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The Journal of Neuroscience, July 13, 2005, 25(28):6561-6575; doi:10.1523/JNEUROSCI.1450-05.2005
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Cellular/Molecular
Mitochondrial Nitric Oxide Mediates Decreased Vulnerability of Hippocampal Neurons from Immature Animals to NMDA
Jeremy D. Marks,1,2,3
Chan Boriboun,1 and
Janice Wang1
1Department of Pediatrics and the Committees on 2Cell Physiology and 3Molecular Medicine, University of Chicago, Chicago, Illinois 60637
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Abstract
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Mitochondrial membrane potential (  m)-dependent Ca2+ uptake plays a central role in neurodegeneration after NMDA receptor activation. NMDA-induced m dissipation increases during postnatal development, coincident with increasing vulnerability to NMDA. NMDA receptor activation also produces nitric oxide (NO), which can inhibit mitochondrial respiration, dissipating m. Because m dissipation reduces mitochondrial Ca2+ uptake, we hypothesized that NO mediates the NMDA-induced m dissipation in immature neurons, underlying their decreased vulnerability to excitotoxicity. Using hippocampal neurons cultured from 5- and 19-d-old rats, we measured NMDA-induced changes in [Ca2+]cytosol, m, NO, and [Ca2+]mito. In postnatal day 5 (P5) neurons, NMDA mildly dissipated m in a NO synthase (NOS)-dependent manner and increased NO. The NMDA-induced NO increase was abolished with carbonyl cyanide 4-(trifluoromethoxy)phenyl-hydrazone and regulated by [Ca2+]mito. Mitochondrial Ca2+ uptake inhibition prevented the NO increase, whereas inhibition of mitochondrial Ca2+ extrusion increased it. Consistent with this mitochondrial regulation, NOS and cytochrome oxidase immunoreactivity demonstrated mitochondrial localization of NOS. Furthermore, NOS blockade increased mitochondrial Ca2+ uptake during NMDA. Finally, at physiologic O2 tensions (3% O2), NMDA had little effect on survival of P5 neurons, but NOS blockade during NMDA markedly worsened survival, demonstrating marked neuroprotection by mitochondrial NO. In P19 neurons, NMDA dissipated m in an NO-insensitive manner. NMDA-induced NO production was not regulated by m, and NOS immunoreactivity was cytosolic, without mitochondrial localization. NOS blockade also protected P19 neurons from NMDA. These data demonstrate that mitochondrial NOS mediates much of the decreased vulnerability to NMDA in immature hippocampal neurons and that cytosolic NOS contributes to NMDA toxicity in mature neurons.
Key words: NMDA; mitochondria; nitric oxide; calcium; development; mtNOS
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Introduction
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Mitochondria play important roles in neuronal death after activation of NMDA receptors, a central mechanism of hypoxic-ischemic brain injury (Rothman, 1984 ; Choi and Rothman, 1990; Beal, 1992). Excitotoxicity-induced mitochondrial dysfunction leads to energy failure (Lang-Rollin et al., 2003), neuronal necrosis (Gwag et al., 1997; Colbourne et al., 1999; Niquet et al., 2003), increased production of reactive oxygen species (Sengpiel et al., 1998; Castilho et al., 1999; Luetjens et al., 2000), and apoptosis (Ankarcrona et al., 1995; Wang et al., 2004).
Mitochondrial dysfunction during excitotoxicity depends on mitochondrial membrane potential (m)-driven uptake of Ca2+ into mitochondria, and excitotoxic neuronal death depends on this Ca2+ uptake (Dessi et al., 1995; Budd and Nicholls, 1996; Pivovarova et al., 2004). Preventing mitochondrial Ca2+ uptake by first dissipating m blocks excitotoxic neuronal death, despite the large increases in cytosolic free calcium concentration ([Ca2+]cytosol) that accompany removal of this Ca2+ sink (Stout et al., 1998). Similarly, overexpression of mitochondrial uncoupling protein 2, which modestly dissipates m, reduces neuronal death from stroke and trauma (Mattiasson et al., 2003).
In hippocampal neurons, vulnerability to excitotoxic death changes markedly during postnatal development (Liu et al., 1996; Marks et al., 1996, 2000). Thus, despite similar NMDA-induced bulk [Ca2+]i increases in immature and mature neurons, death of cultured hippocampal neurons prepared from newborn (0-5 d old) animals is minimal but increases sharply in neurons from increasingly older animals, becoming nearly universal in neurons from mature (19-25 d old) animals (Marks et al., 2000). During maturation, mitochondrial responses to NMDA also change dramatically: in neurons from newborns, NMDA induces mild, transient m dissipation, whereas those from mature animals exhibit profound, long-lasting m dissipation (Marks et al., 2000). The profound m dissipation in mature neurons may reflect mitochondrial Ca2+ uptake, energy failure, and, under some conditions, mitochondrial permeability transition pore opening (Brustovetsky and Dubinsky, 2000; Maciel et al., 2001; Kobayashi et al., 2003). However, mechanisms underlying the mild, NMDA-induced m dissipation in neurons from immature animals are unclear, as are its consequences.
Under some conditions, NMDA-induced m dissipation is abolished by inhibition of nitric oxide (NO) synthase (NOS) (Almeida et al., 1999; Keelan et al., 1999). NO dissipates m at nanomolar concentrations, reversibly competing with O2 for the reduced binuclear center CuB/a3 of cytochrome oxidase (Brown, 1999; Antunes et al., 2004). This competition transiently inhibits oxidative phosphorylation, precluding maintenance of m in the face of ongoing ATP synthesis. By dissipating m during elevations of [Ca2+]cytosol, NO may reduce mitochondrial Ca2+ uptake and subsequent cell death in neurons, a phenomenon reported in cardiomyocytes in vitro during ischemia-reperfusion injury (Rakhit et al., 2001).
Because NMDA induces mild m dissipation in newborn hippocampal neurons with little subsequent death, we hypothesized that this m dissipation results from NMDA-induced NO production and that this NO production protects neurons after NMDA. Accordingly, using cultures of hippocampal neurons from newborn and mature animals, we assessed the role played by NO production in mediating this developmentally regulated resistance to NMDA and ascertained the mechanisms underlying its regulation.
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Materials and Methods
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Culture media and supplements were obtained from Invitrogen (Carlsbad, CA). Fura-2, fura-FF, rhod-2, 3-amino-4-(N-methylamino)-2',7'-difluorofluorescein (DAF-FM), Mitofluor red, tetramethylrhodaminemethylester (TMRM), and Alexa 488-conjugated anti-cytochrome oxidase (subunit I) came from Molecular Probes (Eugene, OR). Ru-360 and Mn(III)tetrakis(4-benzoic acid)porphyrin (MnTBAP) were purchased from EMD Biosciences (San Diego, CA). 7-Chloro-5-(2-chlorophenyl)-1,5-dihydro-4,1-benzothiazepin-2(3H)-one (CGP-37157) and 1 H-[1,2,4]oxadiazolo[4,3-a]quinoxalin-1-one (ODQ) were from Biomol (Plymouth Meeting, PA). Anti-neuronal nitric oxide synthase (nNOS) was obtained from BD Transduction Laboratories (Lexington, KY). All other chemicals were from Sigma (St. Louis, MO). For epifluorescence imaging, all filters and mirrors were obtained from Chroma Technology (Brattleboro, VT).
Postnatal hippocampal neurons. Hippocampal neurons were prepared from immature (5 d old) and mature (19 d old) Sprague Dawley rats as described previously (Marks et al., 2000), with modifications. Briefly, isoflurane-anesthetized rats were decapitated, and the hippocampi were removed, sectioned (400 µm), and incubated in oxygenated, pH-buffered saline. Sections were incubated at room temperature with trypsin type XIII (0.5-1.0 mg/ml) for 30 min, then with Pronase (0.4 mg/ml) for 15 min, and mechanically triturated. Dissociated cells were centrifuged through an iodixanol density gradient (1.055-1.026 g/ml) and plated onto poly-D-lysine-coated coverslips. Coverslips were placed on a layer of cultured cortical astrocytes, maintained in DMEM supplemented with HEPES (15 mM), N2, and ovalbumin, and incubated in a humidified atmosphere containing O2 (5 ± 0.1%) and CO2 (10 ± 0.1%) at 35°C. We have shown previously that these postnatal hippocampal neurons depend on a 5% O2 atmosphere for survival in culture (Marks et al., 2000). Neurons were studied between 4 and 7 d in vitro.
Microscopy, imaging, and fluorescence quantification. Under xenon illumination, dye-loaded neurons were observed under epifluorescence using either a 40x, 1.3 numerical aperture (NA) Plan Fluor objective or a 100x, 1.40 NA Plan Apo objective in an inverted microscope (Nikon, Tokyo, Japan) and imaged with a cooled CCD camera (Photometrics, Tucson, AZ) connected to a computer workstation running Metafluor imaging software (Universal Imaging, Downington, PA). Multiple fluorophores were simultaneously used by means of polychroic mirrors, in conjunction with narrow bandpass filters in computer-controlled excitation and emission wheels. Images of a drop of dye-free perfusate were used for background correction. Non-uniform illumination in the imaging system was corrected by dividing each image by a fluorescence image of a homogenous, uranium oxide slide, and the resultant image was scaled. Background-subtracted, shading-corrected intracellular fluorescence measurements were made every 20 s before, during, and after perfusion of NMDA. For cytosolic dyes, mean somal fluorophore-specific fluorescence was calculated for each cell in the image, and fluorescence intensities were plotted on a region-by-region basis as a function of time.
Time-lapse studies. Coverslips were placed in a closed recording chamber (Warner Instrument, New Haven, CT) on the microscope stage and perfused (1-2 ml/min) with bicarbonate-buffered saline. The composition of the buffer (control buffer) was as follows (in mM): 125 NaCl, 3.0 KCl, 1.25 NaH2PO4, 1.3 Mg2SO4, 2.4 CaCl2, 10 glucose, and 26 NaHCO3. Unless otherwise stated, the perfusate was bubbled with 21% O2/5% CO2. In experiments in which pO2 was manipulated, buffers were equilibrated before the experiment by bubbling with a mixture of 5% CO2 and a calibrated O2 concentration. Perfusate pO2 was controlled using gas-equilibrated solutions that were delivered to the glass-sealed chamber with flexible stainless steel tubing. Neurons were maintained at 34.5 ± 0.2°C.
Measurement of [Ca2+]i. [Ca2+]i was measured with either fura-2 (Kd of 224 nM) or fura-FF (Kd of 5.5 µM), loaded as AM esters for 1 h at 35°C. After loading, cultures were washed in HCO3-buffered saline for at least 15 min to ensure complete hydrolysis of the AM ester. Fura dyes were sequentially excited using 10 nm bands of light centered on 340 and 380 nm, and a 40-nm wide band of fluorescence centered on 535 nm was imaged.
Measurement of changes in [Ca2+]mito. Changes in mitochondrial matrix free calcium concentrations [Ca2+]mito were measured using the cationic fluorescent calcium indicator rhod-2. Rhod-2 was reduced with NaBH4 to the nonfluorescent dihydro-rhod-2 before loading. Neurons were incubated in dihydro-rhod-2 AM (3 µM) for 1 h at room temperature in HEPES-buffered saline and then washed for 15 min in culture medium at 35°C. Neurons were excited with a 20 nm band of light centered on 548 nm, and a 40 nm wide band of fluorescence centered on 600 nm was imaged, using a 100x plan Apo objective. To decrease light emanating from outside the plane of focus, time-lapse images were deconvolved using software using maximum likelihood estimation (Huygens Essential; Scientific Volume Imaging, Hilversum, The Netherlands).
Measurement of cellular nitric oxide. Changes in intracellular NO concentration were monitored using DAF-FM, a non-fluorescent compound that is irreversibly nitrosated by an NO-dependent mechanism to a fluorescent triazole (Itoh et al., 2000). DAF-FM intensity also exhibits no pH dependence over the physiologic range (Kojima et al., 1999). Neurons were loaded with DAF-FM diacetate (10 µM) for 1 h at 35°C in culture media, and the coverslips washed in bicarbonate-buffered saline, pH 7.4, for 15 min at 35°C. Neurons were excited with a 10 nm wide band of light centered on 480 nm, and a 40 nm wide band of fluorescence centered on 535 nm was imaged. Polychroic beam splitters were used to allow simultaneous imaging of fura-2 and DAF-FM and of DAF-FM and Mitofluor red 589. Mean somal DAF-FM intensity was calculated for each neuron in the microscopic field. Time-dependent changes in somal DAF-FM intensity were expressed as percentage change from baseline (F/F). Linear regression was used to quantify the rate of triazole fluorescence rise before and during NMDA. The rate of rise during the 2-3 min immediately before NMDA was used to calculate the baseline slope. Because the rate of rise after NMDA tapered off after 5-7 min, the initial 4 min after the onset of the NMDA-induced [Ca2+]i rise was used to calculate the NMDA response. Statistical tests for repeated measures were used to assess differences between slopes in neurons obtained at baseline and during NMDA.
Measurement of m. To assess changes in m, we used TMRM, a cationic fluorophore that is concentrated within polarized mitochondria as a function of potential. We ensured that neurons were exposed to a constant concentration of TMRM throughout the experiment by diluting TMRM into bicarbonate-buffered saline solution to a concentration of 0.5 nM and then deriving all solutions used in the experiment from this stock. Neurons were incubated at 35°C for 1 h in TMRM-containing saline to allow electrochemical equilibration of TMRM across the plasma and inner mitochondrial membranes. This low concentration ensured that intramitochondrial TMRM was not quenched at baseline (polarized) mitochondrial potentials. In this way, graded m dissipation was evidenced by graded loss of TMRM fluorescence. TMRM-loaded neurons were excited with a 30 nm wide band of light centered on 560 nm, attenuated by neutral density filters to 0.003% of unfiltered intensity, and a 55 nm wide band of fluorescence centered on 605 nm was imaged. The low illumination level enabled time-lapse studies to be performed for up to 1 h without light-induced dissipation of m. We used polychroic beam splitters to allow simultaneous use of fura-2 and TMRM.
TMRM fluorescence intensities were measured over time from mitochondria-rich and -poor regions of individual neurons. To eliminate contributions to changes in mitochondrial TMRM intensity made by plasma membrane depolarization, we divided the TMRM intensity of the mitochondria-rich region by that of the mitochondria-poor region of the neuron. Corrected fluorescence ratios were then normalized to baseline ratio (100%) and the ratio obtained after dissipation of m with carbonyl cyanide 4-(trifluoromethoxy)phenyl-hydrazone (FCCP) (0%) and plotted as a function of time.
Manipulation of mitochondrial [Ca2+]. Mitochondrial Ca2+ uptake was blocked with Ru-360, a cell-permeable oxygen-bridged dinuclear ruthenium amine complex that avidly (IC50 of 184 pM) and specifically blocks Ca2+ uptake into mitochondria in vitro (Matlib et al., 1998). Ru-360 was dissolved in N2-sparged water immediately before use. Neurons were incubated in Ru-360 (10 µM) for 1 h before study. Mitochondrial Ca2+ efflux was blocked with CGP-37157, a specific blocker of the mitochondrial Na+/Ca2+ exchanger. This compound has some blocking activity at plasma membrane Ca2+ channels at the concentrations needed to block mitochondrial Ca2+ efflux (Baron and Thayer, 1997). To prevent CGP-37157 from reducing Ca2+ entry across the plasma membrane, we applied CGP-37157 according to published methods (White and Reynolds, 1997; Wang and Thayer, 2002): first perfusing neurons with NMDA briefly (1 min) and then switching the perfusate to one containing NMDA and CGP-37157 (10 µM). In preliminary experiments, we found that the magnitude and time course of the initial [Ca2+]i rise after the onset of NMDA stimulation was not different from untreated neurons.
Immunohistochemistry. Neurons were fixed in paraformaldehyde (4% for 5 min) and then washed three times in 0.1% Triton X-100. Antigen retrieval was performed by incubating coverslips in 50 mM Tris-buffered saline, pH 7.5, at 95°C for 20 min, followed by three washes in PBS. Nonspecific immunoreactivity was blocked with 10% goat serum. Cultures were incubated overnight at 4°C in PBS containing a polyclonal antibody generated against a C-terminal synthetic peptide sequence corresponding to amino acids 1095-1289 of human nNOS (1:500 dilution) and a monoclonal antibody to subunit I of human cytochrome oxidase, conjugated to the fluorescent molecule Alexa 488 (1:500 dilution). Immunoreactivity to nNOS was amplified and detected using an Alexa 594 conjugate of a goat anti-rabbit IgG antibody. Cytochrome oxidase and nNOS immunoreactivity were imaged using a 60x, 1.4 NA objective, and optical slices through the cultures were obtained using the 488 and 543 nm lines, respectively, of an Olympus Optical (Tokyo, Japan) Fluoview 200 laser scanning confocal microscope.
Induction and assessment of neuronal death. Cultures were incubated for 20 min in a sterile manner to Mg2+-free, bicarbonate-buffered saline containing NMDA (300 µM) and glycine (5 µM) at 35°C in a 5% CO2 atmosphere. Control cultures were incubated in saline without NMDA. To perform these experiments at ambient oxygen tensions, neurons were placed in a standard 5% CO2 incubator for the duration of the exposure. To perform these experiments at 3% O2/5% CO2, neurons were placed into a hypoxic work station, consisting of a glove box and an attached airlock, in which O2 and CO2 levels were continuously regulated to within ±0.1% (Coy Laboratory Products, Grass Lake, MI). Petrie dishes containing saline solutions were placed into the work station for 18 h before the experiment to ensure equilibration of oxygen tensions with the 3% environment. After exposure in either 21 or 3% O2, cultures were placed into their original media and put back into their standard incubator. Neuronal death was assessed 48 h later by means of calcein AM (1 µM) and propidium iodide (1 µM) fluorescence to identify living (green) and dead (red) neurons, respectively. Cells were illuminated with 480 nm light, and the resultant red and green fluorescence was observed using a polychroic beam splitter and narrow emission filters. Living and dead neurons were counted in 36 adjacent high-power fields in a 6 x 6 grid in each coverslip. A minimum of six coverslips per age was counted, and the percentages of survival were averaged and normalized to control survival. Statistical analysis of differences between treatments was performed with ANOVA.
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Results
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m dissipation accompanies the rise in [Ca2+]i
We first assessed the extent to which NMDA receptor activation dissipates m in hippocampal neurons cultured from postnatal day 5 (P5) rats and the temporal relationship of the m dissipation to the NMDA-induced [Ca2+]i increase. We used fura-2 to identify the onset and offset of the NMDA-induced [Ca2+]i rise. Before NMDA stimulation, baseline [Ca2+]i and corrected mitochondrial TMRM intensities were stable. After the onset of NMDA (300 µM), [Ca2+]i abruptly increased, remained elevated for the remainder of the 5 min NMDA stimulation, and then decreased monotonically after NMDA washout (Fig. 1A). NMDA transiently dissipated m, coinciding with, or immediately after (within one time-lapse imaging interval), the onset of the NMDA-induced [Ca2+]i rise. The mean peak corrected TMRM intensity change from baseline (-24.1 ± 5.4% SEM; n = 32) occurred 1-2 min into the NMDA stimulus. After NMDA removal, m returned to baseline over  15 min. NMDA-induced m dissipation and recovery was observed in every neuron tested (n = 32 neurons on 8 coverslips).
NOS activity is required for m dissipation
Dissipation of m after glutamate receptor excitotoxicity has been linked to NO production in embryonic hippocampal neuron cultures (Almeida et al., 1999; Keelan et al., 1999). To assess the role played by NO in P5 neurons, we measured NMDA-induced m dissipation in neurons in which NOS activity had been blocked by pretreatment with N -nitro-L-arginine methyl ester (L-NAME) (100 µM for 3 h). Pretreatment with L-NAME completely abolished the neuronal m dissipation induced by NMDA (-0.13 ± 4.6% SEM; n = 11; p < 0.01) (Fig. 1B), suggesting that NOS activity is required for NMDA-induced m dissipation in these P5 neurons.
Because the L-NAME-induced antagonism of m dissipation may have been attributable to smaller Ca2+ rises after NMDA, we compared NMDA-induced [Ca2+]i rises in L-NAME-incubated neurons with unexposed neurons. However, high-affinity Ca2+ reporters, such as fura-2 (Kd of 224 nM), differentiate poorly between toxic and nontoxic [Ca2+]i levels that are attained during excitotoxic stimulation (Stout and Reynolds, 1999). Consequently, we used the low-affinity Ca2+ reporter fura-FF (Kd of 5.5 µM). At baseline, fura-FF ratios did not differ significantly between control and L-NAME-treated neurons (control, 0.39 ± 0.05 vs L-NAME, 0.33 ± 0.04 arbitrary units, mean ± SEM; n = 20). Most importantly, the fura-FF ratio increase induced by NMDA (300 µM) did not differ significantly between control and L-NAME-treated neurons (control, 1.23 ± 0.28 vs L-NAME, 1.72 ± 0.34 arbitrary units, mean ± SEM; n = 20; p = 0.4). Accordingly, the marked decrease in m dissipation that we observed in the presence of L-NAME was not attributable to an L-NAME-associated decrease in bulk [Ca2+]i. Instead, blockade of m dissipation by L-NAME suggested that NO production underlies NMDA-induced m dissipation in these neurons.
To obtain additional evidence that NO production is the primary mechanism of NMDA-induced m dissipation in these P5 neurons, we measured m during NMDA in the presence of other compounds known to alter NO production (Fig. 1C). We first pretreated cultures with 7-nitroindazole (7-NI) (100 µM for 3 h), a neuronal NOS-selective antagonist structurally unrelated to L-NAME (Babbedge et al., 1993). Similar to L-NAME, we found that 7-NI blocked NMDA-induced m dissipation (3.1 ± 5.3%; n = 15; p < 0.01). We also incubated L-NAME- and 7-NI-treated neurons in a 10-fold molar excess of arginine (1 mM) to overcome the NOS blockade. Not only did arginine supplementation prevent the L-NAME-induced block of m dissipation, arginine significantly increased the degree of NMDA-induced m dissipation compared with control (44.4 ± 4.9%; n = 27; p < 0.05). Similar results were seen with arginine-supplemented neurons incubated in 7-NI.
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Figure 1. Inhibition of NOS prevents NMDA-induced m dissipation. A, Simultaneous measures over time of NMDA-induced changes in [Ca2+]i (fura-2) and m (TMRM) in the absence (left) and presence (right) of L-NAME (100 µM for 3 h). Maximal m dissipation is induced with FCCP (dotted line) at the end of each experiment. To eliminate contributions to changes in mitochondrial TMRM intensity made by plasma membrane depolarization, TMRM intensities from a mitochondria-rich region of each neuron at each point in time was divided by the corresponding intensity from a mitochondria-poor region within the same neuron. Each ratio was normalized to the mean baseline ratio (100%) and the mean ratio obtained after FCCP (0%). NMDA induces a modest m dissipation that is blocked by L-NAME. B, Population summary of mean peak [Ca2+]i increases during NMDA in the presence and absence of NOS blockade. [Ca2+]i increases are reported with fura-FF (Kd of 5.5 µM). NMDA-induced [Ca2+]i increases do not significantly differ between control and L-NAME. Inset, Representative examples of raw fura-FF responses to NMDA in control and L-NAME-treated neurons. Calibration bar, 1 min. C, NMDA-induced m dissipation is decreased during NOS blockade (L-NAME, 7-NI), and the blockade is overcome with supplemental L-arginine (Arg). MnTBAP, a superoxide dismutase mimetic, increases NMDA-induced m dissipation, suggesting that a portion of the NO generated by NMDA is converted to peroxynitrite. Statistical comparisons made between control and each treatment. *p < 0.05;  p < 0.01. A.U., Arbitrary units.
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NO reacts at diffusion-limited rates with superoxide anion (O2.) to form peroxynitrite (Huie and Padmaja, 1993). Consequently, O2. production, known to increase during NMDA (Lafon-Cazal et al., 1993; Bindokas et al., 1996), may, through peroxynitrite formation, reduce NO availability (Fennell et al., 2002). To assess whether peroxynitrite formation during NMDA reduces NO availability, we treated P5 neurons with MnTBAP, a superoxide dismutase mimetic, and measured NMDA-induced m dissipation. Baseline TMRM ratios were not significantly different in MnTBAP-treated neurons compared with untreated neurons. However, NMDA induced a significantly larger m dissipation in MnTBAP-treated neurons compared with untreated neurons (Fig. 1C), suggesting that a portion of the NO generated by NMDA in these neurons is converted to peroxynitrite, decreasing the NO effect on m. Together, these data strongly support the hypothesis that NMDA-induced m dissipation in P5 neurons is attributable to NOS activation and NO production.
NO production increases during NMDA receptor activation in P5 neurons
To characterize the temporal relationship between NO production and m dissipation in P5 neurons, we next measured cellular NO production before and during NMDA. Because m dissipates immediately after the onset of the NMDA-induced [Ca2+]i increase, we used the onset of this [Ca2+]i increase as a proxy for the onset of m dissipation. To estimate NMDA-induced changes in NO production, we simultaneously measured time-dependent changes in fura-2 and DAF-FM fluorescence, a pH-independent, NO-specific indicator (Itoh et al., 2000; Kojima et al., 2001). We used linear regression to quantify the slope of the DAF-FM fluorescence increase before and during the first 4 min of NMDA stimulation, beginning with the onset of the [Ca2+]i rise. To confirm that the low intensity of UV and visible light excitation used in these fura-2/DAF-FM experiments did not induce noticeable DAF-FM nitrosation, we first performed control time-lapse experiments, measuring changes in DAF-FM intensity every 20 s in the absence of NMDA. Each DAF-FM exposure was preceded by acquisition of fura-2 images at 340 and 380 nm excitation. We observed no significant changes in DAF-FM slope from baseline over 30 min, the length of a typical experiment (n = 18). Accordingly, under our experimental conditions, the increases in DAF-FM fluorescence we report are not the result of illumination.
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Figure 2. NMDA increases NO production in postnatal hippocampal neurons. A, Simultaneously obtained measures (every 20 s) of changes in [Ca2+]i (fura-2) and NO (DAF-FM) in response to NMDA (bar). The slope of DAF-FM fluorescence begins to increase coincident with the upstroke of the [Ca2+]i rise. The boxes around the DAF-FM traces identify the regions used to calculate DAF-FM slopes at baseline and during the initial response to NMDA. B, Calculation of DAF-FM slopes. Data comprising the DAF-FM traces within the boxes in A are presented, and lines produced by linear regression of each trace are superimposed on each trace. Beside each line is presented the calculated DAF-FM slope and the correlation coefficient (r2) of each regression. Because of crowding, the calculated slope and r2 for the middle baseline trace has been omitted. C, NMDA-induced increases in DAF-FM slope are prevented by NOS inhibition with L-NAME and increased with MnTBAP, a superoxide dismutase mimetic. Mean ± SEM DAF-FM slopes at baseline and during the initial 4 min of NMDA stimulation obtained by linear regression in untreated neurons and neurons in which NO production has been blocked (L-NAME) or increased (MnTBAP). MnTBAP, by removing O2., prevents NO consumption by decreasing peroxynitrite formation, increasing NO availability. Statistical comparisons are made within treatments, comparing the DAF-FM slope during NMDA with that slope during baseline. *p < 0.05; p < 0.01. A.U., Arbitrary units.
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During NMDA, the rate of rise of DAF-FM fluorescence increased markedly over the baseline slope in 17 of 21 neurons initially studied. This increase occurred immediately on the onset of the [Ca2+]i rise (Fig. 2, top). The mean DAF-FM slope during NMDA was significantly greater compared with the mean baseline slope (n = 34 slopes in 17 neurons; p < 0.01 by t test for repeated measures) (Fig. 2, bottom). To confirm that these DAF-FM fluorescence increases reflect increased NO, we used pharmacological agents to alter NMDA-induced NO production (Fig. 2, bottom). Thus, L-NAME pretreatment (100 µM for 3 h) decreased the DAF-FM slope at baseline and completely blocked the NMDA-induced slope increase (n = 20; p < 0.01). Similar results were obtained with 7-NI pretreatment. Finally, because we had observed that MnTBAP increased the magnitude of NMDA-induced m dissipation, consistent with the reduction of NO availability through its interaction with O2. to form peroxynitrite, we assessed whether MnTBAP pretreatment increased the NMDA-induced DAF-FM slope increase. No significant differences were observed at baseline in MnTBAP-pretreated neurons. However, NMDA induced significantly larger DAF-FM slope increases compared with untreated neurons (n = 25). These findings demonstrate that NMDA increases NO production in P5 hippocampal neurons during the initial [Ca2+]i rise, consistent with our finding of NOS-mediated m dissipation during the same period, and suggest that a portion of this NO production is converted to peroxynitrite.
To assess whether the DAF-FM rise depended on the [Ca2+]i rise induced by NMDA, we measured DAF-FM and fura-2 responses to NMDA in the absence of extracellular Ca2+, using an otherwise identical perfusate containing EGTA (5 mM) and no added Ca2+. Removal of extracellular Ca2+ completely blocked both the NMDA-induced [Ca2+]i rise and the increase in DAF-FM slope during NMDA (n = 41), demonstrating its dependence on the NMDA-induced [Ca2+]i increase. Thus, this Ca2+-dependent increase in NO that occurs during NMDA receptor activation likely mediates the NOS-dependent m dissipation that occurs during NMDA.
Increased NO production and m dissipation are specific to NMDA receptor activation
We next asked whether the m dissipation and increased NO production that we observed after NMDA also occurred after [Ca2+]i increases that were not mediated by NMDA. We induced a [Ca2+]i rise through activation of plasma membrane voltage-gated Ca2+ channels, by depolarizing neurons with an otherwise identical, bicarbonate-buffered saline solution, in which 60 mM NaCl had been replaced with KCl. During 5 min exposures to high K+ solution, the somal fura-2 ratio significantly increased (mean ± SEM ratios, baseline, 0.5 ± 0.06 vs depolarizing solution, 1.05 ± 0.05 arbitrary units; n = 23; p < 0.01) (Fig. 3, left inset). In contrast, the slope of DAF-FM fluorescence did not change significantly (slope increase, 0.52 ± 0.42%/min, mean ± SEM; n = 23; p = 0.23) (Fig. 3, left bottom). Furthermore, in separate experiments using TMRM, we observed no m dissipation during exposure to depolarizing solutions (mean ± SEM loss of TMRM fluorescence, baseline, -2.7 ± 0.8% vs depolarization, -4.6 ± 1.5%; n = 19) (Fig. 3, left top). The lack of m dissipation during plasma membrane depolarization also provides additional evidence that the change in TMRM fluorescence observed during NMDA does not represent an artifact of plasma membrane depolarization but rather m dissipation.
NMDA dissipates m as a function of O2 concentration
Having found an NO increase temporally associated with NMDA-induced m dissipation, we next sought to characterize the mechanisms by which NO dissipates m in this context. We first assessed whether m dissipation depended on NO-mediated activation of soluble guanylate cyclase, by treating neurons, before NMDA, with the guanylate cyclase inhibitor ODQ (10 µM for 30 min). ODQ-treated neurons demonstrated the identical degree of NMDA-induced TMRM decrease compared with untreated neurons (ODQ, 29.1 ± 4.5% vs control, 29.4 ± 5.1%; n = 66; p = 0.95), indicating that guanylate cyclase activation plays no role in NO-mediated m dissipation.
A more likely, well described mechanism (Brown, 2001) is the binding of NO to the binuclear CuB/cytochrome a3 site of cytochrome c oxidase (E.C. 1.9.3.1
[EC]
) (Webb, 1992), the terminal complex of the mitochondrial respiratory chain. Because NO binding to cytochrome c is competitive, the amounts of NO-induced respiratory inhibition and m dissipation vary as a function of O2 concentration (Brown and Cooper, 1994). Using tanks of known O2 concentrations (95, 21, 9, and 1%) and an oxygen-impermeable experimental setup, we clamped the pO2 within the experimental chamber to known values and assessed the relationship between pO2 and the magnitude of NMDA-induced TMRM fluorescence loss. For each O2 concentration studied, we first recorded the level of fura-2 and TMRM fluorescence in 21% oxygen and then switched the perfusate to one equilibrated with a different O2 concentration for 5 min before administering NMDA. In the absence of NMDA, neither fura-2 nor TMRM fluorescence changed as a result of altering chamber O2 concentration. Importantly, however, we did observe that the lower the pO2 concentration, the more NMDA stimulation dissipated m (Fig. 4). Correlation analysis revealed a significant, negative, linear relationship between pO2 and NMDA-induced m dissipation magnitude (r = 0.27; p < 0.01; n = 111). Accordingly, the O2 dependence of this response supports the hypothesis that NMDA-induced NO production dissipates m by competitively binding to cytochrome c oxidase.
NMDA-induced NO production is regulated by m and depends on increases in [Ca2+]mito
Because mitochondrial respiratory inhibition appears central to NO-induced m dissipation in these neurons, we asked whether mitochondria themselves regulate NO production. We first assessed whether mitochondrial polarization is required for NO production by measuring NMDA-induced NO production in neurons in which m was dissipated with the protonophore FCCP. To prevent the ATP consumption that accompanies uncoupling of oxidative phosphorylation from ATP synthesis, neurons were first incubated in oligomycin (2 µg/ml) for 3 min, and the slope of DAF-FM fluorescence increase was measured. Next, cells were exposed to FCCP (1 µM) for 3 min, and the DAF-FM fluorescence slope was measured again. Neither oligomycin alone nor oligomycin with FCCP significantly affected the slope of the DAF-FM fluorescence increase compared with untreated neurons (mean ± SEM, untreated, 1.36 ± 0.07%/min; oligomycin, 1.38 ± 0.13%/min; oligomycin plus FCCP, 1.13 ± 0.15; n = 35; p = NS). Finally, oligomycin and FCCP-treated neurons were exposed to NMDA (300 µM) for 5 min. Under conditions of m dissipation, the NMDA-induced increase in DAF-FM slope was completely blocked (mean ± SEM, untreated, 2.63 ± 0.16%/min vs FCCP, 0.97 ± 0.14%/min; n = 35; p < 0.02) (Fig. 5). Accordingly, NMDA-induced NO production depends on either a polarized m or conditions within the mitochondrion that are abolished with m dissipation.
Dissipation of m abolishes the driving force for Ca2+ entry into the mitochondria, resulting in loss of intramitochondrial free Ca2+ via the mitochondrial Na+/Ca2+ exchanger. Because neuronal NOS activity is Ca2+ dependent (Mayer et al., 1992), we hypothesized that the dependence of NMDA-induced NO production on m reflects a dependence on increased mitochondrial matrix [Ca2+] ([Ca2+]mito). Accordingly, we compared the rates of DAF-FM fluorescence increases in neurons in which mitochondrial Ca2+ uptake and efflux were individually blocked. We first prevented mitochondrial Ca2+ uptake with Ru-360, a cell-permeable, oxygen-bridged dinuclear ruthenium amine complex. In neurons incubated in Ru-360 (10 µM for 1 h), the slope of DAF-FM fluorescence at baseline was not significantly different from untreated neurons. Similar to FCCP-treated neurons, in Ru-360-treated neurons, NMDA failed to increase the slope of DAF-FM fluorescence (Fig. 5), although the NMDA-induced [Ca2+]i rise was unchanged. Thus, NMDA-induced NO production in these P5 neurons depends on Ca2+ influx into mitochondria. Next, mitochondrial Ca2+ efflux was blocked using CGP-37157 (10 µm), a specific inhibitor of mitochondrial Na+/Ca2+ exchange, added after the first minute of the 5 min NMDA stimulus. Consistent with our hypothesis, in CGP-37157-treated neurons, NMDA significantly increased the DAF-FM slope compared with neurons exposed to NMDA alone (mean ± SEM, CGP-37157, 3.23 ± 0.44%/min vs control, 2.63 ± 0.16%/min; n = 24; p < 0.01) (Fig. 5). Together, these data show that NMDA-induced NO production in these immature neurons depends on an increase in [Ca2+]mito.
Localization of neuronal NOS and NO production within mitochondria in P5 neurons
Our finding that [Ca2+]mito regulates NO production suggested that these immature neurons harbor a Ca2+-regulated NOS within mitochondria. Accordingly, we looked for mitochondrial localization of NOS using double immunofluorescence: we simultaneously stained cultures using an anti-nNOS polyclonal antibody and a monoclonal anti-cytochrome oxidase antibody and used confocal microscopy to assess staining patterns and mitochondrial colocalization. P5 neurons did not demonstrate cytosolic staining for nNOS. Instead, punctate staining was seen in most somata that primarily excluded the nucleus. Simultaneous staining for cytochrome oxidase demonstrated that the majority of nNOS staining colocalized with mitochondria (Fig. 6, top). Assessment of the amount of fluorescence occurring from nonspecific binding of the anti-rabbit secondary antibody was performed with the secondary antibody alone. This staining revealed faint labeling of the nucleus only without mitochondrial colocalization. By demonstrating localization of nNOS to mitochondria, these studies provide anatomic evidence for the existence of a mitochondrially localized nNOS within these neurons.
Having found mitochondrial colocalization of nNOS in these neurons, we next looked for physiological evidence of mitochondrially localized NO production during NMDA stimulation using neurons loaded with DAF-FM and Mitofluor red 589, a m-independent mitochondrion-selective dye. To detect localized changes in DAF-FM fluorescence induced by NMDA, we imaged DAF-FM and Mitofluor red 590 every 20 s before and during NMDA (300 µM) stimulation. Images were digitally deconvolved to remove out-of-focus light. To identify regions in which NMDA increased DAF-FM, we subtracted, on a pixel-by-pixel basis, the DAF-FM image obtained immediately before NMDA onset from each DAF-FM image obtained during NMDA stimulation. Within 40-60 s of the onset of NMDA, DAF-FM fluorescence appeared in highly localized regions within neurons and steadily increased over 5 min. To assess mitochondrial localization of this fluorescence, subtracted images were superimposed onto the deconvolved Mitofluor red 589 images obtained at the same points during the experiment. This superimposition revealed that the initial DAF-FM fluorescence was highly localized to mitochondria, both in processes and soma, before spreading to nonmitochondrial regions of the soma (Fig. 6, bottom) (supplemental data, available at www.jneurosci.org as supplemental material). Identical experiments and analyses of NMDA-induced DAF-FM localization within Mitofluor red 589-identified mitochondria, performed using L-NAME-treated P5 neurons (n = 7), demonstrated no cellular DAF-FM increases. Furthermore, the identical image analysis used to detect mitochondrial DAF-FM increases failed to demonstrate any localization of DAF-FM within mitochondria. Thus, the combination of mitochondrial localization of NMDA-induced DAF-FM fluorescence and immunostaining evidence of mitochondrially localized nNOS provides anatomic and physiological evidence of NMDA-induced NO production within mitochondria in these hippocampal neurons.
NMDA-induced NO production decreases vulnerability of P5 neurons to NMDA
Vulnerability to NMDA is decreased in neurons from immature animals compared with those from mature animals (Liu et al., 1996; Marks et al., 2000). Because protonophore-induced m dissipation before excitotoxicity prevents neuronal death in vulnerable neurons (Stout et al., 1998), we hypothesized that the NO-mediated m dissipation we observed during NMDA in these P5 neurons contributed to their decreased vulnerability to NMDA. To assess the role of NO production in neuronal susceptibility to NMDA, NOS activity was blocked in neuronal cultures with L-NAME (100 µM for 3 h). Then, half of the L-NAME-incubated cultures, as well as half of sister cultures not incubated in L-NAME, were exposed to NMDA (300 µM) in ambient (21%) O2 for 20 min, and survival was assessed 48 h later. Mean ± SEM survival of control neurons was 96.3 ± 4.2%. In the absence of NMDA, survival of L-NAME-treated neurons was not significantly different from control neurons, and NMDA decreased survival by 25%. L-NAME pretreatment significantly worsened survival after NMDA but by only 10% (n = 36 coverslips; p < 0.01) (Fig. 7A).
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Figure 6. Anatomic and physiologic evidence of NO production within mitochondria of P5 neurons. A, Staining patterns of immunoreactivity to nNOS and subunit I of mitochondrial cytochrome oxidase as visualized by confocal microscopy. nNOS binding (red) was identified with a fluorescent (Alexa 594) secondary antibody; cytochrome oxidase binding (green) was visualized through direct conjugation to Alexa 488. The yellow in the overlay indicates mitochondrial colocalization of nNOS. Scale bar, 20 µm. B, High-resolution confocal images of NOS and cytochrome oxidase immunoreactivity in the soma of a P5 neuron. Note the extensive colocalization of NOS with cytochrome oxidase and the almost complete absence of extramitochondrial NOS immunoreactivity. Scale bar, 10 µm. Bottom, Mitochondrial localization of NO production during NMDA. Neurons loaded with DAF-FM and Mitofluor red 589, a m-independent mitochondrial dye, were perfused with NMDA (300 µM) for 5 min. DAF-FM fluorescence that had accumulated before NMDA was removed from images obtained during NMDA stimulation by subtracting the DAF-FM image obtained immediately before NMDA from all subsequent images. Mitofluor (red) and DAF-FM (green) images were obtained sequentially every 20 s, deconvolved to remove out-of-focus light, and overlaid to assess mitochondrial colocalization, which appears as yellow. This representative montage shows images obtained at different times (top right corner of each image) immediately before and during NMDA perfusion. Three neurons (outlined, with nuclei labeled N) are shown. By 80s of NMDA stimulation, NO is clearly visualized first within mitochondria (arrows), with little extramitochondrial staining. As NMDA stimulation continues, increasing numbers of mitochondria demonstrate NO production, with NO extending to nonmitochondrial regions only by 160 s.
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Because we had found that the magnitude of NO-mediated m dissipation markedly increased at progressively lower O2 concentrations, we predicted that the magnitude of NO-mediated neuroprotection would similarly depend on O2 concentration. Accordingly, we performed the identical survival assays on P5 neurons (n = 18 coverslips) at 3% O2, an O2 concentration similar to that measured in rodent hippocampus in vivo (Feng et al., 1988; Buerk and Nair, 1993). Mean survival of P5 neurons after a 20 min exposure to control saline in 3% O2 was 89.0 ± 1.6%, and survival of L-NAME-treated neurons was not significantly different from control. Remarkably, NMDA (300 µM) did not reduce survival from control values (Fig. 7B). In L-NAME-treated neurons, however, NMDA markedly decreased neuronal survival to 43% of control (p < 0.01). Thus, at physiologic O2 tensions, NMDA-induced NO production provided robust protection from NMDA toxicity.
To better understand the mechanism of this NO-mediated neuroprotection, we assessed the role played by activation of soluble guanylate cyclase after NMDA-induced NO production. Neuronal cultures were treated with ODQ (10 µM for 30 min) to inhibit soluble guanylate cyclase. Then, half of the ODQ-exposed cultures as well as half of sister cultures not exposed to ODQ were exposed to NMDA (300 µM) in 21% O2 for 20 min, and survival was assessed 48 h later. Survival after ODQ alone (mean ± SEM, 101.2 ± 1.8% of control) was not significantly different from control. As observed in other experiments, survival after NMDA (mean ± SEM, 67.4 ± 3.2% of control) was significantly decreased from control (p < 0.05). However, survival of ODQ-treated neurons after NMDA (mean ± SEM, 69.1 ± 6.1% of control) was not significantly different from survival of NMDA-treated neurons not exposed to ODQ (n = 16 coverslips). Thus, NO-mediated neuroprotection of immature hippocampal neurons after NMDA does not depend on activation of soluble guanylate cyclase.
Mitochondria-regulated NO production decreases mitochondrial Ca2+ uptake
We next assessed whether NO production, by virtue of its mild dissipation of m, decreases NMDA-induced mitochondrial Ca2+ uptake. We measured changes in [Ca2+]mito using rhod-2, a fluorescent cationic Ca2+ indicator that accumulates in mitochondria (Fig. 8A). To restrict our measurements to in-focus mitochondria, we analyzed digitally deconvolved images. To confirm that rhod-2 fluorescence reported changes in [Ca2+]mito, we first measured changes in rhod-2 intensity in response to m dissipation induced by oligomycin (2 mg/ml) and FCCP (1 µM). This mitochondrial inhibition abruptly and uniformly decreased mitochondrial rhod-2 fluorescence to background levels. Subsequently, oligomycin and FCCP were applied at the end of every rhod-2 experiment with the same results. Next, we blocked mitochondrial Ca2+ uptake with Ru-360 incubation (10 µM for 1 h) and applied NMDA (300 µM) for 5 min. In contrast with untreated neurons (see below), Ru-360-treated neurons failed to demonstrate a significant increase in mean peak rhod-2 fluorescence during NMDA (mean ± SEM, 3.7 ± 1.4%; n = 7) (Fig. 8C). Thus, rhod-2 reliably reported changes in [Ca2+]mito.
We next measured NMDA-induced increases in [Ca2+]mito in the presence and absence of previous nNOS blockade (100 µM L-NAME for 3 h). Mitochondrial rhod-2 fluorescence was stable before NMDA. During NMDA stimulation, rhod-2 fluorescence abruptly increased (Fig. 8B). In control neurons, rhod-2 fluorescence increased by an average of 17.0 ± 2.5% (mean ± SEM; n = 14) and remained elevated during NMDA, returning to baseline over the subsequent 5 min (Fig. 7B). In L-NAME-treated neurons, however, the rhod-2 fluorescence increase was almost twice the control increase (mean ± SEM, 30.0 ± 2.8%; n = 25; p < 0.01) (Fig. 8B,C). Furthermore, rhod-2 remained elevated above baseline for 5-7 min longer than control neurons. Thus, NMDA-induced NO production decreased the magnitude of the [Ca2+]mito rise and shortened the length of time during which [Ca2+]mito was elevated.
To obtain additional evidence that NMDA-induced NO production decreases mitochondrial Ca2+ uptake, we stimulated L-NAME-treated and control neurons with NMDA and then measured the amount of Ca2+ released into the cytosol after FCCP-induced m dissipation according to the method of Brocard et al. (2001). FCCP-induced changes in [Ca2+]cytosol were measured with the low-affinity Ca2+ indicator fura-FF. NMDA (300 µM for 5 min) induced an increase in fura-FF ratio that declined after NMDA removal. In control neurons, FCCP, applied 5 min after the end of NMDA, transiently increased fura-FF ratios in a small percentage of neurons; in the majority of control neurons, the fura-FF ratio continued to decline (Fig. 8D). In contrast, in neurons subjected to nNOS blockade, FCCP caused a marked increase in fura-FF ratio in all neurons studied (Fig. 8D). To quantify this Ca2+ release, we measured the baseline-subtracted areas under the curves (AUCs) of fura-FF during FCCP: L-NAME-treated neurons exhibited a significantly larger mean AUC compared with control neurons (n = 61; p < 0.01) (Fig. 8E), indicating that NOS blockade increases the amount of Ca2+ released from the mitochondria and, hence, the amount of m-dependent Ca2+ uptake during NMDA. These data, together with the increased NMDA-induced rhod-2 transients in nNOS-inhibited neurons, indicate that endogenous NO decreases mitochondrial Ca2+ uptake in P5 neurons during NMDA.
In neurons from mature rats, NO does not mediate NMDA-induced m dissipation but does mediate NMDA toxicity
In contrast to protecting neurons from NMDA toxicity, as seen in immature neurons, NMDA-induced NO production has been shown to kill neurons in the brains of mature animals, as well as in cultured embryonic neurons maintained in vitro for >10 d (Dawson et al., 1991; Schulz et al., 1995; Keelan et al., 1999). We wanted, therefore, to define how the role of NMDA-induced NO production changes during postnatal development. Accordingly, we compared our findings in P5 neurons with those of hippocampal neurons cultured from P19 rats and studied at the same time in vitro. These neurons from mature animals demonstrate much greater vulnerability to NMDA toxicity than do P5 neurons (Marks et al., 2000).
We first assessed the extent of NMDA-induced m dissipation and whether NO production played a role in any dissipation. In contrast to the modest m dissipation seen in neurons from 5-d-old animals (-24.1 ± 5.4%, mean ± SEM; see above), neurons from 19-d-old animals demonstrated almost complete m dissipation during NDMA (mean peak dissipation, -73.8 ± 6.6%; n = 6) (Fig. 9A). This dissipation typically lasted for 30-40 min. In marked contrast to P5 neurons, blockade of NOS activity with L-NAME pretreatment (100 µM for 3 h) failed to alter the magnitude or duration of NMDA-induced m dissipation (n = 35) (Fig. 9A). Because this greater m dissipation in P19 neurons compared with that of P5 neurons could be attributable to larger NMDA-induced [Ca2+]i increases, we assessed the magnitude of the [Ca2+]i rise after NMDA with fura-FF. Surprisingly, mean peak fura-FF ratios during NMDA were much smaller in these mature neurons (0.33 ± 0.01, mean ± SEM; n = 14) (Fig. 9B) compared with those ratios in P5 neurons (1.23 ± 0.28, mean ± SEM; see above). These smaller peak ratios suggest that NMDA does not elevate [Ca2+]cytosol in P19 neurons to levels achieved in P5 neurons. However, greater Ca2+ loading into P19 neurons during NMDA compared with P5 neurons cannot be excluded as a contributory mechanism to the increased m dissipation without electrophysiological measurement of whole-cell current densities. Nonetheless, these data demonstrate that NO production does not mediate the profound m dissipation that occurs in these mature neurons during NMDA.
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Figure 8. NMDA-induced NO production decreases mitochondrial Ca2+ loading. A, Neurons loaded with rhod-2. This image and all images used for quantification were deconvolved to remove out-of-focus light. Scale bar, 20 µm. B, NOS blockade with L-NAME (100 µM for 3 h) induces greater increases in [Ca2+]mito (reported by rhod-2) compared with control neurons. Two representative experiments are overlaid for comparison. Each trace is the average of five neurons. Vertical lines represent SDs. In addition to the greater NMDA-induced rhod-2 increase in the L-NAME-treated neurons, note also that, in the L-NAME-treated neurons, [Ca2+]mito has not declined by 5 min after the end of NMDA, whereas, in control neurons, [Ca2+]mito has returned to baseline levels. C, Population summary of mean peak rhod-2 increases during NMDA stimulation comparing control neurons with neurons incubated in Ru-360 (10 µM for 1 h), a specific inhibitor of mitochondrial Ca2+ uptake, and neurons incubated in L-NAME. As predicted, Ru-360 blocks the NMDA-induced rhod-2 rise, whereas nNOS inhibition with L-NAME significantly increases it. D, NOS inhibition increases mitochondrial Ca2+ loading during NMDA. Mitochondrial Ca2+ loading was quantified by stimulating control and L-NAME-treated neurons (100 µM for 3 h) with NMDA (300 µM for 5 min) and then measuring changes in [Ca2+]cytosol after FCCP-induced m dissipation. Changes in [Ca2+]cytosol were reported with fura-FF. With this dye (Kd for Ca2+ of 5.5 µM), FCCP causes a small fluorescence increase in a few control neurons. In contrast, NOS-inhibited neurons exhibit marked fura-FF increases in all neurons, demonstrating greater mitochondrial Ca2+ release and, hence, greater mitochondrial Ca2+ loading during NMDA. E, Quantification of the fura-FF AUC during FCCP stimulation. In L-NAME-treated neurons, the AUC is significantly greater than in control neurons. The AUC is negative in control neurons because the fura-FF fluorescence continued to fall in most neurons during FCCP. *p < 0.05; p < 0.10.
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Having obtained evidence that NO does not mediate the NMDA-induced m dissipation in mature neurons, we assessed what role NO plays in determining neuronal survival after NMDA. We measured survival 48 h after NMDA in cultures exposed and unexposed to previous nNOS blockade (L-NAME, 100 µM for 3 h). We first performed these studies (n = 24 coverslips) in 21% O2. Baseline survival of P19 neurons after a 20 min exposure to saline was 71.6 ± 0.3% (mean ± SEM). In the absence of NMDA, L-NAME had no statistically significant effect on survival. After NMDA in the absence of L-NAME, fewer than 35% of neurons survived (p < 0.01) (Fig. 9C). However, in stark contrast to the neuroprotection seen in P5 neurons, L-NAME pretreatment provided marked neuroprotection, increasing neuronal survival to levels not significantly different from control neurons (Fig. 9C).
Because, in P5 neurons, we had found that NO effects were increased at lower O2 tensions, we confirmed that NO-induced neurotoxicity in P19 neurons did not change at a lower O2 tension. We performed the identical survival studies using 3% O2-equilibrated solutions (n = 18 coverslips). Control survival of P19 neurons 48 h after a 20 min exposure to saline was 76.7 ± 0.02%, slightly higher than under 21% O2. Survival after NMDA in 3% O2 decreased markedly compared with control (p < 0.01) and to a similar extent seen in 21% O2. Similarly, L-NAME pretreatment provided marked neuroprotection, just as observed in 21% O2, with survival after NMDA not significantly different from control (Fig. 9D). Thus, in P19 neurons, and in contrast to P5 neurons, NO production mediates much of the toxicity of NMDA.
NMDA induces greater NO production in P19 neurons
The contrast between NO-mediated neuroprotection in P5 neurons and NO-induced neurotoxicity in P19 neurons suggested that P19 neurons may differ from P5 neurons in either the magnitude or intracellular location of NMDA-induced NO production. Therefore, we first measured changes in NO production during NMDA using DAF-FM and linear regression (Fig. 10). The mean baseline slope of DAF-FM fluorescence increase in P19 neurons was approximately half of that seen in P5 neurons (n = 26; p < 0.01). Similar to P5 neurons, NMDA induced a significantly greater DAF-FM slope compared with baseline (Fig. 10). However, the mean slope increase during NMDA was not significantly different from that observed in P5 neurons (mean ± SEM, P19, 3.1 ± 0.4%/min < |
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Abstract
Introduction
