Novel Role of Vitamin K in Preventing Oxidative Injury to Developing Oligodendrocytes and Neurons

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The Journal of Neuroscience, July 2, 2003, 23(13):5816-5826

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Novel Role of Vitamin K in Preventing Oxidative Injury to Developing Oligodendrocytes and Neurons
Jianrong Li,¹ Judith C. Lin,² Hong Wang,¹ James W. Peterson,³ Barbara C. Furie,² Bruce Furie,² Sara L. Booth,³ Joseph J. Volpe,¹ and Paul A. Rosenberg¹
¹Department of Neurology, Division of Neuroscience, Children's Hospital, and ²Center for Hemostasis and Thrombosis Research, Beth Israel Deaconess Medical Center, Harvard Medical School, Boston, Massachusetts 02115, and ³Department of Agriculture Human Nutrition Research Center on Aging, Tufts University, Boston, Massachusetts 02111

   Abstract

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Abstract
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Materials and Methods
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Discussion
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Oxidative stress is believed to be the cause of cell death inmultiple disorders of the brain, including perinatal hypoxia/ischemia.Glutamate, cystine deprivation, homocysteic acid, and the glutathionesynthesis inhibitor buthionine sulfoximine all cause oxidativeinjury to immature neurons and oligodendrocytes by depletingintracellular glutathione. Although vitamin K is not a classicalantioxidant, we report here the novel finding that vitamin K₁ and K₂ (menaquinone-4) potently inhibit glutathione depletion-mediatedoxidative cell death in primary cultures of oligodendrocyte precursors and immature fetal cortical neurons with EC₅₀ valuesof 30 nM and 2 nM, respectively. The mechanism by which vitaminK blocks oxidative injury is independent of its only known biological function as a cofactor for ${gamma}$ -glutamylcarboxylase, an enzyme responsible for posttranslational modification of specific proteins. Neither oligodendrocytes nor neurons possess significant vitamin K-dependent carboxylase or epoxidase activity. Furthermore, the vitaminK antagonists warfarin and dicoumarol and the direct carboxylaseinhibitor 2-chloro-vitamin K₁ have no effect on the protectivefunction of vitamin K against oxidative injury. Vitamin K doesnot prevent the depletion of intracellular glutathione causedby cystine deprivation but completely blocks free radical accumulationand cell death. The protective and potent efficacy of this naturally occurring vitamin, with no established clinical sideeffects, suggests a potential therapeutic application in preventingoxidative damage to undifferentiated oligodendrocytes in perinatalhypoxic/ischemic brain injury.

Key words: glutathione depletion; oxidative stress; cell death; vitamin K; neuron; oligodendrocyte; white matter; cystine deprivation; menaquinone-4; cerebral palsy

   Introduction

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Oxidative mechanisms of injury are important in many neurological disorders, including cerebral damage caused by ischemia/reperfusion. Hypoxic/ischemic injury to the developing brain is a major neurological disorder in the perinatal period. Neurological deficits in survivorsinclude mental retardation, seizures, and cerebral palsy. Theneuropathology of perinatal hypoxic/ischemic brain injury iscomplex and differentially involves gray and white matter regions,depending on the type and extent of the injury, the age ofthe infant, and the developmental stage of cerebral vascularity (Kinney and Armstrong, 1997). In the premature infant, thecerebral white matter is particularly susceptible to ischemicinjury, resulting in periventricular leukomalacia (PVL) and cerebral palsy, i.e., preferential damage to the cerebral whitematter that is mainly populated at that age with premyelinatingoligodendrocytes (OLs) (Volpe 1997, 2001; Back et al., 2001).We demonstrated previously that these premyelinating OLs aremore sensitive to oxidative damage than are mature, myelinatingcells (Back et al., 1998). There is now emerging evidencesuggesting that oxidative stress plays a key role in the pathogenesisof PVL (Haynes et al., 2003).
Glutathione (GSH) depletion is widely used as a cellular modelof oxidative stress (Murphy et al., 1989, 1990; Kane et al.,1993; Ratan et al., 1994). Reduced GSH is the major intracellularantioxidant and plays a pivotal role in maintaining cellularredox homeostasis. Depletion of GSH results in a time-dependentaccumulation of endogenous reactive oxygen species (ROS) and subsequent oxidative stress. GSH depletion is the underlyingmechanism by which glutamate induces receptor-independent celldeath in neurons and OLs (Murphy et al., 1989, 1990; Okaet al., 1993). Glutamate promotes cystine efflux or competitivelyblocks cystine uptake via an exchanger/antiporter, resultingin loss of intracellular cystine and GSH. Similarly, cystine-freeculture medium, or the GSH synthesis inhibitor buthionine sulfoximine(BSO), results in loss of GSH and oxidative cell death (Yonezawaet al., 1996; Back et al., 1998). A decrease in tissue GSHconcentration has been demonstrated after in vivo ischemia/hypoxia(Orwar et al., 1994; Shivakumar et al., 1995; Wallin et al., 2000) and excitotoxicity (Floreani et al., 1997). Furthermore,a GSH prodrug, YM737, provides protection against cerebral ischemia in rats (Yamamoto et al., 1993).
Our finding of the protective effect of vitamin K against oxidativestress induced by GSH depletion was made serendipitously inthe course of our investigation into the mechanism of celldeath. Vitamin K is a family of fat-soluble vitamins composedof a naphthoquinone with isoprenylacyl side chains of varyinglengths and is required for proper synthesis of vitamin K-dependentproteins involved in blood coagulation and bone metabolism (Suttie, 1991; Furie et al., 1999). It is a cofactor for asingle known enzyme, ${gamma}$ -glutamylcarboxylase, that catalyzes theposttranslational conversion of glutamic acid to ${gamma}$ -carboxyglutamicacid (Gla) in vitamin K-dependent proteins. The enzyme is alsoan epoxidase converting vitamin K to vitamin K epoxide during formation of Gla. The carboxylase is expressed in the CNS during embryogenesis, even before its expression in the liver, thesite for production of many vitamin K-dependent proteins (Romeroet al., 1998). The physiological roles of vitamin K and thecarboxylase in the CNS are not characterized. It is well knownthat vitamin K is developmentally deficient in neonates, especiallyin preterm infants whose risk for PVL is especially high. VitaminK status is important in the maintenance of normal biosynthesisof lipid sulfatide, an important component of CNS myelin, inyoung animals (Sundaram et al., 1996). Moreover, exposureto the vitamin K antagonist warfarin in utero causes CNS malformationsand mental retardation (Hall et al., 1980). These observationssuggest a possible unidentified role of vitamin K in the developingbrain. In this study, we report the discovery of a novel andpotent protective action of vitamin K in preventing oxidativeinjury to primary OL precursors and to immature cortical neuronsthat appears to be independent of the current known functionof vitamin K.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Materials. DMEM, HBSS, Earle's balanced salt solution (EBSS),FBS, penicillin, and streptomycin were purchased from LifeTechnologies, Inc. Antibody against polyADP-ribose was obtainedfrom Chemicon International Inc. (Temecula, CA). 2-Chloro-vitaminK₁ was a generous gift from Dr. John W. Suttie (Universityof Wisconsin, Madison, WI). Primary rat hepatocytes were obtainedfrom Dr. Timothy R. Billiar (University of Pittsburgh, Pittsburgh,PA). Unless otherwise specified, all other chemicals were from Sigma (St. Louis, MO).
OL cultures. Primary rat OLs were prepared from the cerebral hemispheres of Sprague Dawley rats at postnatal days 1–2using a shaking method as described with modifications (McCarthyand de Vellis, 1980; Oka et al., 1993). Briefly, forebrainsfree of meninges were chopped into 1 mm ³ blocks and placedinto HBSS containing 0.01% trypsin and 10 µg/ml DNase.After digestion for 15 min at 37°C, the tissue was collectedby centrifugation and triturated with the plating medium DMEM20Scontaining DMEM, 20% FBS, and 1% penicillin-streptomycin, andpassed through a 70 µm sieve. Cells were plated ontopoly-D-lysine-coated 75 cm ² flasks at a density of 1 pup brainper flask. Cultures were fed with fresh DMEM20S medium everyother day for 10–11 d at 37°C in a humid atmosphereof 5% CO₂ and 95% air.
To isolate OLs, the co-culture flasks were shaken for 1 hr at200 rpm at 37°C to remove adherent microglia/macrophages,and the cultures were washed with the same medium and subjectedto shaking at 200 rpm overnight (18–22 hr) to separateOLs from the astrocyte layer. The suspension was plated ontouncoated Petri dishes and incubated for 1 hr at 37°C to further remove residual microglia and astrocytes that adhereto the dishes. The OLs were then collected by passing througha 15 µm sieve and centrifuged. Isolated OLs were platedonto poly-ornithine (50 µg/ml)-coated culture plates,i.e., 96-well plates (at a density of 3.3 x 10 ³ cell/well,for cell survival assay), 24-well plates with glass coverslips(1.74 x 10 ⁴ cell/well, for imaging), and 60 mm plates (2.75x 10 ⁵ cell/plate, for enzyme assay). Purified OLs were culturedfor 7–9 d in a serum-free basal-defined medium (BDM; DMEM containing 0.1% BSA, 50 µg/ml apo-transferrin, 50µg/ml insulin, 30 nM sodium selenite, 10 nM D-biotin,10 nM hydrocortisone, 200 µM L-cystine, 10 ng/ml PDGF,and 10 ng/ml basic FGF). At 7–9 d, the OL cultures, primarilycomposed of progenitors and pre-OLs [A₂B₅ ⁺,O₄ ⁺, myelin basicprotein ^- (MBP ^-)] but not mature OLs (MBP ⁺), were used inthis study. The purity of OL cultures was consistently >95%OLs with <1% astrocyte contamination.
Oxidative stress in cell cultures. To induce oxidative stress, unless specified otherwise, BDM medium without cystine (Cys^-) was used. Vitamin K₁ and menaqunone-4 were made fresh inanhydrous DMSO as a 1000x working solution. The final concentrationof DMSO in culture medium was 0.1%, and had no effect on cellviability, proliferation, or morphology. The final concentrationof vitamin K was as indicated. When glutamate toxicity wasexamined, the concentration of cystine in the culture mediumwas 20 µM instead of the normal 200 µM, becauseprevious results showed that glutamate toxicity inversely correlates with the concentration of cystine in the culture medium (Murphyet al., 1989; Oka et al., 1993). BDM containing 20 µMcystine was not toxic to OL precursors.
Neuronal cultures. Primary embryonic cortical neurons from E14rat cerebral hemispheres were isolated and cultured accordingto a method described previously (Wang et al., 1998). Theneurons were plated in poly-D-lysine-coated 96-well cultureplates at a density of 2.4 x 10 ⁴ cells/well and used after24–48 hr of plating.
Cell survival assay. Cell survival was determined after treatment for 22–24 hr using Alamar Blue (Southern Biotech, Birmingham,AL), a tetrazolium dye that is reduced by living cells to acolored product. This assay is similar in principle to theMTT cell viability assay and has been previously validatedas an accurate measure of survival of OLs in our culture system(Back et al., 1999). All results of cell death assays werealso confirmed by visual inspection under a light microscope.Briefly, culture medium in the 96-well plate was aspirated, and cells were incubated with 200 µl of assay solutionprepared by diluting 100x stock solution of Alamar Blue intoEBSS for 2 hr at 37°C. The fluorescence of the assay solution,reflecting cell viability, was measured with a fluorescenceplate reader (FluoroCount; Packard Instrument Co., Meridian,CT) using an excitation wavelength of 560 nm and an emission wavelength of 590 nm. All survival assays were performed intriplicate, and cell viability was expressed as mean ±SD. Intracellular GSH levels were determined by a colorimetricmethod as described previously (Back et al., 1998).
Intracellular free radical accumulation measurement. Intracellular free radical generation was evaluated with dichlorohydrofluorescindiacetate (DCFH-DA) and dihydrorhodamine 123 (Rho123; Molecular Probes,Eugene, OR) (LeBel et al., 1992; Wang and Joseph,1999). DCFH-DA and Rho123 were prepared as 100 mM and 10 mM stocks, respectively, in dimethyl sulfoxide and stored in thedark at -20°C. After cells were treated for 10–15hr, DCFH-DA (100 µM) or dihydrorhodamine (10 µM)was added directly to the cells and incubated with the cellsfor 20 min at 37°C. The extracellular DCFH-DA or dihydrorhodaminewas then removed by washing the cells twice with EBSS. Thefluorescence of the cells loaded with DCFH-DA was measuredusing a multiwell fluorescence plate reader (excitation ${lambda}$ = 485 nm; emission ${lambda}$ = 530 nm). For fluorescent imaging of oxidized Rho123, the oxidized form of dihydrorhodamine, cells were immediately visualized using a digital fluorescent microscope equipped witha 40x oil immersion objective. Cells were visualized by excitationat 490 nm and emission at 515 nm. For all images, the microscopesettings, such as brightness, contrast, and exposure time wereheld constant to compare the relative intensity of oxidizedRho123 across all treatment conditions.
Antioxidant activity assay. Antioxidant activity of various reagents was assayed with two different methods. In the firstmethod, we monitored at 517 nm the disappearance of the opticalabsorbance of stable-free radical 1,1-diphenyl-2-picrylhydrazyl(DPPH) on reaction with test compounds (Blois, 1958). The rateof the reaction represents the antioxidant potency of testagents. The known free radical scavenger Trolox was used asa positive control. Briefly, 10 µl of test reagents atindicated final concentrations were added to 300 µl of100 µM DPPH. Optical absorbance of DPPH at 517 nm wasimmediately monitored for 5 min. In the second method, we determinedTrolox equivalent activity concentration of the test agentsaccording to the method of Rice-Evans and Miller (1994). Theinhibition of the absorbance of the radical cation formationof 2,2'-azinobis (3-ethylbenzothiazoline 6-sulfonate) (ABTS ^+·) was monitored continuously for 30 min at 660 nm inPBS containing 150 µM ABTS, 2.5 µM metmyoglobin,75 µM H₂O₂, and the indicated concentration of testreagent.
Immunocytochemistry and immunofluorescence microscopy. Cellswere fixed with 4% paraformaldehyde in PBS for 10 min at roomtemperature, washed three times with PBS, and blocked withTBST (50 mM Tris-HCl, pH 7.4, 150 mM NaCl, and 0.1% TritonX-100) containing 5% goat serum for 1 hr at room temperature.The coverslips were incubated with mouse monoclonal antibodiesA₂B₅ (1:100 dilution; American Type Culture Collection, Manassas,VA), O₄, O₁ (1:100 dilution; gifts from Dr. Steven E. Pfeiffer,University of Connecticut Health Center, Farmington, CT), MBP(1:500 dilution; Boehringer Mannheim, Indianapolis, IN), CD11(1:100), or glial fibrillary acidic protein GFAP (1:4000) for1 hr. After three to four washes at 5 min each, the appropriate secondary antibody conjugated with either fluorescein or OregonGreen (Molecular Probes Inc.) was added to the coverslips andincubated for 1 hr. After extensive washes with TBST, nucleiwere stained by adding Hoechst 33258 at a final concentrationof 2 µg/ml for 1 min. After three more washes, the coverslipswere mounted onto glass slides with FluoroMount and kept inthe dark at 4°C. Cell images were captured with a fluorescencemicroscope (Nikon Eclipse E800) equipped with a Spot RT digitalcamera (Diagnostic Instruments, Inc.).
Cell homogenization and solubilization of microsomal proteins. Three to 5 x 10 ⁷ OL precursors or primary rat hepatocytes (Li et al., 1999) were first rinsed with cold PBS and scrapedinto buffer A (PBS, 20% glycerol, and 1x protease inhibitormixture) (Furie et al., 1997). Microsomes were isolated byhomogenization and differential ultracentrifugation, and microsomalproteins were extracted with buffer A supplemented with 0.5% 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS)and 0.2% phosphatidylcholine, as described previously (Furieet al., 1997). Protein concentration was measured using thelipid- and detergent-compatible Dc protein assay (Bio-Rad,Hercules, CA) with BSA as standard.
${gamma}$ -Glutamylcarboxylase and vitamin K epoxidase assay. Vitamin K-dependent carboxylase activity of the microsomal protein preparationswas evaluated by measuring vitamin K-dependent incorporationof ¹⁴CO₂ into the synthetic peptide substrate FLEEL over 30 min at 25°C (Ulrich et al., 1988). Purified recombinantFlag-tagged bovine carboxylase was used as a standard, as describedpreviously (Furie et al., 1997). The assay mixture (125 µl)contained 25 mM 3-(N-morpholino)propanesulfonic acid, pH 7.0,0.5 mM NaCl, 0.16% CHAPS, 0.16% phosphatidylcholine, 8 mM dithiothreitol,222 µM chemically reduced vitamin K₁ (Abbott Laboratories,North Chicago, IL), and 1.4 mM NaH ¹⁴CO₃ (10 µCi; Amersham).The reaction was initiated by adding the reaction mixture tomicrosomal preparation or recombinant carboxylase. ¹⁴CO₂ incorporationin the absence of vitamin K was considered background and wassubtracted. Inhibition of recombinant carboxylase by 2-Cl-vitmainK₁ was determined using increasing the molar ratio of 2-Cl-vitaminK₁ over the cofactor vitamin K₁ in the assay mixture.
Vitamin K epoxidase activity was determined as described previously (Sugiura et al., 1997). For assay of vitamin K epoxide, NaH¹⁴CO₃ was replaced by NaHCO₃. On completion of the carboxylasereaction, the reaction mixture was extracted with 250 µlof ethanol and then with 750 µl of hexane. The organicand aqueous phases were separated by centrifugation at 1000x g for 10 min. The organic phase was removed, and the solventwas evaporated to dryness. The residue was redissolved in 200µl of methanol. Half of this solution was injected ontoa reverse-phase C18 HPLC column (Hypersil ODS; 5 µm;4.6 x 250 mm; Custom LC, Houston, TX) using a Beckman model126 HPLC equipped with a Beckman model 168 diode array detector.The column was developed with a mobile phase of 10% dichloromethane/90%methanol that had been saturated with nitrogen. Vitamin K derivativeswere detected at 226 nm, and vitamin K epoxide was quantitated using a purified synthetic standard of 2,3-vitamin K₁ epoxide.The identity of vitamin K epoxide in the HPLC fraction wasfurther confirmed by mass spectroscopy.

   Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Characterization of primary OLs in culture
OLs differentiate along a specific lineage, progressing throughfour stages recognized by specific antibodies: progenitors (A₂B₅⁺ or NG₂⁺), pre-OLs (O₄⁺), immature OLs (O₁⁺), and matureOLs (MBP⁺) (Pfeiffer et al., 1993). Each developmental stagepossesses a characteristic morphology. Primary OL culturesused in this study were grown for 7–9 d in vitro. Themajority of cells were OL progenitors (A₂B₅⁺) and pre-OLs (A₂B₅⁺, O₄⁺). Immunocytochemical characterization confirmedthat the majority of OLs in our cultures were positive forthe surface markers recognized by the monoclonal antibodiesA₂B₅ and O₄ and were negative for O₁ (Fig. 1). There wereonly a few mature, differentiated OLs expressing MBP. TheseOLs (A₂B₅ ⁺, O₄ ⁺, MBP ^-) are referred to as OL precursorsin this study. Contamination by astrocytes (GFAP ⁺) and microglia(CD11 ⁺) was <2% (Fig. 1).

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Figure 1. Characterization of primary OL cultures.A,Representative microphotographs of morphology and immunocytochemistry of cells (7–9 d in vitro) labeled with indicated antibodies. B, Composition of developing OL cultures as determined by immunostaining for indicated markers. Total cell number was determined by counting all cells labeled with the nuclei dye Hoechst 33258. Values represent mean ± SEM from three separate experiments.

Vitamin K₁ and menaquinone (MK)-4 protect against cystine depletion-inducedoxidative death to OL precursors
Our discovery of a protective effect of vitamin K against oxidative stress-induced cell death was made serendipitously as follows.Previously, we showed that OL precursors undergo oxidativestress-induced cell death after GSH depletion caused by removalof cystine from the culture medium (Yonezawa et al., 1996; Back et al., 1998). In pursuing the mechanism of the cell deathin this model, we initially hypothesized that activation ofpoly(ADP-ribose) polymerase (PARP) is involved in the toxicity, because it is known that free radicals can cause extensive DNA-strandbreakage and activation of the DNA repair enzyme PARP. Activationof this enzyme, however, also results in ATP depletion, energyfailure, and cell death (Szabo and Dawson, 1998). We found,however, that the known PARP inhibitors, 3-methoxybenzamideand 3-aminobenzamide, did not protect against OL death inducedby cystine depletion (data not shown), indicating that PARPactivation is not involved in this model. Consistent with thisresult, polyADP-riboslyation of multiple proteins was not observedby Western blotting analysis with antibody against polyADP-ribose(data not shown), nor was cellular ATP depletion observed beforecell lysis (data not shown). In addition to PARP inhibitors,we tested in parallel the effect of inhibitors of mono-ADP-ribosyltransferase(MART), activation of which has not been linked to energy failure.Unexpectedly, we found complete protection with the MART inhibitors (Banasik et al., 1992), vitamin K₁ (phylloquinone), and vitaminK₂ (MK-4). Cystine deprivation for 18–20 hr caused completecell death in cultures (Fig. 2B). In the presence of 0.1 µMvitamin K₁ or MK-4, however, the cell death was completelyprevented (Fig. 1A, B). Interestingly, other known MART inhibitors,such as novobiocin, stearic acid, palmitic acid, coumermycin,and m-iodobenzylguanidine, had no or limited protective effecton cystine depletion-induced cell death and were associatedwith cytotoxicity at high concentrations (Fig. 2A).

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Figure 2. Vitamin K protected against cystine deprivation-induced OL death independent of MART. A, Effects of various MART inhibitors on cystine depletion-induced OL death. OLs were subjected to either normal medium (Cys ⁺) or cystine-free medium (Cys ^-) in the presence of indicated concentrations of various MART inhibitors. Cell viability was evaluated after 24 hr. Results are representative of four independent experiments. B, Phase contrast photomicrographs of OLs exposed to normal or cystine-depleted medium with or without 0.1µM vitamin K₁ or MK-4 for 18 hr. Magnification, 400x. Data are representative of at least 10 separate experiments. C, Vitamin K prevented OL death in a concentration-dependent manner. Cell viability was assayed 24 hr after cystine deprivation in the presence of increasing concentrations of K₁ and MK-4. Values are mean ± SEM of six separate experiments.

We next examined the concentration dependence of the protectiveeffect of vitamin K₁ and MK-4. Surprisingly, vitamin K completelyabolished cystine depletion-mediated OL death at remarkablylow concentrations with EC₅₀ ${approx}$ 30 nM and 2 nM for K₁ and MK-4,respectively (Fig. 2C). These EC₅₀ values for protecting OLswere much lower than their IC₅₀ for inhibiting MART (i.e.,1.9 µM and 13 µM for K₁ and MK-4, respectively)in vitro (Banasik et al., 1992). Interestingly, the effectiveconcentrations obtained in this cell death model are closeto the normal adult human serum vitamin K levels (2.9 ±1.4 nM) (Mummah-Schendel and Suttie, 1986). The order of potencyof K₁ and MK-4 to protect OLs against cystine deprivation wasopposite to their order of potency to inhibit MART. Therefore,these results suggest that vitamin K exerts its protectiveeffect by a mechanism other than MART inhibition in these cultures.
Vitamin K₁ and MK-4 prevent GSH depletion-induced oxidative death to both primary OLs and immature neurons
Methods other than cystine depletion are often used to induceintracellular GSH depletion, and it was of interest to testwhether vitamin K₁ and MK-4 could prevent oxidative toxicityin these models. Glutamate has been shown to cause oxidativetoxicity in immature cortical neurons and OLs by decreasingintracellular cystine and, thus, GSH (Murphy et al., 1989, 1990; Oka et al., 1993). Consistent with our previous observations(Oka et al., 1993), OLs exposed to glutamate underwent celldeath (Fig. 3A). This toxicity of glutamate was completelyprevented by 0.1 µM vitamin K₁ or 0.1 µM MK-4 (Fig. 3A). Similarly, blocking GSH biosynthesis with 1 mM BSO,an inhibitor for the rate-limiting enzyme ${gamma}$ -glutamylcysteinesynthetase, induced oxidative cell death that also was completelyblocked by vitamin K₁ or MK-4 (Fig. 3A). The protective effectof vitamin K₁ and MK-4 on oxidative cell death was not specificto OLs, because their presence also completely inhibited glutamate-inducedneuronal death (Fig. 3B). In addition, we found that vitaminK₁ and MK-4 also blocked homocysteic acid- and BSO-inducedneuron degeneration (Fig. 3B).

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Figure 3. Vitamin K₁ and MK-4 protected both OL precursors and neurons from cell death induced by various GSH depletion methods. A, Vitamin K prevented OL cell death induced by cystine depletion, by glutamate (5 mM), and by BSO (1 mM). B, Vitamin K₁ and MK-4 prevented immaturecorticalneuronaldeathinducedbyhomocysteicacid(HA,2.5mM),glutamate(5mM), or BSO (1 mM). Primary cells were incubated with indicated agents for 24 hr in the presence or absence of K₁ (0.1µM) or MK-4 (0.1µM), and cell viability was analyzed after 24 hr. Results are mean ± SEM of three separate experiments. C, Effect of vitamin K₁ and MK-4 on H₂O₂-induced toxicity. OL precursors were incubated with or without 800µM H₂O₂ in the presence of indicated concentrations of vitamin K for 15 hr, and cell viability was evaluated. Data are representative of at least four independent experiments with similar results.

Taken together, these data demonstrate that both vitamin K₁and MK-4 are potent inhibitors of oxidative cell death inducedby GSH depletion in primary OL precursor cultures and in neuronalcultures. In addition to GSH depletion-mediated cell death,we also examined the effect of vitamin K on exogenous oxidantH₂O₂-induced cell death. At concentrations ranging from 0.01µM to 200 µM, vitamin K₁ and MK-4 did not prevent H₂O₂-induced OL death (Fig. 3C). They also did not block kainate-,menadione-, or nitric oxide-induced cytotoxicity to the OLprecursors (data not shown).
Both the naphthoquinone ring and the 3'-side chain are required for vitamin K protection
There are two naturally occurring forms of vitamin K, phylloquinone (vitamin K₁) and MKs (vitamin K₂) (Fig. 4A). Both K₁ and K₂are characterized by a naphthoquinone ring and an aliphaticside chain. Vitamin K₂ is a series of naphthoquinones withside chains of varying numbers of isoprenoid units (n = 2–13;when n = 4, K₂ is also called MK-4). Although vitamin K₁ isthe predominant form of vitamin K in the liver, heart, andpancreas, MK-4 is the predominant form of vitamin K in the brain (Thijssen et al., 1996) and can be synthesized from vitaminK₁, probably by a cellular enzymatic conversion mechanism thathas yet to be identified (Thijssen et al., 1996; Davidsonet al., 1998). To examine the structural requirements for vitaminK protection in culture, we tested several commercially availablecompounds that share some similarity with K₁ and MK-4 (Fig. 4A). Menadione, also known as vitamin K₃, contains the samenaphthoquinone structure as vitamin K₁ and K₂ but without the3'-side chain. This compound was ineffective in the protectionof OL precursors against cystine deprivation (Fig. 4B) andwas, in fact, quite toxic to OLs at a higher concentration(>2 µM; data not shown). Similar results were obtainedwith immature neurons (data not shown). Another lipophilicvitamin, retinoic acid, that has an aliphatic side chain butlacks the naphthoquinone structure also did not show any protection of OL precursors against cystine deprivation (data not shown).Taken together, these results demonstrate that both the nathphoquinonering structure and the isoprenoid chain are essential for inhibitionof GSH depletion-mediated cell death.

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Figure 4. Structural requirement for vitamin K-dependent protection against cystine depletion-induced cell death. A, Structures of vitamin K₁, K₂, and compounds tested in B for their effects on cystine depletion-induced OL death. B, Effect of various compounds on OL cell death induced by cystine depletion. Representative results of two to three independent experiments are shown. No cytotoxicity to OLs in normal culture medium was seen with the test compounds at the concentration used.

Vitamin K protection against oxidative cell death is independentof vitamin K-dependent ${gamma}$ -glutamylcarboxylase
To explore further the mechanism by which vitamin K₁ and MK-4 protect against oxidative cell injury, we investigated whetherthis protection is mediated by the known mechanism for thebiological actions of vitamin K. As mentioned above, vitaminK is an essential cofactor for ${gamma}$ -glutamylcarboxylase, an enzymethat catalyzes the incorporation of CO₂ into certain glutamicacid residues of about a dozen proteins that are involved inblood coagulation, bone metabolism, and cell growth and survival(Suttie, 1985; Furie et al., 1999). This posttranslationalformation of Gla plays an important biological role in proteinfunction. For example, the highly negatively charged Gla residuesare required for Ca²⁺-dependent phospholipid binding of allcoagulation factors, a requirement for their biological activity.The carboxylase requires the reduced, hydroquinone form (KH₂)of vitamin K as the actual cofactor. In the course of carboxylation,KH₂ is stoichiometrically oxidized by the carboxylase to vitaminK-2, 3-epoxide, which is then reduced by a NADPH-dependent,warfarin-sensitive vitamin K reductase back to the quinone(K) and hydroquinone (KH₂) forms (the so-called vitamin K cycle).During this cycle, KH₂ is continuously regenerated. Blockadeof vitamin K epoxide cycling back to vitamin K by warfarin and dicoumarol analogs prevents efficient carboxylation of vitaminK-dependent proteins and, thus, forms the basis of their actionas anticoagulants.
To test for a role of vitamin K-dependent ${gamma}$ -glutamylcarboxylasein protection from oxidative cell death, the effect of warfarinon the protective function of vitamin K was investigated. Treatmentof OLs with increasing concentrations of warfarin or dicoumaroldid not block the protective effect of vitamin K, suggestingthat regeneration of KH₂ is not required for the observed protectionand that carboxylation may not be involved (Fig. 5A). It is possible, however, that even in the absence of efficient recycling,enough vitamin K is present to generate carboxylation of aprotein(s) that confers protection. Because there is evidencesuggesting the existence of a warfarin-resistant vitamin Kreductase (Suttie, 1985), we next tested the effect of 2-chloro-vitaminK₁ (Cl-K₁), an analog of K₁ and a direct inhibitor of the carboxylasein vitro and in vivo (Lowenthal et al., 1960; Suttie, 1985).Even at over 100-fold excess of K₁, Cl-K₁ did not prevent vitaminK₁ protection against cystine depletion-induced cell death(Fig. 5B). At higher concentrations (140 µM), Cl-K₁became cytotoxic. To prove that Cl-K₁ indeed directly inhibitscarboxylase enzyme activity at the concentrations used in ourcultures, we incubated purified recombinant carboxylase withincreasing molar ratios of Cl-K₁ to vitamin K₁ and determinedthe carboxylase activity. We found that Cl-K₁ is indeed a potent inhibitor of the vitamin K-dependent carboxylase (Fig. 5C).Consistent with the above data, we found no measurable vitaminK-dependent carboxylase activity or epoxidase activity usinga purified microsome preparation from cultured OLs. Primaryadult rat hepatocytes, the major cell type expressing the carboxylase,were used as a positive control in these experiments (Fig.5D, E). Therefore, we conclude that vitamin K blocks GSH depletion-inducedoxidative cell death by a mechanism independent of carboxylation.

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Figure 5. Vitamin K protected OLs via a mechanism independent of vitamin K-dependent ${gamma}$ -glutamylcarboxylase.A,Inhibitors of vitamin K cycling, warfarin and dicoumarol, had no effect on vitamin K protection. OL precursors were induced to undergo cystine depletion-induced cell death in the presence or absence of indicated treatment for 24 hr, and cell viability was assayed. Concentrations used were: vitamin K₁, 0.1µM; MK-4, 0.1µM; warfarin, 500µM; dicoumarol, 200µM. Results are representative of at least two separate experiments. B, Carboxylase inhibitor Cl-K₁ did not reverse vitamin K protection. Cells were treated as indicated with or without Cl-K₁ (0–140 µM) and vitamin K₁ (0.2 µM) for 24 hr, and cell viability was analyzed. C, Cl-K₁ directly inhibited enzymatic activity of purified ${gamma}$ -glutamylcarboxylase in vitro. Purified ${gamma}$ -glutamylcarboxylase was incubated in the presence of increasing concentrations of Cl-K₁ versus K₁ and assayed in duplicates for its enzyme activity. Results are mean ± SEM of three independent experiments. D, E, OL precursors express little, if any, ${gamma}$ -glutamylcarboxylase and vitamin K epoxidase activity. Microsomal proteins were extracted from cultured primary OLs, and vitamin K-dependent carboxylase and epoxidase activity of the microsomal preparation were analyzed. Primary rat hepatocyte microsomal preparation was performed in parallel as positive control for the enzyme assays. Results are representative of two independent experiments.

Persistent presence of MK-4 in culture is not required for itspotent protection
We next asked whether pretreatment of cells with MK-4 wouldrender them resistant to subsequent oxidative insult, becausethis would have potential therapeutic implications in vivo.Both vitamin K₁ and MK-4 were readily uptaken by OLs as determinedby HPLC analysis (data not shown). In experiments in whichcells were treated with 0.1 µM MK-4, washed extensively,and then subjected to cystine deprivation, it was observed that pretreatment with 0.1 µM MK-4 for 1 hr was sufficientto provide complete protection against subsequent cystine depletion-inducedcell death (Fig. 6A). Interestingly, similar pretreatmentwith vitamin K₁ was not effective in preventing subsequentcystine depletion-induced cell death.

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Figure 6. Persistent presence of MK-4 was not required for protection. A, Effect of pretreatment with MK-4 on subsequent cystine depletion-induced cell death. OL precursors were preincubated with or without MK-4 (0.1 µM) for 1 hr in cystine-free medium, followed by wash three times with cystine-free medium, when indicated. Cell viability was determined 24 hr later, and the percentage of cell survival was based on the control in which cells were maintained in normal medium. Results are one representative of three independent experiments with similar results. B, Effect of vitamin K treatment at various time intervals after initiation of cystine depletion. Cells were treated with increasing amounts of K₁ or MK-4 (µM) at the time of cystine depletion or the indicated time after cystine depletion. The total cystine deprivation time is 24 hr, and the cell viability was evaluated. L-Cystine (200 µM) was added back to the cystine-free medium at 8 hr after cystine depletion and was used as a control. Results are representative of three experiments.

To examine the time dependence of the protective action of vitaminK against the cystine depletion-induced cell death pathway,increasing concentrations of vitamin K₁ and MK-4 were addedto OLs at indicated intervals after the initiation of cystinedeprivation, and cell viability was determined after 24 hrof cystine depletion (Fig. 6B). Concentrations as low as 100nM for K₁ or 10 nM for MK-4 were completely protective whenadded at the onset of cystine deprivation (i.e., added at T= 0 hr). Vitamin K₁, however, lost its protective potency whenadded after 6 hr. MK-4 at10 nM was no longer protective ifadded after 6 hr, but MK-4 at 100 nM was still fully protective.MK-4 at 100 nM became only marginally effective when addedafter 8 hr. A higher concentration of MK-4 (1 µM) wasrequired to inhibit cell death when added 8 hr after cystinedepletion. Because it has been found that ROS became detectableonly 10–15 hr after the onset of cystine deprivation(data not shown) (Back et al., 1998), these data suggest thatfor maximal effectiveness vitamin K must be present before the generation of ROS.
Vitamin K and MK-4 do not reverse decreases in intracellularGSH level but completely prevent ROS generation
Accumulation of intracellular oxygen free radicals occurs with intracellular GSH depletion initiated by exposure to glutamate,BSO, homocysteic acid, or cystine depletion of the medium (Murphyet al., 1989, 1990; Back et al., 1998). Thus, we testedwhether vitamin K prevents the ROS accumulation caused by GSH depletion. Accumulation of intracellular ROS was assessed byoxidation of Rho123 or DCFH-DA. Rho123 reacts with oxidantsto form the red fluorescent product rhodamine 123 (Hendersonand Chappell, 1993). DCFH-DA, a cell-permeable, nonfluorescentdye, is deesterified, retained inside cells, and becomes fluorescenton oxidation (Royall and Ischiropoulos, 1993). Vitamin K₁and MK-4 completely inhibited the intracellular accumulationof ROS resulting from cystine deprivation (Fig. 7A, B), without sparing cells from depletion of intracellular GSH (Fig. 7D).Consistent with the hypothesis that vitamin K prevents deathby decreasing the cellular oxidant burden, MK-4 (1 µM)rescued the cells when introduced to cells 8 hr after the onsetof cystine deprivation (Fig. 6B); this rescue was associatedwith a significant decrease in ROS accumulation (Fig. 7C).

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Figure 7. Vitamin K blocked cystine deprivation-induced free radical accumulation. OLs were subjected to Cys ⁺ or Cys ^- medium as indicated, with or without vitamin K₁ or MK-4 for 10–15 hr, and cells were then loaded with DCFH-DA (A) or Rho123 (B), and the free radical production was evaluated as described. Both DCFH-DA and Rho123 are nonfluorescent but become fluorescent on oxidation. DCF fluorescence was measured using a microplate reader, and oxidized Rho123 was visualized under a fluorescence microscope with fixed exposure settings to compare the relative production of ROS among cells with different treatments. C, Effect of vitamin K on ROS accumulation when added 8 hr after initiation of cystine depletion. Cells were first subjected to cystine deprivation for 8 hr, followed by the addition of MK-4. ROS accumulation in cells was evaluated 3 hr later, as inA.D,Effect of vitam in K on the loss of intracellular GSH induced by cystine depletion. Cells were treated as indicated for 15 hr, and the GSH level was evaluated as described. E, F, Vitamin K did not react with free radicals. Free radicals are generated by DDPH in solution and have absorption at 517 nm. The scavenging of the radicals was monitored spectrophotometrically after the addition of vitamin K or Trolox. Trolox was used as a positive control. Trolox rapidly scavenged free radicals, whereas vitamin K was unable to react directly with the radicals, and the absorption of free radical remained constant over time (E). Trolox equivalent antioxidant activity was determined by monitoring inhibition by specified reagents of ABTS cation formation with H₂O₂ as oxidant trigger as described (F). Data are representative of at least three independent experiments.

We next examined the possibility of a direct interaction betweenvitamin K and ROS. Unlike ${alpha}$ -tocopherol and its soluble analogTrolox, vitamin K itself is not known to be an antioxidant (Vervoort et al., 1997). To evaluate the antioxidant potentialof vitamin K₁ and MK-4, we used two widely applied radicalscavenging assays (Blois, 1958; Rice-Evans and Miller, 1994). In the first assay, we tested the ability of vitamin K₁ andMK-4 to quench the stable lipoxyl radical DPPH. In the presenceof vitamin K₁ and MK-4 at 5 and 25 µM, the optical absorbanceof a solution of DPPH remained constant. In contrast, Trolox,a known antioxidant, rapidly and efficiently scavenged DPPH,as indicated by the loss of DPPH absorbance (Fig. 7E). Thesecond assay, the Trolox equivalent activity assay, is basedon the inhibition by antioxidants of the formation of the radicalcation ABTS^+·. The ABTS radical cation is formed by the interaction of ABTS with ferrylmyoglobin radical species (^·X - [Fe^IV = O]), generated by the activation of metmyoglobinwith H₂O₂. Antioxidant compounds suppress the absorbance ofthe ABTS radical cation to an extent and on a time scale dependingon their antioxidant capacities. Vitamin K₁ and MK-4 at concentrationsas high as 100 µM had no antioxidant activity, whereastocopherol and Trolox efficiently prevented ABTS^+· formation(Fig. 7F).

   Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

We report here the discovery of a novel role of vitamin K inpreventing GSH depletion-induced oxidative injury to primaryOL precursors and to immature cortical neurons. To our knowledge,this is the first study demonstrating a protective functionof vitamin K against oxidative stress in any cell.
We show that at low nanomolar concentrations, vitamin K₁ and MK-4 block cell death induced by various methods in a concentration-dependent manner: cystine depletion of culture medium, or exposure toexcess glutamate, homocysteic acid, or BSO (Fig. 3). All ofthese treatments result in depletion of intracellular GSH andaccumulation of ROS. In this model, oxidative stress occursbecause of the gradual and progressive accumulation of ROSwithin the cells. We also tested the protective efficacy ofvitamin K in another model of cell death involving oxidativestress. Vitamin K₁ and MK-4 had no effect on cell death inducedby exogenous H₂O₂. The oxidative stress and the death mechanismsin these two models are likely to be different because exogenousH₂O₂ presents a rapid and intense insult.
Vitamin K is required for the vitamin K-dependent ${gamma}$ -glutamylcarboxylasethat catalyzes a functionally important posttranslational modificationof a relatively small number of vitamin K-dependent proteins,including transmembranous proteins with unknown functions,and Gas6 (growth arrest-specific gene product 6) with a survival-promotingfunction (Tsaioun, 1999). Although the involvement of carboxylasewas not explored, low concentrations of vitamin K were foundto have a trophic effect on primary cortical neurons culturedin the absence of serum (Nakajima et al., 1993). On the basisof these observations and current understanding of vitamin K metabolism, it was intriguing to hypothesize that the protectiveaction of vitamin K₁ and MK-4 against oxidative injury wasbecause of vitamin K-dependent carboxylation of a protein thatpromotes cell survival. Several lines of evidence presentedhere, however, demonstrated that this hypothesis was incorrect.First, even at high concentrations, the vitamin K antagonists warfarin and dicoumarol, which inhibit vitamin K reductase,vitamin K cycling, and consequent carboxylation by depletingKH₂, had no effect on the protective function of vitamin K(Fig. 5A). Second, 2-Cl-vitamin K₁, an irreversible inhibitorof vitamin K-dependent ${gamma}$ -glutamylcarboxylase, did not block the protective action of vitamin K (Fig. 5B). The inhibitoryeffectiveness of 2-Cl-vitamin K₁ was confirmed in an enzymeassay using purified ${gamma}$ -glutamylcarboxylase (Fig. 5C). Third,neither OLs nor immature cortical neurons express vitamin K-dependent ${gamma}$ -glutamylcarboxylase activity (Fig. 5D and data not shown).Moreover, the vitamin K epoxidase activity, required for the carboxylation reaction, also was not present in these cells (Fig. 5E and data not shown). Finally, the reported Km valueof ${gamma}$ -glutamylcarboxylase for reduced K is in the range of 20–60µM (Stanley et al., 1997), 1000-fold higher than theconcentration required for protection by vitamin K. Therefore,we conclude that vitamin K prevents oxidative cell death viaa mechanism independent of ${gamma}$ -glutamylcarboxylase.
Depletion of GSH is a necessary step for cell death inducedby glutamate exposure or cystine deprivation (Murphy et al.,1989; Back et al., 1998). The cystine deprivation-induced lossof intracellular GSH is not prevented by treatment with vitaminK. The generation of ROS, however, is completely inhibited(Fig. 7). The origin of the ROS and the molecular events thatlead to ROS generation and cell death in our model are notknown and require further investigation. Other protective agents,such as the antioxidants idebenone and ${alpha}$ -tocopherol, protectagainst glutamate depletion-induced or cystine depletion-inducedoxidative cell death via preventing ROS accumulation without blocking the loss of GSH (Murphy et al., 1989, 1990; Okaet al., 1993; Yonezawa et al., 1996). Studies from severalgroups showed only weak activity (IC₅₀ >> 100 µM)of vitamin K species (including menadione) as inhibitors oflipid peroxidation in various test systems (Wills, 1972; Canfieldet al., 1985; Talcott et al., 1985; Ohyashiki et al., 1991). Consistent with these observations, vitamin K₁ and MK-4 do not possess any antioxidant activity in the two antioxidant assaysused here (Fig. 7E, F). Others, however, have also shown thatthe reduced form of vitamin K, hydroquinone KH₂, has potentanti-lipid peroxidation activity in solution (Mukai et al.,1993) and in microsomes (Vervoort et al., 1997). Whether KH₂can act as an antioxidant in cells has not been studied previously.Nevertheless, it is possible that the prevention of ROS generationin OLs by vitamin K is mediated through a mechanism involvingredox cycling of this vitamin. Direct detection of KH₂ in cellshas not been technically possible because KH₂ is readily oxidizedduring extraction. Whether vitamin K is actually convertedto KH₂ in the OLs is currently unknown, but it appears unlikely.Warfarin, an inhibitor for vitamin K epoxidase/reductase, anddicoumarol, a potent inhibitor of quinone reductase responsiblefor the two-electron reduction of quinone to hydroquinone,had no effect on the vitamin K-dependent protection, even atconcentrations 100-fold higher than those required to blockthe reductase (Fig. 5). Furthermore, staining for quinone reductaseactivity (Murphy et al., 1998) revealed only minor positivityin these OL precursors but profound activity in primary astrocytes,and this activity was completely blocked by the inhibitor dicoumarol(J. Li, A. Greene, J. J. Volpe, and P. A. Rosenberg, unpublished observations). Because vitamin K has also been shown to be metabolizedinto unidentified derivatives (Canfield et al., 1987; Rosset al., 1991), it remains possible that the protective activityof vitamin K observed in our study may because of one of itsunknown metabolites, rather than vitamin K per se.
Another possibility for the action of vitamin K in preventingGSH depletion-induced cell death is that vitamin K at low concentrationsmay interact with early signaling events leading to ROS production.Several lines of evidence suggest that GSH depletion-inducedoxidative death is mediated through a specific cell death signalingpathway. First, the transcriptional and translational inhibitorsactinomycin D and cycloheximide block cystine deprivation-inducedOL death (J. Li, J. J. Volpe, and P. A. Rosenberg, unpublishedobservations). Second, the tyrosine kinase inhibitor geldanamycin (Xiao et al., 1999) prevents GSH depletion-induced neuronaldeath. Third, inhibitors of the MEK signaling pathway protectagainst oxidative death in neurons (Stanciu et al., 2000). Although the detailed molecular cell death pathway in theseoxidative injury models awaits thorough investigation, it hasbeen suggested that vitamin K modulates cellular signalingtransduction pathways in other systems. Using a chick embryogenesismodel, Saxena et al. (1997) demonstrated the existence ofa vitamin K₁-dependent protein–tyrosine phosphorylationcascade that is sensitive to the alteration in levels or metabolismof vitamin K₁. Ni et al. (1998) also showed increased tyrosinephosphorylation of specific proteins in cells treated with vitaminK analogs. Furthermore, the vitamin K-dependent protein, Gas6,binds to its tyrosine kinase receptor and activates a seriesof intracellular signaling pathways that are responsible forits survival-promoting effect in Schwann cells and fibroblasts(Goruppi et al., 1996, 1999; Li et al., 1996; Nakano etal., 1996). Neither tyrosine kinase inhibitors (such as genistein)nor phosphatidylinositol 3'-kinase (PI3K) inhibitors (LY9804902and wortmanin), however, prevented the protective effect ofvitamin K in OL cultures (J. Li, J. J. Volpe, and P. A. Rosenberg,unpublished observations), suggesting that the Gas6-PI3K pathwayis not involved in our system. Again, this finding is consistentwith our conclusion that the function of vitamin K is independent of carboxylation.
Discovery of new approaches to prevent oxidative stress-mediatedinjury to OLs is important for designing clinical strategiesagainst PVL (Volpe, 2001). Using a primary cell culture systemin which the OL lineage closely corresponds to that presentin human cerebral white matter at a developmental stage most vulnerable to PVL (Back et al., 2001), we and others have demonstratedthat these cells are exquisitely sensitive to GSH depletion-mediatedoxidative injury (Back et al., 1998), AMPA–kainate-receptoractivation (Rosenberg et al., 2003), and hypoxia/hypoglycemia-mediatedcell death (Fern and Moller, 2000). The finding of a potentprotective action of vitamin K₁ and MK-4 against oxidativeinjury has potentially important clinical implications. OL precursors are the targets of white matter injury in neonatalhypoxia/ischemia rodent models (Back et al., 2002). Becauseneonates, and especially preterm infants, are developmentallyvitamin K deficient and are at a substantial risk for hemorrhagicdiseases, including intracranial hemorrhage, it is recommendedby the American Academy of Pediatrics that vitamin K be givento newborns at birth to prevent hemorrhage. The ability ofvitamin K to cross the blood brain barrier, its safety, andthe current use in newborns make it an attractive potentialtherapeutic molecule for the prevention and treatment of PVL,for which no current treatment is available. The efficacy ofvitamin K in preventing hypoxic/ischemic white matter injuryin a neonatal animal model is currently under investigation.
In summary, we demonstrate for the first time that oxidativecell death induced by GSH depletion in primary OL precursorsand in primary cortical neurons can be prevented by nanomolarconcentrations of vitamin K₁ and MK-4. The cytoprotective effectof K vitamins in this model is independent of their known biologicalrole in carboxylation. They do not prevent the loss of intracellularGSH caused by cystine depletion but markedly inhibit ROS accumulationand, thus, cell death. These results suggest a new approachto developing potential preventative and therapeutic strategiesfor neurological diseases in which GSH depletion-induced oxidativestress plays a role.

   Footnotes

Received Oct. 31, 2002; revised Apr. 11, 2003; accepted May. 7, 2003.
This work was supported by National Institutes of Health (NIH)Grants HD18655 and NS38475 (to J.J.V.), a Hearst FoundationAward (to J.L.), United Cerebral Palsy Foundation ResearchGrant R-737 (to J.L.), a fellowship from the Howard HughesMedical Institute (to J.C.L.), and NIH Grant HL42443 (to B.C.F.).We thank Dr. Hannah C. Kinney for discussions and comments onthis manuscript. We are grateful to Dr. John W. Suttie forreagents and helpful discussions and to Amanda Greene for technicalassistance.
Correspondence should be addressed to Dr. Paul A. Rosenberg,Department of Neurology, Enders 3, Children's Hospital, 300Longwood Avenue, Boston, MA 02115. E-mail: paul.rosenberg{at}tch.harvard.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235816-11$15.00/0

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Results
Discussion
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