From the
Department of Veterinary and Comparative Anatomy, Pharmacology and Physiology,
Program in Neuroscience, Washington State University, Pullman, Washington 99164-6520
Received for publication, February 19, 2003 , and in revised form, April 23, 2003.
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ABSTRACT |
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INTRODUCTION |
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CNG channels are highly permeable to Ca2+, and Ca2+ entry through CNG channels provides a negative feedback signal that assists in adaptation and recovery in photoreceptors and olfactory sensory neurons (1315). Calmodulin (CaM) is thought to participate in these processes by binding Ca2+ and then targeting to different cellular components including CNG channels (16). Numerous studies have described Ca2+-CaM regulation of the ligand sensitivity of rod and olfactory CNG channels (1725). Olfactory CNG channels are composed of CNGA2 (26), CNGA4 (8, 9), and CNGB1b subunits (10, 11); Ca2+-CaM modulates olfactory channel activity via direct binding to NH2-terminal CaM-binding sites of CNGA2 (20) (and probably CNGB1b) subunits, whereas the presence of CNGA4 and CNGB1b subunits tunes the kinetics of the response to CaM (27, 28). Rod CNG channels contain CNGA1 (29) and CNGB1 (7) subunits. For these channels, Ca2+-CaM modulation is comparatively weaker, and the CNGB1 subunit provides the CaM-binding site in the NH2-terminal cytoplasmic domain that is critical for regulation (3032).
For cone CNG channels, Ca2+-feedback mechanisms are less well defined. Ca2+-dependent regulation of apparent cGMP affinity is robust for native striped bass cone CNG channels and is thought to be of greater significance for cone photoreceptor adaptation than the corresponding changes in rods (3335). Application of CaM to patches excised from cone outer segments inhibits these channels, but CaM only partially mimics the activity of an endogenous modulator(s) (33, 34). In contrast, CaM has no effect on CNG channels in patches excised from catfish cone outer segments (36). Recombinant homomeric CNG channels composed of chick cone CNGA3 subunits are modulated by Ca2+-CaM (37). However, homomeric channels formed by the human or bovine orthologs of CNGA3 are insensitive to CaM regulation, even though these subunits possess an NH2-terminal CaM-binding site (3840). Thus, there appear to be species differences in sensitivity to regulation by Ca2+-CaM both for native cone photoreceptor CNG channels and for heterologously expressed homomeric CNGA3 channels. With recent cloning of the cone photoreceptor subunit (CNGB3) for mice (12) and humans (41, 42), the importance of this subunit for modulation of cone CNG channels by Ca2+-CaM can now be examined.
In this study, we demonstrate that the human CNGB3 (hCNGB3) subunit forms functional heteromeric channels with human CNGA3 (hCNGA3) when co-expressed in Xenopus oocytes. These recombinant heteromeric channels exhibited electrophysiological properties that differed from those of homomeric hCNGA3 channels, including sensitivity to regulation by Ca2+-CaM. Human CNGB3 plus CNGA3 heteromeric channels are shown to be unique compared with other CNG channel types, in that CaM regulation involves functionally important CaM-binding sites in both the NH2- and COOH-terminal cytoplasmic domains of hCNGB3.
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EXPERIMENTAL PROCEDURES |
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CaM Interaction AssaysRecombinant protein expression in bacteria and purification were carried out as previously described (25). Briefly, cells were harvested and resuspended in buffer S (50 mM Tris-HCl (pH 7.8), 150 mM NaCl, 25 mM imidazole, 1% NDSB (Calbiochem, San Diego, CA), 0.5% CHAPS, and 0.25% Tween 20) containing protease inhibitors (Roche Applied Science), then lysed using a French pressure cell (SLM Instruments, Rochester, NY) or sonication. Soluble proteins were isolated by centrifugation at 20,000 x g and 4 °C for 30 min. GST fusion proteins were purified using glutathione-Sepharose beads (Amersham Biosciences); His-tagged CaM was purified using Ni2+-charged Sepharose (Probond resin; Invitrogen), eluted with 0.5 M imidazole (pH 6.0), and then dialyzed with buffer S. GST pull-down assays were performed using immobilized GST fusion proteins and 2 µM recombinant hCaM-FLAG, in the presence of 2 mM Ca2+ or 10 mM EDTA. Pull-down assays were incubated overnight in buffer S at 4 °C with rocking. Beads were centrifuged for 2 min at 700 x g, washed 5 times in 100 µl of buffer S (including either Ca2+ or EDTA), and suspended in SDS-PAGE sample buffer containing 2-mercaptoethanol. Bound proteins were separated using 12 or 420% SDS-PAGE and transferred to nitrocellulose. Gel overlay assays were performed using similarly blotted GST fusion proteins with 1 µg/ml hCaM-FLAG in 20 mM Tris (pH 7.5), 0.15 M NaCl, 0.1% Tween 20, 1% milk, and either 1 mM Ca2+ or 5 mM EDTA (maintained throughout the assay and blot processing). For both assays, interacting hCaM-FLAG was visualized using M2 monoclonal antibody (Eastman Kodak) directed against the FLAG epitope and a chemiluminescent detection system (SuperSignal West Dura Extended Duration Substrate; Pierce). Interaction assays were repeated at least 3 times with reproducible results. CaM-binding site search and analysis was performed using the Calmodulin Target database of M. Ikura and co-workers.2
ElectrophysiologyFor functional expression of hCNGA3 and hCNGB3, Xenopus laevis oocytes were isolated and microinjected with 510 ng of in vitro transcribed mRNA (mMessage mMachine; Ambion, Austin, TX) as previously described (45). The ratio of hCNGA3 to hCNGB3 cRNA was 1:5. Two to 7 days after microinjection of mRNA into oocytes, patch clamp experiments were performed with an Axo-patch 200B patch clamp amplifier (Axon Instruments, Foster City, CA) in the inside-out configuration. Initial pipette resistances were 0.450.75 megohm. Currents were low-pass filtered at 2 kHz and sampled at 10 kHz. Intracellular and extracellular solutions contained 130 mM NaCl, 0.2 mM EDTA, and 3 mM HEPES (pH 7.2). Cyclic nucleotides were added to intracellular solutions as indicated. Intracellular solutions were changed using an RSC-160 rapid solution changer (Molecular Kinetics, Pullman, WA). Currents in the absence of cyclic nucleotide were subtracted. Recordings were made at 20 to 22 °C. For electrophysiological experiments involving CaM, bovine CaM (Calbiochem, San Diego, CA) was used at 250 nM. EDTA was substituted by 2 mM nitrilotriacetic acid and 704 µM CaCl2 for 50 µM buffered free Ca2+ in the intracellular solution. Excised patches were first exposed to 5 mM EDTA for 210 min to remove soluble, endogenous Ca2+-dependent modulators. In addition, any changes because of Ca2+ alone were permitted to occur before CaM was applied (1040 min). After CaM experiments, the channels were typically tested for sensitivity to L-cis-diltiazem (RBI, Natick, MA) applied in the intracellular solution to verify the subunit composition of the channel, i.e. whether hCNGB3 and deletion constructs of hCNGB3 participated in the formation of the expressed channels. Dose-response relationships were obtained by plotting the current as a function of cyclic nucleotide concentration. Dose-response data were fitted to the Hill equation, I/Imax = ([cNMP]n/(Kn + [cNMP]n)), where I is the current amplitude, Imax is the maximum current, [cNMP] is the ligand concentration, K1/2 is the apparent affinity for ligand, and n is the Hill slope. For current inhibition by L-cis-diltiazem, data were fit to the Hill equation in the form: Idiltiazem/I = (K
n/(K
n + [diltiazem]n)). Data were acquired using Pulse (HEKA Elektronik, Lambrecht, Germany), and analyzed using Igor Pro (Wave-metrics, Lake Oswego, OR) and SigmaPlot (SPSS, Chicago, IL). The data were expressed as mean ± S.D. unless otherwise indicated. Statistical significance was determined using a Mann-Whitney rank sum or Student's t test (SigmaStat; SPSS), and a p value of <0.05 was considered significant.
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RESULTS |
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hCNGB3 Plus hCNGA3 Heteromeric Channels Are Inhibited by Ca2+-CaMWe examined the sensitivity of both homomeric hCNGA3 channels and heteromeric hCNGA3 + hCNGB3 channels to regulation by Ca2+-CaM. Consistent with previous studies (39), homomeric channels formed by hCNGA3 subunits alone were not inhibited by 250 nM CaM in the presence of 50 µM Ca2+ (Fig. 2, A and C, left). In contrast, heteromeric hCNGA3 + hCNGB3 channels displayed significant inhibition by Ca2+-CaM under identical conditions (Fig. 2, B and C, right). The time course for maximum current inhibition by Ca2+-CaM varied between seconds and minutes. The ratio of the current elicited by 10 µM cGMP at +80 mV with and without 250 nM CaM, i.e. ICaM/I, was 0.96 ± 0.01 (n = 2) for homomeric hCNGA3 channels and 0.62 ± 0.09 (n = 8) for heteromeric hCNGA3 + hCNGB3 channels. Inhibition by Ca2+-CaM was relieved by perfusion of the patch with calcium-free solution (Fig. 2, B and C, right). The apparent affinity of the heteromeric channel for cGMP was decreased slightly by Ca2+-CaM (Fig. 2D), from a K of 19.0 ± 2.7 µM, n = 2.0 ± 0.2 (n = 5) in the absence of CaM (see also Table I) to 25.8 ± 6.7 µM, n = 2.1 ± 0.2 (n = 5) in the presence of CaM (p < 0.05, paired t test). No change in the maximum current at a saturating concentration of cGMP (1 mM) was observed with Ca2+-CaM compared with Ca2+ alone (data not shown). These results indicate that the presence of the cone photoreceptor hCNGB3 subunit conferred sensitivity to regulation by Ca2+-CaM in the context of recombinant heteromeric channels.
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Identification of Region in the hCNGB3 NH2-terminal Domain Important for Interaction with Ca2+-CaMTo test the hypothesis that hCNGB3 subunits provide sites for direct binding of Ca2+-CaM, we used epitope-tagged human CaM in gel overlay and pull-down interaction assays with GST fusion proteins representing cytoplasmic domains of hCNGB3 and hCNGA3. hCNGA3 subunits are known to possess a CaM-binding site in the NH2-terminal cytoplasmic domain that is functionally silent in the context of homomeric channels (39). As expected, the NH2-terminal domain of hCNGA3 interacted with CaM in the presence of calcium, and deletion of a region including the previously identified Ca2+-CaM-binding site prevented this interaction (Fig. 3, B and C). The NH2-terminal cytoplasmic domain of hCNGB3 (hCNGB3 N) also was able to physically associate with Ca2+-CaM (Fig. 3, B and C). Next, we localized the CaM-binding site within the hCNGB3 NH2-terminal domain. GST fusion proteins representing various hCNGB3 N deletion constructs were generated and tested for interaction with CaM in vitro (Fig. 3A). Deletion of amino acids 2 to 107 of hCNGB3 N did not disrupt binding of Ca2+-CaM. However, deletion of amino acids 108159 in hCNGB3 N completely abolished the interaction with Ca2+-CaM (Fig. 3, B and C). Moreover, a GST fusion protein including only amino acids 108154 of hCNGB3 N was able to associate with Ca2+-CaM. Thus, these results show that this region of hCNGB3 N is both necessary and sufficient for direct binding of Ca2+-CaM. No CaM binding was observed for any of the fusion proteins in the absence of Ca2+, confirming that the interaction was entirely Ca2+-dependent (Fig. 3, B, middle, and C, bottom). Sequence alignment of the probable CaM-binding site in the hCNGB3 NH2-terminal domain with those of CNGB1, CNGA3, and CNGA2 is shown in Fig. 3D. This site in hCNGB3 N resembles a 114 CaM-binding motif, exhibiting bulky hydrophobic residues at positions 1 and 14, a net charge of +4, and a predicted propensity to form an amphiphilic -helix (47, 48). This pattern in hCNGB3 N appears to conform better to these common CaM-binding motifs than the previously characterized "unconventional" CaM-binding site in the NH2-terminal domain of CNGB1 (30, 31).
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Localization of a CaM-binding Site in the hCNGB3 COOH-terminal DomainBecause a functionally silent CaM-binding site was previously identified in the COOH-terminal cytoplasmic domain of the rod CNG channel subunit (CNGB1) (30, 31), we investigated the possibility that the carboxyl-terminal domain of hCNGB3 (hCNGB3 C) may also bind Ca2+-CaM. Gel-overlay experiments with full-length hCNGB3 C demonstrated an interaction with Ca2+-CaM in vitro (Fig. 4B). Similar to hCNGB3 N, CaM binding to hCNGB3 C depended on the presence of calcium. As expected, the hCNGA3 COOH-terminal domain did not interact with CaM. To localize which regions of hCNGB3 C were necessary for binding of Ca2+-CaM, GST fusion proteins representing hCNGB3 C deletion mutants were engineered and tested using in vitro protein-protein interaction assays (Fig. 4). Assays carried out with fusion proteins including the C-linker region and the cyclic nucleotide-binding (CNB) domain, or the CNB domain alone, revealed no binding to Ca2+-CaM. Instead, Ca2+-CaM specifically interacted with a fusion protein representing the region of hCNGB3 C distal to the CNB domain (amino acids 637809). A fusion protein limited to amino acids 661757 of hCNGB3 was sufficient for interaction with Ca2+-CaM, whereas proteins including amino acids 637681 or 680809 of hCNGB3 C were unable to bind CaM. Similar results were obtained using GST pull-down assays (data not shown). In all cases, CaM binding did not occur in the absence of calcium (Fig. 4B, middle). These results, summarized in Fig. 4A (right), identify a region distal to the cyclic nucleotide-binding domain that is necessary for Ca2+-CaM binding in vitro. Consistent with these findings, a search for likely CaM-binding sites in hCNGB3 C highlighted this sequence as a candidate CaM target (Fig. 4A, bottom). This Ca2+-CaM-binding site in hCNGB3 is positioned similar to the functionally silent CaM-binding site in the COOH-terminal domain of CNGB1, but this region of CNGB3 exhibits little sequence homology with CNGB1.
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Effects of hCNGB3 NH2- and COOH-terminal Deletions on Ca2+-CaM Modulation of Heteromeric CNG ChannelsTo determine the functional importance of the CaM-binding sites identified within hCNGB3 NH2- and COOH-terminal cytoplasmic domains, hCNGB3 deletion mutants were engineered and individually co-expressed with hCNGA3 in Xenopus oocytes. As shown in Table I, the functional properties of these channels, as indicated by the K for cGMP, the K
for cAMP, IcAMP/IcGMP, and the sensitivity to block by L-cis-diltiazem, were roughly similar to wild type hCNGA3 + hCNGB3 channels, demonstrating that all hCNGB3 deletion mutants studied were able to participate in the formation of heteromeric channels. An
subunit with deletion of its Ca2+-CaM-binding site, hCNGA3
N, also formed functional homomeric channels (data not shown) as well as heteromeric channels when co-expressed with hCNGB3.
Sensitivity to regulation by CaM for these mutant CNG channels was examined in the presence of 25 µM cGMP and 50 µM Ca2+. Inhibition by Ca2+-CaM was still observed for heteromeric hCNGA3 + hCNGB3 N, hCNGA3 + hCNGB3
C, and hCNGA3
N + hCNGB3
N channels (Fig. 5, A, C, and E). For some patches, slow recovery of the current after Ca2+-CaM inhibition was apparent with removal of CaM even in the presence of Ca2+ (Fig. 5A). Thus, neither individual deletion of NH2- or COOH-terminal CaM-binding sites in hCNGB3, nor of the NH2-terminal CaM-binding site in hCNGA3, eliminated sensitivity to regulation by Ca2+-CaM. Furthermore, the extent of inhibition by Ca2+-CaM of hCNGA3 + hCNGB3
C and hCNGA3
N + hCNGB3
N channels resembled that of wild type heteromeric channels. These results suggest that either CaM-binding site in hCNGB3 is sufficient for the full range of CaM regulation of heteromeric channels. However, co-expression of hCNGA3 with hCNGB3 subunits having both NH2- and COOH-terminal CaM-binding sites deleted (hCNGB3
N
C) gave rise to channels that were no longer sensitive to regulation by Ca2+-CaM (ICaM/I was 0.95 ± 0.02, n = 8) (Fig. 5, B, D, and E). Together, these results imply that both CaM-binding sites in hCNGB3 can contribute to modulation by CaM, but that the CaM-binding site in hCNGA3 is not sufficient for CaM regulation in the context of these heteromeric channels.
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To ensure that channels arising from this combination of subunits had characteristics consistent with heteromeric rather than homomeric hCNGA3 channels, the activation properties and sensitivity to block by L-cis-diltiazem were examined more closely. hCNGA3 + hCNGB3 N
C channels displayed greater relative cAMP efficacy compared with homomeric hCNGA3 channels (p < 0.001) (Table I). Furthermore, the K
for L-cis-diltiazem block of currents at +80 mV for hCNGA3 + hCNGB3
N
C channels (6.6 ± 4.2 µM, n = 0.74 ± 0.17; n = 5) was similar to that of wild-type heteromeric channels. These results confirm that hCNGB3
N
C subunits were fully competent for assembly into functional heteromeric channels. Yet, the basic properties of hCNGB3
N
C-containing channels differed somewhat from wild-type heteromeric channels. In particular, there was a significant decrease in both apparent affinity for cGMP (p = 0.001) and relative agonist efficacy, IcAMP/IcGMP (p < 0.01) (Table I). These changes indicate that deletion of both CaM-binding sites in hCNGB3 has an effect on channel gating that parallels the effect of Ca2+-CaM on the activation of wild-type heteromeric channels.
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DISCUSSION |
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With completion of this study and comparison to previous studies (for review, see Ref. 50), similarities and differences in CaM binding and regulation among olfactory, rod, and cone CNG channels are now evident. All three sensory transduction channels contain one or more subunits with NH2-terminal CaM-binding sites located a short distance from the first putative transmembrane domain: CNGA2 and CNGB1b for the olfactory channel, CNGB1 for the rod channel, and CNGA3 and CNGB3 for the cone channel. The cone channel is in several ways unique among these CNG channel types. First, the NH2- terminal CaM-binding site of the human CNGA3 subunit is functionally silent not only for homomeric channels (39), but also, as shown in this paper, for heteromeric channels containing hCNGB3 subunits. Second, the sequence of the hCNGB3 NH2-terminal CaM-binding site conforms better to typical 114 type motifs than the NH2-terminal CaM-binding site of CNGB1, which has been previously described as unconventional in that its sequence is in part similar to an IQ-type motif yet CaM binding to this site is calcium-dependent (30, 31). Third, whereas CNGB3 and CNGB1 subunits both possess a COOH-terminal CaM-binding site located distal to the CNB domain, only the site in the CNGB3 subunit is functionally important for Ca2+-CaM regulation. For the rod CNG channel, the CNGB1 COOH-terminal CaM-binding site is not necessary or sufficient for regulation by Ca2+-CaM (30, 31). In contrast, the COOH-terminal CaM-binding site of the CNGB3 subunit contributes to the sensitivity of the cone channel to Ca2+-CaM regulation and is sufficient for regulation in the absence of the NH2-terminal CaM-binding site. Thus, our results suggest that both NH2- and COOH-terminal CaM-binding sites of hCNGB3 are equally important for regulation. Because single deletions of the individual CaM-binding sites gave rise to heteromeric channels that exhibited sensitivity to modulation roughly similar to that of wild-type channels, we favor a model where each CaM-target site in hCNGB3 is independently capable of conferring regulation, rather than the two sites acting in a synergistic or additive manner.
CaM also decreases the ligand sensitivity of rod, cone, and olfactory CNG channels to different extents. Ca2+-CaM reduces the apparent affinity of the olfactory CNG channel for cAMP by up to 20-fold (18, 20), whereas it has a more modest effect on channels formed by rod photoreceptor CNGB1 plus CNGA1 subunits (19, 22, 3032). The magnitude of cone channel modulation by Ca2+-CaM is much smaller than that of olfactory CNG channels but similar to that of rod channels. Although the sensitivity of cone photoreceptor CNG channels to regulation by CaM may vary with different species, our results indicate that channels formed by human CNGB3 and CNGA3 subunits are modulated by Ca2+-CaM to an extent similar to recombinant bovine and human rod CNG channels. As previously suggested (25, 27, 32, 39, 51), CNG channel sensitivity to regulation by Ca2+-CaM is dependent not merely on the presence, number, or location of CaM-binding sites but also other structural features and interactions.
As is the case for CNGA2 homomeric channels (20, 25), deletion of the CaM-binding sites in hCNGB3 subunits alters the activation properties of heteromeric channels in a way that parallels the effect of Ca2+-CaM binding on gating of wild-type channels. Previous evidence suggests that an interaction occurs between NH2- and COOH-terminal cytoplasmic domains of olfactory CNGA2 subunits that promotes channel opening and helps control gating of the channels. Ca2+-CaM modulates olfactory CNG channels by direct binding to an NH2-terminal autoexcitatory domain (20, 52, 53), disrupting interdomain coupling with the COOH-terminal CNB domain (25). For rod CNG channels, Ca2+-CaM binding to an NH2-terminal site in CNGB1 also disrupts an interaction between this domain and the distal COOH-terminal region of CNGA1 (32). It remains to be determined if a similar mechanism is involved in CaM regulation of cone CNG channels.
Whereas the simplest explanation for the observations described in this paper is that Ca2+-CaM can regulate the activity of cone CNG channels by direct binding to NH2- and COOH-terminal CaM-binding sites of hCNGB3 subunits, other mechanisms remain possible. Ca2+-CaM may alter channel activity by binding to a channel-associated protein rather than, or in addition to, docking at the hCNGB3 subunit itself. In this regard, hCNGB3 deletions may prevent interactions between the channel and proteins other than CaM. Another possibility is that Ca2+-CaM may stimulate patch-associated CaM-dependent kinase activity, which in turn may modulate cone CNG channels via phosphorylation. CaM kinase II activity has been implicated in circadian regulation of the ligand sensitivity of native chick cone CNG channels (54); whether the reported effect is because of direct phosphorylation of the channel protein or occurs via an indirect pathway remains to be determined. Muller and co-workers (40) have demonstrated that the ligand sensitivity of homomeric bovine CNGA3 channels is regulated by protein kinase C-mediated phosphorylation. Therefore, like rod CNG channels (Refs. 55 and 56, for review, see Ref. 57), cone CNG channels may be the targets of several regulatory pathways that include but are not limited to direct binding of CaM.
An additional consideration is that at least in some species other physiologically important effectors for Ca2+-dependent regulation of cone CNG channels may act in concert with CaM. There is evidence suggesting that a Ca2+-binding protein other than CaM may regulate native CNG channels of striped bass cone photoreceptors, particularly because CaM application to patches excised from cone outer segments does not completely recapitulate the effect of the endogenous calcium-dependent modulator(s) (33, 34). For CNG channels of intact cone outer segments, changes in cytoplasmic Ca2+ concentration can alter apparent cGMP affinity over a 4-fold range (34). The more modest extent of CaM-mediated inhibition of heterologously expressed CNGB3 plus CNGA3 channels suggests that CaM can account for some but not all of this Ca2+-dependent modulation of ligand sensitivity. It has also been suggested that an unknown endogenous factor may be important for Ca2+-dependent regulation of native rod (21) and olfactory (58) CNG channels. Warren and Molday (59), however, have recently shown that soluble extracts from bovine rod outer segments that have been depleted of endogenous CaM do not contain an additional endogenous factor sufficient to regulate rod CNG channel activity. Several other Ca2+-binding proteins related to CaM are expressed in the retina (60). One of these, CaBP1, has recently been shown to compete with CaM for binding to a region within the cytoplasmic COOH-terminal domain of neuronal Cav2.1 channels (61). Further studies are needed to identify and characterize potential interactions between CNG channels and other calcium-sensitive regulatory proteins that may augment or compete with the action of CaM.
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FOOTNOTES |
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¶ To whom correspondence should be addressed. Tel.: 509-335-0701; Fax: 509-335-4650; E-mail: varnum{at}wsu.edu.
1 The abbreviations used are: CNG, cyclic nucleotide-gated; CNB, cyclic nucleotide-binding; hCaM, human calmodulin; GST, glutathione S-transferase; N, amino; C, carboxyl; CHAPS, 3-[(3-cholamidopropyl)-dimethylammonio]-1-propanesulfonic acid.
2 calcium.uhnres.utoronto.ca/ctdb/pub_pages/classify/index.htm.
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ACKNOWLEDGMENTS |
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REFERENCES |
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