Enantioselectivity of Pregnanolone-Induced gamma -Aminobutyric AcidA Receptor Modulation and Anesthesia

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Vol. 293, Issue 3, 1009-1016, June 2000

Enantioselectivity of Pregnanolone-Induced $gamma$ -Aminobutyric Acid_A Receptor Modulation and Anesthesia¹

Douglas F. Covey, Devi Nathan, Melissa Kalkbrenner, Kent R. Nilsson, Yuefei Hu, Charles F. Zorumski and Alex S. Evers

Departments of Molecular Biology and Pharmacology (D.F.C., Y.H., K.R.N., A.S.E.), Anesthesiology (D.N., M.K., A.S.E.), and Psychiatry (C.F.Z.), Washington University School of Medicine, St. Louis, Missouri

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

This study reports the actions of enantiomer pairs of anesthetic steroids 3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P as modulatorsof $gamma$ -aminobutyric acid (GABA)_A receptors and as anesthetics. Theenantiomers of structurally related 17-carbonitrile analogs alsoare examined. These studies were aimed at 1) determining whetherthe steroid recognition site could distinguish between moleculesdiffering in shape, but not other physical properties (enantioselectivity);2) providing further insight into the structure-activity relationshipsof anesthetic steroids; and 3) determining whether modulationof GABA_A receptor function correlates with anesthetic potencyfor anesthetic steroid enantiomers. Stereoselective actions ofthe compounds were evaluated in four different bioassays: 1) noncompetitivedisplacement of [³⁵S]t-butylbicyclophosphorothionate from the picrotoxin site ofGABA_A receptors present in rat brain membrane preparations; 2)modulation of GABA currents in cultured rat hippocampal neurons;3) loss of righting reflex in tadpoles; and 4) loss of rightingreflex in mice. The data indicate that 5 $alpha$ -reduced steroids, butnot 5 $beta$ -reduced steroids, show a high degree of enantioselectivity/enantiospecificityin their actions as modulators of GABA_A receptors and as anesthetics.For all compounds studied, the effects on GABA_A receptor functionclosely tracked with anesthetic effects. These data show thatthe anesthetic steroid recognition site is capable of distinguishingenantiomers, suggesting a protein-binding site of specific dimensionsand shape. The results are compatible either with a structuralmodel of the binding site that can accommodate 3 $alpha$ 5 $alpha$ P, 3 $alpha$ 5 $beta$ P, andent-3 $alpha$ 5 $beta$ P, but not ent-3 $alpha$ 5 $alpha$ P, or with two different binding sitesfor steroidanesthetics.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

The steroids 3 $alpha$ 5 $alpha$ P (allopregnan-3 $alpha$ -ol-20-one) and 3 $alpha$ 5 $beta$ P (pregnanolone) are potent anesthetics (Phillipps, 1974). A large amountof data supports the hypothesis that the anesthetic actions ofthese steroids are correlated with their enhancement of $gamma$ -aminobutyricacid (GABA)_A receptor-mediated neuronal inhibition (Lambert etal., 1995). The number of binding sites for these steroids andtheir location on GABA_A receptors are not known. Moreover, whetherthe steroids share a common site is not known. Molecular-modelingstudies suggest that the anesthetic activities of these steroidsresult from binding at a common binding site (Purdy et al., 1990;Han et al., 1996). However, binding studies for steroid-inducednoncompetitive displacement of t-butylbicyclophosphorothionate(TBPS) from the picrotoxin-binding site on GABA_A receptors indicatethat, although these steroids may share a common binding site,multiple binding sites are detectable for some steroids (Morrowet al., 1990; Hawkinson et al., 1994a,b, 1998).

Because 3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ P are molecules that each contain eight chiral centers (C-3, C-5, C-8, C-9, C-10, C-13, C-14, and C-17),their stereoselective modulation of GABA_A receptor function canbe studied by inverting each, some, or all of the chiral centersin the molecules. Inversion of one center in a molecule containingmultiple chiral centers gives compounds called epimers. Epimersare a subset of compounds called diastereomers. Diastereomersare compounds with multiple chiral centers that differ in configurationat one or some, but not all, chiral centers. Studies of the C-3(inversion of the 3-hydroxyl group) and C-17 (inversion of theacetyl group) epimers of 3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ P have been very informativein establishing the structure-activity relationships for anestheticsteroids (Phillipps, 1974). No doubt, studies of additional diastereomersof 3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ P will further define these structure-activityrelationships. However, because diastereomers have different physicalproperties due to the relative positions of some atoms in eachdiastereomer being different, the membrane-perturbing effectsas well as the direct effects of these steroids on GABA_A receptorfunction will be different. Thus, C-3 epimers (3 $beta$ -OH) of 3 $alpha$ 5 $alpha$ Pand 3 $alpha$ 5 $beta$ P not only fail to potentiate GABA effects at GABA_A receptorsbut also interact differently with membrane phospholipids (Makriyanniset al., 1991).

To avoid the membrane-perturbing effects caused by studying anesthetic steroid diastereomers having different physical properties,we have studied anesthetic steroid enantiomers (Fig. 1). Enantiomersare the stereoisomers of optically active compounds that are mirrorimages of each other (all chiral centers have the opposite absoluteconfiguration). Enantiomers have identical physical propertiesbecause the relative positions of all atoms in each enantiomerare identical. For example, any group having an axial configurationin one enantiomer also has an axial configuration in the otherenantiomer.

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Fig. 1. Structures of the four pairs of anesthetic steroid enantiomers studied.

Enantioselectivity of 3 $alpha$ 5 $alpha$ P-induced GABA_A receptor modulation and anesthesia in Xenopus laevis tadpoles and mice has beenreported previously (Wittmer et al., 1996). Herein, we reportthe corresponding actions of the 3 $alpha$ 5 $beta$ P enantiomers. Additionally,new information for the displacement of TBPS binding by both pairsof enantiomers is reported. Some comparative data for the correspondingenantiomers of the 17-carbonitrile analogs of 3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ Palso are presented. The new data show that enantioselectivity[comparison of 3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $alpha$ P with 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P) and diastereoselectivity(comparison of 3 $alpha$ 5 $alpha$ P/3 $alpha$ 5 $beta$ P with ent-3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $beta$ P) for modulationof GABA_A receptor function by these anesthetic steroids are different.The enantioselective actions of 3 $alpha$ 5 $alpha$ P are significantly greaterthan the enantioselective actions of 3 $alpha$ 5 $beta$ P. The diastereoselectiveactions of the 3 $alpha$ 5 $alpha$ P/3 $alpha$ 5 $beta$ P steroid pair are not significant andthose of the ent-3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $beta$ P pair are significantlydifferent.

	Materials and Methods

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Chemicals. The ent-3 $alpha$ 5 $beta$ P, ent-3 $alpha$ 5 $alpha$ P, 3 $alpha$ 5 $alpha$ ACN [(3 $alpha$ ,5 $alpha$ ,17 $beta$ )-3-hydroxyandrostane-17-carbonitrile], ent-3 $alpha$ 5 $alpha$ ACN, and 3 $alpha$ 5 $beta$ ACN [(3 $alpha$ ,5 $beta$ ,17 $beta$ )-3-hydroxyandrostane-17-carbonitrile]were prepared and characterized as described previously (Hu etal., 1993, 1997; Han et al., 1996; Nilsson et al., 1998). Theent-3 $alpha$ 5 $beta$ ACN was prepared from ent-(3 $alpha$ ,5 $beta$ )-3-hydroxyandrostan-17-onewith the methods described for the preparation of 3 $alpha$ 5 $beta$ ACN (Hanet al., 1996). The infrared, ¹H NMR, and ¹³C NMR spectra of the 3 $alpha$ 5 $beta$ ACN and ent-3 $alpha$ 5 $beta$ ACN were identical. The3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ P were purchased from either Sigma Chemical Co.(St. Louis, MO) or Steraloids (Newport, RI). The [³⁵S]TBPS was purchased from NEN Life Science Products (Boston, MA)and TBPS was purchased from Research Biochemicals International(Natick,MA).

[³⁵S]TBPS Binding. Rat brain cortical membranes were prepared with minor modifications of the method previously reported (Hawkinson et al., 1994a).Briefly, frozen rat cerebral cortices (Pel-freez, Rogers, AK)were thawed and homogenized in 10 volumes of ice-cold 0.32 M sucrosewith a glass/Teflon pestle. The homogenate was centrifuged at1500g for 10 min at 4°C. The resultant supernatant was centrifugedat 10,000g for 30 min at 4°C. The pellet (P2) from this centrifugationwas resuspended in 200 mM NaCl, 50 mM potassium phosphate buffer,pH 7.4, and centrifuged at 10,000g for 20 min at 4°C. This washingprocedure was done three times, and then pellets were resuspendedin buffer (~4 ml/brain) with a glass/Teflon pestle. The membranesuspension was aliquoted, frozen in liquid nitrogen, and storedat $-$ 80°C before use. [³⁵S]TBPS binding assays were done according to the procedure describedpreviously (Hawkinson et al., 1994a) with modifications. Briefly,aliquots of membrane solution (0.5 mg/ml final protein concentrationin assay) were incubated with 5 µM GABA, 2 nM [³⁵S]TBPS (45-120 Ci/mmol), and 5 µl-aliquots of steroid in dimethylsulfoxide (DMSO) solution (final assay concentrations ranged from1 nM to 10 µM), and brought to a final volume of 1 ml with 200mM NaCl, 50 mM potassium phosphate buffer, pH 7.4. Control bindingwas defined as binding observed in the presence of 0.5% DMSO andthe absence of steroid. Nonspecific binding was defined as bindingobserved in the presence of 200 µM picrotoxin and ranged from6.1 to 14.3% of total binding. Assay tubes were incubated for2 h at room temperature. A Brandel (Gaithersburg, MD) cell harvesterwas used for filtration of the assay tubes through Whatman/GF/Cglass filter paper. Filter paper was rinsed with 4 ml of ice-coldbuffer three times. Radioactivity bound to the filters was readby liquid scintillation counter and data were fit with Sigma Plotversion 3.0 to the Hill equation

f=R<UP>max</UP>/{1+([<UP>conc</UP>]/<UP>IC</UP>50)n}

where R_max is the maximal effect, [conc] is steroid concentration, IC₅₀ is the half-maximal inhibitor concentration, andn is the Hill coefficient. Each data point was determined in triplicateand two or three full concentration-response curves were generatedfor eachsteroid.

Electrophysiological Recording. Hippocampal neurons were cultured from 1- to 2-day-old Sprague-Dawley albino rats with methods described previously (Thioet al., 1991). After 4 to 7 days in culture, neurons were voltageclamped at $-$ 60 mV with whole-cell patch-clamp recording techniques.The extracellular recording solution contained 140 mM NaCl, 4mM KCl, 2 mM MgCl₂, 2 mM CaCl₂, 10 mM HEPES, and 10 mM glucose,pH 7.3. Recording pipettes were filled with a solution containing140 mM CsCl, 4 mM NaCl, 0.5 mM CaCl₂, 4 mM MgCl₂, and 10 mM HEPES,pH 7.3. GABA and steroids were applied for 500 ms with a pressure(20 psi of air) ejection drug delivery system with patch pipettespositioned ~5 µm from the recorded neuron. This system allowedreliable drug application while minimizing exposure of neuronsto steroids. The concentrations reported are those in the pipetteand are ~2- to 3-fold higher than the concentrations bathing thecell. Steroids were prepared in a DMSO stock at 10 to 100 mM anddiluted so that the final concentration of DMSO was <0.5%. DMSOat this concentration had no effect on GABA responses. Concentration-responsedata were fit to an equation of the form

f=R<UP>max</UP>×{[<UP>conc</UP>]n/([<UP>conc</UP>]n+<UP>EC</UP>50n)}

where R_max is the maximum effect, [conc] is the steroid concentration, EC₅₀ is the half-maximal effective concentration,and n is the Hillcoefficient.

Tadpole Loss of Righting Reflex (LRR) Anesthesia Assay. Tadpole LRR was measured as described previously (Wittmer et al., 1996). Briefly, groups of 10 early prelimb-bud stage Xenopuslaevis tadpoles (Nasco, Fort Atkinson, WI) were placed in 100ml of oxygenated Ringer's stock solution containing various concentrationsof compound. Compounds were added from a 10 mM DMSO stock (finalconcentration of DMSO in test solutions was 0.1%). After equilibratingat room temperature for 3 h, tadpoles were evaluated with theLRR behavioral endpoint. LRR was defined as failure of the tadpoleto right itself within 5 s after being flipped by a smooth glassrod. In all cases, the tadpoles regained their righting reflexwhen placed in fresh oxygenated Ringer's solution. Control beakerscontaining up to 0.6% DMSO produced no LRR in tadpoles. Concentration-responsecurves were fit with Sigma Plot version 3.0 to the Hill equation

f=R<UP>max</UP>/{1+([<UP>conc</UP>]/<UP>EC</UP>50)n}

where R_max is the maximum effect, [conc] is the steroid concentration, EC₅₀ is the half-maximal effective concentration,and n is the Hillcoefficient.

Mouse Anesthesia Assay. BALB/c mice (Sprague-Dawley; Harlan Breeders, Indianapolis, IN) weighing 20 to 30 g each were placed under a heat lamp for1 to 2 min. Compounds were injected i.v. through a tail vein withvarious doses of either 3 $alpha$ 5 $beta$ P or ent-3 $alpha$ 5 $beta$ P in an 8% ethanol, 16%Cremaphor EL (Sigma Chemical Co.) solution at a rate of 50 to250 µl/5 to 10 s. Sleep time was measured from the moment micedisplayed LRR until they were able to right themselves. All micerecovered fully without observable neurological deficits. Controlsolutions without steroids were administered with no observableneurobehavioraleffect.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

[³⁵S]TBPS Binding. Anesthetic steroids are known to be noncompetitive displacers of [³⁵S]TBPS from the picrotoxin-binding site of GABA_A receptors (Majewskaet al., 1986). In this study, the enantioselectivity for [³⁵S]TBPS displacement by four pairs of anesthetic steroid enantiomerswas examined (Fig. 2). For the two 5 $beta$ -reduced steroid enantiomerpairs, 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P and 3 $alpha$ 5 $beta$ ACN/ent-3 $alpha$ 5 $beta$ ACN, the natural enantiomerswere each ~4-fold more potent displacers of [³⁵S]TBPS. For the two 5 $alpha$ -reduced steroid enantiomer pairs, 3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $alpha$ Pand 3 $alpha$ 5 $alpha$ ACN/ent-3 $alpha$ 5 $alpha$ ACN, the natural enantiomers were the morepotent displacers by factors of 26 and 80, respectively. Thus,enantioselectivity for [³⁵S]TBPS displacement was found for all enantiomer pairs, but thedegree of enantioselectivity was much higher for the 5 $alpha$ -reducedsteroids.

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Fig. 2. Inhibition of [³⁵S]TBPS binding to rat brain cortical membranes by steroid enantiomers. The enantiomers of 3 $alpha$ 5 $alpha$ ACN and 3 $alpha$ 5 $alpha$ P show a larger degree of enantioselectivity than do the enantiomers of 3 $alpha$ 5 $beta$ ACN and 3 $alpha$ 5 $beta$ P. The figure shows a representative concentration-response curve for each steroid. The IC₅₀ ± S.E. values reported are from the fit of data points from two or three experiments. A, the 3 $alpha$ 5 $beta$ ACN (

) and ent-3 $alpha$ 5 $beta$ ACN ( $open circle$ ) show an ~4-fold difference in IC₅₀ (72 ± 8 versus 292 ± 21 nM) for inhibition of [³⁵S]TBPS binding. B, the 3 $alpha$ 5 $beta$ P (

) and ent-3 $alpha$ 5 $beta$ P ( $open circle$ ) enantiomer pair also show an ~4-fold difference in IC₅₀ (71 ± 18 versus 276 ± 34 nM) for inhibition of [³⁵S]TBPS binding. C, an 80-fold difference in IC₅₀ (50 ± 5 versus 4020 ± 310 nM) for inhibition of [³⁵S]TBPS binding is demonstrated between 3 $alpha$ 5 $alpha$ ACN (

) and ent-3 $alpha$ 5 $alpha$ ACN ( $open circle$ ). D, an ~26-fold difference in IC₅₀ (74 ± 7 versus 1910 ± 270 nM) is seen between 3 $alpha$ 5 $alpha$ P (

) and ent-3 $alpha$ 5 $alpha$ P ( $open circle$ ).

Steroid Effects on GABA_A Currents. The enantioselectivity found for modulation of GABA_A receptor function in cultured rat hippocampal neurons by the enantiomerpairs is shown in Figs. 3 and 4. At a steroid concentration of10 µM, there was no enantioselectivity for potentiation of 2 µMGABA-mediated currents by the 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P pair (Fig. 3). Incontrast, an ~4-fold enantioselectivity for the degree of potentiationunder the same experimental conditions was found for the 3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $alpha$ Ppair (Fig. 3). This last result is in close agreement with resultspreviously reported from a more extensive electrophysiologicalevaluation of GABA_A receptor modulation in these cells by the3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $alpha$ P pair (Wittmer et al., 1996).

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Fig. 3. A, traces show the enhancement of GABA-mediated currents (2 µM; ~EC₁₀) by 10 µM 3 $alpha$ 5 $beta$ P and ent-3 $alpha$ 5 $beta$ P in hippocampal neurons recorded at a holding potential of $-$ 60 mV. GABA, either alone or in the presence of the steroids, was applied for 500 ms. B, average potentiation of 2 µM GABA currents by 10 µM enantiomers of 3 $alpha$ 5 $beta$ P (right columns). For comparison, the effects of 10 µM 3 $alpha$ 5 $alpha$ P enantiomers on currents gated by 2 µM GABA are shown (left columns). Results represent the mean ± S.E. of four to six cells per experimental condition.

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Fig. 4. Concentration-response curves for the potentiation of currents gated by 1 µM (~EC₅) GABA (A) and for direct chloride-channel gating in the absence of GABA (B) by 3 $alpha$ 5 $beta$ P (

) and ent-3 $alpha$ 5 $beta$ P ( $black-triangle$ ). A, points represent the percentage of increase ± S.E. in GABA response produced by the steroid for three to five cells per concentration. The solid lines represent the best fit of the logistic concentration-response equation. For 3 $alpha$ 5 $beta$ P, the maximal response, Hill coefficient, and EC₅₀ were 1725 ± 111%, 1.0 ± 0.3 µM, and 1.2 ± 0.4 µM, respectively, whereas for ent-3 $alpha$ 5 $beta$ P these values were 1737 ± 1%, 1.4 ± 0.1 µM, and 3.6 ± 0.1 µM, respectively. B, responses to the steroids were normalized with respect to the response obtained at 10 µM steroid and represent data (points are the mean ± S.E.) from four or five cells per concentration. The responses to 10 and 100 µM 3 $alpha$ 5 $beta$ P were 316 ± 64 pA and 1234 ± 224 pA, respectively (n = 4 each). The responses to 10 and 100 µM ent-3 $alpha$ 5 $beta$ P were 346 ± 53 pA and 2010 ± 254 pA, respectively, (n = 4 each). The solid lines represent best fits with maximal responses of 1429 ± 1 and 1337 ± 1%, Hill coefficients of 0.8 ± 0.01 and 1.0 ± 0.01, and EC₅₀ values of 272 ± 1 and 125 ± 1 µM for 3 $alpha$ 5 $beta$ P and ent-3 $alpha$ 5 $beta$ P, respectively. For the best fits, values ± S.E. given are from the fit of the data points.

A concentration-response curve for potentiation of GABA-mediated currents by the 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P pair is shown in Fig. 4A.The 3 $alpha$ 5 $beta$ P enantiomer was 3-fold more potent than the ent-3 $alpha$ 5 $beta$ Penantiomer (EC₅₀ = 1.2 and 3.6 µM, respectively). In Fig. 4B,the concentration-response curve for gating of GABA_A receptorsin the absence of added GABA is shown. The ent-3 $alpha$ 5 $beta$ P gates a currentat the same concentration as 3 $alpha$ 5 $beta$ P and does so to a very similarextent. This contrasts with the results previously obtained withent-3 $alpha$ 5 $alpha$ P and ent-3 $alpha$ 5 $alpha$ ACN, neither of which gates GABA_A receptorsat a concentration of up to 100 µM (Wittmer et al., 1996

Tadpole LRR. The concentration-response relationships for the loss of tadpole LRR were determined for the 3 $alpha$ 5 $beta$ ACN/ent-3 $alpha$ 5 $beta$ ACN and 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ Ppairs. Little, if any, enantioselectivity was observed for theseenantiomer pairs (Fig. 5). The results contrast with the significantdegrees of enantioselectivity found previously (Wittmer et al.,1996) for tadpole LRR with the 3 $alpha$ 5 $alpha$ ACN/ent-3 $alpha$ 5 $alpha$ ACN and 3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $alpha$ Ppairs (10- and 2.8-fold, respectively).

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Fig. 5. 3 $alpha$ 5 $beta$ ACN and 3 $alpha$ 5 $beta$ P enantiomers cause tadpole LRR but do not act enantioselectively. Points on the tadpole concentration-response curves represent mean response of 10 to 40 animals, scored quantally. A, concentration-response curves for LRR in tadpoles showing the effects of 3 $alpha$ 5 $beta$ ACN (

) versus ent-3 $alpha$ 5 $beta$ ACN ( $open circle$ ). The EC₅₀ values ± S.E. of the fit data were 80 ± 13 and 115 ± 19 nM, respectively. B, concentration-response curves for LRR in tadpoles showing the effects of 3 $alpha$ 5 $beta$ P (

) versus ent-3 $alpha$ 5 $beta$ P ( $open circle$ ). The EC₅₀ values ± S.E. of the fit data were 61 ± 4 and 58 ± 18 nM, respectively.

Mouse LRR. When injected into mice, both 3 $alpha$ 5 $beta$ P and ent-3 $alpha$ 5 $beta$ P produced anesthesia (as indicated by LRR) in a dose-dependent manner (Fig.6). The slopes of the lines from a regression analysis of thedose-response data for this enantiomer pair differ by a factorof 2. The 3 $alpha$ 5 $beta$ ACN/ent-3 $alpha$ 5 $beta$ ACN pair was not tested for anestheticactivity in mice because adequate amounts of ent-3 $alpha$ 5 $beta$ ACN werenot available. These 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P results for mouse anesthesiaare different from those obtained previously for the 3 $alpha$ 5 $alpha$ ACN/ent-3 $alpha$ 5 $alpha$ ACNpair in this bioassay (Wittmer et al., 1996). In that study, thelowest dose of 3 $alpha$ 5 $alpha$ ACN shown to cause LRR was 4 mg/kg; whereasent-3 $alpha$ 5 $alpha$ ACN did not cause LRR at a dose as high as 80 mg/kg.

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Fig. 6. Intravenous injection of 3 $alpha$ 5 $beta$ P (

) or its enantiomer ent-3 $alpha$ 5 $beta$ P ( $open circle$ ) each produced dose-dependent LRR (sleep times) in mice. Points ± S.E. on mouse dose-response curves represent the average sleep time for three or four animals and were fit to a straight line.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The results from this and our previous enantioselectivity study (Wittmer et al., 1996) provide new information about the enantioselectiveand diastereoselective interactions of anesthetic steroids withGABA_A receptors. Enantioselective interactions can be examinedby comparing the results obtained with the 3 $alpha$ 5 $alpha$ /ent-3 $alpha$ 5 $alpha$ and 3 $alpha$ 5 $beta$ /ent-3 $alpha$ 5 $beta$ steroid pairs. Diastereoselective interactions can be examinedby comparing the results obtained for the 3 $alpha$ 5 $alpha$ /3 $alpha$ 5 $beta$ and ent-3 $alpha$ 5 $alpha$ /ent-3 $alpha$ 5 $beta$ steroid pairs because only the chiral center at C-5 is differentin each of these steroidpairs.

As summarized in Table 1, all pairs of anesthetic steroid enantiomers studied in this and our previous study (Wittmer etal., 1996) exhibit some degree of enantioselectivity in electrophysiology,[³⁵S]TBPS binding, and when performed, the mouse anesthesia tests.Significant enantioselectivity was not found in the tadpole LRRexperiments for the 5 $beta$ -reduced enantiomer pairs. Notably, thedegree of enantioselectivity is uniformly greater across the variousassays for the steroids in the 5 $alpha$ -reduced series. The consistencyof these results is remarkable considering that different speciesand preparations were used in the bioassays. Of course, differencesin species and preparation also limit interpretation of the results.For example, the enantioselectivity for anesthetic steroid effectson TBPS binding may differ for different GABA_A receptor subtypes.Additonal studies with different subtypes of GABA_A receptors areneeded to address this possibility.

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TABLE 1
Summary of enantioselectivity results

In the electrophysiological experiments, the enantioselectivity is manifested in different ways for the 5 $alpha$ - and 5 $beta$ -seriesof compounds. For potentiation of GABA-mediated currents, enantioselectivityis detected as a difference in maximal response for the steroidsin the 5 $alpha$ -reduced series, whereas it is detected as a differencein the EC₅₀ values for the 3 $alpha$ 5 $beta$ P/ent-3 $alpha$ 5 $beta$ P enantiomer pair inthe 5 $beta$ -reduced series. Based on prior studies (Wittmer et al.,1996; Zorumski et al., 1998), there are likely to be significantdifferences in the potencies of the 5 $alpha$ -reduced enantiomers forpotentiating GABA responses, but poor solubility at concentrations $>=$ 100 µM limits the ability to generate accurate concentration-responsedata for the ent-steroids. There is also a marked enantioselectivitydifference in the gating of GABA_A receptors by the two seriesof steroids. The ent-steroids in the 5 $alpha$ -reduced series do notgate these ion channels at concentrations up to 100 µM, whereasent-3 $alpha$ 5 $beta$ P was found to gate the ion channels at least as wellas 3 $alpha$ 5 $beta$ P over the concentration range of 1 to 100 µM.

Comparing the IC₅₀ values from the [³⁵S]TBPS binding experiments and the EC₅₀ values from tadpole LRR and electrophysiologicalexperiments shows that the effects of the compounds occur in thesame concentration range throughout these bioassays. However,the enantioselectivity for [³⁵S]TBPS displacement by the 3 $alpha$ 5 $alpha$ ACN and 3 $alpha$ 5 $alpha$ P enantiomer pairsis much greater than the enantioselectivity found for the anestheticeffects of these compounds in the tadpole LRR test. Additionally,whereas a small degree of enantioselectivity is found for the5 $beta$ -reduced steroids in the [³⁵S]TBPS-binding experiments, significant enantioselectivity forthese compounds was not found in the tadpole LRR test. The reasonsfor the failure of the tadpole LRR results to more closely correlatewith those of the [³⁵S]TBPS binding experiment are not clear, although the complexityof factors involved in behavioral responses is likely tocontribute.

Overall the results show that 3 $alpha$ 5 $alpha$ -, 3 $alpha$ 5 $beta$ - and ent-3 $alpha$ 5 $beta$ -steroids potently modulate GABA_A receptors, whereas ent-3 $alpha$ 5 $alpha$ -steroidsdo not effectively modulate these receptors. Enantioselectivityfor GABA_A receptor modulation/anesthesia by anesthetic steroidsin the 5 $alpha$ - and 5 $beta$ -reduced steroid series is different (5 $alpha$ > 5 $beta$ ).Because of this enantioselectivity difference, the diastereoselectiveinteractions of the ent-3 $alpha$ 5 $alpha$ /ent-3 $alpha$ 5 $beta$ and 3 $alpha$ 5 $alpha$ /3 $alpha$ 5 $beta$ steroid pairsare also different (ent-pairs > natural pairs). These stereoselectivityresults raise interesting questions. Do these stereoselectivitydifferences imply different mechanisms (direct versus indirect)for modulation of GABA_A receptor function and the correlated anestheticactions of the two series of anesthetic steroids? Do these stereoselectivitydifferences suggest different binding sites for the two seriesof anesthetic steroids on GABA_A receptors? These questions areaddressed in the followingdiscussion.

Our studies of the enantioselectivity of anesthetic steroid effects on GABA_A receptor function were initiated as a way todistinguish between direct (a steroid-binding site on the receptor)and indirect (membrane perturbation) effects of these compoundson receptor function. We define direct effects as those arisingfrom molecular interactions involving the steroid and amino acidsof the receptor. We define indirect effects as those arising frommolecular interactions involving the steroid and other nonproteinmembrane constituents such as cholesterol and phospholipids. Thedegree to which enantioselectivity can be used to make the distinctionbetween the two types of interactions is dependent on how largea difference is expected for the direct and indirect actions ofthe steroid on receptorfunction.

Binding interactions of ligands with receptors are expected to be highly enantioselective because receptor proteins are madeof only L-amino acids. For substrates binding to enzymes, whereboth the initial binding and then a subsequent chemical reactionmust occur, the expected result is complete enantioselectivity(i.e., the enzymatic transformation is expected to be enantiospecific).However, there are exceptions to the expected results for thesetypes of interactions. For example, the binding of nornicotineto nicotinic acetylcholine receptors is not enantioselective.Both (+)- and ( $-$ )-nornicotine displace ( $-$ )-[³H]nicotine with equal potency and efficacy (Zhang and Nordberg,1993; Badio and Daly, 1994; Abreo et al., 1996).

Many examples of esterases that demonstrate varying degrees of enantioselectivity for the hydrolysis of racemic esters arereported in the literature. Indeed, the effective separation ofracemic esters by enzymes (one ester enantiomer is preferentiallyhydrolyzed and readily separated from the unreacted ester enantiomeras the corresponding alcohol enantiomer) as a method for the resolutionof the optically active components may require the screening ofdifferent esterases to identify the most enantioselective esterasefor a particular separation (Chen et al., 1982 and referencestherein). The implication of these examples for this study isthat the varying degrees of enantioselectivity found for the anestheticsteroids are all consistent with a direct steroid-receptor interaction.Indeed, even if enantioselectivity had not been observed in thisstudy, the possibility of a direct steroid-receptor interactioncould not be unequivocally ruledout.

Based on information currently available, no enantioselectivity would be expected for the indirect modulation of GABA_A receptorfunction by anesthetic steroid enantiomers. This conclusion isbased on the following reasoning and supporting evidence. Becauseenantiomers have identical physical properties, they alter thephysical properties of a membrane (e.g., fluidity) in an identicalmanner unless the physical properties of the membrane are alreadydependent on preexisting enantiospecific interactions betweenmembrane constituents. Most obviously, because the cholesteroland phospholipids found in cell membranes occur in enantiomericallypure form, interactions between these molecules could fulfillthe preexisting enantiospecificity requirement. The extent towhich the different anesthetic steroid enantiomers altered thesepreexisting enantiospecific cholesterol-phospholipid interactionswould then determine the anesthetic steroid enantioselectivityfor indirect modulation of channelfunction.

Is there any evidence that enantiospecific cholesterol-phospholipid interactions are determinants of membrane physical properties?Because of the difficulty involved in addressing this question(the unnatural enantiomers of cholesterol and/or a phospholipidare required for the studies), few experiments have been conductedto examine this question. However, the few available experiments(lipid monolayer and NMR studies) provide no evidence that enantiospecificcholesterol-phospholipid interactions have any effect on the physicalproperties of the membrane (Ghosh et al., 1971; Arnett and Gold,1982). Thus, we have referred previously to the membrane as anonchiral environment and we have concluded that no enantioselectivityfor anesthetic steroid action is expected if the effects of thesecompounds are indirectly caused by membrane perturbation (Wittmeret al., 1996). Realizing that this conclusion is based on verylimited experimental data, we recently reported a new method forpreparing the unnatural enantiomer of cholesterol (Kumar and Covey,1999) and we plan to address the biological significance of enantiospecificinteractions between cholesterol and different classes of phospholipidsin future studies. Because, in this study, we find some degreeof enantioselectivity for both series of anesthetic steroids,we find no compelling reasons to conclude that either series ofanesthetic steroids modulates GABA_A receptor function by an indirectmechanism.

Whether the different degrees of enantioselectivity imply different receptor-binding sites for the two series of anestheticsteroids is the final question to address. Although there aredata from previous studies suggesting the existence of more thanone class of binding sites for some steroids on GABA_A receptors(Morrow et al., 1990; Hawkinson et al., 1994a,b, 1998), the enantioselectivityresults we have obtained thus far present no new evidence forthis phenomenon. Previous data from studies of the diastereoselectivemodulation of GABA_A receptor function by 3 $alpha$ 5 $alpha$ P and 3 $alpha$ 5 $beta$ P havebeen reasonably explained by a common binding-site hypothesisdeveloped from molecular modeling studies (Purdy et al., 1990;Han et al., 1996). The results from this and the previous enantioselectivitystudy of 5 $alpha$ -reduced anesthetic steroids (Wittmer et al., 1996)establish new criteria that must be satisfied by molecular modelsof a common binding site for 5 $alpha$ - and 5 $beta$ -reduced anesthetic steroids.Molecular models of a common binding site for both classes ofanesthetic steroids also must be able to explain the greater enantioselectivityof 5 $alpha$ -reduced anesthetic steroids and the greater diastereoselectivityobserved for the ent-3 $alpha$ 5 $alpha$ P/ent-3 $alpha$ 5 $beta$ P steroid pair versus the 3 $alpha$ 5 $alpha$ P/3 $alpha$ 5 $beta$ Psteroidpair.

	Footnotes

Accepted for publication February 22, 2000.

Received for publication November 17, 1999.

¹ This study was supported by U.S. Public Health Service Grant GM47969, Research Scientist Development Award MH00964, and theBantlyFoundation.

Send reprint requests to: Douglas F. Covey, Ph.D., Department of Molecular Biology and Pharmacology, Box 8103, Washington University School of Medicine, 660 S. Euclid Ave., St. Louis, MO 63110. E-mail: dcovey{at}molecool.wustl.edu

	Abbreviations

3 $alpha$ 5 $alpha$ P, (3 $alpha$ ,5 $alpha$ )-3-hydroxypregnan-20-one; 3 $alpha$ 5 $beta$ P, (3 $alpha$ ,5 $beta$ )-3-hydroxypregnan-20-one; GABA, $gamma$ -aminobutyric acid; TBPS, t-butylbicyclophosphorothionate; ent-3 $alpha$ 5 $alpha$ P, (3 $beta$ ,5 $beta$ ,8 $alpha$ ,9 $beta$ ,10 $alpha$ ,13 $beta$ ,14 $alpha$ ,17 $alpha$ )-3-hydroxypregnan-20-one; ent-3 $alpha$ 5 $beta$ P, (3 $beta$ ,5 $alpha$ ,8 $alpha$ ,9 $beta$ ,10 $alpha$ ,13 $beta$ , 14 $alpha$ ,17 $alpha$ )-3-hydroxypregnan-20-one; 3 $alpha$ 5 $alpha$ ACN, (3 $alpha$ ,5 $alpha$ ,17 $beta$ )-3-hydroxyandrostane-17-carbonitrile; 3 $alpha$ 5 $beta$ ACN, (3 $alpha$ ,5 $beta$ ,17 $beta$ )-3-hydroxyandrostane-17-carbonitrile; ent-3 $alpha$ 5 $alpha$ ACN, (3 $beta$ ,5 $beta$ ,8 $alpha$ ,9 $beta$ ,10 $alpha$ ,13 $beta$ ,14 $alpha$ ,17 $alpha$ )-3-hydroxyandrostane-17-carbonitrile; ent-3 $alpha$ 5 $beta$ ACN, (3 $beta$ ,5 $alpha$ ,8 $alpha$ ,9 $beta$ , 10 $alpha$ ,13 $beta$ ,14 $alpha$ ,17 $alpha$ )-3-hydroxyandrostane-17-carbonitrile; DMSO, dimethylsulfoxide; LRR, loss of righting reflex.

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Enantioselectivity of Pregnanolone-Induced -Aminobutyric AcidA Receptor Modulation and Anesthesia1

Enantioselectivity of Pregnanolone-Induced $gamma$ -Aminobutyric Acid_A Receptor Modulation and Anesthesia¹