Abstract
Heme oxygenase (HO) converts heme to carbon monoxide (CO) and biliverdin, which is metabolized rapidly to bilirubin. CO is implicated as an intercellular messenger, whereas bilirubin could function as an antioxidant. These cellular functions differ significantly from those of HO in peripheral tissues, in which it degrades heme from senescent erythrocytes, suggesting that the regulation of HO may differ in neurons from that in other tissues. Among neurons, olfactory receptor neurons have the highest level of HO activity. Metabolic labeling with [2-14C]glycine or δ-[3H]aminolevulinic acid ([3H]ALA) was used to investigate heme metabolic turnover and CO biosynthesis in primary cultures of olfactory receptor neurons. The production rates of heme precursors and metabolites from [14C]glycine over 6 hr were (in pmol/mg protein): 100 for ALA, 8.2 for heme, and 2.9 for CO. Taking into account endogenous heme content, the amount of total CO production was determined to be 1.6 nmol/mg protein per 6 hr. Heme biosynthesis usually is subject to end-product negative feedback at the level of ALA synthase. However, metabolic control in these neurons is different. Both heme concentration (heme formation) and HO activity (heme degradation) were enhanced significantly during immature stage of neuronal differentiation in culture. Neuronal maturation, which is accelerated by transforming growth factor-β2 (TGF-β2), suppressed the activities of both heme biosynthesis and degradation. To explore the physiological importance of this endogenous production of CO, we examined the potency of CO as a soluble guanylyl cyclase activator. Exogenous CO (10–30 μm), comparable to endogenous CO production, significantly activated guanylyl cyclase, suggesting that HO activity may regulate cGMP levels in the nervous system.
Recent interest has focused on the role of CO as a member of the class of diffusible messenger molecules involved in intercellular neuronal communication (Stevens and Wang, 1993; Zhuo et al., 1993; Leinders-Zufall et al., 1995; Nathanson et al., 1995;Prabhakar et al., 1995; Ingi et al., 1996). CO is generated by the action of heme oxygenase (HO), which degrades heme to CO and biliverdin, which is then converted to bilirubin. Because CO shares some of the chemical and biological properties of nitric oxide (NO), it is able to bind to the iron in heme associated with soluble guanylyl cyclase, leading to activation of the enzyme (Brüne and Ullrich, 1987; Furchgott and Jothianandan, 1991; Kharitonov et al., 1995). A role for CO as a physiological messenger was suggested in long-term potentiation in hippocampus (Stevens and Wang, 1993; Zhuo et al., 1993), chemosensors of the carotid body (Prabhakar et al., 1995), regulation of cyclic nucleotide-gated channels in olfactory receptor neurons (Leinders-Zufall et al., 1995), and regulation of Na, K-ATPase in cerebellum (Nathanson et al., 1995). In addition, bilirubin has been proposed to function as a neuronal antioxidant. These roles differ substantially from that of heme metabolism in peripheral tissues (in which it acts to degrade heme from senescent blood cells), suggesting that the regulation of HO may be different in brain, as well. HO consists of two homologous isozymes (Maines, 1988). Whereas type 1 (HO-1) is induced by heme and is most abundant in the spleen and liver, where it is responsible for destruction of heme from senescent red blood cells (Cruse and Maines, 1988), type 2 (HO-2) is the constitutive form expressed at high levels in the brain. The colocalization of ALA synthase (ALAS) with HO-2 in the brain indicates that the machinery for porphyrin turnover and CO biosynthesis occurs together (Verma et al., 1993).
Cultures of olfactory receptor neurons have been used to investigate the relationship of CO to cGMP levels, because these cells have high levels of HO activity but no NOS activity (Verma et al., 1993; Ingi and Ronnett, 1995; Leinders-Zufall et al., 1995). Thus, the relevance of CO as a mediator of cGMP can be studied in this cell in the absence of NO, a more potent activator of soluble guanylyl cyclase, which could confound results. Inhibition of HO activity and CO production significantly lowered endogenous cGMP levels in these cells (Verma et al., 1993; Ingi and Ronnett, 1995). These lines of evidence suggest that CO may function as an endogenous regulator of cGMP levels.
In this study, metabolic labeling of heme was used to investigate the regulatory mechanism of porphyrin turnover and CO production caused by heme degradation under physiological conditions in primary cultures of olfactory receptor neurons. With this approach, we directly demonstrate the significant level of both endogenous heme production and turnover in neurons, the neuronal regulatory mechanism of heme turnover, and the involvement of heme turnover in neuronal differentiation. On the basis of these results, we have gone on to demonstrate that addition of exogenous CO at the determined physiological concentrations can augment cGMP production. Our observations suggest the physiological relevance of heme turnover in the nervous system and the role of CO as a cGMP regulator. These biochemical data provide a first step toward further studies aimed at the physiological relationship of CO production with odors stimulation and other neurotransmitters, including their possible involvement in olfactory neuronal development and signal transduction.
MATERIALS AND METHODS
Materials. [2-14C]-glycine (57 mCi/mmol) was purchased from ICN Biomedicals (Cleveland, OH), and δ-[3,5-3H]aminolevulinic acid (1.87 Ci/mmol) was obtained from DuPont NEN Radiochemicals (Wilmington, DE). Zn protoporphyrin 9 (ZnPP9) was obtained from Porphyrin Products.
Assay of heme oxygenase activity. Microsomes were prepared from each tissue as previously described (Schacter, 1978). Heme oxygenase activity was measured by the method of Tenhunen et al. (1970a). Briefly, the 1.0 ml reaction mixture contained 0.1 m potassium phosphate buffer (pH 7.4), microsomes (1 mg of protein), 17 μm hemin, 180 μm NADPH, and purified biliverdin reductase (step 3, 1 mg of protein) (Tenhunen et al., 1970b). The reaction was performed for 10 min at 37°C. Blank assays were conducted in the absence of NADPH. The rate of bilirubin formation was calculated from the rate of increase in absorbance (468 nm). The extinction coefficient, obtained with standards in the reaction mixture, was 13.9 mm−1cm−1.
Cell culture. Primary cultures of olfactory receptor neurons were prepared from neonatal rats, as previously described (Ronnett et al., 1991), and cultured for 5 d in 24 well plates, 6 well plates, 9 cm dishes (for extraction assays and RT-PCR), or slide flasks (for 14CO assay), with modified Eagle’s medium containing D-valine (MDV; Life Technologies, Grand Island, NY) containing 15% (v/v) dialyzed fetal calf serum (Life Technologies), gentamycin, kanamycin, nerve growth factor (Collaborative Research, Bedford, MA), and cytosine arabinoside. These cultures contained <5% glial contaminants (Ronnett et al., 1991).
Cellular uptakes of [14C]glycine and [3H]ALA. Olfactory receptor neuron cultures in 24 well plates were incubated with 2 μCi/ml of [14C]glycine or 40 μCi/ml of [3H]ALA for 6 hr. At indicated time intervals after the addition of radiolabeled materials, cells were transferred into eppendorfs and washed three times in ice-cold PBS, and the cellular radioactivity was counted.
Extraction and quantitation of labeled ALA. This procedure was performed essentially as described (Ebert et al., 1970; Gardner et al., 1991). Briefly, cultures were incubated with [14C]glycine as described above. After stopping the incubation with [14C]glycine by addition of ice-cold PBS and rapid centrifugation, the cell pellets were washed three times by centrifugation and lysed in 200 μl of 0.2% (w/v) aqueous sodium deoxycholate. The solubilized protein was precipitated by addition of 50% (w/v) trichloroacetic acid (TCA) to a final concentration of 5% (w/v). ALA was isolated by ion exchange chromatography on columns (0.5 ml gel bed) of Dowex resin (type 50W × 8, mesh size 200–400; Sigma, St. Louis, MO) that had been prepared by twice heating in 2 m NaOH to 50°C and washing in distilled water. Before use, the stored resin was equilibrated in 0.05 m sodium acetate, pH 3.9. TCA supernatants containing ALA were applied to Dowex columns that then were washed with 30 ml of acetate buffer to remove the unconverted glycine label and other radiolabeled material. Then ALA was eluted with a pulse of 600 μl of 0.25 m sodium phosphate buffer, pH 6.8. The eluates were assayed for14C-radioactivity in a scintillation counter.
Extraction and quantitation of heme. The extraction of heme from the various tissues and 14C-labeled culture was performed essentially as described (Ponka and Schulman, 1985). Briefly, cultures in 6 well plates or 10 cm dishes were incubated with [14C]glycine as described. Cells were washed twice with ice-cold PBS, lysed with 500 μl of distilled water, and kept frozen overnight. After the samples were thawed, heme was extracted from 500 μl of these cell homogenates by vigorously mixing with 1 ml of ethyl acetate–glacial acetic acid (3:1). One additional extraction was done with 1 ml of the same reagent, and the extracts then were pooled. The extracts were washed three times with 1 ml of 0.3% sodium acetate and twice with 2 ml of 1.5 N HCl. The total heme content in the extracts was quantitated fluorometrically by the method of Morrison, as described (Sassa et al., 1975). Samples were added to 2 moxalic acid and heated at 100°C for 30 min. After cooling, the fluorescence was measured at 662 nm during excitation at 400 nm with a Perkin-Elmer LS50 luminescence spectrometer. For the measurement of14C-labeled heme, heme crystallizations were performed by the method of Labbe and Nishida (1957) with modification (Falk, 1975). [14C]heme was crystallized in the presence of carrier heme, and the radioactivity of this material was counted.
Extraction and quantitation of 3H-labeled heme and bile pigment. The cultures plated in 10 cm dishes were incubated with 40 μCi/ml [3H]ALA. At 6 hr after the addition of [3H]ALA, cells were scraped into 1 ml of PBS. After addition of 0.1 ml of carrier pigment in the form of normal bile containing ∼15 mg/dl total bilirubin, mono- and diglucuronide conjugates were converted quantitatively to the corresponding methyl esters by alkaline methanolysis (Blanckaert, 1980). Heme, unconjugated bilirubin, and the bilirubin methyl esters were extracted into chloroform (Blanckaert, 1980), and the solution was reduced to dryness under nitrogen. The residue was dissolved in 30 ml of chloroform/methanol (1:1) and applied to thin-layer plates (Silica Gel IB2, J.T. Baker, Phillipsburg, NJ) that were developed immediately in one of two different solvent systems. Chloroform/methanol/acetic acid (97:2:1) was used for separation of bilirubin and its mono- and dimethyl esters. In this system, heme migrates <1 cm. To separate heme from the origin, a second system consisting of chloroform/methanol/water/acetic acid (40:20:4:1) was used. Under these conditions, heme migrates with RF = 0.65, whereas bilirubin and its methyl esters migrate in a single band withRF = 0.9.
14CO measurement. On each culture day, cultures in slide flasks were preincubated with 5 μCi of [2-14C] glycine for various times, and the radioactivity incorporated into14CO was measured as described (Lincoln et al., 1989). Briefly, the gases from cultured flasks were drawn through the following series of traps: ethanolamine–methanol (trap for CO2), H2SO4, CaCl2, heated Hopcalite, and ethanolamine–methanol (trap for CO).14CO was converted to 14CO2 by hopcalite and collected in the second ethanolamine–methanol trap. Each trapping solution was counted. No radioactivity over background (30 cpm) was detected in the CO trap when Hopcalite was removed from the series of traps. When inhibitors were used, cultures were incubated with [14C]glycine in the presence of ZnPP9 at the indicated concentrations for 6 hr. Then the gases were drawn from the flasks.
Reverse transcriptase-PCR (RT-PCR). Primary cultures of olfactory receptor neurons were plated as described, except that cells were plated in a medium that did not contain exogenous growth factors. After cell plating (∼6 hr), the feeding medium was replaced with fresh medium with or without 10 ng/ml TGF-β2. Cultures were maintained for 1–5 d, at which time [14C]heme production and HO activity were measured as previously described to determine the effects of neuronal maturation and TGF-β2. On day 3, poly(A) RNA was prepared from cultured olfactory receptor neurons. cDNA was synthesized in a 50 μl reaction using 1 μg of poly(A) RNA. The RNA mixed with 100 ng oligo(dT) primer was denatured for 10 min at 70°C and cooled to 37°C. Reverse transcription was performed at 37°C for 1 hr after addition of 10 μl of 5 × reverse transcription buffer (Bethesda Research Labs, Bethesda, MD), 5 μl of 0.1 m DTT, 2 μl of 2.5 mm dNTPs, 20 U of RNasin, and 2 μl of MMLV reverse transcriptase (Superscript; Bethesda Research Labs). After first-strand cDNA synthesis, HO-2 and β-actin PCR products were generated from these cDNAs. cDNA (5 μl) was used as a template in subsequent 50-μl-reaction volumes. PCR amplifications were performed for 30 cycles with the following specific oligo primers (0.5 μm): P16 and P17 for HO-2, and Act-5 and Act-3 for β-actin. Under the condition used, PCR products increased linearly between 28–33 cycles.
Oligonucleotides used as PCR primers were synthesized from the following positions in the cDNAs:
HO-2 (Rotenberg and Maines, 1988):
P16 = 5′-CACTTGGGATAGGATGCAAACA AC-3′ (from 984 to 961 on cDNA)
P17 = 5′-TTTGAATGAGCCAAGGACCGAAGTG-3′ (−49 to −25 on cDNA).
The predicted size of PCR products with P16 and P17 is 1033 bp. β-actin (Nudel et al., 1983):
Act-5 = 5′-ATGGATGACGATATCGCTGCGCTC-3′ (from 1242 to 1265 on gene)
Act-3 = 5′-GGCCAGGATAGAGCCACCAATCCA-3′ (from 3045 to 3022 on gene).
The predicted size of PCR products with Act-5 and Act-3 is 1042 bp.
Guanylyl cyclase activity assay. The brain was excised from adults rats and immediately placed in ice-cold 50 mmTris-HCl, pH 7.4, containing 1 mm DTT, finely minced, washed twice with this buffer, and homogenized. The homogenate was centrifuged for 10 min at 10,000 × g, and the supernatant was ultracentrifuged for 60 min at 105,000 × g. Guanylyl cyclase activity in the obtained cytosolic fraction (0.75 mg of protein per assay tube) was determined by incubation for 10 min at 37°C in the presence of 50 mmTris-HCl, pH 7.4, containing (in mm): 1 DTT, 1 GTP, and 5 MgCl2. The incubation was terminated with a 0.3 volume of 18% TCA, and cGMP was quantitated by radioimmunoassay (Amersham, Arlington Heights, IL). The indicated concentrations of exogenous CO were achieved by adding a series of diluted CO-containing buffers. To make CO-equilibrated buffer, Tris-HCl buffer was bubbled with 100% CO gas for 1 min.
RESULTS
Comparison of heme and HO in peripheral and neural tissues
Throughout the body, high levels of HO activity are distributed in the spleen and liver, where HO is responsible for the destruction of heme from senescent red blood cells. To evaluate the activity of heme turnover in the nervous system, we determined the cellular concentrations of heme and microsomal HO enzymatic activities in tissue preparations from spleen, liver, brain, cerebellum, and olfactory epithelium (Table 1). Spleen displayed the highest values for both the level of heme and HO activity. In whole brain, HO activity and heme levels were similar to those of liver. These values for HO activities obtained by this assay resemble those previously reported by others (Maines, 1988). Olfactory neuroepithelium and cerebellum have relatively high HO activity. This agrees with the finding that HO-2 is expressed abundantly in olfactory receptor neurons by in situ hybridization and immunohistochemistry (Ewing and Maines, 1992; Verma et al., 1993). These results indicate that brain has significant levels of heme (1.3 nmol/mg protein) and high HO activity (280 pmol of bilirubin/mg protein per min), providing evidence for the physiological importance of heme function in neurons.
Heme turnover and CO biosynthesis in olfactory receptor neurons
In addition to heme and HO-2, olfactory receptor neurons contain a high level of heme-metabolizing enzymes such as ALAS and cytochrome P-450 reductase (Verma et al., 1993). This suggests that heme metabolic turnover is significant in olfactory receptor neurons, providing us with an excellent model in which to study neuronal control of heme turnover and CO biosynthesis. Because the colocalization of ALAS with HO-2 in these neurons indicates that the machinery for porphyrin turnover and CO biosynthesis occur together, primary cultures of olfactory receptor neurons were incubated with [2-14C]glycine to label heme precursors, heme, and CO. As shown in Figure 1, cellular uptake of [14C]glycine and biosynthesis of [14C]ALA, [14C]heme, and 14CO were measured in these cell cultures at the indicated time intervals. All of these14C-labeled heme precursors and metabolites increased in a similar manner over this time period.
The amounts labeled in 6 hr were (in pmol/mg protein): 100 [14C]ALA, 5.3 [14C]heme, and 2.9 14CO (Table 2). Both unlabeled and14C-labeled levels of cellular heme (the substrate of HO) were measured in cultures to determine the specific activity of CO production. The total cellular heme was determined spectrophotometrically to be 1.5 nmol/mg protein (Table 2). Under the conditions used, incorporation of [14C]glycine into cellular heme increased over 6 hr, as shown in Figure 1C; the average concentration of [14C]heme during this period was 2.7 pmol/mg protein. As summarized in Table 2, the amount of total CO production was determined to be 1.6 nmol/mg protein per 6 hr, taking into account the ratio of total heme to [14C]heme. Similar adjustment for the dilution of [14C]glycine (1.2 nmol/mg protein) by endogenous free glycine (20 nmol/mg protein; Hall et al., 1979; Freeman et al., 1983) yielded the following synthetic rates (in nmol/mg protein per 6 hr): 3.4 for ALA, 180 for heme, and 95 for CO (Table 2). These results indicate that the total amount of newly synthesized heme for 6 hr was 275 (180 + 95) pmol/mg protein and that 35% (95/275) of this synthesized heme was rapidly degraded to CO and biliverdin.
To verify these values obtained by labeling cells with [14C]glycine, olfactory receptor neuron cultures were incubated independently with [3H]ALA to label heme and bilirubin. As summarized in Table 2, cellular uptake of [3H]ALA was measured in these cultures, and the biosynthesis of [3H]heme and [3H]bilirubin was determined by thin-layer chromatography. The ratio of [3H]heme to [3H]ALA (1.2/36 = 3.3%) in this experiment is equivalent statistically to that of [14C]heme to [14C]ALA (5.3/100 = 5.3%), which confirms the rate of the cellular heme synthetic pathway in Table 2. Taking into account the ratio of total heme to [3H]heme, we determined the amount of total bilirubin production to be 0.57 nmol/mg protein per 6 hr, a value of similar magnitude to that obtained for the total CO production calculated from14CO measurement (1.6 nmol/mg protein per 6 hr). Thus, these two approaches for measurement of metabolic labeling yielded comparable results. These studies verify that endogenous heme synthesis is significant in neurons.
Regulation of heme metabolism by exogenous heme and inhibitors
Heme formation is subject to end-product regulation by negative feedback, but the exact point of metabolic control differs between tissues (May and Bawden, 1989). As shown in Figure3, studies in liver culture provided strong evidence that the rate-limiting enzyme of the heme biosynthetic pathway, ALAS, is regulated by heme, the end product of the pathway (Granick, 1966;Granick et al., 1975). To investigate the regulatory mechanism of heme in olfactory receptor neurons, we incubated primary cultures of olfactory receptor neurons with [14C]glycine in the presence or absence of exogenous heme or inhibitors of this pathway (Fig. 3). As shown in Figure 2B, 50 μm of hemin inhibited [14C]heme synthesis to 54% of control, which indicates the existence of a negative feedback system in olfactory receptor neurons. However, 50 μm hemin had little inhibitory effect on the incorporation of [14C]glycine into cellular ALA in this neuron culture (Fig. 2A), although hemin concentrations lower than 50 μm repressed the ALAS activity to 50% of control in liver cell cultures (Granick et al., 1975).
These results indicate that hemin regulates the heme synthetic pathway in neurons, not at the level of ALAS but at other sites. One mm succinyl acetone (SA) clearly elevated cellular [14C]ALA level to 280% of control (Fig. 2A), which agrees with its potent inhibitory effect on ALA dehydratase. ZnPP9 (10 μm), a potent inhibitor of HO activity, had a significant inhibitory effect on 14CO production and elevated [14C]heme level to 140% of control (Fig.2B,C). However, the same concentration of ZnPP9 had little effect on cellular [14C]ALA levels (Fig. 2A). Although 50 μm of hemin significantly suppressed14CO production, this may be attributable to its competitive effect on [14C]heme (substrates) binding to HO (enzyme) rather than by direct inhibition of HO.
Regulation of heme turnover in neuronal differentiation
To investigate the change of heme turnover during growth and differentiation of olfactory receptor neurons, we determined the effects of neuronal maturation and TGF-β2 (an olfactory neurogenic/survival factor) on heme biosynthesis and degradation in cultures over time as cells matured. Olfactory receptor neurons were cultured in the presence or absence of 10 ng/ml TGF-β2 from days 1 to 5. On each day, cultures were incubated with [14C]glycine to label heme. At 6 hr after addition of [14C]glycine, [14C]heme was measured in these neuronal cultures. As shown in Figure 4A, there was an increase of [14C]heme production, from 1.2 pmol/mg protein at day 1 in culture to 3.0 pmol/mg protein at day 3. Afterward, [14C]heme production fell until day 5. Whereas TGF-β2 potentiated the increase of [14C]heme production at day 3, it potentiated the decrease of [14C]heme production at days 4 and 5.
The level of HO expression was determined by measuring the level of HO-2 mRNA in culture on each culture day. As shown in Figure4B, HO-2 mRNA is expressed abundantly during the early phase of culture (days 2 and 3) with the highest concentration at day 3, identical to the changes in [14C]heme production in culture. TGF-β2 consistently suppressed the expression of HO-2 in culture at days 3 and 5 (Fig. 4C). Although TGF-β2 elevated [14C]heme levels at day 3, this effect may be attributable to its potent inhibitory effect on HO-2 expression rather than to a change in heme synthetic rate. These findings indicate that both heme biosynthesis and degradation are enhanced significantly during the immature stages of culture and that, as neuronal maturation occurs, heme biosynthesis and degradation are coordinately down-regulated, further confirming that these activities are important in neurons.
Effect of physiological level of exogenous CO on cGMP level
Like NO, CO binds to the iron of the heme moiety in soluble guanylyl cyclase to activate this enzyme (Brüne and Ullrich, 1987; Furchgott and Jothianandan, 1991; Kharitonov et al., 1995). However, the potency of CO as a guanylyl cyclase activator is weaker, raising the question as to whether CO could have any effect on soluble guanylyl cyclase at physiological concentrations (Stone and Marletta, 1994). As shown in Table 2, the total amount of CO production was determined to be 1.6 nmol/mg protein per 6 hr. Because of the gaseous nature of CO and its high affinity for hemoprotein, it is very difficult to determine the exact intracellular concentration of CO. However, taking into account the diffusion of CO, it may be reasonable to assume that the amount of CO produced for 10–30 min is an effective concentration in the cell. On this assumption, the endogenous CO level was calculated to be 50–160 pmol/mg protein or 10–30 μm. To investigate whether this physiological level of CO can affect guanylyl cyclase activity, we examined the effect of CO at various concentrations on soluble guanylyl cyclase activation (Fig.5). CO (10–30 μm), which corresponds to endogenous CO levels, significantly elevated guanylyl cyclase activity up to 190–220% of control. This result, together with the chemical stability of CO, suggests that CO does not work as a rapid stimulator of cGMP but, rather, works as a modulator that could produce slower, long-term effects.
DISCUSSION
There are several major findings of the present study. (1) Quantitative analysis has demonstrated that high levels of heme synthesis and CO production occur in olfactory receptor neurons, consistent with its postulated role as a neurotransmitter. (2) The regulation of heme biosynthesis in this neuron is subject to negative feedback regulation at a site different from that in liver, consistent with the hypothesis that HO does not function simply in heme degradation in neurons. (3) Heme synthesis and degradation are enhanced during immature stages of neuronal development in culture and are suppressed during the mature stage. (4) The total amount of CO that is produced physiologically by this neuron is clearly enough to activate guanylyl cyclase.
A necessary prerequisite for a functional role of CO as a neuronal messenger is the significant expression of heme and heme metabolic enzymes in the nervous system. For this reason, we measured the levels of cellular heme and HO activity in spleen, liver, and the nervous system. Although HO has been detected in all tissues, the relative abundance of HO varies greatly among different sources (Maines, 1988). Hemoglobin heme from senescent red blood cells is degraded mainly by the phagocytic cells that line the sinusoids of the spleen, liver, and bone marrow. Therefore, HO activity of these tissues is >10-fold higher than that of other HO-poor tissues, such as the small intestine (Maines, 1988). HO activity in brain was high and equivalent to that of liver, and it colocalized with significant levels of cellular heme there, which suggests active local heme synthesis and turnover. As a result, we attempted to elucidate the mechanism and role of this heme turnover and resultant CO production in the nervous system, which had been unclear.
In animal cells the regulation of the heme biosynthetic pathway differs between erythroid and nonerythroid tissues (May and Bawden, 1989). In the liver and other nonerythroid cells, the rate of heme biosynthesis is controlled by the level of ALAS (Ponka and Schulman, 1985). Heme may regulate its own synthesis by feedback inhibition of ALAS and by controlling the synthesis of ALAS. In contrast, it is now generally agreed that ALAS is not under the same regulatory mechanism in differentiating erythroid cells (Granick and Sassa, 1978; Ponka and Schulman, 1985; Gardner and Cox, 1988), but at present there is no clear consensus as to what and how many factors may limit heme production. Our results demonstrate that the regulatory mechanism of heme biosynthesis by olfactory receptor neurons is similar to that in the erythroid cell type, in which degradation is not the primary goal. In olfactory receptor neurons, exogenous heme clearly suppressed heme biosynthesis, which indicates that the overall rate of heme synthesis in this cell is subject to negative feedback control. However, exogenous heme did not affect ALAS activity, suggesting that the action site of this negative feedback control is not at the level of ALAS. This is the first evidence that neurons are able to regulate heme synthesis by a mechanism similar to that of erythroid cells, and this process of regulation may be applicable to other types of neurons.
SA significantly inhibited ALA dehydratase activity in olfactory receptor neurons, which resulted in the accumulation of ALA. SA is an abnormal metabolite produced in patients with hereditary tyrosinemia as a consequence of an inherited deficiency of fumaryl acetate hydrolase (Sassa and Kappas, 1983). Because SA is an extremely potent inhibitor of ALA dehydratase, patients with this disease excrete excessive amounts of urinary ALA and have low ALA dehydratase activity in erythrocytes and liver. Neurological dysfunction is one of the clinical manifestations of this disorder. Together with this background, our results confirm the potent inhibitory effect of SA on ALA dehydratase in the nervous system and implicate the physiological importance of heme metabolism in neuronal function.
It has now been shown that, in cultured primary olfactory receptor neurons, both formation and degradation of heme are enhanced in the immature stages of neuron culture, after which they progressively declined as the neurons matured. It has becoming increasingly evident that heme synthesis and degradation play pivotal roles in the regulation of growth and differentiation of erythroid and nonerythroid cells (Abraham, 1991). During erythropoietic differentiation one of the key events is the increase in the synthesis of heme for hemoglobin production. The vital, ubiquitous role of heme in mammalian physiology is attested to by its function as the prosthetic group in a variety of important hemoproteins. However, the effect of heme on erythropoiesis is distinct from its direct involvement as a prosthetic group. The expression of specific heme metabolic enzymes determines the level of cellular heme that is necessary for proper erythropoiesis (Sassa et al., 1975; Conder et al., 1991). The heme metabolic enzymes participate in the implementation of both stimulation and suppression of erythropoiesis. Enhancement of erythropoiesis obtained with erythropoietin and some growth factors results in increased levels of ALAS and porphobilinogen deaminase, the proposed rate-limiting enzymes in the heme biosynthetic pathway. Suppression of erythropoiesis is observed by either insufficient levels of one of the heme biosynthetic enzymes or by increased heme degradation.
In hematopoietic cells, HO level may play a crucial role during stem cell proliferation and differentiation (Abraham, 1991). In humanin vitro erythroid colony development systems, HO activity was elevated in the early phases of erythroid culture, after which it declined. A similar observation was made in olfactory receptor neurons and in cerebellar granule cell cultures. A decrement in HO activity may be an important feature of the differentiation process. In human erythroleukemia cells, the inducers of differentiation, such as heme, cause a repression in HO activity and concomitant appearance of staining (Abraham, 1991). TGF-β2 is known to be an olfactory neurogenic/survival factor that initiates terminal differentiation in olfactory receptor neurons (Mahanthappa and Schwarting, 1993). In olfactory receptor neuron cultures, TGF-β2 caused an increase in neuron cell adhesion molecule (N-CAM)-positive cells; N-CAM is a marker of olfactory neurogenesis. In our data, TGF-β2 significantly suppressed the expression of HO-2 at the phases of neuronal differentiation in culture. This result agrees with the report that TGF-β2 suppressed CO production in olfactory receptor neuron (Ingi and Ronnett, 1995). These lines of evidence suggest that the repression of HO in neurons and erythroid cells may work as a trigger of the differentiation of these cells.
CO is a weak activator of soluble guanylyl cyclase. In vitro, CO activation of purified soluble guanylyl cyclase is 1/30-fold less potent than NO (Stone and Marletta, 1994). Therefore, it was questioned whether CO will have any effect on soluble guanylyl cyclase at physiological concentration. As shown in Figure 5, 3–30 μm CO actually activated soluble guanylyl cyclase significantly. These results suggest that CO can affect guanylyl cyclase activity effectively in the range of 3–30 μm and agree with the recent report that CO regulates cyclic nucleotide-gated channels via cGMP formation with a K1/2 value of 2.9 μm in olfactory receptor neurons (Leinders-Zufall et al., 1995). Although NO can work as a very potent and short-lived stimulator of cGMP, the chemical stability of CO may have the advantage of working as a modulator that could produce long-term or tonic effects. CO may serve as a neuromodulator that produces long-term effects on cGMP level in the nervous system. It has been proposed that CO, either alone or in combination with NO, may act as a retrograde messenger that produces activity-dependent enhancement of synaptic transmission during long-term potentiation in the hippocampus (Stevens and Wang, 1993; Zhuo et al., 1993). By altering the cyclic nucleotide-gated channel activity via changes in the level of cGMP, CO may modulate the excitable properties of olfactory receptor neurons (Leinders-Zufall et al., 1995).
Although the amplitude of CO induced-activation of soluble guanylyl cyclase is not so drastic (approximately two- to threefold), the action of CO may be more complicated than the simple activation of this enzyme. Recently, we have observed that, in the presence of NO, low micrometers of CO actually suppressed NO-mediated activation of soluble guanylyl cyclase in cerebellar granule cells (Ingi et al., 1996). Collectively, these results indicate that the level of CO produced by olfactory receptor neurons is significant enough to work as a regulator of cGMP levels in the nervous system.
Footnotes
T.I. is a Postdoctoral Fellow for Research Abroad, supported by Japan Society for the Promotion of Science. G.V.R. is supported by a National Institutes of Health grant, a McKnight Scholars Award, and grants from the Whitehall Foundation, the Develbiss Fund, and the W. M. Keck Foundation. We thank M. Angelyn Bethel for technical assistance and Lana Kramer for manuscript preparation.
Correspondence should be addressed to Dr. Gabriele V. Ronnett, Department of Neuroscience, The Johns Hopkins University School of Medicine, 725 North Wolfe Street, Baltimore, MD 21205.