Activity-Dependent Modulation of Rod Photoreceptor Cyclic Nucleotide-Gated Channels Mediated by Phosphorylation of a Specific Tyrosine Residue

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The Journal of Neuroscience, June 15, 1999, 19(12):4786-4795

Activity-Dependent Modulation of Rod Photoreceptor Cyclic Nucleotide-Gated Channels Mediated by Phosphorylation of a Specific Tyrosine Residue
Elena Molokanova, Floyd Maddox, Charles W. Luetje, and Richard H. Kramer
Department of Molecular and Cellular Pharmacology, University of Miami School of Medicine, Miami, Florida 33101

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cyclic nucleotide-gated (CNG) channels are crucial for phototransduction in vertebrate rod photoreceptors. The cGMP sensitivityof these channels is modulated by diffusible intracellular messengers,including Ca²⁺/calmodulin, contributing to negative feedback during sensoryadaptation. Membrane-associated protein tyrosine kinases and phosphatasesalso modulate rod CNG channels, but whether this results fromdirect changes in the phosphorylation state of the channel proteinhas been unclear. Here, we show that bovine rod CNG channel $alpha$ -subunits(bRET) contain a tyrosine phosphorylation site crucial for modulation.bRET channels expressed in Xenopus oocytes exhibit modulation,whereas rat olfactory CNG channels (rOLF) do not. Chimeric channelsreveal that differences in the C terminus, containing the cyclicnucleotide-binding domain, account for this difference. One specifictyrosine in bRET (Y498) appears to be crucial; replacement ofthis tyrosine in bRET curtails modulation, whereas installationinto rOLF confers modulability. As the channel becomes dephosphorylated,there is an increase in the rate of spontaneous openings in theabsence of ligand, indicating that changes in the phosphorylationstate affect the allosteric gating equilibrium. Moreover, we findthat dephosphorylation, which favors channel opening, requiresopen channels, whereas phosphorylation, which promotes channelclosing, requires closed channels. Hence, modulation by changesin tyrosine phosphorylation is activity-dependent and may constitutea positive feedback mechanism, contrasting with negative feedbacksystems underlyingadaptation.

Key words: rod photoreceptor; protein kinase; cyclic GMP; phototransduction; tyrosine kinase; phosphorylation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cyclic nucleotide-gated (CNG) channels in vertebrate photoreceptors and olfactory receptor neurons generate changes in membranepotential and intracellular Ca²⁺ concentration in response to sensory stimuli. The change in internalCa²⁺, in conjunction with calmodulin and other Ca²⁺-binding proteins, feeds back on CNG channels to lower their sensitivityto cyclic nucleotides during sensory adaptation (Kramer and Siegelbaum,1992; Hsu and Molday, 1993; Chen and Yau, 1994; Nakatani et al.,1995; Kurahashi and Menini, 1997). Other diffusible intracellularmessengers, such as diacylglycerol (Gordon et al., 1995) and nitricoxide (Broillet and Firestein, 1996) can also directly affectCNG channels and may play additional roles in sensory transductionand/oradaptation.

CNG channels are also modulated by changes in phosphorylation state catalyzed by Ser/Thr kinases (Muller et al., 1998) andphosphatases (Gordon et al., 1992) and by protein tyrosine kinases(PTKs) and protein tyrosine phosphatases (PTPs) (Molokanova etal., 1997). Rod CNG channels expressed in Xenopus oocytes exhibitan increase in cGMP sensitivity that occurs spontaneously afterexcision of membrane patches containing the channels. This increasein cGMP sensitivity is unaffected by Ser/Thr phosphatase inhibitorsbut is suppressed by a PTP inhibitor, suggesting that it resultsfrom tyrosine dephosphorylation (Molokanova et al., 1997). Inaddition, oocyte patches contain active PTKs that reverse theeffect, decreasing cGMP sensitivity after ATP application. Thisis prevented by specific inhibitors of PTKs but not by inhibitorsof Ser/Thr kinases. These results indicate that rod CNG channelsexpressed in oocytes are associated with active PTPs and PTKsthat catalyze changes in tyrosine phosphorylation state, therebyaltering cGMP sensitivity. Additional studies (Molokanova et al.,1997) suggest that rod outer segments also contain PTPs and PTKsthat modulate native CNG channels, but these enzymes are lostor inactive in excised patches fromrods.

It has been unclear whether the CNG channel protein, or a distinct protein associated with the channels, is the substratefor PTPs and PTKs. Native rod CNG channels are heteromeric, composedof $alpha$ - and $beta$ -subunits (Chen et al., 1993; Koerschen et al., 1995),but functional homomeric CNG channels with similar propertiescan be formed in Xenopus oocytes by expression of the $alpha$ -subunitalone (Kaupp et al., 1989). Here, we show that the $alpha$ -subunit ofthe bovine rod channel (bRET) contains crucial phosphorylationsites responsible for altering cGMP sensitivity. First, we showthat modulation is dependent on the activation state of the channel,such that cGMP profoundly alters the ability of PTPs and PTKsto modulate the channel. This activity-dependence of phosphorylationand dephosphorylation may be physiologically important for regulatingthe extent of modulation in rods. Second, we exploit our observationthat the rat olfactory CNG channel expressed in oocytes (rOLF)does not exhibit modulation by tyrosine phosphorylation. By studyingchimeric bRET-rOLF channels, we have identified a specific tyrosineresidue (Y498) within the cyclic nucleotide binding site of therod channel that is crucial for modulation. Thus, cGMP sensitivityis dynamically regulated by changes in the phosphorylation stateof a specific tyrosine in the rod CNG channelprotein.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression and recording from oocyte CNG channels. A cDNA clone encoding the bovine rod photoreceptor CNG channel $alpha$ -subunit(Kaupp et al., 1989) was used for in vitro transcription of mRNA,as described previously (Goulding et al., 1992), which was injectedinto Xenopus oocytes (50 nl per oocyte at 1 ng/nl). After 2-7d, the vitelline membrane was removed from injected oocytes, whichwere then placed in a chamber for patch-clamp recording at 21-24°C.Glass patch pipettes (2-3 M $Omega$ ) were filled with a solution containing(in mM): 115 NaCl, 5 EGTA, and 10 HEPES, pH 7.5. This also servedas the standard bath solution and cGMP perfusion solution, unlessnoted otherwise. After formation of a gigaohm seal, inside-outpatches were excised, and the patch pipette was quickly (<30 sec)placed in the outlet of a 1 mm diameter tube for cGMP application.We used a perfusion manifold containing up to 15 different solutionsthat is capable of solution changes within 50 msec. A series offour to five cGMP concentrations (10-2000 µM cGMP) was appliedto the patch. Application of the series required 20-30 sec andwas repeated at 1 min intervals. In many experiments, 200 µM ATP(Mg salt) was applied transiently for 3 min starting 10.5 minafter patch excision. cGMP, ATP, and sodium orthovanadate wereobtained from Sigma (St. Louis,MO).

Current responses through CNG channels were obtained with an Axopatch 200A patch clamp (Axon Instruments, Foster City, CA),digitized, stored, and later analyzed on a 486 personal computerusing pClamp 6.0 software. Membrane potential was held at $-$ 75mV. Current responses were normalized to the maximal CNG current(I_max), elicited by saturating (2 mM) cGMP. Normalized dose-responsecurves were fit to the Hill equation: I/I_max = 1/(1 + (K_1/2/[A])ⁿ), where A is the cGMP concentration and n is the Hill coefficient,using a nonlinear least squares fitting routine (Origin; MicrocalSoftware, Inc., Northampton, MA). Variability among measurementsis expressed as mean ±SEM.

Fitting dose-response data to the allosteric Monod-Wyman-Changeux model. To fit dose-response curves to the Monod-Wyman-Changeux(1965) (MWC) model, we first needed to estimate spontaneous openprobability (P_sp) and maximal open probability (P_max). To estimateP_sp, spontaneous openings were recorded with patch pipettes coatedwith Sylgard (Dow Corning Co., Midland, MI) at a holding potentialof $-$ 80 mV and pipette and test solutions containing (in mM): 67KCl, 30 NaCl, 10 EGTA, 1 EDTA, and 10 HEPES, pH 7.2. Mean spontaneouscurrents (I_sp) resulting from unliganded channel openings (filteredat 4 kHz, digitized at 20 kHz) were determined from the integralof the difference between the channel current and zero currentbaseline. P_sp was calculated from the equation: P_sp = (I_sp/I_max)P_max, where I_max is the current elicited by saturatingcGMP.

Spontaneous currents were measured at 1 min after excision in the absence of cGMP, and 2 mM cGMP was applied for ~8 min, followedby 1 min of extensive and continuous washing with cGMP-free solution,which flowed 2 ml/min. The patch pipette was inserted directlyinto the perfusion tube, and from the initial rate at which themacroscopic current deactivates after washout (<50 msec), we estimatethat by 2 min later cGMP is completelyremoved.

To estimate P_max, we used noise analysis. Membrane currents, filtered at 10 kHz, were recorded over 60 sec in the absenceand presence of 25-2000 µM cGMP and analyzed using StrathclydeElectrophysiological Software (Dr. John Dempster, University ofStrathclyde, Glasgow, Scotland). Current variance values werefit according to the relation: $sigma$ ² = Ii $-$ I²/N, where N is the number of CNG channels, and i is the unitarycurrent, estimated from i = V_m $gamma$ , where V_m is the driving force( $-$ 80 mV) and $gamma$ is the single channel conductance (57 pS) (Liuet al., 1998). P_max was calculated as follows: P_max = I_max/(Ni).

Currents through CNG channels at various concentrations of cGMP were expressed as open probability (P_o) according to P_o =(I_A/I_max) (P_max $-$ P_sp) + P_sp, where I_A is the current at a givenligand concentration. Open probabilities as a function of theligand concentration were fit by the MWC model according to P_o= (1 + [A]/K_o)ⁿ/(L_o (1 + [A]/K_c)ⁿ + (1 + [A]/K_o)ⁿ), where K_o and K_c are dissociation constants of ligand bindingto the channel in the open and close states, respectively, and[A] is ligand concentration. Parameters of the MWC model wereeither directly determined (L_o, P_max) or obtained from the fitsof the model (K_o/K_c). The equation L_o = 1/P_sp $-$ 1 provides a valuefor the allosteric equilibrium constant (L_o) between the unligandedclosed and open states of thechannel.

Mutagenesis and construction of chimeric receptors. Mutant CNG channel subunits were constructed using PCR (Higuchi, 1990)and Pfu DNA polymerase. Our notation for mutant subunits is tolist the naturally occurring residue, followed by the positionof that residue, followed by the change that has been made. Forexample, the mutant bRET-Y498F is bRET in which tyrosine 498 hasbeen changed to a phenylalanine. To minimize the amount of PCRproduct in the final construct that would have to be sequenced,a small cassette containing the mutation was cut from the PCRproduct and inserted into the wild-type construct using existingrestriction sites. All PCR-derived portions of final constructswere confirmed by sequencing using Sequenase 2.0 from AmershamLife Sciences (Cleveland, OH). Pfu DNA polymerase was from Stratagene(La Jolla,CA).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activity-dependence of modulation by tyrosine dephosphorylation

bRET channels expressed in Xenopus oocytes exhibit a gradual increase in their sensitivity to cGMP (a decrease in K_1/2) whenmembrane patches containing the channels are excised from thecell. Our previous studies (Molokanova et al., 1997) suggest thatthis decrease in K_1/2 results from tyrosine dephosphorylationby PTPs that are constitutively active in excised patches. Brieflyexposing patches to ATP reverses this process, resulting in adecrease in the sensitivity to cGMP (an increase in K_1/2). Ourevidence also suggests that this increase in K_1/2 is attributableto tyrosine phosphorylation by constitutively active PTKs in excisedpatches. To better understand whether bRET channels are modulateddirectly by acting as substrates for these PTK(s) and PTP(s),we examined how modulation is affected by the presence of ligandsthat selectively bind to CNG channels (i.e., cyclicnucleotides).

We first investigated whether the decrease in K_1/2 after patch excision, which results from tyrosine dephosphorylation, isinfluenced by the presence of cGMP. Changes in the K_1/2 afterpatch excision were monitored by repeatedly applying various concentrationsof cGMP onto the patch (Fig. 1A). When these cGMP concentrationswere applied at 1 min intervals, the change in K_1/2 occurred quickly( $tau$ of 2.4 min), stabilizing at 52 ± 5% (n = 55) of its initialvalue within 10 min after excision. However, when the cGMP concentrationswere applied less frequently, at 3 min intervals, the K_1/2 declinedmore slowly ( $tau$ of 6.1 min), decreasing to 66 ± 4% (n = 7) of itsinitial value after 13 min. At 2 min intervals, the K_1/2 declinedat a rate that was intermediate to that elicited by 1 or 3 minapplication intervals. These observations suggest that the declinein K_1/2 associated with tyrosine dephosphorylation occurs morequickly when cGMP is present, accounting for the faster rate ofdecline when cGMP is applied more frequently.

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Figure 1. Activity-dependence of modulation by tyrosine dephosphorylation of bRET channels. A, Decline of K_1/2 for activation by cGMP (increase in sensitivity) with time after excision of membrane patches. To determine K_1/2 values, four concentrations of cGMP (50, 100, 250, and 2000 µM) were repeatedly applied on different patches at 1 (n = 55), 2 (n = 8), or 3 (n = 7) min intervals, starting 1 min after patch excision. In this and other figures, data are normalized to the initial K_1/2 value obtained 1 min after excision, unless indicated otherwise. Note that K_1/2 declines more quickly with more frequent cGMP application. B, Application of ligand (2 mM cGMP) during treatment period (9 min) promotes the decline of K_1/2 for cGMP, whereas with no ligand, K_1/2 changes little (n = 10-14 each). C, cGMP and cAMP treatment promote similar changes in the K_1/2 for cGMP, depending only on the integrated open time of CNG channels. Integrated open time is defined as the total current activated by ligand during the treatment period, divided by the maximal integrated current activated by saturating (2 mM) cGMP. Each point represents an individual patch with the final K_1/2 normalized to the initial K_1/2 value obtained at 1 min after patch excision. Patches were examined over a 10 min period, except for those treated with cAMP for 19 min. Patches were repeatedly exposed to various concentrations of ligand (interval paradigm, as in A) or continuously exposed to saturating ligand (continuous treatment, as in B). The dashed line is a single exponential fit to the data with a time constant of 0.4 min.

To further examine the effect of ligands, we used a different paradigm, illustrated in Figure 1B. The initial K_1/2 was measured1 min after patch excision, ligand was applied continuously duringa "treatment" period for the subsequent 9 min, and then K_1/2 valueswere again monitored at 1 min intervals. When saturating cGMP(2 mM) was present during the treatment period, the K_1/2 declineddramatically during the first 10 min after excision. In contrast,when ligands were absent during the treatment period, the K_1/2exhibited little change during the first 10 min, but subsequentexposure to cGMP could elicit a decline. With no ligand presentduring the treatment period, the K_1/2 declined by 12 ± 4% (n =12), whereas with cGMP present, the K_1/2 declined by 52 ± 3% (n=14).

Activation of CNG channels involves two processes: binding of ligands and opening of the channel. Whereas binding of cGMPto rod CNG channels is tightly coupled to opening, cAMP is lesseffective in triggering opening, such that saturating cAMP elicitsonly ~2% of the current activated by saturating cGMP (Kaupp etal., 1989; Goulding et al., 1992). To distinguish whether theacceleration of dephosphorylation results from ligand bindingor channel opening, we compared the effects of cGMP and cAMP.We observed that saturating cAMP was much less effective thansaturating cGMP in promoting a decline in K_1/2 as a result ofdephosphorylation, suggesting that simple occupancy of the bindingsites is insufficient to account for effect of ligand. In Figure1C, we take into account the different efficacies of cAMP versuscGMP and the different application paradigms (e.g., continuousvs interval application) by determining the integrated open timefor each experiment. The integrated open time represents the averagetime spent by each channel in the open state and was estimatedby calculating the total current activated by ligand during thetreatment period (usually 10 min), divided by the maximal integratedcurrent activated by saturating cGMP. Figure 1C shows that thedecrease in K_1/2 is promoted equally well by cAMP and cGMP oncethe difference in efficacy of these ligands is accounted for bycalculating integrated open time. The decrease in K_1/2 dependsonly on the integrated open time with either ligand and followsthe same trajectory, with a time constant of ~0.4 min. At integratedopen times greater than ~1.5 min, additional exposure to ligandresults in no further change in K_1/2, suggesting that dephosphorylationis complete. These experiments strongly suggest that channel openingrather than ligand binding is the crucial factor that promotesdephosphorylation.

Activity-dependence of modulation by tyrosine phosphorylation

We next examined whether the effect of ATP exposure on K_1/2 is influenced by the presence of cGMP. In previous work (Molokanovaet al., 1997), we showed that treatment of patches with ATP couldsuppress or reverse the decrease in K_1/2 that occurs after patchexcision and that the effect of ATP is blocked by specific inhibitorsof PTKs. Figure 2A shows that treatment with ATP increases theK_1/2 of RET channels for cGMP, partially reversing the declinein K_1/2 that occurs during the first 10 min after patch excision.However, if a saturating concentration of cGMP (2 mM) is includedalong with ATP during the treatment period, no change in K_1/2occurs. Thus, cGMP can completely suppress the increase in K_1/2attributed to tyrosine phosphorylation.

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Figure 2. Activity-dependence of modulation by tyrosine phosphorylation of bRET channels. A, Increase in K_1/2 for activation by cGMP (decrease in sensitivity) after exposure to 200 µM ATP. Note that the presence of 2 mM cGMP during the treatment period (3 min) prevents the change in K_1/2 in response to ATP (n = 12 each). B, Summary data for experimental protocol illustrated in A. Change in normalized K_1/2 during the treatment period (10-13 min after excision) with the different treatments indicated. n = 38 for ATP alone; n = 8-12 for other treatments.

How does addition of cGMP prevent the effect of ATP on the channels? Because tyrosine dephosphorylation is promoted by openingthe channels (Fig. 1), it is possible that cGMP inhibits the ATPeffect not by inhibiting PTK, but rather by promoting PTP activity.According to this scenario, even if the channels are tyrosinephosphorylated in the presence of ATP plus cGMP, they are morerapidly dephosphorylated by the enhanced PTP activity. If thiswere true, addition of vanadate, which inhibits PTPs (Swarup etal., 1982) and suppresses the apparent dephosphorylation of therod CNG channel (Molokanova et al., 1997), should restore theeffect of ATP. However, Figure 2B shows that there was no significantchange in K_1/2 when ATP and cGMP were coapplied, even when 200µM vanadate was added (p < 0.05). Hence, it is likely that inhibitionof the ATP effect by saturating cGMP results from suppressionof PTK activity rather than promotion of PTPactivity.

Further studies (Fig. 2B) show that saturating cAMP (20 mM) also prevented the increase in K_1/2 during ATP treatment. Thesimilarity of the actions of cAMP and cGMP suggest that simpleoccupancy of the ligand binding site could account for the preventionof modulation by tyrosine phosphorylation. Our observation thatdephosphorylation is accelerated by ligands rules out the possibilitythat ligands simply indiscriminately occlude access to the phosphorylationsite by both PTK and PTP enzymes. However, we cannot rule outthe possibility that bound ligand selectively prevents accessby PTKs. An additional possibility is that cAMP prevents tyrosinephosphorylation by inducing conformational changes that are notassociated with full activation of the channels. The observationthat the rates of both dephosphorylation and phosphorylation areprofoundly altered by cyclic nucleotides strongly suggests thatthe CNG channel proteins themselves are substrates for PTPs andPTKs.

Identification of a protein region containing the tyrosine phosphorylation site

To investigate the molecular basis of modulation, we investigated the behavior of the related CNG channel rOLF and exploitedthe observation that this channel does not exhibit modulationby tyrosine phosphorylation. Figure 3 shows the behavior of rOLFchannels expressed in Xenopus oocytes after patch excision. Variousconcentrations of cGMP or cAMP were applied at 1 min intervals,and resulting dose-response curves were fit with the Hill equation,and the three free parameters, K_1/2, Hill coefficient, and maximalcurrent, were analyzed. Unlike bRET channels, the K_1/2 valuesof activation were stable after patch excision and showed no significantchanges after application of ATP, either with cGMP or cAMP asthe ligand (Fig. 3A). Likewise, the Hill coefficient exhibitedno significant change over time (Fig. 3B). The maximal currentelicited by saturating concentrations of cGMP or cAMP (I_max) didchange, increasing progressively with time after excision (Fig.3C). However, this increase was unaffected by vanadate, a PTPinhibitor (data not shown), or by ATP, indicating that the increasein I_max is unrelated to tyrosine phosphorylation or dephosphorylation.Thus, rOLF channels expressed in oocytes do not appear to be modulatedby tyrosine phosphorylation. One of several possible explanationsis that they may be lacking one or more critical tyrosine residuesthat constitute the phosphorylation site.

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Figure 3. The rOLF channel does not exhibit modulation by tyrosine phosphorylation or dephosphorylation. A, K_1/2 values for activation by cGMP and cAMP measured at 1 min intervals after patch excision. Note that there is no significant change after either excision or ATP application. B, There is also no significant change in Hill coefficient values after excision and ATP application. C, Maximal current (I_max) elicited by saturating cGMP (2 mM) or cAMP (20 mM) increase with time after excision. I_max values were normalized to the initial I_max, measured at 1 min after patch excision. n = 14 for cGMP; n = 9 for cAMP.

To test this possibility, we used chimeric CNG channels containing segments of the rOLF sequence substituted into the correspondingpositions of bRET and segments of bRET substituted into the correspondingpositions of rOLF (Gordon and Zagotta, 1995b). We found that substitutionof the cytoplasmic C-terminal segment, which contains the conservedcyclic nucleotide binding site, was capable of conferring sensitivityto tyrosine phosphorylation. Thus, bRET channels containing theC terminus of rOLF behaved like rOLF channels, exhibiting no changesin K_1/2 after patch excision or ATP application (Fig. 4A). Incontrast, rOLF channels containing the C terminus of bRET exhibitedstriking changes in K_1/2 after excision and ATP application (Fig.4B). Hence, chimeric channels containing the C terminus of bRETexhibited modulation, whereas channels that contained the C terminusof rOLF did not.

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Figure 4. The difference in modulability of bRET and rOLF channels results from differences in the cytoplasmic C-terminal domain. A-D, Changes in K_1/2 for cGMP with time after patch excision and after application of 200 µM ATP. The icons illustrate each chimeric construct, with gray representing portions of the bRET channel and black indicating portions of the rOLF channel. The chimeras used in parts A-D correspond to CHM1, CHM18, CHM15, and CHM16 of Gordon and Zagotta (1995). n = 8-10 patches for each panel.

We also examined chimeras of the N-terminal cytoplasmic domain, which has also been implicated in the activation of CNG channels(Goulding et al., 1994; Gordon and Zagotta, 1995; Gordon et al.,1997). The N terminus of rOLF also contains a domain that bindscalmodulin, which can modulate cyclic nucleotide sensitivity (Liuet al., 1994). We found that substitution of the N-terminal domainhad no effect on modulation by tyrosine phosphorylation. Thus,bRET channels containing the N terminus of rOLF exhibited largechanges in K_1/2 after excision and ATP application (Fig. 4C),whereas rOLF channels containing the N terminus of bRET did notexhibit changes in K_1/2 (Fig. 4D). Hence, whereas the specificsequence of the C terminus of bRET appears to be crucial for determiningwhether modulation by tyrosine phosphorylation can occur, thespecific nature of the N terminus appears to be less importantand may not contain relevant tyrosine phosphorylationsites.

Identification of a specific tyrosine residue involved in modulation

The cytoplasmic C-terminal domain of bRET contains 10 tyrosine residues. Three of these are not conserved with respect tothe rOLF sequence. Because modulability by tyrosine phosphorylationmaps to this region of the channel protein, we generated threenew channel constructs in which each of these tyrosines in bRETwas substituted with the amino acid in the complementary positionof rOLF. One of the mutant constructs (bRET-Y541C) could not befunctionally expressed in Xenopus oocytes and therefore couldnot be analyzed. Figure 5A shows a comparison of the behaviorof the remaining two constructs with that of bRET and rOLF. ThebRET-Y454N channel exhibits changes in K_1/2 after excision andATP application that are indistinguishable from those observedin bRET. In contrast, the bRET-Y498F channel exhibited very littlemodulation, with only a minor decrease in K_1/2 during the first10 min after excision and no significant change resulting fromapplication of ATP. The modulability of bRET-Y498F is greatlyreduced with respect to bRET, but comparison with rOLF shows thatit is not completely eliminated. In other respects, the bRET-Y498Fchannels are similar to bRET channels. Thus, the initial K_1/2after excision was 132 ± 8 µM (n = 12), slightly higher than theinitial K_1/2 of bRET (117 ± 6 µM; n = 55). Moreover, the maximalopen probability of bRET-Y498F channels at saturating cGMP was~0.85, similar to that of bRET (Goulding et al., 1994), and thechannels retained their selective activation by cGMP versus cAMP(data not shown). The simplest explanation for these observationsis that Y498 is a phosphorylation site that contributes to modulationof the rod CNG channel.

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Figure 5. Identification as Y498 as a site crucial for modulation by phosphorylation. Decline in K_1/2 for cGMP with time after patch excision and increase in K_1/2 with 200 µM ATP application, indicative of tyrosine dephosphorylation and phosphorylation, respectively. Changes in K_1/2 resulting from both processes are shown for mutant bRET (A) and mutant rOLF (B) channels. Data from wild-type bRET (n = 55) and rOLF (n = 14) are shown in both A and B for comparison. n = 12 patches for each mutant.

To test whether this tyrosine is sufficient for inducing modulation, we constructed a mutant of the rOLF channel in whicha tyrosine residue was introduced into the appropriate position,substituting for a phenylalanine (rOLF-F477Y). We find that this"reverse mutant" channel does exhibit changes in K_1/2 after patchexcision and ATP application that are significantly larger thanthose seen in rOLF, although the modulation is not as profoundas that exhibited by bRET (Fig. 5B). To determine whether thechanges in K_1/2 in rOLF-F477Y indeed result from introductionof a tyrosine phosphorylation site, we tested the effects of vanadate,a PTP inhibitor, and erbstatin, a PTK inhibitor. In the presenceof 100 µM vanadate, the K_1/2 for cGMP decreased only by 8 ± 4%(n = 4) during the first 10 min after excision compared with 23± 7% (n = 8) without vanadate present. Moreover, in four experiments,application of 50 µM erbstatin completely blocked the effect ofATP on the K_1/2 for cGMP, consistent with introduction of a tyrosinephosphorylation site. These results strongly support the hypothesisthat Y498 of the bRET channel is a tyrosine phosphorylation sitethat regulates cGMPsensitivity.

Figure 6 quantifies the results of our mutagenesis experiments. Modulation resulting from dephosphorylation and phosphorylationwere both large in bRET channels but insignificant in rOLF channels.Mutant bRET-Y541C did not functionally express. Modulation ofmutant bRET-Y454N (n = 12) by both dephosphorylation and phosphorylationwere similar to bRET. In contrast, modulation of bRET-Y498F wasgreatly reduced compared with bRET (p < 0.05). After patch excision,the K_1/2 of rOLF and bRET channels decreased by 6 ± 7 (n = 14)and 48 ± 3% (n = 55), respectively. The decrease in K_1/2 of thebRET-Y498F channel was only 16 ± 5% (n = 12), accounting for atleast 75% of the difference between bRET and rOLF.

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Figure 6. Modulation by dephosphorylation and phosphorylation of bRET and rOLF point mutants. Top, Dephosphorylation was estimated by monitoring the change in K_1/2 for cGMP during the first 10 min after patch excision, normalized to the initial K_1/2 (1 min after excision). Bottom, Phosphorylation was estimated by monitoring the change in K_1/2 for cGMP evoked by a 3 min application of 200 µM ATP, as shown in Figure 5. K_1/2 values after ATP were normalized to values immediately before ATP application. There was no expression (N.E.) of mutant bRET-Y541C. Numbers of experiments for each bar are the same as Figure 5, except rOLF-C520Y in which n = 8.

Introduction of the tyrosine into rOLF (rOLF-F477Y) had the opposite effect, installing modulability by both phosphorylationand dephosphorylation. The decrease in K_1/2 evoked by dephosphorylationof this channel was ~23 ± 7% (n = 8), approximately half the decreaseobserved in bRET channels. The rOLF-F477Y channel exhibited a31 ± 7% increase in K_1/2 resulting from phosphorylation, ~75%as large as the increase observed with bRET. Hence, this datastrongly implicates residue Y498 of bRET as a phosphorylationsite that modulates cGMPsensitivity.

The failure of bRET-Y541C to express functionally prevented us from obtaining information about a potential role for Y541.As an additional attempt to gain information about this site,we constructed rOLF-C520Y, inserting a tyrosine into rOLF at aposition equivalent to Y541 of bRET. This construct was capableof functional expression but did not show any modulation. Hence,this tyrosine residue cannot confer modulability on rOLF, suggestingthat it is not involved in modulation ofbRET.

Modulation by tyrosine phosphorylation results from changes in the allosteric channel opening transition

To understand how tyrosine phosphorylation affects the activation of CNG channels, we used the classic allosteric model ofMonod et al. (1965), which was adapted for CNG channels (Stryer,1987; Goulding et al., 1994). According to this model, all foursubunits of a CNG channel undergo a concerted allosteric transitionbetween open (O) and closed (C) states. In the absence of ligand,the equilibrium gating constant of this transition is termed L_o.Ligand can bind to both closed and open channels, but the dissociationconstant of binding to the open channel (K_o) is lower than thatfor the closed channel (K_c). Sequential binding of ligand to eachof the four subunits causes a progressive shift in the equilibriumgating constant by the factor (K_o/K_c)ⁿ, where n is the number of ligand molecules bound to the channel.According to this model, changes in the apparent affinity of ligandas a result of phosphorylation could be caused by altering theallosteric opening equilibrium (change in L_o) and/or by alteringthe ratio of dissociation constants of binding to open versusclosed states (change in K_o/K_c).

To determine whether the value of L_o changes during dephosphorylation, we examined spontaneous opening of CNG channels (Tibbset al., 1997) in the complete absence of ligand at 1 and 10 minafter patch excision. Because these openings do not involve ligandbinding, they can be used as a unambiguous indicator of channelgating. The small single channel conductance of bRET channelsmakes it very difficult to measure current through spontaneousopen channels. Therefore, we used a chimeric channel (RO133; Gouldinget al., 1993) composed of the bRET channel substituted with thepore-forming region of the catfish olfactory channel, which hasa threefold larger single channel conductance that bRET. We findthat RO133 exhibits behaviors characteristic of tyrosine dephosphorylationand phosphorylation that are qualitatively and quantitativelysimilar to those observed in bRET, namely a decrease in K_1/2 afterpatch excision and an increase in K_1/2 after ATP application (datanotshown).

Figure 7A shows how open probability of RO133 channels changes during the first 10 min after patch excision. The spontaneousopen probability of these channels increased from 5.3 × 10⁵ to 1.37 × 10⁴ (160% increase). As a control, we performed the same analysison patches from oocytes expressing rOLF channels, which are muchmore sensitive to cGMP but do not exhibit modulation by tyrosinephosphorylation. For rOLF channels, spontaneous open probabilitywas 2.31 × 10³ ± 0.91 × 10³ at 1 min and 2.19 × 10³ ± 0.88 × 10³ at 10 min after patch excision (n = 4). Thus, using the sameprocedure, we find no increase in spontaneous openings between1 and 10 min after excision. Our observation that the increasein spontaneous openings is specific for bRET also indicates thatchannels native to oocytes are unlikely to contribute, becausethey should be present in both RO133 and rOLF patches.

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Figure 7. The MWC model of CNG channel activation suggests that modulation of cGMP-sensitivity results from a change in the equilibrium of the allosteric gating transition. A, Open probability of RO133 channels in the complete absence of ligand (spontaneous open probability, left panel) and in the presence of 2 mM cGMP (maximal open probability, right panel), determined at 1 and 10 min after patch excision. See Materials and Methods for how these parameters are calculated. B, Equilibrium gating constant (L_o) at 1 and 10 min after patch excision, calculated from spontaneous open probability. C, Fits of the MWC model (solid lines) to data representing activation of RO133 channels obtained 1 min (closed circles) and 10 min (open circles) after patch excision. Inset represents MWC model with C and O representing closed and open channels, with zero to n ligands bound, A representing agonist, and K_o and K_c representing dissociation constants for binding to the open and closed states. D, Ratio of dissociation constants (K_o/K_c) as a result of fits to the model. n = 7 patches for 1 and 10 min for each panel.

The maximal open probability of RO133 channels, determined from noise analysis of current in the presence of saturating ligand(2 mM cGMP), increased from 0.86 to 0.95 (10% increase) duringthe first 10 min after patch excision. We observed a similar increasein maximal current in bRET channels of 13 ± 5%; (n = 55), althoughwe previously presented data from a single patch that showed nosignificant increase (Molokanova et al., 1997). With cAMP as theagonist, which has a much lower efficacy that cGMP, we observeda much larger increase in maximal current of 122 ± 17% (n = 10)over the first 10min.

Our measurement of spontaneous open probability allows the direct determination of L_o. Figure 7B shows that L_o decreases 2.6-foldafter channel dephosphorylation. Using the calculated values forL_o and the directly determined values of maximal open probability,dose-response curves of RO133 channel activation at 1 and 10 minafter excision were fitted with the MWC model (Fig. 7C). The ratioof dissociation constants for binding to open versus closed states(K_o/K_c) was a free parameter, and this value was obtained fromthe best fit of the model to our data. Figure 7D shows that thevalues of K_o/K_c required for the best fit were not significantlydifferent at 1 versus 10 min after patch excision (p < 0.01).Therefore, the decrease in K_1/2 resulting from tyrosine dephosphorylationcan be fully accounted for by changes in L_o without requiringa change in K_o/K_c. Hence, the increase in apparent affinity forcGMP caused by tyrosine dephosphorylation results, at least inpart, from an energetically more favorable openingreaction.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of the tyrosine phosphorylation site responsible for modulation

Our results indicate that modulation of bRET channels expressed in oocytes results from direct phosphorylation and dephosphorylationof tyrosine residues located in the bRET polypeptide. One particulartyrosine, Y498, appears to have a major importance for modulation.When this tyrosine is removed from bRET (bRET-Y498F), modulationis reduced by 75%. When a tyrosine is introduced into the correspondingposition of rOLF (rOLF-F477Y), modulation appears, although thechanges in cGMP sensitivity are only ~50% as great as those observedin bRET. The simplest interpretation of our results is that Y498is a phosphorylation site that alters cGMP sensitivity in bRET.The residual modulation observed when this site is removed frombRET suggests that phosphorylation of additional tyrosines alsocontributes. The partial introduction of modulability to rOLFafter installation of the tyrosine is also consistent with thisidea. Additional tyrosines that may contribute to modulation arelikely to reside in the C terminus because the chimeric bRET channelcontaining the rOLF C terminus exhibits a complete loss of modulation,and the chimeric rOLF channel containing the bRET C terminus exhibitsa complete gain ofmodulation.

Many cyclic nucleotide-binding proteins, including CNG channels, cAMP and cGMP-dependent protein kinases (PKA and PKG, respectively),and the catabolite gene activator protein (CAP), a bacterial transcriptionfactor, contain a conserved cyclic nucleotide binding site (Shabband Corbin, 1992). In each of these proteins, the amino acid positioncorresponding to Y498 is highly conserved, containing either atyrosine or a phenylalanine. Type I PKG and CAP both contain atyrosine, but it is not known whether the activities of theseproteins are modulated by tyrosine phosphorylation. Whereas therat olfactory CNG channel (rOLF) contains a phenylalanine (Dhallanet al., 1990), the catfish olfactory channel contains a tyrosine(Goulding et al., 1992), and studies have shown that this channelexpressed in Xenopus oocytes does exhibit changes in K_1/2 afterpatch excision and ATP application (R. Kramer, unpublished observations),suggesting that it too is susceptible to modulation by tyrosinephosphorylation.

The crystal structure of CAP shows that cyclic nucleotides bind in a pocket between an eight-stranded $beta$ -roll and a long $alpha$ -helix(the C-helix), with two additional $alpha$ -helices supporting the structure(Weber and Steitz, 1987). The amino acid corresponding to Y498(Y23 in CAP) is located in the $beta$ 1 strand, with the side groupon the periphery of the $beta$ -roll, accessible to the aqueous environment.The predicted position of Y498 in CNG channels is removed fromcontact sites with cyclic nucleotides, consistent with our findingthat phosphorylation affects allosteric gating transitions butnot necessarily binding of ligands. The $beta$ 1 strand is located closeto the N-terminal end of the cyclic nucleotide-binding domain.Hence, by occurring between the ligand binding site and the restof the channel protein, the tyrosine phosphorylation site is locatedin a strategic position for influencing coupling of ligand bindingto channelgating.

Molecular basis for the difference in modulability of bRET and rOLF channels

The absence of a tyrosine in the position of rOLF (F477) corresponding to Y498 of bRET partly explains why rOLF does not exhibitmodulation. We have considered several other structural and functionaldifferences between bRET and rOLF that could also contribute tothe difference in modulability. First, the binding of ligandsappears to be coupled more tightly to the opening of rOLF channelsthan in bRET channels (Zagotta and Siegelbaum, 1996). It is conceivablethat even if tyrosine phosphorylation occurred in rOLF as it doesin bRET, it would have less of an impact in the context of suchfavorable gating. Our results suggests that this cannot explainthe lack of modulation in rOLF. The free energy change of channelopening in rOLF channels with bound cAMP is much less than withbound cGMP, making the allosteric opening transition much lessfavorable and similar to that of the bRET channel with cGMP asthe agonist (Goulding et al., 1994; Gordon and Zagotta, 1995).However, even with cAMP as the agonist, the rOLF channel stilldoes not exhibitmodulation.

Second, modulation may be impaired in rOLF because of a possible lack of recognition sites for binding PTKs and PTPs. Severaltypes of ion channels, including nicotinic acetylcholine receptors(Swope and Huganir, 1994; Fuhrer and Hall, 1996) and certain voltage-gatedK⁺ channels (Holmes et al., 1996), contain specific domains thatmediate "docking" to src homology domains 2 and 3 (SH2 and SH3)that are common in PTKs and PTPs (Fantl et al., 1993). The bindingsite for an SH2 domain is characterized by proline-rich regions,and examination of the predicted bRET and rOLF sequences failto reveal such motifs in cytoplasmic portions of the proteins,suggesting that other uncharacterized binding domains mediateinteraction with PTKs and PTPs. The observation that introductionof a tyrosine into rOLF can confer modulability implies that atleast to some extent PTKs and PTPs can effectively bind and recognizethe rOLF channel as asubstrate.

Activity-dependence of tyrosine phosphorylation and dephosphorylation

Both phosphorylation and dephosphorylation of bRET are activity-dependent, such that cyclic nucleotides alter the abilityof PTKs and PTPs to modulate the channel. Cyclic nucleotides preventphosphorylation by PTKs, which could occur if bound ligand occludedthe phosphorylation site, sterically preventing access by theenzymes. We cannot distinguish between this possibility and anadditional one in which the binding of ligands produces conformationalchanges short of channel opening, which influence the abilityof PTKs to catalyze phosphorylation byPTKs.

In contrast, PTP activity is accelerated by cyclic nucleotides. Our studies comparing cGMP and cAMP suggest that the activity-dependenceof dephosphorylation results from channel activation rather thanligand binding per se. Hence, the extent to which a ligand promotesdephosphorylation is directly related to its ability to open CNGchannels (Fig. 1C). The catalytic rates of PTPs appear to be dependenton the specific conformation of the channel (e.g., closed vs open),which can be altered much more effectively by cGMP than bycAMP.

The conformation of the channel might differentially alter the accessibility of a specific phosphorylation site to PTKs andPTPs that are already bound to the channel. An alternate, moresimple possibility is that the conformation of the channel determineswhether PTKs or PTPs can bind to the channel in the first place.Figure 8 illustrates a model in which the PTKs and PTPs can bindand unbind from the bRET channel, with the closed state allowingPTK binding and the open state allowing PTP binding. The activity-dependencereflects the exclusivity of PTK or PTP binding. The slow kineticsof phosphorylation and dephosphorylation could result from theslow kinetics of association of the enzymes with the channel,which may be rate-limiting.

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Figure 8. Schematic model illustrating positive feedback resulting from activity-dependence of modulation by tyrosine phosphorylation and dephosphorylation. The top and bottom represent closed and open channels, respectively, and the left and right represent phosphorylated and dephosphorylated channels, respectively. The ovals represent cGMP molecules. The relative thickness of arrowheads represents changes in the favorability of gating.

One interesting feature of the model is that it is capable of exhibiting positive feedback. Thus, when the channel opens (e.g.,in the presence of cGMP), binding of PTP, which dephosphorylatesthe channel, promotes channel opening, further accelerating dephosphorylation.In contrast, when the channel is closed (and/or when ligand isabsent), binding of PTK leads to phosphorylation, promoting channelclosing and further phosphorylation. The channel potentially hasfour tyrosine phosphorylation sites, so according to the abovescheme, it is possible that dephosphorylation of one site increasesthe likelihood of dephosphorylation of additional sites. To testthis possibility, it will be necessary to determine how many phosphorylationevents are required to change the cGMP sensitivity of a singlechannel.

The positive feedback implied in this model is in sharp contrast to negative feedback systems, such as those mediated by intracellularCa²⁺, which contribute to relatively rapid (seconds to minutes) adaptationprocesses in photoreceptors (Koutalos and Yau, 1996). It is interestingto speculate about the functional role of modulation by tyrosinephosphorylation and what its positive feedback characteristicsmight play in rods. Our previous studies show that native CNGchannels in rods can be modulated by native PTKs and PTPs in amanner similar to that observed in expressed bRET channels (Molokanovaet al., 1997). Recent studies show that certain growth factors,especially insulin-like growth factor I (IGF-1), modulate cGMP-sensitivityof native rod channels, apparently by changing their tyrosinephosphorylation state (A. Savchenko and R. Kramer, unpublishedobservations). From these observations, we predict that the effectsof growth factors, such as IGF-1, on rod CNG channels should exhibitpositive feedback. The positive feedback feature of modulationby tyrosine phosphorylation may provide a mechanism for offsettingor overriding the homeostatic negative feedback mechanisms ofadaptation.

  FOOTNOTES

Received Jan. 22, 1999; revised March 31, 1999; accepted April 7, 1999.

This work was supported by grants from the National Institutes of Health (EY11877 to R.H.K. and DA08102 to C.W.L.) and theAmerican Heart Association, Florida Affiliate (9502002 to R.H.K.).We thank Michael Vendiola for technical assistance, Alexei Savchenkofor help with figures, and William Zagotta for providing chimericchannelconstructs.
Correspondence should be addressed to Dr. Richard H. Kramer, P.O. Box 016189, University of Miami School of Medicine, Miami,FL 33101.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Broillet M-C, Firestein S (1996) Direct activation of the olfactory cyclic nucleotide-gated channel through modification of sulfhydryl groups by NO compounds. Neuron 16:377-385[ISI][Medline].
Chen T-Y, Yau K-W (1994) Direct modulation by Ca²⁺-calmodulin of cyclic nucleotide-activated channel of rat olfactory receptor neurons. Nature 368:545-548[Medline].
Chen T-Y, Peng Y-W, Dhallan RS, Ahamed B, Reed RR, Yau K-W (1993) A new subunit of the cyclic nucleotide-gated cation channel in retinal rods. Nature 362:764-767[Medline].
Dhallan RS, Yau K-W, Schrader K, Reed R (1990) Primary structure and functional expression of a cyclic nucleotide-activated channel from olfactory neurons. Nature 347:184-187[Medline].
Fantl WF, Johnson DE, Williams LT (1993) Signaling by tyrosine kinases. Annu Rev Biochem 62:453-481[ISI][Medline].
Fuhrer C, Hall ZW (1996) Functional interaction of Src family kinases with the acetylcholine receptor in C2 myocytes. J Biol Chem 271:32474-32481[Abstract/Free Full Text].
Gordon SE, Zagotta WN (1995) Localizations of regions affecting an allosteric transitions in cyclic nucleotide-activated channels. Neuron 14:857-864[ISI][Medline].
Gordon SE, Brautigan DL, Zimmerman AL (1992) Protein phosphatases modulate the apparent agonist affinity of the light-regulated ion channel in retinal rods. Neuron 9:739-748[ISI][Medline].
Gordon SE, Downing-Park J, Tam B, Zimmerman AL (1995) Diacylglycerol analogs inhibit the rod cGMP-gated channel by a phosphorylation-independent mechanism. Biophys J 69:409-417[Abstract/Free Full Text].
Gordon SE, Varnum MD, Zagotta WN (1997) Direct interactions between amino- and carboxyl-terminal domains of cyclic nucleotide-gated channels. Neuron 19:431-441[ISI][Medline].
Goulding EH, Ngai J, Kramer RH, Colicos S, Siegelbaum SA, Axel R, Chess A (1992) Molecular cloning and single channel properties of a cyclic nucleotide-gated cation channel from catfish olfactory receptor neurons. Neuron 8:45-58[ISI][Medline].
Goulding EH, Tibbs G, Liu D, Siegelbaum SA (1993) Role of H5 domain in determining pore diameter and ion permeation through cyclic nucleotide-gated channels. Nature 364:61-64[Medline].
Goulding EH, Tibbs GR, Siegelbaum SA (1994) Molecular mechanism of cyclic-nucleotide-gated channel activation. Nature 372:369-374[Medline].
Higuchi R (1990) Recombinant PCR. In: PCR protocols, a guide to methods and applications (Innis MA, Gelfand GH, Sninsky JJ, White TJ, eds), pp 177-183. San Diego: Academic.
Holmes TC, Fadool DA, Ren R, Levitan IB (1996) Association of Src tyrosine kinase with a human potassium channel mediated by SH3 domain. Science 274:2089-2091[Abstract/Free Full Text].
Hsu YT, Molday RS (1993) Modulation of the cGMP-gated channel of rod photoreceptor cells by calmodulin. Nature 361:76-79[Medline].
Kaupp BU, Niidome T, Tanabe T, Terada S, Bonigk W, Stuhmer W, Cook NJ, Kangawa K, Matsuo H, Hirode T, Miyata T, Numa S (1989) Primary structure and functional expression from complementary DNA of the rod photoreceptor cGMP-gated channel. Nature 342:762-766[Medline].
Koerschen HG, Illing M, Seifert R, Sesti F, Williams A, Gotzes S, Colville C, Muller F, Dose A, Godde M, Molday L, Kaupp UB, Molday RS (1995) A 240 kDa protein represents the complete $beta$ subunit of the cyclic nucleotide-gated channel from rod photoreceptor. Neuron 15:627-636[ISI][Medline].
Koutalos Y, Yau K-W (1996) Regulation of sensitivity in vertebrate rod photoreceptors by calcium. Trends Neurosci 19:73-81[ISI][Medline].
Kramer RH, Siegelbaum SA (1992) Intracellular Ca²⁺ regulates sensitivity of cyclic nucleotide-gated channels in olfactory receptor neurons. Neuron 9:897-906[ISI][Medline].
Kurahashi T, Menini A (1997) Mechanism of odorant adaptation in the olfactory receptor cell. Nature 385:725-729[Medline].
Liu DT, Tibbs GR, Paoletti P, Siegelbaum SA (1998) Constraining ligand-binding site stoichiometry suggests that a cyclic nucleotide-gated channel is composed of two functional dimers. Neuron 21:235-248[ISI][Medline].
Liu M, Chen T-Y, Ahamed B, Li J, Yau K-W (1994) Calcium-calmodulin modulation of the olfactory cyclic nucleotide-gated cation channel. Science 266:1348-1354[Abstract/Free Full Text].
Molokanova E, Trivedi B, Savchenko A, Kramer RH (1997) Modulation of rod photoreceptor cyclic nucleotide-gated channels by tyrosine phosphorylation. J Neurosci 17:9068-9076[Abstract/Free Full Text].
Monod J, Wyman J, Changeux JP (1965) On the nature of allosteric transitions: a plausible model. J Mol Biol 12:88-118[ISI][Medline].
Muller F, Bonigk W, Sesti F, Frings S (1998) Phosphorylation of mammalian olfactory cyclic nucleotide-gated channels increases ligand sensitivity. J Neurosci 18:164-173[Abstract/Free Full Text].
Nakatani K, Koutalos Y, Yau K-W (1995) Ca²⁺ modulation of the cGMP-gated channels of bullfrog retinal rod photoreceptors. J Physiol (Lond) 484:69-76[ISI][Medline].
Shabb JB, Corbin JD (1992) Cyclic nucleotide-binding domains in proteins having diverse functions. J Biol Chem 267:5723-5726[Free Full Text].
Stryer L (1987) Visual transduction: design and recurring motifs. Chem Scr 27B:161-171.
Swarup G, Cohen S, Garbers DL (1982) Inhibition of membrane phosphotyrosyl-protein phosphatase activity by vanadate. Biochem Biophys Res Commun 107:1104-1109[ISI][Medline].
Swope SL, Huganir RL (1994) Binding of the nicotinic acetylcholine receptor to SH2 domains of Fyn and Fyk protein tyrosine kinases. J Biol Chem 269:29817-29824[Abstract/Free Full Text].
Tibbs GR, Goulding EH, Siegelbaum SA (1997) Allosteric activation and tuning of ligand efficacy in cyclic-nucleotide-gated channels. Nature 386:612-615[Medline].
Weber IT, Steitz TA (1987) Structure of a complex of catabolite gene activator protein and cyclic AMP refined at 2.5 Å resolution. J Mol Biol 198:311-326[ISI][Medline].
Zagotta WN, Siegelbaum SA (1996) Structure and function of cyclic nucleotide-gated channels. Annu Rev Neurosci 19:235-263[ISI][Medline].

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