Desensitization Mechanism of GABA Receptors Revealed by Single Oocyte Binding and Receptor Function

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

A correction has been published

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (18)

Citing Articles via Google Scholar

Google Scholar

Articles by Chang, Y.

Articles by Weiss, D. S.

Search for Related Content

PubMed

PubMed Citation

Articles by Chang, Y.

Articles by Weiss, D. S.

Previous Article  |  Next Article

The Journal of Neuroscience, September 15, 2002, 22(18):7982-7990

Desensitization Mechanism of GABA Receptors Revealed by Single Oocyte Binding and Receptor Function
YongChang Chang, Emmanuel Ghansah, Yonghui Chen, Jiawei Ye, and David S. Weiss
Departments of Neurobiology and Physiology, and Biophysics, University of Alabama at Birmingham, Birmingham, Alabama 35294

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Prolonged exposure of most fast neurotransmitter-operated ion channels to agonist drives the receptors into a nonfunctional,or desensitized, state. Despite extensive investigation, desensitizationremains a thoroughly characterized, yet poorly understood, process.Part of the difficulty in elucidating the mechanism of desensitizationhas been an inability to resolve the kinetics of both agonistbinding and functional desensitization in the same set of operablereceptors. To overcome this limitation, we applied single oocyte³H-ligand binding and two-electrode voltage clamp to oocytes expressingrecombinant $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors. Using this approach, we reportseveral observations fundamental to the mechanism of desensitization.First, we confirm that desensitization reversibly shifts GABAreceptors into a high-affinity state. For [³H]GABA binding, the half-maximal binding of the desensitized statewas ~0.040 µM. Second, we show that, upon agonist removal, thishigh-affinity state disappears with a time constant of 127 ± 12sec (n = 4), similar to the time constant for functional recoveryfrom desensitization of 124 ± 26 sec (n = 5). [³H]GABA, however, dissociates fourfold faster ( $tau$ = 30 ± 2 sec;n = 3) than functional recovery, indicating that desensitizedreceptors need not be bound by GABA. These data provide directevidence for a cyclical model of receptordesensitization.

Key words: GABA_A receptor; desensitization; binding; kinetics; affinity; oocyte

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Early studies of endplate nicotinic acetylcholine (nACh) receptors demonstrated that prolonged exposure to agonist drove thereceptors into a refractory, or desensitized, state (Katz andThesleff, 1957). Recovery from desensitization was a time-dependentprocess that first required removal of the agonist. It is nowclear that desensitization is a general feature of most ligand-activatedion channels (Changeux and Edelstein, 1998). In GABA receptors,it has been suggested that desensitization may play an importantrole in shaping synaptic inhibition (Jones and Westbrook, 1995;Overstreet et al., 2000), and desensitization has also been implicatedin the mechanism by which allosteric modulators exert their effects(Birnir et al., 1997; Zhu and Vicini, 1997). Still, despite extensiveinvestigation, desensitization remains a thoroughly characterized,yet poorly understood,process.

In their pioneering studies, Katz and Thesleff (1957) proposed the following

View larger version (9K):
[in this window]
[in a new window]

cyclical model for desensitization: where R is the activatable receptor, A is the agonist molecule, and D is the desensitized receptor. They postulated that,if the affinity for the agonist in the desensitized state wasgreater than that of the activatable state, then this scheme couldaccount for the following: (1) the profound desensitization inthe absence of significant activation and (2) the slow rate ofonset of desensitization compared with the rate of recovery whenagonist was removed. Although evidence has accumulated that suggeststhe desensitized state has a higher affinity for agonist thanthat of the nondesensitized closed state (Rang and Ritter, 1970;Weber et al., 1975; Weiland et al., 1975; Quast et al., 1978;Neubig et al., 1982; Heidmann et al., 1983), the issue is farfrom resolved. Scheme 1 also predicts that agonist can dissociatedirectly from the desensitized state. In this scenario, a receptormay no longer be bound by agonist but yet still functionally desensitized.Again, direct evidence for this hypothesis islacking.

We developed previously a technique that allows one to perform repeated radioactive ligand binding measurements in singleintact oocytes expressing recombinant GABA receptors (Chang andWeiss, 1999a). One can then submit these oocytes to electrophysiologicalrecording, allowing a direct correlation between binding and functionin the same set of operable surface receptors. Here, we use thisapproach to investigate the desensitization of recombinant GABAreceptors comprising rat $alpha$ 1, $beta$ 2, and $gamma$ 2subunits.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

cDNA and cRNA preparation. The wild-type cDNAs of rat $alpha$ 1, $beta$ 2, and $gamma$ 2 subunits were subcloned into the vector pGEMHE for highexpression (Liman et al., 1992). The plasmids were linearizedby NheI, which left a >200 base pair tail for cRNA stability.RNase-free cDNA templates were prepared by treating linearizedcDNA with proteinase K. Capped cRNAs were then transcribed byT7 RNA polymerase. After degradation of the DNA template by RNase-freeDNase I, the cRNAs were purified and resuspended in diethyl pyrocarbonate(DEPC)-treated water. cRNA yield and integrity were examined ona 1% agarosegel.

Oocyte preparation and cRNA injection. Female Xenopus laevis (Xenopus I, Ann Arbor, MI) were anesthetized by 0.2% MS-222.The ovarian lobes were surgically removed from the frog and placedin calcium-free OR2 incubation solution consisting of 92.5 mMNaCl, 2.5 mM KCl, 1 mM MgCl₂, 1 mM Na₂HPO₄, 5 mM HEPES, 50 U/mlpenicillin, and 50 µg/ml streptomycin, pH 7.5. The lobes werecut into small pieces and digested with 0.3% Collagenase A (BoehringerMannheim, Indianapolis, IN) with constant stirring at room temperaturefor 1.5-2 hr. The dispersed oocytes were thoroughly rinsed withthe above solution containing 1 mM CaCl₂. Stage VI oocytes wereselected, and the follicular layer, if still present, was manuallyremoved with fine forceps. The oocytes were incubated at 18°C.

Micropipettes for cRNA injection were pulled from borosilicate glass (Drummond Scientific, Broomall, PA) on a Sutter Instruments(Novato, CA) P87 horizontal puller, and the tips were cut withscissors to an ~40 µm outer diameter The cRNA with dilution inDEPC-treated water (for voltage clamp) or without dilution (forbinding) was drawn up into the micropipette and injected intooocytes with a Nanoject microinjection system (Drummond Scientific)at a total injection volume of 20-60nl.

Electrophysiology. One to 2 d after injection, the oocyte expressing $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors was voltage clamped at $-$ 70 mV.Dose-response relationships were determined by measuring the currentinduced by a range of agonist concentrations. The EC₅₀ and Hillcoefficient were determined by fitting the data to the Hill equationof the following form:

(1)

where I is the current amplitude for that particular agonist concentration ([A]), I_max is the maximum current amplitude,EC₅₀ is the agonist concentration that induces a 50% maximal response,and n is the Hillcoefficient.

Single oocyte binding. Two to 3 d after injection, the expression level of the $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors was examined by two-electrodevoltage clamp at $-$ 70 mV. Oocytes with a current in response to10 µM GABA of >3000 nA were selected for the binding assay. Mostof the oocytes tested had a current amplitude in the 4000-6000nA range. The single oocyte binding was performed as describedpreviously (Chang and Weiss, 1999a). Briefly, the oocyte expressing $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors was held by gentle suction to the end ofa sequencing gel loading pipette tip. The oocyte was then incubatedin OR2 containing [³H]GABA or [³H]muscimol for 30 sec at room temperature, rinsed for 5 sec ina 0°C OR2 bath with constant stirring (to remove unbound ³H-ligand), and finally placed in 250 µl of OR2 at room temperaturefor 85 sec to let the bound ³H-ligand dissociate. The 250 µl of OR2 was then thoroughly mixedwith 4 ml of scintillation fluid, and the radioactivity (in countsper minute) was determined in a liquid scintillation counter.This binding paradigm was followed by an accompanying run withthe initial incubation in the same concentration of ³H-ligand plus 300 µM nonradiolabeled gabazine (SR95531) or bicuculline,antagonists of the GABA_A receptor (Research Biochemicals, NatickMA). In this case, the counts per minute released is a measureof the nonspecific ³H-ligand binding and, when subtracted from the total binding (countsper minute measured in the absence of the antagonist), provideda measure of the specific binding. Except for the experimentsexamining the dose dependence of ³H-ligand binding, 1 µM ³H-ligand was typically used to assess changes in the amount ofbound ligand. Based on our estimate of the apparent K_D (0.04 µM)and the k_off ( $tau$ = 30 sec) and the relationship k_obs = k_on * [GABA]+ k_off, we determined an association time constant for 1 µM GABAof 1.2 sec. Thus, our typical 30 sec incubation in 1 µM GABA ismore than sufficient to reach equilibrium for binding to receptorsalready in the high-affinity state. However, during the incubationin ³H-agonist, more receptors enter the desensitized state. In thiscase, the measurements were not at steady state. In addition,we demonstrate that GABA dissociates from the high-affinity statewith a time constant of ~30 sec at room temperature. Thus, welose <15% of the bound [³H]GABA in the 5 sec cold rinse. In all binding paradigms, calculationsconfirmed that there would be no significant depletion of the³H-agonist.

For the measurement of the apparent binding affinity, a concentration range of ³H-ligand was examined. The relationship between the concentrationof ³H-ligand and the specific binding (B) were fit with the followingform of the Hill equation:

(2)

in which K_D is the concentration of ligand (A) required for half-maximal binding, B_max is the maximum binding of ³H-agonist, and n is the Hill coefficient. We will use the termapparent K_D (half-maximal binding) because this experiment doesnot necessarily measure the receptor affinity because the agonist-receptorinteraction is not a simple bimolecular process (Colquhoun, 1998;Chang and Weiss, 1999a). The rate of dissociation was determinedusing the same binding protocol as described above, except thatthe final release of ³H-ligand was into sequential 250 µl wells of OR2. The dissociationdata were least-squares fit by an exponential decayfunction.

The equilibrium dose-response relationship for [³H]GABA was determined by placing the oocyte in a 96 V-shaped well plate. TheOR2 in the well was removed and replaced with 12 µl of OR2 withthe desired [³H]GABA concentration. After a 30 min incubation, the solutionwas removed, and the oocyte was rinsed five times with 300 µlof cold OR2 over a 10 sec time period. Finally, 250 µl of roomtemperature OR2 was added to the well, and 10 min was allowedfor the release of [³H]GABA. The OR2 was then collected, and radioactivity was determinedin a liquid scintillation counter. The process was repeated butwith the 30 min [³H]GABA incubation in the presence of 300 µM SR95531 to determinethe nonspecific binding in the sameoocyte.

Predictions of the proposed kinetic scheme. The prediction of the EC₅₀ for functional desensitization by Scheme 2 (presentedin Discussion) was determined from the following relationship:

(3)

where D is the fraction of receptors in the desensitized state for a given GABA concentration, K_R and K_D are the agonistbinding affinities of the resting and desensitized receptor, respectively,M is [R]/[D] or the ratio of the equilibrium occupancies of theresting and desensitized forms of the unbound receptor, and nis the maximum number of GABA molecules that can bind to the receptor,two in our case (Edelstein and Changeux, 1996).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Detection of specific binding in single oocytes expressing $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors

Oocytes were injected with cRNA encoding for $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors. Figure 1A demonstrates that we can obtain specific bindingof [³H]GABA or [³H]muscimol to individual oocytes expressing recombinant $alpha$ 1 $beta$ 2 $gamma$ 2GABA receptors. We previously used this single oocyte radioactiveligand binding technique to study $rho$ 1 GABA receptors in which,because of the lack of desensitization and extremely slow dissociationof GABA from its binding site, we were able to examine agonistassociation and dissociation to and from nondesensitized openand closed states (Chang and Weiss, 1999a). In contrast, the GABA-activatedchloride currents from $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors decay much fasterthan $rho$ 1 receptors when agonist is removed (Amin and Weiss, 1994).Figure 1B shows a sample current response at 8°C in which onesmall drop (~10 µl) of 20 µM GABA was added to an oocyte in arapidly flowing 100 µl bath. The current decay was well fit bya single exponential function with a time constant of 0.56 ± 0.03and 0.85 ± 0.08 sec at 23 and 8°C, respectively (n = 8). This1.5-fold difference in the time constant of decay at the two temperatureswas partly attributable to the measured 1.2-fold slower perfusionrate at 8°C compared with 23°C and was likely attributable toa slight shrinkage of the diameter of the tubing at the lowertemperature. Recombinant $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors expressed in HEK293cells and assayed with the patch-clamp technique (allowing a fastersolution exchange than oocyte recording) exhibit a biexponentialdeactivation with the slowest time constant on the order of 180msec (Tia et al., 1996). Thus, the current decay we observed inoocytes expressing $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors likely represents, inlarge part, the rate of agonist removal from the bath rather thanthe underlying receptor kinetics.

View larger version (12K):
[in this window]
[in a new window]
Figure 1. Specific binding to individual oocytes expressing recombinant GABA_A receptors. A, Oocytes were incubated in 1 µM [³H]GABA or 2 µM [³H]muscimol for 30 sec as described in Materials and Methods. Nonspecific binding was determined in the presence of 300 µM SR95531. Specific binding would be the difference between the total and nonspecific binding (in counts per minute). B, An oocyte expressing GABA_A receptors was voltage clamped at $-$ 70 mV at 8°C, and 10 µl of 20 µM GABA was added in a rapidly flowing 100 µl bath. The current decay was well fit by a single exponential function with a time constant of 0.85 ± 0.08 sec (n = 8). The arrow indicates 5 sec, the duration of the cold rinse in the binding experiments. Note that, by 5 sec, the current returned to baseline.

In the binding assay, the initial incubation in ³H-ligand was followed by a 5 sec 0°C rinse to wash away the free ³H-ligand from the surface of the oocyte. The rinse time was approximatelysixfold longer than the observed time constant of current decay(Fig. 1B, arrow), indicating that ~99.7% of the receptors wouldhave closed by the end of the rinse. (This percentage is likelyto be a lower limit given that the observed current decay reflectsagonist removal in the perfusion chamber rather than agonist dissociation,and, in addition, the rinse with 150 ml of OR2 in a beaker withconstant stirring should have a faster exchange rate around theoocyte surface than that of the recording chamber.) So, if channelsare closing and agonist is dissociating within 5 sec, what isthe source of the specific binding in Figure 1A? One possibleexplanation is that the ³H-ligand is binding to a state of the receptor with higher affinitythan that of the state(s) along the activation pathway. The datain Figure 1B demonstrates that the binding is clearly not to thepresumed high-affinity open state (Chang and Weiss, 1999b). Althoughwe cannot completely rule out that a small fraction of the bindingin Figure 1A is to nondesensitized states (closed or open), evidencewill be provided that the majority of the binding is to the high-affinitydesensitizedstate.

Increased binding in desensitized receptors

Figure 2A shows a current in response to a 150 sec application of 500 µM GABA in an oocyte expressing $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors.Note that, by the end of the prolonged GABA application, the currentdecayed toward a steady-state level that was ~5% of the peak current.Thus, a majority of the receptors were functionally desensitized.This current decay was not attributable to a change in the chloridegradient because we compared the reversal potentials during amaintained application of 2 µM GABA ( $-$ 20.7 ± 1.7; n = 3), whichshows little decline in current, and at the end of the prolongedapplication of 500 µM GABA ( $-$ 23.4 ± 2.0; n = 3). This representsa 5.6 ± 1.4% decrease in the driving force at the end of the 500µM GABA application, which would only account for a small fractionof the >95% decrease in current amplitude. The filled bar in Figure2B plots the specific binding in single oocytes expressing $alpha$ 1 $beta$ 2 $gamma$ 2GABA receptors that were first exposed to 500 µM nonradiolabeledGABA for 150 sec, rinsed for 30 sec, and then tested for specificbinding of 1 µM [³H]GABA using the same protocol as in Figure 1A. The open bar plotsthe specific binding from the same oocytes but before the 150sec 500 µM GABA incubation. Desensitization of the receptors increasedthe specific binding from 163 ± 25 to 1253 ± 309 cpm (n = 8),a 7.7-fold increase. In the case of the desensitized receptors,a fraction of the binding sites would still be bound by unlabeledGABA at the end of the 30 sec rinse. Thus, we would be measuringbinding in the fraction of receptors from which GABA has dissociated.The observation that the specific binding increased with the 500µM GABA preincubation suggests that, although the receptors releasedGABA, they are still desensitized. In a subsequent section, amore direct demonstration of this will be provided. Nevertheless,an interpretation of this increased binding is that the desensitizedreceptors have a higher affinity for agonist.

View larger version (15K):
[in this window]
[in a new window]
Figure 2. Increased binding of 1 µM [³H]GABA after receptor desensitization. A, Application of 500 µM GABA for 150 sec desensitized the GABA receptors. B, Specific binding of 1 µM [³H]GABA was determined in an oocyte, and then the oocyte was incubated in 500 µM GABA for 150 sec and rinsed for 30 sec, and the specific binding of 1 µM [³H]GABA was determined again in the same oocyte. Desensitization increased the specific binding from 163 ± 25 to 1253 ± 309 cpm (n = 8), a 7.7-fold increase.

Relationship between the concentration dependence of the increased binding and functional desensitization

If the increase in binding in Figure 2B were to the desensitized state of the receptor, then the concentration dependenceof the increased binding should be similar to the concentrationdependence of functional desensitization. Figure 3A shows ourmethod for assessing the concentration dependence of functionaldesensitization. First, we measured the current in response to1 µM GABA. Next, a variable concentration of GABA was appliedfor 150 sec to desensitize the receptors. Thirty seconds fromthe termination of the GABA application, the current in responseto 1 µM GABA was tested again. The level of functional desensitizationwas the ratio of the 1 µM GABA applications after and before desensitization.This ratio is normalized and plotted in Figure 3B (open circles).The solid line is a fit of Equation 1 to these data and yieldedan EC₅₀ for functional desensitization of 9.8 ± 3.4 µM. We usedthe same protocol (agonist concentrations and incubation times)to examine the concentration dependence of the increased binding.The filled circles in Figure 3B plot the increase in binding of1 µM [³H]GABA (B) normalized to the maximum binding increase (B_max) asa function of the concentration of nonlabeled GABA used to desensitizethe receptors. The continuous line is a least-squares fit of Equation2 to these data and yielded an apparent K_D of 10.1 ± 1.2 µM (n= 4). Equilibrium was likely not achieved at the lower GABA concentrationsin either the functional or binding experiments of Figure 3. Thus,the EC₅₀s and apparent K_D values are not accurate determinationsof the GABA concentration required to desensitize half the receptorsor the GABA concentration required for a half-maximal increasein binding. Nevertheless, the goal was to correlate the concentrationdependence of functional desensitization and [³H]GABA binding. Because the relationships are remarkably similar,these data further support the notion that the measured bindingis to the desensitized state of the receptor.

View larger version (18K):
[in this window]
[in a new window]
Figure 3. Correlation of the concentration dependence of the increased binding and functional desensitization. A, Oocytes were first tested with 1 µM GABA and desensitized for 150 sec with 1, 3.16, 10, 31.6, and 100 µM GABA, and then retested with 1 µM GABA to assess the fraction of functionally desensitized receptors. Three representative traces from an oocyte desensitized with 1, 3.16, and 10 µM GABA are superimposed. B, The open circles plot the fraction of desensitized receptors as a function of the concentration of GABA used in the desensitizing application. The same protocol was used to assess the concentration dependence of increased binding (filled circles). Both functional desensitization and increased binding show the same concentration dependence with an EC₅₀ of 9.8 ± 3.4 µM (n = 3) and an apparent K_D of 10.1 ± 3.2 µM (n = 4), respectively.

Relationship between the time course of the disappearance of the increased binding and the time course of functional recovery

If the increased binding is to desensitized receptors, then the time course of the disappearance of the increased bindingshould be similar to the time course of functional recovery fromdesensitization. Figure 4A shows the paradigm for assessing thetime course of recovery from the functionally desensitized state.After a stable response to 1 µM GABA was obtained, the receptorswere desensitized for 150 sec in 500 µM GABA. At the end of thisprolonged GABA application and a 30 sec rinse, 30 sec pulses of1 µM GABA were applied at 2 min intervals. The filled circlesin Figure 4A plot the fractional recovery of the current versustime. The recovery was well described by a single exponentialfunction with a time constant of 124 ± 26 sec (n = 5). A similarprotocol (30 sec incubation, 5 sec rinse, 85 sec release) wasused to assess the disappearance of the increased binding aftera 150 sec incubation of 500 µM GABA and 30 sec rinse (Fig. 4B).The decay of the increased binding was dominated by an exponentialfunction with a time constant of 127 ± 12 sec (n = 4). Note that,after 600 sec, the binding was still slightly elevated over theoriginal baseline, suggesting the presence of an additional slowercomponent. Nevertheless, the similarity of the time constantsthat dominate the recoveries further supports the hypothesis thatthe observed ³H-ligand binding reflects the desensitized state of the receptor.

View larger version (19K):
[in this window]
[in a new window]
Figure 4. Correlation of the time course of the recovery of function and increased binding after receptor desensitization. A, After a stable response to 1 µM GABA was obtained, 500 µM GABA was applied for 150 sec, followed by a 30 sec rinse, and a 1 µM 30 sec test pulse of GABA was applied in 2 min intervals. The filled circles plot the recovery, and the solid line is from a fit of a single exponential function yielding the indicated time constant. B, The same protocol was performed to assess the decay of the increased binding, which also decreased as a single exponential function (solid line) with a time constant very similar to that observed for functional recovery.

Comparison of muscimol activation and binding

The EC₅₀ for $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors is ~46 µM for GABA compared with ~14 µM for muscimol (Amin and Weiss, 1993). Furthermore,the available stock concentrations of [³H]GABA is 11 µM compared with 51 µM for [³H]muscimol. Thus, we can examine [³H]muscimol binding to the receptor across a wider activation rangethan for [³H]GABA. The open circles in Figure 5A plot the normalized currentamplitude as a function of muscimol concentration in oocytes expressing $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptors. These data were fit with a Hill equation(continuous line) yielding an EC₅₀ of 5.3 ± 1.0 µM and a Hillcoefficient of 1.60 ± 0.10 (n = 5). We next conducted bindingstudies over a comparable range of [³H]muscimol concentrations. The filled circles in Figure 5A plotthe specific binding as a function of the [³H]muscimol concentration. Fitting a Hill equation to the meanof the binding data yielded a dominant apparent K_D of 6.3 µM (n= 6), which agreed well with that determined in the electrophysiologicalanalysis of muscimol-mediated activation.

View larger version (20K):
[in this window]
[in a new window]
Figure 5. Muscimol binding and activation. A, Correlation of the concentration dependence of activation and binding by muscimol. The open circles plot the dose-response relationship for muscimol. The solid line is a fit of the Hill equation yielding an EC₅₀ of 5.3 ± 1.0 µM and a Hill coefficient of 1.60 ± 0.10 (n = 5). The specific binding for [³H]muscimol (filled symbols) demonstrated a dominant apparent K_D of 6.3 µM and a Hill coefficient of 1.76. The reported binding parameters represent fits to the mean rather than the mean of the fits to individual oocytes. For both binding and activation, the data were normalized to the maximum predicted from a least-squares fit to the data points. B, Desensitization shifts the receptors into a high-affinity state. Specific binding is plotted as a function of [³H]muscimol. For the resting (open symbols) and recovered (shaded symbols) states, oocytes were incubated with the indicated concentrations of [³H]muscimol and specific binding was determined as in Figure 1A. In the desensitized case (filled symbols), the oocyte was incubated in 500 µM GABA for 150 sec and rinsed for 30 sec before each test concentration. For all three relationships, the data were well described by the sum of two Hill equations with EC₅₀ values and Hill coefficients provided in Table 1. For each oocyte, the data were normalized to the value at 6.3 µM in the resting state.

If the desensitized state is of higher affinity than the resting closed state, the question arises as to why the EC₅₀ foractivation and the apparent K_D for binding in Figure 5A are inexcellent agreement. In the binding studies, prolonged exposureto muscimol drives the receptors to the high-affinity desensitizedstate to which we can measure bound [³H]muscimol. In the electrophysiological studies, the receptorsmust be driven through the same set of states on the pathway tochannel opening. Thus, a possible interpretation of the data inFigure 5A is that the concentration dependence is similar forboth activation and desensitization because they share commonagonist concentration-dependent bindingsteps.

Direct demonstration that desensitization increases the apparent affinity of the receptor

The data thus far suggests that the desensitized state has an increased agonist affinity. To directly test this hypothesis,we examined binding as a function of [³H]muscimol concentration as in Figure 5A, except each test concentrationof [³H]muscimol was preceded by a 150 sec preincubation in 500 µM GABA,followed by a 30 sec rinse. The open circles in Figure 5B plotthe binding as a function of [³H]muscimol concentration without predesensitization (resting).The filled circles plot the binding as a function of [³H]muscimol with predesensitization before each test concentrationof [³H]muscimol (desensitized). Note that the dose-binding relationshipshifted to the left, indicating a higher apparent affinity. Thereceptors were then allowed to recover, and the binding as a functionof [³H]muscimol (without predesensitization) was reexamined (Fig. 5B,shaded circles, Recovered). The dose-binding relationship returnedto the control, restinglevel.

For all three conditions in Figure 5B (Resting, Desensitized, and Recovered), the sum of two Hill equations was required tofit the binding curves, suggesting a minimum of two apparent affinities.Fitting a single component gave an inadequate description of thedata. Table 1 provides the parameters for the two components.These data indicate a high-affinity component of <200 nM and alow-affinity component in the 6-9 µM range (Table 1). In theresting and recovered curves, the fraction of the high-affinitycomponent was 0.15 in both cases, whereas the fraction of thehigh-affinity component after desensitization was 0.58. Becauseof the small amplitude of the high-affinity component in the restingand recovered states, as well as the low number of data points,the fitting failed to converge to a solution. To estimate theparameters, we fixed the apparent K_D of the high-affinity componentto the value we determined in the desensitized state. Regardlessof the specific values of the parameters, we interpret the twocomponents as follows. Without predesensitization, a small populationof receptors may already exist in the desensitized state (seeDiscussion). Thus, we measure a minor high-affinity componentand a dominant low-affinity component. The same is true for therecovered state. During desensitization, however, receptors shiftto a high-affinity state, and, therefore, the fraction of thehigh-affinity component was increased. In the desensitized situation,the low-affinity component was still significant because recoveryis occurring during both the 30 sec rinse after the 500 µM GABAdesensitization and the 30 sec incubation in [³H]muscimol.


View this table:
[in this window]
[in a new window]
Table 1. Parameters from the fit of the sum of two Hill equations to the relationship between the concentration dependence of [³H]muscimol binding

Rate of dissociation of [³H]GABA from desensitized receptors

As demonstrated in Figure 2, desensitized receptors show an enhanced binding of [³H]GABA. Unless new binding sites are being uncovered by desensitization(an unlikely scenario), these data suggest that GABA must dissociatefrom the desensitized receptor faster than the disappearance ofthe high-affinity state (Fig. 4B). To quantify the rate of dissociation,we examined the time course of [³H]GABA dissociation from the desensitized receptors. Oocytes wereexposed to 500 µM nonradiolabeled GABA for 150 sec, rinsed for30 sec, and then incubated in 1 µM [³H]GABA for 30 sec. Figure 6 shows the time course of dissociationof [³H]GABA. The continuous line is the best fit of a single exponentialcomponent, which yielded a time constant of 30 ± 2 sec (n = 3).There is evidence of a faster component, but we do not have thetemporal resolution to establish its kinetics. Nevertheless, thesedata, coupled with the data in Figure 4 demonstrating a functionalrecovery with a time constant of 124 sec, indicate that receptorscan remain in a desensitized state long after agonist has dissociatedfrom its binding site.

View larger version (21K):
[in this window]
[in a new window]
Figure 6. Dissociation rate of [³H]GABA from desensitized receptors. Receptors were first desensitized with 500 µM GABA and then bound with 1 µM [³H]GABA. The filled symbols plot the [³H]GABA released in 6 sec intervals. The dissociation was well described by a single exponential component (solid line) yielding the indicated time constant. The data were normalized to the first point of the control run before desensitization of the receptors. The plotted value is actually the absolute value of the derivative of dissociation. However, the derivative of an exponential function has the same time constant, so the reported $tau$ is the same as that for the dissociation.

In a previous study using single oocyte binding and concomitant two-electrode voltage clamp on oocytes expressing recombinant $rho$ 1 GABA receptors, we identified an ~10-fold excess in the numberof receptors determined by binding compared with electrophysiology(Chang and Weiss, 1999a). This comparison was possible becauseof the slow agonist dissociation and lack of desensitization ofthe receptor. Unfortunately, because of the rapid activation anddesensitization kinetics of the $alpha$ 1 $beta$ 2 $gamma$ 2 receptor and because desensitizedreceptors do not conduct current, we were unable to make a similarcomparison. Although we cannot rule out excess binding, the highcorrelation between the concentration and time dependence of desensitizationas assessed by binding and electrophysiology (Figs. 3, 4) givesus confidence that we are probing the same process(es) with thetwomeasurements.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Part of the difficulty in elucidating the mechanism of desensitization has been an inability to resolve the kinetics of bothagonist binding and functional desensitization in the same setof operable receptors. To this end, we used the single oocytebinding technique (Chang and Weiss, 1999a), along with the two-electrodevoltage clamp, to investigate the mechanism of GABA receptordesensitization.

We were able to measure specific binding of [³H]GABA and [³H]muscimol in individual oocytes expressing recombinant $alpha$ 1 $beta$ 2 $gamma$ 2 GABAreceptors. We concluded that the observed specific binding wasto the desensitized state of the receptor based on the followingobservations. First, the specific binding increased dramatically(approximately eightfold) after the receptors were desensitized.Second, the concentration dependence of functional desensitization(EC₅₀ of 9.8 µM) and increased binding (apparent K_D of 10.1 µM)were similar. And third, the increase in binding after desensitizationrecovered with a time constant of 127 sec, similar to the 124sec time constant of recovery from functional desensitization.Having established that the observed binding was to the functionallydesensitized state, we addressed two fundamental issues regardingthe mechanism of GABA receptor desensitization: (1) the dissociationrate of agonist and its relationship to functional recovery and(2) the affinity of the desensitizedstate.

Relationship between the dissociation rate of agonist and the lifetime of the functionally desensitized state

A cyclical model of receptor desensitization (Scheme 1) (Katz and Thesleff, 1957) implies that agonist can dissociate directlyfrom the desensitized receptor. Thus, a receptor may have releasedagonist yet still be functionally desensitized. Previous evidencein support of this notion is that the recovery rate of desensitizednACh receptors does not depend on the particular agonist (Rangand Ritter, 1970). The basis for this argument is that, if agonistremained bound, the affinities of the different agonists woulddetermine their rates of recovery. Additional evidence for thecyclical model is that the observed rate of agonist dissociationfrom desensitized receptors in membrane preparations was fasterthan the rate of functional recovery (Quast et al., 1978; Boydand Cohen, 1980). The extent to which this holds true for operablesurface receptors was unclear. This is an important considerationbecause membrane isolation can alter the apparent receptor affinity(Fenster et al., 1999).

In this study, we were able to directly correlate dissociation and recovery in intact surface receptors. We found that agonistdissociation from desensitized GABA receptors was dominated bya single exponential component with a time constant of 30 ± 2sec, whereas GABA receptors recovered from functional desensitizationwith a time constant of 124 ± 26 sec. These data indicate thata basic model of GABA receptor desensitization must be cyclicaland include the ability of agonist to dissociate directly fromthe desensitized receptor (AD $right-arrow$ D in Scheme I). In fact, thismust be the dominant pathway for recovery, otherwise the rateof recovery and the rate of dissociation would be the same. Forexample, receptors recovering from AD to AR (Scheme I) will movealong a pathway from which they can be reactivated. Some reactivationmay occur, and this is evident in Figure 3A in which the tailof the GABA-activated current, because of the increased levelof desensitization, is slowed with increasing GABAconcentration.

Jones and Westbrook (1995) observed that GABA receptor deactivation was slowed by desensitization and modeled their data usinga noncyclical model. Because they did not examine binding andthe relationship between dissociation and functional recovery,we do not know whether a cyclical model would be more appropriate.The desensitization and recovery in the Jones and Westbrook studywere dominated by rates faster than we could resolve in our bindingand electrophysiological analyses. The question remains as tohow their findings relate to the present study. It should be keptin mind that they probed a heterogeneous population of nativeGABA receptors in mammalian neurons with brief GABA applications,whereas we examined a homogeneous population of recombinant receptorsexpressed in oocytes desensitized for extended time periods. Furthermore,we are studying GABA receptors in an exogenous expression systemthat may lack components (cytoskeletal elements, linker proteins,and kinases) that contribute to the properties of receptor activationand desensitization. The relationship between their mechanismand the mechanism we presented here and the degree to which thisdifference can be attributed to the expression system, receptorsubtype, and/or temporal resolution must await future studies.More recently, a slow component of desensitization ( $tau$ _recovery~15 sec) was investigated in hippocampal neurons and shown toinfluence synaptic inhibition by decreasing GABA receptor availability.Therefore, slow components of desensitization may serve a physiologicalrole (Overstreet et al., 2000).

Does desensitization increase the affinity of the receptor for agonist?

Indeed, evidence has supported the hypothesis that desensitized receptors have a higher agonist affinity than the restingclosed state (Rang and Ritter, 1970; Weber et al., 1975; Weilandet al., 1975; Quast et al., 1978; Sine and Taylor, 1979; Neubiget al., 1982; Heidmann et al., 1983), although these measurementshave been typically performed in membrane or vesicle preparationsin which the functional integrity of the receptors was unknown.Using the single oocyte binding technique, we have been able tocompare the apparent affinity of the same set of surface receptors,before and after receptor desensitization. In both cases, therelationship between the concentration of [³H]muscimol and the specific binding was described by the sum oftwo Hill equations: a component with an apparent K_D of ~8.0 µMand a higher-affinity component with a apparent K_D of ~0.20 µM.The fraction of the specific binding in the high-affinity componentincreased with receptor desensitization. The simplest interpretationof these data are that desensitization shifted receptors froma low- to high-affinity state. Although a minimum of two apparentaffinities seems inescapable from the data in Figure 5B, cautionmust be exercised in interpreting the parameters of these components.First, by the nature of the binding assay, the relative amplitudesof the two components reflect a partial recovery of the receptorsfrom desensitization. Second, some fraction of the receptors weredesensitized by the [³H]muscimol incubation used to assess the level of desensitization.Third, in the case of the specific binding before receptor desensitizationin which the high-affinity component was relatively small, itwas necessary to constrain the apparent K_D for the fitting algorithmto converge. Finally, caution must be exercised in interpretingthe apparent K_D values because they do not represent true bindingaffinities, and their values must be considered in light of aspecific kinetic scheme for receptor desensitization (Colquhoun,1998). It should be mentioned that, at steady state, only a singlecomponent would be observed in the dose dependence of agonistbinding. However, these measurements were not taken at steadystate, thus permitting the appearance of the two apparentaffinities.

Working hypothesis for desensitization of GABA_A receptors

Although the consideration of a complete model with transitions between the resting, open, and desensitized states is beyondthe scope of this study, we can consider select transitions toand from the desensitized states, begin to define the most likelypathways, and put some limitations on select rates. Scheme

View larger version (12K):
[in this window]
[in a new window]

2 is similar to Scheme 1 but has been modified to account for the two agonist binding steps. In this allosteric scheme, K_Rrepresents the affinity of the resting state (the open statesare not depicted in this scheme), K_D represents the affinity forbinding to the desensitized states, M is [R]/[D], and a is K_D/K_R.

In a previous study, taking advantage of a mutation that promotes spontaneous opening of the $alpha$ 1 $beta$ 2 $gamma$ 2 GABA receptor, we wereable to estimate K_R (Chang and Weiss, 1999b). The desensitizedstates were not included in the derivation of these parameters.If entry into desensitized states are significant along the activationpathway (R $right-arrow$ AR $right-arrow$ A₂R $right-arrow$ A₂O), then desensitization would affectthe derivation of these values. Nevertheless, we estimated K_Rto be ~78.5 µM.

In the present study, we examined receptors under conditions that favor receptor desensitization. We approximated the K_D formuscimol (Fig. 5B), but, because a majority of the experimentswe presented in this study were with GABA, we set out to determinethe apparent affinity of the desensitized receptor for [³H]GABA (Fig. 7A). In this case, the binding was performed witha 30 min incubation at each concentration of [³H]GABA to ensure that equilibrium was obtained. The relationshipbetween specific binding and concentration was well describedby a single Hill equation with a apparent K_D of 0.04 µM and aHill coefficient of 1.22. In contrast to muscimol (Fig. 5B), asecond component was not seen because the resting state affinity(~78 µM) would be too low to resolve in this assay. Early studiesexamining [³H]GABA binding in synaptic membrane fractions revealed a K_D onthe order of 100 nM (Zukin et al., 1974). Subsequently, a heterogeneityof binding sites was observed with K_D values in the 10-20 and100-200 nM range (Olsen et al., 1981). Whether these two affinitiesrepresent an interconvertible pool or distinct receptor populationswas unclear. The interpretation of K_D values determined from membranepreparations is further complicated by a study in which the apparentbinding affinity of nicotine to nACh receptors expressed in oocyteswas compared in both intact oocytes and membranes prepared fromthese oocytes. In this case, the membrane preparation demonstratedan ~25-fold higher affinity for nicotine, suggesting that membraneisolation may alter the apparent receptor affinity or uncovernew high-affinity binding sites (Fenster et al., 1999).

View larger version (15K):
[in this window]
[in a new window]
Figure 7. Equilibrium binding and steady-state desensitization. A, Equilibrium binding of [³H]GABA. Oocytes were incubated for 30 min with the indicated concentrations of [³H]GABA. The filled symbols represent the average of three oocytes. The continuous line is a fit of the Hill equation of these data yielding a apparent K_D of 0.040 µM and a Hill coefficient of 1.22. B, Determination of the steady-state level of desensitization. An oocyte was voltage clamped at $-$ 70 mV, and the indicated concentrations of GABA were applied successively. All four concentrations of GABA were saturating in terms of desensitization. The amplitude of the baseline current at the end of the application was used to calculate the maximum fraction of receptors in the desensitized state, which was 0.049 of the peak GABA-activated current.

The K_D is the ratio of the microscopic off and on rates. Because we determined the dissociation rate for GABA (~0.03 sec¹) (Fig. 6), the k_on for the desensitized state would be ~0.75µM¹ sec¹. In Scheme 2, a = K_D/K_R or 0.00051. At saturating concentrationsof GABA, the receptors would be at equilibrium between A₂D andA₂R. We can estimate the population of state A₂D from the experimentshown in Figure 7B in which receptors were exposed to 316, 1000,3160, and 10000 µM GABA. These are all saturating concentrationsof GABA in terms of desensitization because the steady-state currentlevel did not change. At the end of the series of applications,0.049 of the peak current remained. This value is an upper limitbecause we likely underestimated the peak attributable to thenecessarily slow application rate of GABA to oocytes. Nevertheless,after correction for the maximum open probability of 0.84 (Changand Weiss, 1999b) based on Scheme 2, Ma² = [A₂R]/[A₂D] = 0.043 and therefore M = 165320. This model suggeststhat, in the absence of GABA, 6.0 × 10⁶ of the receptors would be in the desensitized state. Again, theseparameters are only approximations, and the equilibrium constantswould depend on the specific kinetic scheme. For example, it isconceivable that the desensitized states communicate mainly withthe open states. Nevertheless, our demonstration of a cyclicalmodel for desensitization would still hold, as would our estimationof the apparent affinity of the desensitized state. From our previousanalysis of receptor activation and the present considerationof desensitization, we provided estimates of the apparent K_D valuesof the resting, open, and desensitized states to be ~78.5 µM,120 nM, and 40 nM, respectively. It is interesting that a biochemicalstudy of [³H]GABA binding in native membranes from bovine cortex suggestedthree sites in terms of affinity with K_D values of 1 µM, 100 nM,and 10 nM. These affinities were hypothesized to represent theresting, open, and desensitized states, respectively (Olsen etal., 1984).

Can Scheme 2 account for our experimental data? Using Scheme 2, the derived equilibrium constants, and, in Equation 3, wepredicted an EC₅₀ for functional desensitization of 19.4 µM (seeMaterials and Methods) that is close to the experimentally observedvalue of 9.8 µM. Clearly this is a simplified model because itdoes not include the open states. Inclusion of transitions fromthe open states to desensitized states could shift the predictedestimate toward the observed value. A complete description ofthe experimental results must await a more comprehensive modelof receptor activation anddesensitization.

  FOOTNOTES

Received March 15, 2002; revised June 21, 2002; accepted June 26, 2002.

This work was supported in part by National Institutes of Health Grants NS35291, NS36195 (D.S.W.), and DK07545 (Y.C.).

Correspondence should be addressed to Dr. David S. Weiss, Department of Neurobiology, University of Alabama at Birmingham,1719 Sixth Avenue South, CIRC410, Birmingham, AL 35294-0021. E-mail:dweiss{at}nrc.uab.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Amin J, Weiss DS (1993) GABA_A receptor needs two homologous domains of the $beta$ -subunit for activation by GABA but not by pentobarbital. Nature 366:565-569[Medline].
Amin J, Weiss DS (1994) Homomeric $rho$ 1 GABA channels: activation properties and domains. Receptors Channels 2:227-236[Web of Science][Medline].
Birnir B, Tieney ML, Dalziel JE, Cox GB, Gage PW (1997) A structural determinant of desensitization and allosteric regulation by pentobarbitone of the GABA_A receptor. J Membr Biol 155:157-166[Web of Science][Medline].
Boyd ND, Cohen JB (1980) Kinetics of binding of [³H]acetylcholine to Torpedo postsynaptic membranes: association and dissociation rate constants by rapid mixing and ultrafiltration. Biochemistry 19:5353-5358[Medline].
Chang Y, Weiss DS (1999a) Channel opening locks agonist onto the GABA_C receptor. Nat Neurosci 2:219-225[Web of Science][Medline].
Chang Y, Weiss DS (1999b) Allosteric activation mechanism of the $alpha$ 1 $beta$ 2 $gamma$ 2 GABA_A receptor revealed by mutation of the conserved M2 leucine. Biophys J 77:2542-2551[Web of Science][Medline].
Changeux J-P, Edelstein SJ (1998) Allosteric receptors after 30 years. Neuron 21:959-980[Web of Science][Medline].
Colquhoun D (1998) Binding, gating, affinity, and efficacy: the interpretation of structure-activity relationships for agonists and of the effects of mutating receptors. Br J Pharmacol 125:923-948.
Edelstein SJ, Changeux J-P (1996) Allosteric proteins after thirty years: the binding and state functions of the neuronal $alpha$ 7 nicotinic acetylcholine receptors. Experientia 52:1083-1090[Web of Science][Medline].
Fenster CP, Whitworth TL, Sheffield EB, Quick MW, Lester RAJ (1999) Upregulation of surface $alpha$ 4 $beta$ 2 nicotinic receptors is initiated by receptor desensitization after chronic exposure to nicotine. J Neurosci 19:4804-4814[Abstract/Free Full Text].
Heidmann T, Bernhardt J, Neumann E, Changeux JP (1983) Rapid kinetics of agonist binding and permeability response analyzed in parallel on acetylcholine rich membranes from Torpedo marmorata. Biochemistry 22:5452-5459[Medline].
Jones MV, Westbrook GL (1995) Desensitized states prolong GABA_A channel responses to brief agonist pulses. Neuron 15:181-191[Web of Science][Medline].
Katz B, Thesleff S (1957) A study of the desensitization produced by acetylcholine at the motor end-plate. J Physiol (Lond) 138:63-80[Free Full Text].
Liman ER, Tytgat J, Hess P (1992) Subunit stoichiometry of a mammalian K⁺ channel determined by construction of multimeric cDNAs. Neuron 9:861-871[Web of Science][Medline].
Neubig RR, Boyd ND, Cohen JB (1982) Conformations of Torpedo acetylcholine receptor associated with ion transport and desensitization. Biochemistry 21:3460-3467[Medline].
Olsen RW, Bergman MO, Van Ness PC, Lummis SC, Watkins AE, Napias C, Greenlee DV (1981) $gamma$ -aminobutyric acid receptor binding in mammalian brain. heterogeneity of binding sites. Mol Pharmacol 19:217-227[Abstract/Free Full Text].
Olsen RW, Wong EHF, Stauber GB, King RG (1984) Biochemical pharmacology of the $gamma$ -aminobutyric acid receptor/ionophore protein. Fed Proc 43:2773-2778[Web of Science][Medline].
Overstreet LS, Jones MV, Westbrook GL (2000) Slow desensitization regulates the availability of synaptic GABA_A receptors. J Neurosci 20:7914-7921[Abstract/Free Full Text].
Quast U, Schimerlik M, Witzemann V, Blanchard S, Raftery MA (1978) Ligand-induced conformation changes in Torpedo californica membrane-bound acetylcholine receptor. Biochemistry 17:2405-2414[Medline].
Rang HP, Ritter JM (1970) On the mechanism of desensitization at cholinergic receptors. Mol Pharmacol 6:357-382[Abstract/Free Full Text].
Sine SM, Taylor P (1979) Functional consequences of agonist-mediated state transitions in the cholinergic receptor. Studies in cultured muscle cells. J Biol Chem 254:3315-3325[Abstract/Free Full Text].
Tia S, Wang JF, Kotchabhakdi N, Vicini S (1996) Distinct deactivation and desensitization kinetics of recombinant GABA_A receptors. Neuropharmacology 35:1375-1382[Web of Science][Medline].
Weber M, David-Pfeuty T, Changeux J (1975) Regulation of binding properties of the nicotinic receptor protein by cholinergic ligands in membrane fragments from Torpedo marmorata. Proc Natl Acad Sci USA 72:3443-3447[Abstract/Free Full Text].
Weiland G, Georgia B, Lappi S, Chignell C, Taylor P (1975) Kinetics of agonist-mediated transitions in state of the cholinergic receptor. J Biol Chem 252:7648-7656[Free Full Text].
Zhu WJ, Vicini S (1997) Neurosteroid prolongs GABA_A channel deactivation by altering kinetics of desensitized states. J Neurosci 17:4022-4031[Abstract/Free Full Text].
Zukin SR, Young AB, Snyder SH (1974) Gamma-aminobutyric acid binding to receptor sites in the rat central nervous system. Proc Natl Acad Sci USA 71:4802-4807[Abstract/Free Full Text].

Copyright © 2002 Society for Neuroscience 0270-6474/02/22187982-09$05.00/0

This article has been cited by other articles:

K. Solt, D. Ruesch, S. A. Forman, P. A. Davies, and D. E. Raines
Differential Effects of Serotonin and Dopamine on Human 5-HT3A Receptor Kinetics: Interpretation within an Allosteric Kinetic Model
J. Neurosci., November 28, 2007; 27(48): 13151 - 13160.
[Abstract] [Full Text] [PDF]

M. T. Bianchi, E. J. Botzolakis, K. F. Haas, J. L. Fisher, and R. L. Macdonald
Microscopic kinetic determinants of macroscopic currents: insights from coupling and uncoupling of GABAA receptor desensitization and deactivation
J. Physiol., November 1, 2007; 584(3): 769 - 787.
[Abstract] [Full Text] [PDF]

M. Bali and M. H. Akabas
The Location of a Closed Channel Gate in the GABAA Receptor Channel
J. Gen. Physiol., January 29, 2007; 129(2): 145 - 159.
[Abstract] [Full Text] [PDF]

A. Keramidas, T. L. Kash, and N. L. Harrison
The pre-M1 segment of the {alpha}1 subunit is a transduction element in the activation of the GABAA receptor
J. Physiol., August 15, 2006; 575(1): 11 - 22.
[Abstract] [Full Text] [PDF]

E. B. Pratt, T. S. Brink, P. Bergson, M. M. Voigt, and S. P. Cook
Use-Dependent Inhibition of P2X3 Receptors by Nanomolar Agonist
J. Neurosci., August 10, 2005; 25(32): 7359 - 7365.
[Abstract] [Full Text] [PDF]

S. S Smith and Q. H. Gong
Neurosteroid administration and withdrawal alter GABAA receptor kinetics in CA1 hippocampus of female rats
J. Physiol., April 15, 2005; 564(2): 421 - 436.
[Abstract] [Full Text] [PDF]

A. Sedelnikova, C. D. Smith, S. O. Zakharkin, D. Davis, D. S. Weiss, and Y. Chang
Mapping the {rho}1 GABAC Receptor Agonist Binding Pocket: CONSTRUCTING A COMPLETE MODEL
J. Biol. Chem., January 14, 2005; 280(2): 1535 - 1542.
[Abstract] [Full Text] [PDF]

D. S. Dahan, M. I. Dibas, E. J. Petersson, V. C. Auyeung, B. Chanda, F. Bezanilla, D. A. Dougherty, and H. A. Lester
A fluorophore attached to nicotinic acetylcholine receptor {beta}M2 detects productive binding of agonist to the {alpha}{delta} site
PNAS, July 6, 2004; 101(27): 10195 - 10200.
[Abstract] [Full Text] [PDF]

J. W. Mozrzymas, E. D. Zarmowska, M. Pytel, and K. Mercik
Modulation of GABAA Receptors by Hydrogen Ions Reveals Synaptic GABA Transient and a Crucial Role of the Desensitization Process
J. Neurosci., September 3, 2003; 23(22): 7981 - 7992.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

A correction has been published

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (18)

Citing Articles via Google Scholar

Google Scholar

Articles by Chang, Y.

Articles by Weiss, D. S.

Search for Related Content

PubMed

PubMed Citation

Articles by Chang, Y.

Articles by Weiss, D. S.