Gene transfer of Cu/Zn SOD to cerebral vessels prevents FPI-induced CBF autoregulatory dysfunction

doi:10.1152/ajpheart.00590.2001

Gene transfer of Cu/Zn SOD to cerebral vessels prevents FPI-induced CBF autoregulatory dysfunction

Chi Dae Kim¹^,^*, Hwa Kyoung Shin¹^,³^,^*, Hyun Seung Lee¹, Jeong Hyun Lee¹, Tae Ho Lee³, and Ki Whan Hong¹^,²

¹ Department of Pharmacology, College of Medicine, ² Research Institute of Genetic Engineering, and ³ Department of Microbiology, College of Natural Sciences, Pusan National University, Pusan 602-739, South Korea

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The goal of this study was to determine whether gene transfer of human copper-zinc (Cu/Zn) superoxide dismutase (SOD) haspreventive effects on cerebral blood flow (CBF) autoregulatorydysfunction after fluid percussion injury (FPI). Rats subjectedto FPI (2-2.5 atm) exhibited enhanced activity of reduced NADP(NADPH) oxidase in the cerebral vasculature. In line with thesefindings, the rats showed not only reduced vasodilation of thepial artery in response to calcitonin gene-related peptide andlevcromakalim but also impaired autoregulatory vasodilation inresponse to acute hypotension. The FPI-induced hemodynamic alterationswere significantly prevented by pretreatment with diphenyleneiodonium(10 µmol/l), an NAD(P)H oxidase inhibitor. Intracisternal applicationof recombinant adenovirus (100 µl of 1 × 10¹⁰ pfu/ml)-encoding human Cu/Zn SOD 3 days before FPI preventedthe impairment of vasodilation to hypotension and vasorelaxants,resulting in the restoration of CBF autoregulation. Our findingsdemonstrate that FPI-induced impairment of CBF autoregulationis closely related with NAD(P)H oxidase-derived superoxide anion,and these alterations can be prevented by the recombinant adenovirus-mediatedtransfer of human Cu/Zn SOD gene to the cerebralvasculature.

cerebral autoregulation; reduced NAD(P)H oxidase

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

ALTERATIONS IN CEREBRAL BLOOD FLOW (CBF) after traumatic brain injury may be one factor that affects the pathophysiology andneurological outcomes associated with brain trauma. Reductionof CBF after brain injury is well documented in rats (17, 33).Fluid percussion-induced brain injury (FPI), as a model of humanconcussive trauma, has been reported (1, 3) to cause considerablealterations in neurohumoral control of the cerebral circulation,including impairment of K⁺ channel function with reduced vasorelaxation. Several studieshave revealed that oxygen radical-mediated cerebrovascular abnormalitiesoccur in the first few hours after brain trauma (8, 16),which is associated with a reduction of CBF (31, 33). We (14)recently demonstrated an altered autoregulatory vasodilation inresponse to acute hypotension in association with reduced vasodilationin response to calcitonin gene-related peptide (CGRP) and levcromakalimafter FPI. In our previous experiment, we (14) demonstrateda mechanistic result that FPI-induced activation of tyrosine kinaselinks the inhibition of K⁺ channels to impaired CBF autoregulation in rat pialartery.

On the other hand, FPI has been observed to be associated with the generation of superoxide on the cerebral cortex, whichis at least one mechanism contributing to altered reactivity ofcerebral arterioles (2, 3, 10, 16). In addition, itwas revealed that transgenic mice overexpressing copper-zinc (Cu/Zn)superoxide dismutase (SOD) showed significantly attenuated neurologicaldeficits following traumatic brain injury (5), suggesting thatoxidative stress plays a deleterious role. Reduced NADP (NADPH)oxidase has recently been demonstrated in adventitial smooth musclecells (4, 20) and is considered a major source of superoxidein vascular cells (12). However, its participation in FPI-inducedCBF autoregulatory dysfunction isunknown.

Adenoviral vectors have been used to achieve efficient transfer and expression of recombinant genes in different vasculaturesin both ex vivo and in vivo experiments, raising the possibilityof this approach to treat vascular disorders (21, 27). Recentresults (29, 30) have described the perivascular adenoviraltransfection of reporter gene encoding $beta$ -galactosidase to rabbit,mice, and rat cerebralvasculatures.

On the basis of these results, it is hypothesized that acute elevation of intracellular superoxide anion after brain injuryresults in activation of tyrosine kinase-linked inhibition ofK⁺ channels and impairment of autoregulatory vasodilation in responseto acute hypotension and to K⁺ channel openers in the rat pial artery. Thus the present studywas designed to test the involvement of NAD(P)H oxidase-derivedsuperoxide anion in the development of the functional impairmentof vasodilatory responses. To address this hypothesis, we employeddiphenyleneiodonium (DPI), an NAD(P)H oxidase inhibitor, and therecombinant adenovirus encoding human Cu/Zn SOD. We thereby provedtheir effectiveness in the recovery of the pial arteries to vasodilatein response to CGRP and levcromakalim and acute hypotension inassociation with restoration of CBF autoregulation in the ratssubjected toFPI.

	MATERIALS AND METHODS

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Preparation of animals. The animal experimentation committee of the College of Medicine, Pusan National University, approved the experimental designof this study and the guiding principles for research. Male Sprague-Dawleyrats (250-300 g) were anesthetized with urethane (1 g/kg ip) andplaced on a heating pad to maintain a constant rectal temperature(37 ± 0.5°C). After a tracheostomy was performed, the animal wasmechanically ventilated with room air with the use of a respirator(model 683, Harvard Apparatus; South Natick, MA). Catheters wereplaced in carotid and femoral arteries for measurement of bloodpressure and for withdrawing and sampling of the arterial blood,respectively. The blood was collected before and after installationof a cranial window for blood gas and pH analysis (STAT Profile3, Nova Biomedicals; Boston, MA). FPI was induced as previouslydescribed (14). In brief, a 4.5-kg pendulum was used to strikea piston that was connected to the female Leuer-Loc fitting, whichhad been implanted over the exposed dura of the rat cerebral cortex.The intensity of the blow was adjusted to 2.0-2.5atm.

Measurement of vessel diameter and CBF. The details for the measurements of pial arterial diameter and CBF have been published previously (14). Briefly, after theclosed cranial window was installed over the contralateral sideof parietal cortex to the side of injury, the image of pial arterioleswas visualized through the cranial window and captured with acharge-coupled device videocamera (model VDC 3900, Sanyo) througha stereomicroscope (model SMZ-2T, Nikon). The caliber was measuredwith the use of a width analyzer (model C3161, Hamamatsu Photonics;Hamamatsu, Japan) after the image was fed to a televisionmonitor.

CBF to the pial artery was measured with the use of laser-Doppler flowmetry (Laserflo BPM², Vasamedics; St. Paul, MN) equipped with a 1-mm-diameter needleprobe (model P-433-5, Vasamedics). After the dura mater was carefullysectioned, the probe was placed near and lateral to the pial arteryin the open window and advanced into the cerebrospinal fluid (CSF)~0.2 mm above the cortical surface. The changes in CBF were monitoredduring controlled hypotension. Stepwise hypotension was achievedby bleeding of the arterial blood into the reservoir. Blood (1ml) was withdrawn every 2 min while the systemic arterial bloodpressure was being monitored until it lowered to ~50%. In thecase of infusion, the reservoir blood was infused back 1 ml every2 min. The laser-Doppler flowmetry outputs were regarded as arbitraryunits and the changes in CBF were expressed as a percentage ofthe baselineCBF.

Three hours after FPI, the vasodilatory responses of the pial artery to vasodilators (0.001-0.1 µmol/l CGRP and 0.1-10 µmol/llevcromakalim) and to stepwise hypotension were determined. Thechanges in the pial arterial blood flow in response to stepwisehypotension and to its reverse of blood pressure were also measured.Thereafter, we reexamined the vasodilatory and autoregulatoryresponses in rats injected with adenovirus vector-encoding humanCu/Zn SOD (AdCMVSOD) or treated with DPI (1 µmol/l). In the presentexperiment, AdCMVSOD was administered via cisterna magna 3 daysbefore FPI, and DPI was applied 30 min before application of vasodilatorsand hypotensive procedure. Alterations in pial arterial diameterand blood pressure were expressed as percent changes in the baselinediameter and mean arterial blood pressure, respectively. The intracranialpressure was maintained constant at 5-6 mmHg throughout the experimentby adjustment of the height of the free end of plastic tube connectedto the outlet of the window. Only one arteriole was observed underthe window in eachrat.

Measurement of NAD(P)H oxidase activity. In a separate experimental system, cerebral vasculature including basilar artery, cerebral arteries (anterior, middle, andposterior cerebral arteries), and pial arterioles was isolatedand homogenized in 50 mmol/l phosphate buffer, and NAD(P)H-inducedproduction of superoxide in the vascular homogenates was measuredas an index for NAD(P)H oxidase activity as described previously(24). Briefly, the vascular homogenates were placed in 200 µlof HEPES buffer containing lucigenin (5 µmol/l) and placed intoa luminometer (Microlumat LB96P, Berthold). After dark adaptation,both NADH (100 µmol/l) and NADPH (100 µmol/l) were added to thevial. Counts were recorded every 30 s for 15 min, and the respectivebackground counts were subtracted. Chemiluminescence was expressedas counts per second per milligram of protein. In some experiments,inhibitors were added to the samples 10 min beforereadings.

Preparation of adenoviral vector and in vivo gene transfer. Replication-deficient recombinant adenoviral vector (serotype 5, produced in HEK-293 cells) driven by the cytomegalovirusimmediate early promoter was used to transfer the genes to thecerebral vasculature. AdCMVSOD and AdCMV Escherichia coli $beta$ -galactosidase(AdCMVLacZ) genes were obtained from Dr. John Engelhardt (GeneTherapy Core Center, University of Iowa). The DNA constructs ofreplication-deficient adenovirus comprise almost a full-lengthcopy of the adenoviral genome, in which a Cu/Zn SOD and LacZ expressioncassette is incorporated at the site of E1 region deletions. Foreach vector, high-titer adenoviral vector stocks were preparedby double-cesium gradient purification, and viral titer [plaque-formingunits (pfu/ml)] was determined by standardmethods.

To transfer the gene to the cerebral vasculature in vivo, rats were anesthetized with thiopental sodium (50 mg/kg ip) anda 27-gauge needle was aseptically inserted into the cisterna magnaas previously described (23). An equal volume (100 µl) of CSFwas removed before injection of viral suspension (100 µl of 1× 10¹⁰ pfu/ml) to avoid an increase in intracranialpressure.

Immunohistochemistry for Cu/Zn SOD. For immunohistochemical analysis for Cu/Zn SOD, serial 5-µm-thick frozen sections of the pial artery were adhered to poly-L-lysine-coatedslides, allowed to dry in room air, and fixed in acetone. Aftertreatment with H₂O₂ (0.6%) and bovine serum albumin (2%), thepreparations were incubated in the goat anti-rat Cu/Zn SOD polyclonalantibody (Santa Cruz Biotechnology). After the primary incubation,the slides were incubated with the biotinylated anti-goat secondaryantibody (Santa Cruz Biotechnology). The slides were then incubatedwith avidin and biotinylated horseradish peroxidase complex (VectorLaboratories; Burlingame, CA) for 1 h. The slides were washedin phosphate-buffered saline, incubated with diaminobenzidine(Vector Laboratories), and then washed with water. Vessel sectionswere counterstained with hematoxyline (purple) and examined forpositive staining of Cu/Zn SOD (gray-black) by light microscopy.Immunoreactivity for Cu/Zn SOD was quantitated by ImagePro PlusImaging software (Media Cybernetics; Silver Spring, MD) and thestain density was expressed as pixels per squared micrometer oftissue.

Drugs. CGRP and DPI were purchased from Sigma (St. Louis, MO). CGRP was dissolved in 0.1% bovine serum albumin to make a stock solutionof 0.01 mmol/l. Levcromakalim, a K⁺ channel opener, was generously donated by the Korea ResearchInstitute of Chemical Technology (Daejon, Korea) and dissolvedin ethanol-polyethylene glycol (50:50% vol/vol) to make a stocksolution of 1 mmol/l.

Statistical analysis. Results were expressed as means ± SE. Student's t-test was used for analyzing values between the data of vehicle- and inhibitor-treatedgroups [concentration giving 25% maximal response (EC₂₅) and lowerlimit of CBF autoregulation]. Two-way repeated-measures analysisof variance (ANOVA) was used for the comparison of time-dependentarterial diameter changes in response to agonists between inhibitor-treatedand vehicle groups. Data presented as the percentage of changewere compared by nonparametric means with Wilcoxon's signed-ranksum test. Repeated-measures ANOVA, followed by Dunnett's t-test,were used for statistical analysis of CBF between baseline valueand the value at each blood pressure level. P < 0.05 was acceptedas statisticallysignificant.

	RESULTS

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Mean arterial blood pressure, PCO₂, PO₂, and pH in the control group were not significantly different from those in the ratssubjected to FPI (Table 1). Baseline pial arterial diameter ofthe FPI group (44.5 ± 6.3 µm, n = 43) was not significantly differentfrom the control value (41.2 ± 4.4 µm, n = 25).

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Table 1. Physiological variables: MABP, blood gas, and pH analysis before and after FPI

NAD(P)H oxidase activity. As shown in Fig. 1, cerebral vessels exposed to FPI exhibited increased superoxide production (12.7 ± 1.4 counts · s¹ · mg protein¹, P < 0.01; n = 7) higher than the control value (4.3 ± 0.2 counts· s¹ · mg protein¹; n = 7). The FPI-induced increase in superoxide production wassignificantly suppressed to 5.5 ± 1.3 counts · s¹ · mg protein¹ (P < 0.01) by pretreatment with DPI (10 µmol/l, n = 7). However,the FPI-induced superoxide production was little affected by 10µmol/l allopurinol (an inhibitor of xanthine oxidase), 10 µmol/lsulfaphenazole (a selective cytochrome P-450 2C9 inhibitor), and10 µmol/l indomethacin (a cyclooxygenase inhibitor), respectively.

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Fig. 1. The activity of reduced NADP (NADPH) oxidase in the cerebral vasculature was accessed by measuring superoxide production with lucigenin chemiluminescence. Values were expressed as counts per second per milligram of protein. The fluid percussion injury (FPI)-induced increase (Veh) in superoxide production was significantly decreased by 10 µmol/l pretreatment with diphenyleneiodonium (DPI), but not by allopurinol (Allo), sulfaphenazole (SFP), and indomethacin (IND), respectively. Values are means ± SE from 7 experiments. ** P < 0.01 vs. control; ##P < 0.01 vs. FPI vehicle.

Effect of DPI on vascular reactivity. Suffusion with artificial CSF containing CGRP (0.001-0.1 µmol/l) or levcromakalim (0.1-10 µmol/l) exerted concentration-dependentvasodilations of the pial arteries with the EC₂₅ values of 0.002± 0.001 and 0.91 ± 0.36 µmol/l, respectively. CGRP and levcromakalimat concentration ranges used in this study caused little changein systemic arterial blood pressure. Vasodilation induced by eitherCGRP or levcromakalim was markedly blunted after FPI with significantlyincreased EC₂₅ values of 0.113 ± 0.024 µmol/l (P < 0.001) and41.35 ± 13.23 µmol/l (P < 0.05), respectively. In turn, theseblunted vasodilations to vasodilators were largely restored undersuffusion with artificial CSF containing 1 µmol/l DPI, with significantlydecreased EC₂₅ values of 0.004 ± 0.002 µmol/l (P < 0.01) and 0.85± 0.24 µmol/l (P < 0.05), respectively (Fig. 2). The pial arterialdiameter was little changed under suffusion with artificial CSFcontaining 1 µmol/l DPI.

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Fig. 2. Percent changes in pial arterial diameter in response to calcitonin gene-related peptide (CGRP) and levcromakalim in the control and FPI rats without and with pretreatment with DPI. Cortical surface was suffused with artificial cerebrospinal fluid (CSF) containing CGRP or levcromakalim in the absence and presence of DPI (1 µmol/l) 3 h after FPI. Values are means ± SE from 6 experiments. The vasodilations induced by CGRP and levcromakalim were markedly blunted after FPI, which were largely restored by pretreatment with DPI.

AdCMVSOD-mediated transgene expression on the pial artery. In the pial artery from the vehicle-treated group, positive staining for Cu/Zn SOD was observed in the endothelium but notin the media or adventitia. Positive staining for Cu/Zn SOD wasobserved in both endothelial and adventitial cells in vesselsfrom the AdCMVSOD-treated group (Fig. 3). The amount of Cu/ZnSOD expression in the endothelium in AdCMVSOD-treated group wasnot different from those in vehicle-treated group. Transgene expressionin the adventitial cells was observed 1 day after and maximized3 days after intracisternal administration of AdCMVSOD (100 µlof 1 × 10¹⁰ pfu/ml).

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Fig. 3. Comparison of densities of immunohistochemical staining for copper-zinc (Cu/Zn) superoxide dismutase (SOD) in pial arteries from vehicle (control) and adenovirus vector-encoding human Cu/Zn SOD (AdCMVSOD)-treated rats. A: in vessels from the vehicle-treated group, positive staining (gray-black) for Cu/Zn SOD was observed in the endothelium, but not in the media or adventitia. B: positive staining for Cu/Zn SOD was observed in both endothelial and adventitial cells in vessels from the AdCMVSOD-treated group. The density of staining in pial arterial section was expressed as pixels per squared micrometer of tissue. Values are means ± SE from 5 experiments.** P < 0.01 vs. control.

Effect of AdCMVSOD-mediated gene transfer on vascular reactivity. In rats treated with AdCMVSOD (100 µl of 1 × 10¹⁰ pfu/ml, intracisternal administration), the FPI-induced blunted vasodilationto CGRP or levcromakalim was significantly restored with decreasedEC₂₅ values of 0.011 ± 0.003 µmol/l (P < 0.01) and 1.81 ± 0.28µmol/l (P < 0.05), respectively (Fig. 4).

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Fig. 4. Percent changes in pial arterial diameter in response to CGRP and levcromakalim in the control and FPI rats without and with pretreatment with AdCMVSOD. AdCMVSOD (100 µl of 1 × 10¹⁰ pfu/ml) was applied 3 days before FPI. Cortical surface was suffused with artificial CSF containing CGRP or levcromakalim 3 h after FPI. Values are means ± SE from 4 experiments. The vasodilations induced by CGRP and levcromakalim were markedly blunted following FPI, which were largely restored by pretreatment with AdCMVSOD.

Effect of AdCMVSOD-mediated gene transfer on autoregulatory vasodilation. Changes in pial arterial diameter in response to a stepwise hypotension were plotted as a function of changes in systemicmean arterial blood pressure, and mean slope was calculated fromlinear regression. Three hours after FPI, the pial artery showedreduced vasodilation to lowering of blood pressure, as evidencedby reduced slopes of regression lines (slope for vasodilation, $-$ 1.99 ± 0.27 in control to $-$ 0.43 ± 0.14, P < 0.001, and that forvasoconstriction, from $-$ 1.60 ± 0.17 to $-$ 0.58 ± 0.14, P < 0.001;n = 6). Markedly blunted autoregulatory vasodilation to hypotensionafter FPI was largely recovered after pretreatment with 1 µmol/lDPI (slope for vasodilation to $-$ 1.25 ± 0.19, P < 0.01, and thatfor vasoconstriction to $-$ 0.93 ± 0.13; n = 5). Application of AdCMVSOD(100 µl of 1 × 10¹⁰ pfu/ml) 3 days before FPI prevented reduction in the autoregulatoryvasodilation of the pial microvessels to hypotension with therestored slopes for vasodilation to $-$ 1.35 ± 0.19 (P < 0.01; n= 5) and for vasoconstriction to $-$ 1.11 ± 0.13 (P < 0.05; n = 5)(Fig. 5). Suffusion with artificial CSF containing DPI (<1 µmol/l)showed little effect on the pial arterial diameter.

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Fig. 5. Graph showing alterations in the autoregulatory vasodilator and vasoconstrictor responses to changes in mean arterial blood pressure (MABP) after FPI without and with pretreatment with DPI (1 µmol/l). The cortical surface was suffused with artificial CSF with DPI from 30 min before and during stepwise hypotension and reverse of blood pressure. Otherwise, either AdCMVLacZ (100 µl of 1 × 10¹⁰ pfu/ml) or AdCMVSOD (100 µl of 1 × 10¹⁰ pfu/ml) was applied 3 days before FPI. Values are means ± SE from 5-6 experiments. Significant differences (P < 0.001) were shown between the blood pressure-diameter relations of the control and FPI groups, between those of the FPI and DPI + FPI groups, and between those of the FPI and AdCMVSOD + FPI groups by two-way repeated-measures ANOVA.

Effect of AdCMVSOD-mediated gene transfer on lower limit of CBF autoregulation. Mean arterial blood pressure was 118.5 ± 9.3 mmHg under resting conditions. CBF to the pial arteries was well preserved despitea decrease in mean arterial blood pressure up to 50-60 mmHg. Whenblood pressure levels decreased further, CBF fell steeply dependingon the fall in blood pressure thereafter. The lower limit of autoregulation,defined as the blood pressure where CBF decreased by 10% of thebaseline, was 55.7 ± 3.5 mmHg in the control group, which wasshifted to 81.9 ± 3.6 mmHg after FPI (P < 0.001). After applicationof AdCMVLacZ, the lower limit of CBF autoregulation was littleaffected. However, after pretreatment with AdCMVSOD (100 µl of1 × 10¹⁰ pfu/ml) 3 days before FPI, the lower limit of CBF autoregulationwas significantly restored to 64.6 ± 1.6 mmHg (P < 0.01), comparableto the level with DPI treatment (60.3 ± 2.1 mmHg, P < 0.001) (Fig.6).

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Fig. 6. Relationship of MABP to cerebral blood flow (CBF) in rat pial arteries after FPI under pretreatment with AdCMVLacZ (100 µl of 1 × 10¹⁰ pfu/ml, AdLacZ), AdCMVSOD (100 µl of 1 × 10¹⁰ pfu/ml, AdSOD), and DPI (1 µmol/l, DPI + FPI) during stepwise hypotension compared with FPI alone. Arrows indicate lower limits of autoregulation defined as the MABP at which CBF decreased by 10% of the baseline value. Values are means ± SE from 4 experiments. Significant difference (P < 0.05) was identified between blood pressure-CBF relationships of control and FPI groups, FPI and DPI + FPI groups, and FPI and AdSOD + FPI groups by two-way repeated-measures ANOVA.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The major findings of this study were the following: 1) FPI caused a significant increase in the activity of NAD(P)H oxidasein the cerebral vasculature, 2) vasodilations of the pial arteryto CGRP and levcromakalim were significantly suppressed in associationwith impairment of autoregulatory vasodilation in response toacute hypotension, and 3) these impaired vasodilations in FPIrats were significantly restored with the recovery of lower limitof CBF autoregulation, after pretreatment with recombinant AdCMVSODand DPI, an NAD(P)H oxidaseinhibitor.

Cerebral autoregulation may be altered in systemic diseases, including hypertension, diabetes mellitus, and some disordersof central nervous system. Maintenance of CBF has been consideredto be very important from a therapeutic point of view, accordingto a report by Heiss et al. (13) that the severity of neuroticsymptoms in the chronic stage of cerebral infarction correlatedwith CBF levels. On the other hand, FPI causes a partial or completeimpairment of the capacity of cerebral vessels to autoregulateCBF (9, 11). The magnitude of vasodilatory reserves availablefor autoregulation is significantly decreased in FPI, and thebrain may be more vulnerable to the effects of secondary insults,such as hypotension (6). In line with these facts, the morbidityand mortality of severe head trauma increase when hypotensionaccompanies the brain injury (26). Consistent with the resultsof Prat et al. (25), in that loss of cerebral autoregulationoccurred during the first 4 h after injury, our (14) previousdata clearly showed that cerebral autoregulatory dysfunction wasmaximized 3 h after brain injury. Considering these results, immediatetherapeutic approaches to preserve the autoregulatory vasodilation(CBF autoregulation) in response to hypotension appear to be veryimportant in reducing the morbidity and mortality of patientsafter braintrauma.

Although the mechanism(s) contributing to posttraumatic changes in CBF autoregulation is still unknown, there is evidencethat oxygen free radicals play a role in brain injury. Brain injuryin cats has been reported (16) to enhance superoxide production,and sustained dilation and abnormal responsiveness of the pialarterioles were observed after injury. Furthermore, in transgenicmice overexpressing human Cu/Zn SOD, significant attenuation ofacute injuries (i.e., brain edema and increased blood-brain barrierpermeability) and chronic neurological deficits were demonstrated(5). Thus it was concluded that FPI-induced superoxide generationon the cerebral cortical surface might contribute to impairedreactivity of cerebral arterioles (10, 15). Consistent withthese earlier reports, our results clearly showed that rats exposedto FPI exhibited enhanced NAD(P)H oxidase activity in the cerebralvasculature. Furthermore, both FPI-induced activation of vascularNAD(P)H oxidase and reduced vasodilatory hemodynamics to CGRPand levcromakalim and to acute hypotension were significantlysuppressed by treatment with DPI, an NAD(P)H oxidase inhibitor.These results suggest the role of NADPH oxidase-derived oxygenfree radicals in the FPI-induced CBF autoregulatory dysfunction.However, it remains unclear about the involvement of other mechanisms,including endothelin-1, prostanoids, opiates, and other excitatoryneurotransmitters.

Ellison et al. (8) and Muir et al. (18) have reported that SOD could restore the posttraumatic cortical blood flow inrats, suggestive of the role of oxygen radicals in cerebrovascularabnormality in brain trauma. According to the results of Sprangeret al. (28), SOD activity was significantly lower in patientswith ischemic stroke and the endogenous antioxidants were depletedas a consequence of an excessive production of oxygen free radicals.SOD has also been demonstrated to improve outcome after traumaticbrain injury in phase II clinical trials (19). Although SODhas been reported (22) to be effective in preventing alterationsin CBF after brain trauma, native SOD has a plasma half-life of~6 min in rats. Furthermore, the entry of exogenous SOD into thebrain is normally very limited by the blood-brain barrier, althoughthe amount of SOD that enters the brain after moderate FPI isincreased severalfold due to the altered vascular permeability(32). Therefore, it is not easy to maintain therapeutic concentrationof SOD in the targeted tissues after the bolusinjection.

Adenoviral vectors have been widely used to achieve efficient transfer and expression of recombinant genes in different vasculaturesboth in ex vivo and in vivo experiments, thereby raising the possibilityof their use to treat vascular disorders (21, 27). It hasrecently been demonstrated (7, 23, 29) that intracisternaladministration of AdCMVLacZ effectively transfers recombinantgenes to the cerebral vasculatures of rat, mice, and rabbit. Inthe present study, after intracisternal administration of recombinantAdCMVSOD, expression of Cu/Zn SOD was demonstrated 1 day laterand maximized after 3 days in the adventitial cells of pialartery.

Considering the fact that an NAD(P)H oxidase in adventitial cells is a major source of superoxide in the vascular cells (12),periadventitial transfer of the Cu/Zn SOD gene is expected toprevent oxygen radical-mediated alterations in vascular function.In our results, recombinant adenovirus-mediated transfer to thecerebral vasculature of Cu/Zn SOD cDNA has prevented alterationsin CBF autoregulation with restoration of vasodilation to vasodilators.These results suggest that alterations in CBF autoregulation andvascular reactivity to vasodilators were ascribed to the productionof an NAD(P)H oxidase-derived superoxide anion. Furthermore, recombinantadenovirus-mediated transfer of Cu/Zn SOD cDNA to cerebral vasculaturemay have the therapeutic potential to minimize the oxidative injurycaused by oxygen free radicals until the endogenous free radicalscavenger system recovers. This approach may contribute dramaticallyto mortality reduction and to improved outcome following traumaticbraininjury.

In summary, a FPI-induced NAD(P)H oxidase-derived superoxide anion is at least one mechanism underlying the FPI-induced cerebralautoregulatory dysfunction, and such impaired function of thepial artery can be prevented by recombinant adenovirus-mediatedtransfer of the Cu/Zn SOD gene to the cerebralvasculature.

	ACKNOWLEDGEMENTS

We thank Dr. John Engelhardt, Gene Therapy Core Center, University of Iowa, for the generous donation of adenoviral vectorscontainingtransgenes.

	FOOTNOTES

^* C. D. Kim and H. K. Shin contributed equally to thisstudy.

This study was supported in part by grants from the Korea Science and Engineering Foundation (to C.D. Kim and K. W. Hong),Korea Research Foundation, Ministry of Health and Welfare, andResearch Institute of Genetic Engineering (all to K. W.Hong).

Address for reprint requests and other correspondence: K. W. Hong, Dept. of Pharmacology, College of Medicine, Pusan NationalUniversity, Pusan 602-739, South Korea (E-mail: kwhong{at}pusan.ac.kr).

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.

10.1152/ajpheart.00590.2001

Received 4 July 2001; accepted in final form 17 January 2002.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

1. Armstead, WM. Brain injury impaires ATP-sensitive K⁺ channel function in piglet cerebral arteries. Stroke 28: 2273-2279, 1997[Abstract/Free Full Text].

2. Armstead, WM. Superoxide generation links protein kinase C activation to impaired ATP-sensitive K⁺ channel function after brain injury. Stroke 30: 153-159, 1999[Abstract/Free Full Text].

3. Armstead, WM, and Kurth CD. Different cerebral hemodynamic responses following fluid percussion brain injury in the newborn and juvenile pig. J Neurotrauma 11: 487-497, 1994[ISI][Medline].

4. Azumi, H, Inoue N, Takeshita S, Rikitake Y, Kawashima S, Hayashi Y, Itoh H, and Yokoyama M. Expression of NADH/NADPH oxidase p22^phox in human coronary arteries. Circulation 100: 1494-1498, 1999[Abstract/Free Full Text].

5. Chan, PH, Epstein CJ, Li Y, Huang TT, Carlson E, Kinouchi H, Yang G, Kamii H, Mikawa S, Kondo T, Copin JC, Chen SF, Chan T, Gafni J, Gobbel G, and Reola E. Transgenic mice and knockout mutants in the study of oxidative stress in brain injury. J Neurotrauma 12: 815-824, 1995[ISI][Medline].

6. Chesnut, RM, Marshall SB, Piek J, Blunt BA, Klauber MR, and Marshall LF. Early and late systemic hypotension as a frequent and fundamental source of cerebral ischemia following severe brain injury in the traumatic coma data bank. Acta Neurochir Suppl (Wien) 59: 121-125, 1993[Medline].

7. Christenson, SD, Lake KD, Ooboshi H, Faraci FM, Davidson BL, and Heistad DD. Adenovirus-mediated gene transfer in vivo to cerebral blood vessels and perivascular tissue in mice. Stroke 29: 1411-1415, 1998[Abstract/Free Full Text].

8. Ellison, MD, Erb DE, Kontos HA, and Povlishock JT. Recovery of impaired endothelium-dependent relaxation after fluid-percussion brain injury in cats. Stroke 20: 911-917, 1989[Abstract/Free Full Text].

9. Engelborghs, K, Haseldonckx M, Reempts JV, Rossem KV, Wouters L, Borgers M, and Verlooy J. Impaired autoregulation of cerebral blood flow in an experimental model of traumatic brain injury. J Neurotrauma 17: 667-677, 2000[ISI][Medline].

10. Fabian, RH, DeWitt DS, and Kent TA. In vivo detection of superoxide anion production by the brain using a cytochrome c electrode. J Cereb Blood Flow Metab 15: 242-247, 1995[ISI][Medline].

11. Golding, EM, Robertson CS, and Bryan RM. The consequences of traumatic brain injury on cerebral blood flow and autoregulation: a review. Clin Exp Hypertens 21: 299-332, 1999.

12. Griendling, KK, Sorescu D, and Ushi-Fukai M. NAD(P)H oxidase: role in cardiovascular biology and disease. Circ Res 86: 494-501, 2000[Abstract/Free Full Text].

13. Heiss, WD, Zeiler K, Havelec L, Reisner T, and Bruck J. Long-term prognosis in stroke related to cerebral blood flow. Arch Neurol 34: 671-676, 1977[Abstract].

14. Hong, KW, Shin HK, Kim CD, Lee WS, and Rhim BY. Restoration of vasodilation and cerebral blood flow autoregulation by genistein in rat pial artery after brain injury. Am J Physiol Heart Circ Physiol 281: H308-H315, 2001[Abstract/Free Full Text].

15. Kasemsri, T, and Armstead WM. Endothelin production links superoxide generation to altered opioid-induced pial artery vasodilation after brain injury in pigs. Stroke 28: 190-197, 1997[Abstract/Free Full Text].

16. Kontos, HA, and Wei EP. Superoxide production in experimental brain injury. J Neurosurg 64: 803-807, 1986[ISI][Medline].

17. Muir, JK, Boerschel M, and Ellis EF. Continuous monitoring of posttraumatic cerebral blood flow using laser-doppler flowmetry. J Neurotrauma 9: 355-362, 1992[ISI][Medline].

18. Muir, JK, Tynan M, Caldwell R, and Ellis EF. Superoxide dismutase improves posttraumatic cortical blood flow in rats. J Neurotrauma 12: 179-188, 1995[ISI][Medline].

19. Muizelaar, JP, Marmarou A, Young HF, Choi SC, Wolf A, Schneider RL, and Kontos HA. Improving the outcome of severe head injury with the oxygen radical scavenger polyethylene glycol-conjugated superoxide dismutase: a phase II trial. J Neurosurg 78: 375-382, 1993[ISI][Medline].

20. Muramo, T, Schini-Kerth VB, Brandes RP, and Busse R. Glucocorticoids inhibit superoxide anion production and p22^phox mRNA expression in human aortic smooth muscle cells. Hypertension 32: 1083-1088, 1998[Abstract/Free Full Text].

21. Nabel, EG, and Nabel GJ. Complex models for the study of gene function in cardiovascular biology. Annu Rev Physiol 56: 741-761, 1994[ISI][Medline].

22. Odlind, B, Appelgren L, and Wolgast M. Tissue distribution of ¹²⁵I-labeled bovine superoxide dismutase (SOD) in the rat. Pharmacol Toxicol 62: 95-100, 1988[ISI][Medline].

23. Ooboshi, H, Welsh MJ, Rios CD, Davidson BL, and Heistad DD. Adenovirus-mediated gene transfer in vivo to cerebral blood vessels and perivascular tissue. Circ Res 77: 7-13, 1995[Abstract/Free Full Text].

24. Pagano, PJ, Ito Y, Tornheim K, Gallop PM, Tauber AI, and Cohen RA. An NADPH oxidase superoxide-generating system in the rabbit aorta. Am J Physiol Heart Circ Physiol 268: H2274-H2280, 1995[Abstract/Free Full Text].

25. Prat, R, Markiv V, Dujovny M, and Misra M. Evaluation of cerebral autoregulation following diffuse brain injury in rats. Neurol Res 19: 393-402, 1997[ISI][Medline].

26. Schmoker, JD, Zhuang J, and Shackford SR. Hemorrhagic hypotension after brain injury causes an early and sustained reduction in cerebral oxygen delivery despite normalization of systemic oxygen delivery. J Trauma 32: 714-720, 1992[ISI][Medline].

27. Schneider, MD, and French BA. The advent of adenovirus: gene therapy for cardiovascular disease. Circulation 88: 1937-1942, 1993[Free Full Text].

28. Spranger, M, Krempien S, Schwab S, Donneberg S, and Hacke W. Superoxide dismutase activity in serum of patients with acute cerebral ischemic injury: correlation with clinical course and infarct size. Stroke 28: 2425-2428, 1997[Abstract/Free Full Text].

29. Toyoda, K, Faraci FM, Russo AF, Davidson BL, and Heistad DD. Gene transfer of calcitonin gene-related peptide to cerebral arteries. Am J Physiol Heart Circ Physiol 278: H586-H594, 2000[Abstract/Free Full Text].

30. Weihl, C, Macdonald RL, Stoodley M, Luders J, and Lin G. Gene therapy for cerebrovascular disease. Neurosurgery 44: 239-252, 1999[ISI][Medline].

31. Yamakami, I, and McIntosh TK. Effects of traumatic brain injury on regional cerebral blood flow in rats as measured with radiolabeled microspheres. J Cereb Blood Flow Metab 9: 117-124, 1989[ISI][Medline].

32. Yoshida, K, Burton GF, Young H, and Ellis EF. Brain levels of polyethylene glycol-conjugated superoxide dismutase following fluid percussion brain injury in rats. J Neurotrauma 9: 85-92, 1992[ISI][Medline].

33. Yuan, XQ, Prough DS, Smith TL, and DeWitt DS. The effect of traumatic brain injury on regional cerebral blood flow in rats. J Neurotrauma 5: 289-301, 1988[Medline].

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