themselves hadno noticeable effect on taurine transporter activity (data notshown). Incubation of ARPE-19 cells with SIN-1 for 2 h followedby immunohistochemical detection of nitrotyrosine revealed thepresence of higher levels of nitrotyrosine in cells treated withSIN-1 (Fig. 6A) than in cells not exposed to SIN-1 (Fig. 6B).A positive nitrotyrosine reaction is considered an indicator ofNO production. These data further support the belief that theSIN-1-induced stimulation of taurine transporter in ARPE-19 cellsis mediated through NO. In experiments in which ARPE-19 cellswere exposed to 8-BrcGMP (100 µM), the uptake of taurine (80 nM)was stimulated 23% (2.67 ± 0.10 pmol/mg protein) compared withcontrol cells (2.17 ± 0.14 pmol/mg protein), suggesting that theinfluence of NO on taurine transporter is mediated, at least inpart, by cGMP.

View larger version (22K):
[in this window]
[in a new window]

Fig. 5. Effects of antioxidants and nitric oxide (NO) scavengers on SIN-1-induced stimulation of taurine uptake in ARPE-19 cells. Confluent cells were treated with or without 1 mM SIN-1 for 24 h. Cells were incubated at the same time in the presence or absence of ascorbate, glutathione, or methylene blue. Uptake of [³H]taurine (80 nM) was measured for 15 min. Values are means ± SE for 3 determinations from 2 independent experiments.

View larger version (125K):
[in this window]
[in a new window]

Fig. 6. Immunodetection of nitrotyrosine in ARPE-19 cells exposed to SIN-1. ARPE-19 cells were grown to confluency on laminin-coated chamber slides and then exposed to 1 mM SIN-1 for 2 h. Cells were processed for immunohistochemistry using a primary antibody against nitrotyrosine followed by an FITC-labeled secondary antibody. A: SIN-1 treated cells. B: control cells. Magnification ×600.

Specificity of NO-induced stimulation of taurine transporter. The NO-induced stimulation of [³H]taurine uptake in ARPE-19 cells was not a nonspecific effect, because the uptake of othernutrients, glutamine, glutamate, alanine, arginine, carnitine,and leucine, was not affected under identical experimental conditions(Table 2). Because the uptake of taurine was actually stimulatedin the presence of SIN-1, while uptake of other compounds wasnot affected, it is not likely that SIN-1 damaged the RPE cells.Total protein levels measured in cells (n = 8) exposed to SIN-1(0.21 ± 0.02 mg) did not differ significantly from protein levelsin cells not exposed to SIN-1 (0.23 ± 0.02, P > 0.5). Moreover,when cells were cultured in the presence or absence of SIN-1 for24 h and subjected to the trypan blue exclusion assay (0.2% wt/vol)to assess cell viability, there was no significant differencein the number of cells excluding the dye (data not shown).

View this table:
[in this window]
[in a new window]

Table 2. Specificity of SIN-1-induced stimulation of taurine uptake

Kinetic analysis of NO-induced stimulation of taurine transporter activity. We then analyzed the kinetics of taurine transporter in control cells and in cells treated for 24 h with 1 mM SIN-1 (Fig.7). The analysis showed that the increase in the transport activityof the taurine transporter observed in SIN-1-treated ARPE-19 cellscompared with control cells was primarily associated with an increasein the maximal velocity of the transporter with no significantchange in the substrate affinity. The maximal velocity of taurineuptake was 3.5-fold greater in SIN-1-treated cells than in controlcells (697.8 ± 61.9 vs. 194.3 ± 25.6 pmol · mg protein¹ · 15 min¹). The Michaelis-Menten constant for taurine remained almost thesame in SIN-1-treated and control cells (9.4 ± 1.9 vs. 8.9 ± 2.7µM).

View larger version (15K):
[in this window]
[in a new window]

Fig. 7. Kinetic analysis of taurine uptake in control and SIN-1-treated ARPE-19 cells. Confluent cells were treated with or without 1 mM SIN-1 for 24 h. Uptake of taurine was measured for 15 min over a taurine concentration range of 0.5-20 µM. Values are means ± SE for 3 determinations from 3 independent experiments. Results are presented as plots describing the relationship between taurine concentration and taurine uptake rate and also as Eadie-Hofstee plots: V/S vs. V, where V is taurine uptake (in pmol · mg protein¹ · 15 min¹) and S is taurine concentration (in µM).

We next examined the influence of cycloheximide (an inhibitor of translation) and actinomycin D (an inhibitor of transcription)on the SIN-1-induced increase in taurine transporter activity.Both compounds significantly decreased the stimulatory effectof SIN-1. As shown in Fig. 8, incubation of cells with SIN-1 inthe absence of actinomycin D or cycloheximide (control) resultedin a stimulation of taurine transport as described above. Whencells were pretreated with either of the inhibitors for 2 h andthen incubated with these compounds in the presence of SIN-1,the stimulatory effect of SIN-1 was eliminated. These data suggestthat the stimulatory effect of SIN-1 on taurine transporter activityinvolves de novo synthesis of RNA and protein.

View larger version (9K):
[in this window]
[in a new window]

Fig. 8. Effects of cycloheximide and actinomycin D on SIN-1-induced increase in taurine transporter activity. Confluent ARPE-19 cells were pretreated with cycloheximide (100 µg/ml) or actinomycin D (10 µg/ml) for 2 h and then incubated with these compounds in the presence or absence of 1 mM SIN-1. Uptake of [³H]taurine (80 nM) was then measured for 15 min. Values are means ± SE for 3 determinations from 3 independent experiments.

Semiquantitative RT-PCR analysis of NO-induced stimulation of the taurine transporter. We then investigated the influence of SIN-1 treatment on the steady-state levels of mRNA transcripts specific for the taurinetransporter. mRNA samples isolated from control and SIN-1-treatedARPE-19 cells were used for semiquantitative RT-PCR for the determinationof the levels of mRNA transcripts. As an internal control, wedetermined the steady-state levels of the GAPDH mRNA in the samplesin parallel. RT-PCR was done with a wide range of PCR cycles (i.e.,9-30). The resultant products were run on a gel and then subjectedto Southern hybridization with ³²P-labeled cDNA probes specific for the taurine transporter andGAPDH. The hybridization signals were quantified using the STORMPhosphorImaging System, and the intensities that were in the linearrange with the PCR cycle number were used for analysis. The resultsof these experiments (Fig. 9) showed that in the cells treatedwith SIN-1, the steady-state levels of taurine transporter mRNAincreased markedly compared with control cells. These resultsdemonstrate that the SIN-1-induced increase in taurine transporteractivity is likely due to increased expression of the gene codingfor the transporter.

View larger version (42K):
[in this window]
[in a new window]

Fig. 9. Analysis of steady-state levels of mRNA for taurine transporter (TAUT) and glyceraldehyde-3-phosphate dehydrogenase (GAPDH) in control ( $-$ SIN-1) and SIN-1 treated (+SIN-1) ARPE-19 cells. Confluent cells were treated with or without 1 mM SIN-1 for 24 h. Poly(A)⁺ RNA was then isolated from these cells and used for semiquantitative RT-PCR. Primer pairs specific for human TAUT mRNA and human GAPDH mRNA were used. RT-PCR was done with a wide range of PCR cycles (9-30). Resultant products were run on a gel and then subjected to Southern hybridization with ³²P-labeled cDNA probes specific for TAUT and GAPDH. Hybridization signals were quantified using the STORM PhosphorImaging System, and intensities that were in the linear range with the PCR cycle number were used for analysis. GAPDH-specific band intensity was used as an internal control. Ratios of TAUT-specific band intensity to GAPDH-specific band intensity were then compared between control and SIN-1 treated cells. Ratio in control cells was taken as 1.

Nuclear run-on assay. To confirm the results of the semiquantitative RT-PCR data, we used the nuclear run-on transcription assay, which is a sensitivemethod for direct measurement and comparison of specific genetranscription in cells (17). We isolated nuclei from ARPE-19cells that had been incubated for 24 h in the presence or absenceof SIN-1 and prepared ³²P-labeled nascent RNA as described by Greenberg and Bender (17).The RNA was subsequently used in slot-blot analysis on membranesto which the human taurine transporter cDNA had been applied toquantitate specifically the taurine transporter mRNA in the nascentRNA samples. As shown in Fig. 10, the intensity of the signal forthe taurine transporter mRNA from ARPE-19 cells incubated withSIN-1 was much greater than that in cells not incubated in SIN-1.Densitometric scans of the bands revealed a 12-fold greater intensityin the SIN-1-treated than in the control cells. This experimentwas carried out twice, and the results were the same in both cases.The data provide strong support that transcription of the taurinetransporter gene is stimulated in the presence of the NO donorSIN-1.

View larger version (57K):
[in this window]
[in a new window]

Fig. 10. Nuclear run-on transcription assay. ARPE-19 cells were incubated for 24 h with or without 1 mM SIN-1. Nuclei were isolated, and nascent RNA was labeled with [ $alpha$ -³²P]UTP. This radiolabeled RNA was then hybridized to membranes with cross-linked human taurine transporter cDNA. Membranes were hybridized overnight at 68°C and exposed to X-ray film.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The present study was designed to assess the effects of NO on the transport of taurine by cultured human RPE cells. NO isa mediator of many physiological processes, such as vasodilationand neurotransmission; it is recognized also for its toxic effects(14). NO has been implicated in the pathogenesis of diabeticretinopathy (2, 14, 29, 42, 48, 57, 58). We haveshown recently that, in cultured RPE cells, NO stimulates thetransport of cystine, the disulfide form of cysteine, which isrequired for synthesis of the antioxidant glutathione (4).In the present study, we asked whether the transport of taurinewould be affected similarly. Taurine is thought to have antioxidantproperties (28, 37). Moreover, there is convincing evidencethat it functions in osmoregulation (5, 39, 50).

To determine whether NO altered the activity of the taurine transporter, we used the well-differentiated ARPE-19 cell line.These cells are a rapidly growing RPE cell line established inthe laboratory of Dr. Larry Hjelmeland (University of California,Davis). They form a uniform population of polarized epithelialmonolayers on porous filter supports. They retain features characteristicof RPE cells, including defined cell borders, a cobblestone appearance,noticeable pigmentation (9, 10), and the capacity to phagocytoseouter segment disks (11). The usefulness of these cells in studyingthe transport of folate was established recently (6). In thepresent study, we used immunohistochemical methods to determinewhether the taurine transporter is present in ARPE-19 cells. Withthe use of an affinity-purified antibody against the transporter,our confocal microscopic analysis clearly showed that the transporteris present in ARPE-19 cells. The horizontal scans suggested thatthe protein was available on the apical membrane and was presentalso throughout the cells. A number of functional studies fromour laboratory and others had suggested the presence of the transporteron the apical surface of cultured RPE cells (30, 32, 33);however, this report represents the first immunohistochemicalevidence to that effect. To confirm the localization of the taurinetransporter to RPE in vivo, we used cryosections of normal mouseeye. The antibody detected a strong positive signal in severallayers of the retina, including the retinal ganglion cells, outerplexiform layer, photoreceptor cell inner segments, and the RPE.Although recent in situ hybridization studies have localized themRNA encoding mouse taurine transporter to these same retinallayers (54), our data represent the first immunohistochemicalevidence of the location of the transporter in any mammalian retina.The detection of the taurine transporter in intact RPE is importantconfirmation of the presence of the protein in RPE in vivo andvalidates the use of RPE cells to study its function invitro.

Having established the presence of the transporter in ARPE-19 cells, we sought to address the effects of NO on taurine transport.We used the NO donors SIN-1 and SNP. Incubation of ARPE-19 cellswith SIN-1 or SNP caused a marked stimulation of uptake of taurineby the transporter. Inasmuch as SIN-1 was more potent than SNPin triggering this effect, the remaining experiments were conductedwith SIN-1. The effects on taurine transporter activity by SIN-1were not immediate. Rather, the increased activity was observedafter 18 h of incubation with the NO donor. Incubation of cellsfor 24 h with SIN-1 led to a 3.5-fold stimulation of taurine transporteractivity. Incubation with SIN-1 did not affect the Na⁺ or Cl dependency of the taurine transporter, the Na⁺- and Cl-activation kinetics, or the capacity of $beta$ -alanine to competewith taurine for the uptake process. Taurine uptake in ARPE-19cells was not only stimulated by NO donors directly, but alsoby exposure of the cells to agents such as LPS that are knownto induce NOS (45). Additional experiments suggested that theSIN-1 effects on taurine transporter activity were mediated viaNO. Treatment of ARPE-19 cells with NO scavengers inhibited SIN-1stimulation of taurine transporter activity. Moreover, immunohistochemicalanalysis assessing nitrotyrosine production in SIN-1-treated cellsshowed positive reactivity, indicating that NO wasproduced.

Kinetic analysis showed that the increased activity of the taurine transporter in the presence of SIN-1 was not due to anincrease in substrate affinity but, rather, to an increase inthe maximal velocity of taurine uptake. Such data suggest thatsynthesis of the taurine transporter may be increased in the presenceof NO donors. To test this further, we cultured ARPE-19 cellsin the presence of SIN-1 plus agents that inhibit transcriptionand translation, actinomycin D and cycloheximide, respectively.In both cases, the SIN-1-induced increase in taurine transporteractivity was completely inhibited. Semiquantitative RT-PCR providedfurther evidence that NO increases the steady-state levels oftaurine transporter mRNA ~3.5-fold. Although NO stimulated theuptake of taurine by ARPE-19 cells, it had little effect on thetransport of other amino acids such as alanine or glutamate. Theobserved increase in steady-state levels of taurine transportermRNA levels may be due to an increase in the transcription rateof the taurine transporter gene or an increase in the stabilityof the taurine transporter mRNA. The finding that the increasedmRNA levels are completely abolished by the transcription inhibitoractinomycin D argues in favor of the gene expression as the siteof regulation of the NO-mediated increase in mRNA levels. Moreover,the data obtained from the nuclear run-on transcription assayprovide strong evidence that the increase in taurine transportermRNA levels is due to increased transcriptionalactivity.

These data provide the first evidence that taurine transporter activity is regulated by NO. They are important, because NOlevels are increased in diabetic retinopathy, the leading causeof blindness among working-aged Americans (56). Other investigatorshave examined taurine transporter activity under hyperglycemicconditions. Stevens et al. (47) showed that taurine transporteractivity decreased within 4 h of exposure of human RPE cells to30 mM glucose. On the other hand, Vilchis and Salceda (53) studieduptake of taurine in RPE isolated from rats that had been diabeticfor 3 and 6 wk. They found a stimulation of taurine uptake indiabetic RPE compared with normal RPE. The differences in theexperimental outcomes from these two laboratories may reflectdifferences in the length of time RPE cells were exposed to hyperglycemicconditions. In the case of cultured cells (47), the earliesteffect of high glucose appears to be a downregulation of the transporter.Thus the acute effect of hyperglycemia on the taurine transporterin RPE cells seems to be a downregulation of the transporter expression.This effect was accompanied by a decrease in intracellular levelsof taurine. The long-term effects of hyperglycemia on the taurinetransporter in the RPE cells used in that study are not known.Interestingly, in the present study, exposure of ARPE-19 cellsto high glucose for 24 h did not affect taurine transporter function.In the case of the studies of diabetic rats (53), taurine transporteractivity increased. In this in vivo model, the retinas would havebeen subjected constantly to a hyperglycemic state for severalweeks. It is noteworthy that the increased taurine transporteractivity was greater after 6 wk of diabetes than after 3 wk. Becauseanimal studies have shown that chronic hyperglycemia increasestaurine transport activity in RPE cells (53), we speculate thatlong-term diabetes may be associated with elevated NO production,which in turn stimulates the taurine transporter expression. Ourexperimental findings showing NO-induced stimulation of taurineuptake in cultured RPE cells support this speculation. That is,they may suggest that, in diabetic retinopathy, NO is one of themolecules responsible for the observed upregulation of taurinetransporter expression and activity. Our experiments address animportant aspect of the altered diabetic state on RPE cells, thatof increased levels of NO. Thus our data showing an upregulationof taurine transport in cultured cells may reflect conditionsof longer-standing diabetes, rather than immediate effects ofthe initial exposure of the cells tohyperglycemia.

Because NO is known to function as a vasodilator (14) and because diabetic retinopathy has an ischemic component in whichNO levels may be decreased, it may seem paradoxical to implicateNO in the pathogenesis of diabetic retinopathy. This paradox isresolved when it is recognized that the increased level of NOobserved in the vitreous of diabetic patients is not an earlyevent (58). During the early stages of diabetic retinopathy,typically called the nonproliferative stage, platelets clump togetherto form small stable aggregates that can lead to capillary closure(21). During this period of ischemia, there may be a reductionof vascular NO. The nonproliferative stage is followed, however,by a proliferative stage in which new blood vessels are formed.It is this proliferative stage that is associated with increasedlevels of NO (57). The proliferative stage is associated alsowith an increase in vascular endothelial growth factor, whichhas been shown to upregulate NO (22, 52). In addition, proliferativediabetic retinopathy is associated with elevated intravitreallevels of cytokine tumor necrosis factor, interferon, and interleukin-1(1, 12). These compounds have been shown also to induce productionof NO by the expression of iNOS, which is found in Müller andRPE cells (16, 45, 57).

The present study did not address the specific mechanism by which NO regulates the expression of the taurine transporter gene.It is known that NO activates guanylate cyclase. Our data showingthat 8-BrcGMP, a cell-permeable cGMP analog, stimulated taurineuptake suggest that the effects of NO donors may be at least partiallymediated by cGMP. It is well known also that, in addition to thissignaling role, NO interacts with cellular redox systems, especiallythiol groups. NO exposure or synthesis may impose a nitrosativestress similar to that imposed by oxygen-derived species. Theattenuation of the stimulatory effect of NO on taurine transporterexpression by the antioxidants ascorbic acid and glutathione suggeststhat nitrosative stress may contribute also to the NO-inducedaction observed in the present study. In summary, these data showthat NO regulates the expression and activity of the taurine transporterin RPE cells in vivo. It is becoming apparent that NO regulatesother transporters in RPE as well. For example, NO stimulatesthe transport by RPE of cystine, the disulfide form of cysteine,which is required for synthesis of the antioxidant glutathione(4). On the other hand, NO inhibits the activity of the reduced-folatetransporter in cultured RPE cells (44). Studies of the regulationof transporter activity by NO may provide important insights foraltered cellular function that occurs in conditions such as diabetes,when NO iselevated.

	ACKNOWLEDGEMENTS

The authors thank Susan Johnson for assistance in preparation of the manuscript and Penny Roon for preparation of the mousetissuesections.

	FOOTNOTES

This research was supported by an unrestricted award from Research to Prevent Blindness to the Department of Ophthalmology,Medical College of Georgia, by an award from the Medical Collegeof Georgia Research Institute, and National Eye Institute GrantsEY-13089 and EY-12830.

Address for reprint requests and other correspondence: S. B. Smith, Dept. of Cellular Biology and Anatomy, Medical Collegeof Georgia, Augusta, GA 30912 (E-mail: sbsmith{at}mail.mcg.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 5 March 2001; accepted in final form 8 August 2001.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

1. Abu el Asrar, AM, Maimone D, Morse PH, Gregory S, and Reder AT. Cytokines in the vitreous of patients with proliferative diabetic retinopathy. Am J Ophthalmol 114: 731-736, 1992[ISI][Medline].

2. Bank, N, and Aynedjian HS. Role of EDRF (nitric oxide) in diabetic renal hyperfiltration. Kidney Int 43: 1306-1312, 1993[ISI][Medline].

3. Brandsch, M, Miyamoto Y, Ganapathy V, and Leibach FH. Regulation of taurine transport in human colon carcinoma cell lines (HT-29 and Caco-2) by protein kinase C. Am J Physiol Gastrointest Liver Physiol 264: G939-G946, 1993[Abstract/Free Full Text].

4. Bridges, CC, Kekuda R, Wang H, Prasad P, Mehta P, Huang W, Smith SB, and Ganapathy V. Structure, function and regulation of human cystine/glutamate transporter in retinal pigment epithelial cells. Invest Ophthalmol Vis Sci 42: 47-54, 2001[Abstract/Free Full Text].

5. Burg, MB, and Kador PF. Sorbitol, osmoregulation, and the complications of diabetes. J Clin Invest 81: 635-640, 1988.

6. Chancy, CD, Kekuda R, Huang W, Prasad PD, Kuhnel J-M, Sirotnak FM, Roon P, Ganapathy V, and Smith SB. Expression and differential polarization of the reduced-folate transporter-1 and the folate receptor $alpha$ in mammalian retinal pigment epithelium. J Biol Chem 275: 20676-20684, 2000[Abstract/Free Full Text].

7. Davidson, AN, and Kaczmarek LN. Taurine a possible neurotransmitter? Nature 234: 107-108, 1971[Medline].

8. Do Carmo, A, Lopes C, Santos M, Proenca R, Cunha-Vaz J, and Carvalho AP. Nitric oxide synthase activity and L-arginine metabolism in the retinas from streptozotocin-induced diabetic rats. Gen Pharmacol 3: 319-324, 1998.

9. Dunn, KC, Aotaki-Keen AE, Putkey FR, and Hjelmeland LM. ARPE-19, a human retinal pigment epithelial cell line with differentiated properties. Exp Eye Res 62: 155-169, 1996[ISI][Medline].

10. Dunn, KC, Marmorstein AD, Bonilha VL, Rodriguez-Boulan E, Giordano F, and Hjelmeland LM. Use of the ARPE-19 cell line as a model of RPE polarity: basolateral secretion of FGF5. Invest Ophthalmol Vis Sci 39: 2744-2749, 1998[Abstract/Free Full Text].

11. Finnemann, SC, Bonilha VL, Marmorstein AD, and Rodriguez-Boulan E. Phagocytosis of rod outer segments by retinal pigment epithelial cells requires $alpha$ _v $beta$ ₅ integrin for binding but not for internalization. Proc Natl Acad Sci USA 94: 12932-12937, 1997[Abstract/Free Full Text].

12. Franks, WA, Limb GA, Stanford MR, Ogilvie J, Wolstencroft RA, Chignell AH, and Dumonde DC. Cytokines in human intraocular inflammation. Curr Eye Res 11 Suppl: 187-191, 1992.

13. Ganapathy, V, Ramamoorthy JD, Del Monte MA, Leibach FH, and Ramamoorthy S. Cyclic AMP-dependent up-regulation of the taurine transporter in a human retinal pigment epithelial cell line. Curr Eye Res 14: 843-850, 1995[ISI][Medline].

14. Goldstein, IM, Ostwald P, and Roth S. Nitric oxide: a review of its role in retinal function and disease. Vision Res 36: 2979-2994, 1996[ISI][Medline].

15. Goto, H, Wu GS, Chen F, Kristeva M, Sevanian A, and Rao NA. Lipid peroxidation in experimental uveitis: sequential studies. Curr Eye Res 11: 489-499, 1992[ISI][Medline].

16. Goureau, O, Hicks D, Courtois Y, and de Kozak Y. Induction and regulation of nitric oxide synthase in retinal Müller glial cells. J Neurochem 63: 310-317, 1994[ISI][Medline].

17. Greenberg, ME, and Bender TP. Identification of newly transcribed RNA. In: Current Protocols in Molecular Biology. New York: Wiley, 1997, sect. 4.10.1-4.10.11.

18. Greenberg, ME, and Ziff EB. Stimulation of 3T3 cells induces transcription of the c-fos protooncogene. Nature 311: 433-438, 1984[Medline].

19. Han, X, Budreau AM, and Chesney RW. Adaptive regulation of MDCK cell taurine transporter (pNCT)mRNA: transcription of pNCT gene is regulated by external taurine concentration. Biochim Biophys Acta 1351: 296-304, 1997[Medline].

20. Hayes, KC, Carey RE, and Schmidt SY. Retinal degeneration associated with taurine deficiency in the cat. Science 188: 949-951, 1975[Abstract/Free Full Text].

21. Heath, H, Brigden WD, Canever JV, Pollock J, Hunter PR, Kelsey J, and Bloom A. Platelet adhesiveness and aggregation in relation to diabetic retinopathy. Diabetologia 7: 308-315, 1971[ISI][Medline].

22. Hood, JD, Meininger CJ, Ziche M, and Granger HJ. VEGF upregulates ecNOS message, protein, and NO production in human endothelial cells. Am J Physiol Heart Circ Physiol 274: H1054-H1058, 1998[Abstract/Free Full Text].

23. Huxtable, RJ. From heart to hypothesis: a mechanism for the calcium modulatory actions of taurine. In: The Biology of Taurine: Methods and Mechanisms, , edited by Huxtable RJ, Franconi F, and Giotti A.. New York: Plenum, 1987, p. 371-388.

24. Ito, T, Nakano M, Yamamoto Y, Hiramitsu T, and Mizuno Y. Hemoglobin-induced lipid peroxidation in the retina: a possible mechanism for macular degeneration. Arch Biochem Biophys 316: 864-872, 1995[ISI][Medline].

25. Jhaing, SM, Fithian L, Smanik P, McGill J, Tong Q, and Mazzaferri EL. Cloning of the human taurine transporter and characterization of taurine uptake in thyroid cells. FEBS Lett 318: 139-144, 1993[ISI][Medline].

26. Jones, DP, Miller LA, Dowling C, and Chesney RW. Regulation of taurine transporter activity in LLC-PK1 cells: role of protein synthesis and protein kinase C activation. J Am Soc Nephrol 2: 1021-1029, 1991[Abstract].

27. Kennedy, AJ, and Voaden MJ. Free amino acids in the photoreceptor cells of the frog retina. J Neurochem 23: 1093-1095, 1974[ISI][Medline].

28. Keys, SA, and Zimmerman WF. Antioxidant activity of retinol, glutathione, and taurine in bovine photoreceptor cell membranes. Exp Eye Res 68: 693-702, 1999[ISI][Medline].

29. Komers, R, Allen TJ, and Cooper ME. Role of endothelium-derived nitric oxide in the pathogenesis of renal hemodynamic changes of experimental diabetes. Diabetes 43: 1190-1197, 1994[Abstract].

30. Leibach, JW, Cool DR, Del Monte MA, Ganapathy V, Leibach FH, and Miyamoto Y. Properties of taurine transport in a human retinal pigment epithelial cell line. Curr Eye Res 12: 29-36, 1993[ISI][Medline].

31. Li, Y-P, and Lombardini JB. Inhibition by taurine of the phosphorylation of specific synaptosomal proteins in the rat cortex: effects of taurine on the stimulation of calcium uptake in the mitochondria and inhibition of phosphoinositide turnover. Brain Res 553: 89-96, 1991[ISI][Medline].

32. Miller, SS, and Steinberg RH. Potassium modulation of taurine transport across the frog retinal pigment epithelium. J Gen Physiol 74: 237-259, 1979[Abstract/Free Full Text].

33. Miyamoto, Y, Kulanthaivel P, Leibach FH, and Ganapathy V. Taurine uptake in apical membrane vesicles from the bovine retinal pigment epithelium. Invest Ophthalmol Vis Sci 32: 2542-2551, 1991[Abstract/Free Full Text].

34. Neuringer, M, and Sturman J. Visual acuity loss in rhesus monkey infants fed a taurine-free human infant formula. J Neurosci Res 18: 597-601, 1987[ISI][Medline].

35. Orr, HT, Cohen AI, and Lowry OH. The distribution of taurine in the vertebrate retina. J Neurochem 26: 609-611, 1976[ISI][Medline].

36. Pasantes-Morales, H. Current concepts on the role of taurine in the retina. Prog Retinal Res 5: 207-229, 1986.

37. Pasantes-Morales, H, and Cruz C. Protective effect of taurine and zinc on peroxidation-induced damage in photoreceptor outer segments. J Neurosci Res 11: 303-311, 1984[ISI][Medline].

38. Pasantes-Morales, H, Klethi J, Ledig M, and Mandel P. Free amino acids of chicken and rat retina. Brain Res 41: 494-497, 1972[ISI][Medline].

39. Pasantes-Morales, H, Ochoa de la Paz LD, Sepulveda J, and Quesada O. Amino acids as osmolytes in the retina. Neurochem Res 24: 1339-1346, 1999[ISI][Medline].

40. Ramamoorthy, S, Del Monte MA, Leibach FH, and Ganapathy V. Molecular identity and calmodulin-mediated regulation of the taurine transporter in a human retinal pigment epithelial cell line. Curr Eye Res 13: 523-529, 1994[ISI][Medline].

41. Ramamoorthy, S, Leibach FH, Mahesh VB, Han H, Yang-Feng T, Blakely RD, and Ganapathy V. Functional characterization and chromosomal localization of a cloned taurine transporter from human placenta. Biochem J 300: 893-900, 1994.

42. Schmetterer, L, Findl O, Fasching P, Ferber W, Strenn K, Breiteneder H, Adam H, Eichler HG, and Wolzt M. Nitric oxide and ocular blood flow in patients with IDDM. Diabetes 46: 653-658, 1997[Abstract].

43. Smith, KE, Borden LA, Wang CH, Hartig PR, Branchek TA, and Weinshank RL. Cloning and expression of a high-affinity taurine transporter from rat brain. Mol Pharmacol 42: 563-569, 1992[Abstract].

44. Smith, SB, Huang W, Chancy C, and Ganapathy V. Regulation of the reduced folate transporter by nitric oxide in cultured human retinal pigment epithelial cells. Biochem Biophys Res Commun 257: 279-283, 1999[ISI][Medline].

45. Sparrow, JR, Nathan CF, and Vodovotz Y. Cytokine regulation of nitric oxide synthase in mouse retinal pigment epithelial cells in culture. Exp Eye Res 59: 129-139, 1994[ISI][Medline].

46. Stevens, MJ, Henry DN, Thomas TP, Killen PD, and Greene DA. Aldose reductase gene expression and osmotic dysregulation in cultured human retinal pigment epithelial cells. Am J Physiol Endocrinol Metab 265: E428-E438, 1993[Abstract/Free Full Text].

47. Stevens, MJ, Hosaka Y, Masterson JA, Jones SM, Thomas TP, and Larkin DD. Downregulation of the human taurine transporter by glucose in cultured retinal pigment epithelial cells. Am J Physiol Endocrinol Metab 277: E760-E771, 1999[Abstract/Free Full Text].

48. Tilton, RG, Chang K, Hasan KS, Smith SR, Petrash JM, Misko TP, Moore WM, Currie MG, Corbett JA, and McDaniel ML. Prevention of diabetic vascular dysfunction by guanidines. Inhibition of nitric oxide synthase versus advanced glycation end-product formation. Diabetes 42: 221-232, 1993[Abstract].

49. Tokunaga, K, Nakamura Y, Sakata K, Fujimori K, Ohkubo M, Sawada K, and Sakiyama S. Enhanced expression of a glyceraldehyde-3-phosphate dehydrogenase gene in human lung cancers. Cancer Res 47: 5616-5619, 1987[Abstract/Free Full Text].

50. Uchida, S, Moo Kwon HM, Preston AS, and Handler JS. Taurine behaves as an osmolyte in MDCK cells: protection by polarized, regulated transport of taurine. J Clin Invest 88: 656-662, 1991.

51. Uchida, S, Moo Kwon H, Yamauchi A, Preston AS, Marumo F, and Handler JS. Molecular cloning of the cDNA for an MDCK cell Na⁺- and Cl-dependent taurine transporter that is regulated by hypertonicity. Proc Natl Acad Sci USA 89: 8230-8234, 1992[Abstract/Free Full Text].

52. Van der Zee, R, Murohara T, Luo Z, Zollmann F, Passeri J, Lekutat C, and I