Synaptically Released and Exogenous ACh Activates Different Nicotinic Receptors to Enhance Evoked Glutamatergic Transmission in the Lateral Geniculate Nucleus

doi:10.1152/jn.00339.2005

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Synaptically Released and Exogenous ACh Activates Different Nicotinic Receptors to Enhance Evoked Glutamatergic Transmission in the Lateral Geniculate Nucleus

Jian-Zhong Guo, Yingbing Liu, Eva M. Sorenson and Vincent A. Chiappinelli

Department of Pharmacology and Physiology, The George Washington University, School of Medicine and Health Sciences, Washington, DC

Submitted 31 March 2005; accepted in final form 13 June 2005

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

The effects of activation of nicotinic acetylcholine receptors(nAChRs) on glutamatergic transmission in the ventral lateralgeniculate nucleus (LGNv) were examined in chick brain slices.Whole cell recordings showed that monosynaptic postsynapticcurrents (PSCs) evoked in LGNv neurons by optic tract stimulationwere blocked by glutamate receptor antagonists. Exogenouslyapplied nicotine (0.5 µM), choline (1 mM), or acetylcholine(ACh, 100 µM) markedly increased (>3-fold) these evokedPSCs. Potentiation by ACh was dose-dependent and did not desensitizeduring a 5-min application. In a second set of experiments,the effect of releasing endogenous ACh by stimulating the lateralportion of the LGNv through a separate conditioning electrodebefore optic tract stimulation was examined. Conditioning stimulationtrains increased PSCs by an average of 5.2-fold, an effect dependenton both the intensity and number of conditioning pulses. Thisincrease in PSC amplitude was most likely caused by releasedACh activating ${alpha}$ 6- and/or ${alpha}$ 3-containing nAChRs because it wasblocked by 100 nM ${alpha}$ -conotoxin MII, 100 nM dihydro- ${beta}$ -erythroidine(DH ${beta}$ E), and 0.1–1.0 µM methyllycaconitine (MLA).In contrast, exogenously applied ACh increased PSC amplitudeby activating a pharmacologically different population of nAChRsbecause this effect was inhibited by 100 nM ${alpha}$ -bungarotoxin, 50nM MLA, and a high concentration (30 µM) of DH ${beta}$ E, indicatingthat ${alpha}$ 7- and/or ${alpha}$ 8-containing receptors were involved. The resultsare consistent with a model whereby ${alpha}$ 6- and/or ${alpha}$ 3-containing nAChRson retinal ganglion cell nerve terminals are located preferentiallyat cholinergic synapses, whereas ${alpha}$ 7- and/or ${alpha}$ 8-containing receptorsare primarily extrasynaptic.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Nicotinic transmission plays a key role during the developmentof mammalian and avian visual systems. Cholinergic nerve fibersand nicotinic acetylcholine receptors (nAChRs) are present throughoutthe vertebrate visual nervous system, including the retina,lateral geniculate nucleus (LGN), and certain layers of thevisual cortex. Nicotinic receptors mediate the initiation ofspontaneous bursts of wave-like activity in the developing retina(Feller et al. 1996; Sernagor et al. 2000). In mice lackingthe ${beta}$ 2 nAChR subunit, these retinal waves are absent, and thepattern of innervation of the LGN by retinal ganglion cellsis abnormal (McLaughlin et al. 2003; Muir-Robinson et al. 2002;Rossi et al. 2001). In ferret visual cortex, fast, evoked nicotinictransmission is observed before and during innervation by thalamicafferents (Roerig et al. 1997).

The chick ventral LGN (LGNv) contains a high density of cholinergicnerve fibers (Sorenson et al. 1989) and at least three subtypesof nAChRs that can be differentially labeled by radioactivenicotine, ${alpha}$ -bungarotoxin ( ${alpha}$ -BgTx), and ${kappa}$ -BgTx (Sorenson and Chiappinelli1992). Functional studies have shown that exogenous nicotinicagonists can increase the frequency of glutamatergic spontaneouspostsynaptic currents (SPSCs) in LGNv neurons by activationof ${alpha}$ -BgTx–sensitive nAChRs (Guo et al. 1998; McMahon etal. 1994). A major source of glutamatergic innervation of LGNvneurons is the optic tract, which contains the axons of retinalganglion cells. The optic tract is well defined in brain slicesand provides an excellent opportunity to study synaptic activitybetween retinal ganglion cells and LGNv neurons.

Our goal in this study was to examine a possible functionalrole for cholinergic nerve fibers and nAChRs in the modulationof evoked neurotransmission at this synapse. We report thatactivation of nAChRs markedly enhanced electrically evoked glutamatergictransmission between retinal ganglion cell nerve terminals andLGNv neurons. Furthermore, we found that exogenous nicotinicagonists and endogenously released ACh modulated this glutamatergicsynaptic transmission by activation of pharmacologically differentnAChRs.

METHODS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Brain slice preparation

Eighteen- to 20-day embryonic White Leghorn chicks were rapidlydecapitated, and their brains were removed and immediately placedin 4°C Mg²⁺-enriched artificial cerebrospinal fluid (ACSF;in mM): 126 NaCl, 2.5 KCl, 1.24 NaH₂PO₄, 10.0 MgSO₄, 2.4 CaCl₂,26 NaHCO₃, and 10 D-glucose, pH 7.3 when bubbled with 95% O₂-5%CO₂. The brains were blocked and attached to the stage of avibrating tissue slicer. Coronal slices (350–400 µm)containing the LGNv were placed in fresh standard ACSF (in mM):126 NaCl, 2.5 KCl, 1.24 NaH₂PO₄, 1.3 MgSO₄, 2.4 CaCl₂, 26 NaHCO₃,10 D-glucose, and 1.0 µM atropine sulfate to block allmuscarinic responses, pH 7.3 when bubbled with 95% O₂-5% CO₂,at room temperature for at least 1 h before use in experiments.Slices were placed in the center of a submerged recording chamber(Warner Instruments, Hamden, CT) and stabilized with a U-shapedplatinum holder. Slices were continuously superfused (2–3ml/min) at room temperature with ACSF, and bicuculline (10 µM)was included in most experiments to eliminate GABAergic currents.All efforts were made to minimize both the suffering and thenumber of animals used in these experiments, and all experimentsconformed to National Institutes of Health guidelines on theethical use of animals.

Electrophysiological methods

Whole cell patch-clamp recordings in brain slices were madefrom LGNv neurons visualized with Nomarski optics as describedin Guo et al. 1998. Patch pipettes were fabricated from borosilicateglass with a two-stage microelectrode puller to produce a tipopening of 1–2 µm with a resistance of 4–8M ${Omega}$ . The pipette solution contained (in mM) 150 K-gluconate, 2MgCl₂, 2 EGTA, 2 Mg-ATP, and 10 HEPES, adjusted to pH 7.3 with1.0 N KOH. Biocytin (0.3%) was added to the recording solutionto facilitate postrecording morphological studies. When examiningthe voltage dependence of the evoked PSCs, 150 mM Cs-gluconatewas used instead of K-gluconate. Electrical stimulation of retinalganglion cell afferents to the LGNv was accomplished with aconcentric bipolar electrode (50-µm tip; FHC Corp.) placedonto the surface of the optic tract about 1 mm ventral to theLGNv (Fig. 1), similar to the approach described by Dye andKarten (1996). Stimulation pulses (5- to 200-µA intensity,200- to 300-µs duration) were triggered at a frequencyof 0.008–0.033 Hz, and evoked PSCs were recorded in LGNvneurons. In experiments examining the effects of endogenouslyreleased ACh, a second stimulating electrode was placed ontothe surface of the lateral portion of the LGNv (Fig. 1). Thiselectrode was used to provide conditioning stimulation trains.Conditioning stimulation trains (3–8 pulses long, 50-to 200-µA intensity, 200- to 300-µs duration at25 Hz) were triggered at a frequency of 0.008–0.017 Hzand were delivered 0.2–1.0 s before optic tract stimulation.Signals were obtained with an Axopatch-200B amplifier (AxonInstruments, Foster City, CA) in voltage-clamp mode. Data wereacquired with Clampex Ver.7.0 (Axon Instruments).

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FIG. 1. Placement of stimulating and recording electrodes. Image is a coronal section of the chick brain that has been immunohistochemically stained for choline acetyltransferase using a cobalt-enhanced diamino-benzidine reaction (Sorenson et al. 1989

). There is a dense network of cholinergic fibers throughout the ventral lateral geniculate nucleus (LGNv). Stimulating electrodes were positioned with micromanipulators onto the optic tract (optic tract stimulation) and the lateral portion of the LGNv (conditioning stimulation). A patch pipette (recording pipette) was used to record electrical activity in individual LGNv lamina interna neurons. li, lamina interna; ne, neuropil; Rt, nucleus rotundus.

Data analysis

To quantitate evoked glutamatergic synaptic transmission, threeto five consecutive responses evoked by optic tract stimulationwere obtained before and during exposure to an exogenous nicotinicagonist, either in normal ACSF or in the presence of variousnicotinic antagonists. These responses were averaged and plottedwith Origin 7.0. A similar approach was taken for conditioningstimulation experiments, except that the conditioning stimulustrain took the place of the exogenous nicotinic agonist. Risetime was calculated at 10–90% of the peak amplitude. Whencomparing only two data sets, a two-tailed t-test was used withP < 0.05 chosen as the level of significance. For nicotinicantagonist experiments, evoked current amplitudes under controlconditions were compared with both those in the presence ofACh (or conditioned stimulation) and those determined in thepresence of ACh (or conditioned stimulation) + antagonist. Statisticaldifferences between these multiple amplitudes were determinedusing the two-tailed ANOVA with the Tukey-Kramer multiple comparisonstest as a posttest. The level of significance chosen was P <0.05. Results are expressed as means ± SE.

Agonist and antagonist application

Nicotinic antagonist application was done by bath superfusionfor $≥$ 15 min before application of agonist. Agonist solutionscontained the antagonist at the appropriate concentration wheneverthe effects of an antagonist were being examined. A separate,gravity-fed U-tube system was used to deliver agonists to LGNvneurons (Alkondon and Albuquerque 1993). The tip of the U-tubehad a diameter of 150 µm, and the lower rim of the U-tubetip was placed 2–3 mm from the LGNv neuron being recordedfrom. The in-flow for all solutions delivered by U-tube intothe recording chamber was gravity-fed, whereas the U-tube out-flowfrom the chamber was regulated by vacuum to provide a steadyout-flow suction pressure. This out-flow suction system preventedany leakage of agonist solutions into the bath between agonistapplications.

Visualization of LGNv neurons

After electrophysiological recordings were completed, the brainslices were placed in 4% paraformaldehyde in 0.1 M phosphatebuffer. To visualize LGNv neurons that were filled with biocytinduring recording, brain slices were washed three times in 0.1M PBS and incubated for at least 1 h in streptavidin conjugatedto Alexa 568 (1 µg/ml; Molecular Probes) and Nissl green(1:100; Molecular Probes) in 0.1 M PBS. The slices were washed,mounted on slides, and coverslipped using 90% glycerol, 10%PBS, and 4% propyl gallate for the mounting media. An epi-fluorescentmicroscope equipped with a digital camera connected to a computerrunning Adobe Photoshop was used to capture low-power imagesshowing the localization of filled neurons within the LGNv.A Bio-Rad 1024 scanning laser confocal microscope equipped witha krypton-argon laser was used to image filled cells in moredetail. Z stacks of optical sections were collected for eachfilled neuron. Each Z stack was converted into a projectionimage. The projection images making up each individual neuronwere imported to Adobe Photoshop 7.0, where they were alignedto create a photomontage of each neuron.

Materials

Drugs used were obtained from the following sources: acetylcholinechloride, atropine sulfate (atropine), bicuculline methiodide,choline chloride (choline), methyllycaconitine (MLA), and (–)-nicotinebitartrate were purchased from Sigma (St. Louis, MO); dihydro- ${beta}$ -erythroidine(DH ${beta}$ E), 6,7-dinitroquinoxaline-2,3-dione (DNQX), and AP5 werefrom RBI/Sigma (Natick, MA); and TTX was from Calbiochem (SanDiego, CA). Purified ${alpha}$ -conotoxins ( ${alpha}$ -CTxs) were gifts from Dr.J. M. McIntosh, University of Utah. ${alpha}$ -BgTx and ${kappa}$ -BgTx were purifiedfrom the crude venom of Bungarus multicinctus as described (Chiappinelli1983). Atropine, DH ${beta}$ E, and nicotine were prepared in deionizedwater to make a 10 mM stock solution. Choline and ACh were preparedin deionized water to make a 1 M stock solution. MLA was preparedin DMSO to make a 10 mM stock solution. Dilution of these stocksin ACSF produced the final working concentration. Lyophilized ${alpha}$ -CTxs were made up to their final concentrations in ACSF containing0.01 mg/ml protease-free bovine serum albumin.

RESULTS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Stimulation of optic tract evokes both glutamatergic and GABAergic postsynaptic currents in LGN neurons

The LGNv receives a major sensory input from the optic tract,which consists of the axons of retinal ganglion cells (Guiloff1991; Gunturkun and Karten 1991; Wu et al. 1999). We placeda stimulating electrode onto the optic tract ventromedial tothe LGNv in a coronal brain slice and examined electricallyevoked responses using whole cell voltage-clamp recordings fromvisually identified LGNv lamina interna neurons (Fig. 1). Whenthese LGNv neurons were clamped at –50 mV, single-pulsestimulation of the optic tract evoked biphasic PSCs under controlconditions (ACSF with 1 µM atropine; Fig. 2 Aa, n = 4).

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FIG. 2. Optic tract stimulation evokes direct monosynaptic glutamatergic and indirect polysynaptic GABAergic postsynaptic currents in LGNv neurons. A: LGNv neuron receives both glutamatergic and GABAergic input. Aa: electrical stimulation of the optic tract (10 µA; 200 µs) evoked a postsynaptic response in an LGNv neuron consisting of a short-latency inward current (<10 ms) followed by a longer-latency outward current lasting $≤$ 300 ms. Neuron was held at –50 mV in standard artificial cerebrospinal fluid (ACSF; contains 1 µM atropine). Ab: bicuculline (10 µM, U-tube) for 30 s before electrical stimulation blocked only the outward going currents. Ac: recovery after 10 min washout of bicuculline. Ad: 6,7-dinitroquinoxaline-2,3-dione (DNQX; 20 µM, U-tube) for 30 s before stimulation substantially blocked both inward and outward evoked currents. Ae: both inward and outward currents recovered after 30 min washout of DNQX. (a-e from same neuron). Ba: in another LGNv neuron, stimulation of the optic tract (40 µA; 200 µs) elicits inward and outward currents. Bb: both inward and outward currents were completely blocked in the presence of DNQX (40 µM) and AP5 (50 µM). C: evoked (15 µA; 200 µs) glutamatergic currents recorded at different holding potentials in the presence of bicuculline (10 µM). Cs-gluconate pipette solution was used and the neuron was held at –70, –40, +10, and +50 mV. D: evoked synaptic currents recorded in response to stimulation pulses of increasing intensities had uniformly short and nearly constant latency. Superfusion ACSF contained atropine (1 µM) and bicuculline (10 µM). Neuron was held at –70 mV. E: latency and initial slope of the evoked (25 µA; 200 µs) synaptic current recorded in the presence of bicuculline (10 µM) did not change after superfusion with high divalent cation solution (12 mM Ca²⁺ and 12 mM Mg²⁺). Neuron was held at –70 mV.

The short-latency, inward PSCs had a duration of <10 ms,whereas the longer-latency outward PSCs lasted $≤$ 300 ms. The GABA_Areceptor antagonist bicuculline (10 µM) blocked the outwardPSCs but had little or no effect on inward PSCs (Fig. 2Ab; n= 3). In contrast, DNQX (20 µM), an antagonist of non–N-methyl-D-aspartate(NMDA) receptors, substantially blocked both inward and outwardPSCs (Fig. 2Ad; n = 3). After slices were treated with bothDNQX and AP5 (an NMDA receptor antagonist), all evoked responseswere completely blocked (Fig. 2Bb; n = 3). These results suggestedthat the short-latency inward current was glutamatergic andthe longer-latency GABAergic response was caused by indirectactivation of GABAergic neurons after optic tract stimulation.In the presence of bicuculline (10 µM), the remainingshort-latency evoked PSCs reversed between –10 and +10mV (Fig. 2C; n = 4). The PSCs decayed rapidly at negative holdingpotentials (–70 to –40 mV) but persisted much longerat positive holding potentials (+50 mV, n = 4, Fig. 2C), indicatingthat glutamate released from optic tract stimulation was actingon both non-NMDA and NMDA receptors present on LGNv neurons.The evoked PSCs recorded in the presence of bicuculline seemedto reflect the activity of a monosynaptic glutamatergic connection.The PSCs had a constant and short latency (<5 ms) and theinitial slope of the PSCs was smoothly graded with changingintensity of the stimulus (Fig. 2D; n = 3). Moreover, therewas no change in latency or rise time of the PSCs when divalentcation concentrations were increased to 12 mM (Sah and Nicoll1991

) to raise the firing threshold and thereby reduce the likelihoodof interneurons participating in the stimulus pathway (Fig.2E, rise time: 4.4 ± 0.1 ms for control, 4.0 ±0.4 ms for high divalent cations, P > 0.5 by t-test, n =3).

Morphology of electrophysiologically characterized neurons

The morphology of neurons filled with biocytin during patchrecording was examined, and most of these neurons (15 of 20)exhibited many of the characteristics of projection neuronsin the lamina interna of the chick LGNv as visualized with Golgiimpregnation (Tombol et al. 2004), while the remaining fiveneurons could not be completely characterized. Cell bodies werelocated in the lamina interna and processes left the dorsaland ventral aspects of the soma (Fig. 3). The ventrally projectingdendrites reached down into different levels within the neuropillayer of the LGNv such that some were found in the third ofthe neuropil under the lamina interna (Fig. 3B), whereas otherswere in the middle of the neuropil (Fig. 3, A and C) or in LGNvneuropil closer to the optic tract (Fig. 3D). Many of theseventral dendrites formed "balls" (Fig. 3, A'–C') withinthe neuropil. The dorsally oriented dendrites appeared to projectpast the lamina interna to the area between the nucleus rotundusand the LGNv (Fig. 3, B and C). Initial axon segments couldbe seen in 7 of the 20 neurons. The axons left the cell somaor one of the primary dorsal dendrites and ran medial to thenucleus rotundus (Fig. 3, A, A', B, B', and D). Axons that wereintact some distance from the cell bodies had collaterals thatran either medial and ventral to the nucleus rotundus or intothe lamina interna and neuropil of the LGNv (Fig. 3, A, A',B, B', and D).

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FIG. 3. Morphology of electrophysiologically characterized LGNv neurons. Four representative LGNv neurons filled with biocytin during electrophysiological recording are shown. A–C: low-power photomicrographs showing localization of somas and their processes within the LGNv and surrounding area. Sections are stained with fluorescent Nissl green to allow localization of neurons within the architecture of sections. A'–C': photomontages of corresponding neurons in A–C, respectively. Cell somas are localized in the lamina interna (li) of the LGNv. Note vertical orientation of cell processes. Ventral dendrites descend to varying levels within the neuropil (ne) between the li and the optic tract (TrO). They often form a clump or ball of fibers within the ne when the neurons were viewed as projections made from z stacks (A'–C'). Neuron in D does not appear to have a dense clump of ventral dendritic processes, but it is unclear whether this is a subclass of li neurons or whether it is a limitation of reconstructing neurons in 350-µm-thick brain sections because neuronal processes may well be lost during sectioning. Dorsal dendrites appeared to have branches not only in the li but also projections in the area dorsal of the LGNv (B and C). Arrows in A and B indicate main axon collaterals of visualized neurons. Main branch of axons leaves LGNv in the dorsal direction and runs medial to the nucleus rotundus (Rt). Axons have collaterals (A', B', and D). Arrows in A', B', and D indicate axonal branching points. Collaterals could be found in the LGNv ne (A' and D), in the li (A' and B'), and/or in the area ventral and ventromedial to the Rt. In B', it appears that the more distal portions of the main axon no longer have axon collaterals. Scale bar represents 100 µm in A–C and 25 µm in A', B' C', and D.

Activation of nicotinic receptors potentiates evoked glutamatergic PSCs

We used a U-tube drug application system for agonist applicationsto facilitate detection of possible fast-desensitizing nicotinicresponses. Bicuculline (10 µM) and atropine (1 µM)were present in all solutions throughout the following experimentsto block the evoked GABAergic currents as well as any muscarinicresponses. U-tube application of ACh (100 µM) producedvery little or no direct effect on membrane current but greatlypotentiated the evoked glutamatergic responses (3.7 ±0.7-fold increase vs. control; P < 0.002 by t-test; n = 18;Fig. 4A). The time-course for this nicotinic effect on evokedresponses was examined. During perfusion for 10 s with ACh (100µM), the potentiation of evoked responses reached a maximumat 2 s and persisted at that level for the remainder of agonistapplication (Fig. 4B; n = 3). Even after 5-min preexposure to100 µM ACh, there was little change in the level of potentiationobserved (Fig. 4C; n = 3). The onset of the response to AChappeared to be determined primarily by how fast the drug wasdelivered to the neurons, which depended on the gravity-feedpressure and the distance of the U-tube from the neuron. Becausethe nicotinic response did not desensitize over 10 s, electricalstimulation of the optic tract was routinely carried out after4–5 s of agonist application in the following experiments.The potentiation by ACh of glutamatergic-evoked transmissionexhibited dose dependence between 0.1 and 10 mM ACh (Fig. 5A;n = 3). It is important to note that, because the U-tube waspositioned in the flowing bath at a considerable distance (2–3mm) from the recorded neuron, a significant dilution of theagonist occurred before reaching the neuron. We estimate thisdilution to be three- to fourfold, based on a comparison ofthe maximum inward current generated by glutamate when appliedby our U-tube method versus when applied by whole bath perfusion(n = 3). U-tube application of other nicotinic agonists, includingnicotine (0.5–1.0 µM; 4.6 ± 2.3-fold increase;P < 0.05; n = 4) and choline (0.3–1 mM; 3.4 ±1.7-fold increase; P < 0.02; n = 9), also greatly potentiatedevoked glutamatergic responses (Fig. 5B). To determine whetherpostsynaptic nAChRs played any role in this enhancement, weexamined the effect of ACh on the response of LGNv neurons toexogenously applied glutamate in the presence of TTX. As shownin Fig. 5C, U-tube application of glutamate (200 µM) for5 s produced inward currents of consistent amplitude. A 10-sapplication of the same concentration of glutamate produceda larger response (4th response in Fig. 5C), indicating thatthe response to 5 s of glutamate was submaximal. Bath applicationof ACh (100 µM) did not alter the current produced byexogenously applied glutamate (n = 3). The results are consistentwith the hypothesis that activation of nicotinic receptors locatedon glutamatergic retinal ganglion cell terminals was responsiblefor the observed modulation of evoked transmission in the LGNv.

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FIG. 4. U-tube application of acetylcholine (ACh) potentiates evoked glutamatergic postsynaptic currents (PSCs) without rapid desensitization of effect. A: U-tube application of ACh (100 µM) for 1, 5, or 10 s before electrical stimulation markedly potentiated evoked glutamatergic PSCs. B: amplitudes of evoked glutamatergic responses at various times during continuous application of ACh (100 µM) for 10 s through U-tube. Responses were normalized to evoked response measured after 5 s of ACh exposure. Each point and vertical bar represent means ± SE (n = 3) from different LGNv neurons. C: potentiation of evoked glutamatergic response by 100 µM ACh persisted after a 5-min exposure to ACh.

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FIG. 5. Activation of nicotinic acetylcholine receptors (nAChRs) on glutamatergic terminals by exogenous ACh, nicotine, or choline potentiates evoked glutamatergic PSCs. A: U-tube application of ACh (0.1–10 mM) potentiated evoked glutamatergic PSCs in a dose-dependent manner. B: U-tube application of nicotine (0.5 µM) greatly potentiated evoked glutamatergic PSCs (2nd trace). After washout of nicotine (middle trace), U-tube application of choline (1 mM) markedly potentiated the evoked response. C: U-tube application of glutamate (200 µM) for 5 s in the presence of 0.3 µM TTX and 1 µM atropine produced an inward current that was unchanged when 100 µM ACh was present in the bath (bar above record). U-tube application of glutamate (200 µM) for 10 s produced a larger inward current (final response in record).

Pharmacology of presynaptic nAChRs mediating responses to exogenously applied nicotinic agonists

Because the LGNv contains at least three different subtypesof nAChRs based on ³H-nicotine–, ¹²⁵I- ${alpha}$ -BgTx–, and¹²⁵I- ${kappa}$ -BgTx–specific binding (Sorenson and Chiappinelli1992), selective antagonists were used to pharmacologicallycharacterize the nAChR subtype(s) mediating the responses toexogenously applied nicotinic agonists. Low concentrations (0.1and 1.0 µM) of DH ${beta}$ E that are selective for non- ${alpha}$ 7 nAChRs(Harvey et al. 1996; Pereira et al. 1994; Sabey et al. 1999)did not significantly block the potentiation produced by 100µM ACh (Fig. 6A; n = 4 at 0.1 µM and n = 6 at 1.0µM; both P > 0.05 by ANOVA). At a higher concentrationof DH ${beta}$ E (30 µM), where most nAChRs should be inhibited,the potentiation was completely blocked (Fig. 6Ad; n = 4; P< 0.01 by ANOVA).

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FIG. 6. Potentiation of evoked glutamatergic PSCs by exogenous ACh is blocked by nicotinic antagonists. A–D: effects of a nicotinic antagonist on the potentiation produced by 100 µM ACh in a different LGNv neuron. Row a: control glutamatergic PSCs in response to optic tract stimulation are shown. These PSCs were recorded 5 s after U-tube application of ACSF was begun. Row b: U-tube application of ACh (100 µM) for 5 s before electrical stimulation markedly potentiated evoked glutamatergic PSCs. Row c: 1 µM dihydro- ${beta}$ -erythroidine (DH ${beta}$ E) and 10 nM methyllycaconitine (MLA) had no significant effect on the ACh-induced potentiation of the evoked response. Row d: complete blockade of the ACh-induced potentiation by 30 µM DH ${beta}$ E, 50 nM MLA, and 100 nM ${alpha}$ -BgTx. Row e: recovery of ACh-induced potentiation after washout of antagonists. Row f: control ACSF responses at the end of experiments. Row g: summary data for all neurons with similar antagonist treatment. For each graph, ACh significantly potentiated the control PSC by $≥$ 3-fold (data reported as mean ± SE of control; n = 4–7, significance determined by ANOVA; *P < 0.05; **P < 0.01; ***P < 0.001). Effects of antagonists on the ACh-potentiation are shown, and only the following concentrations of antagonists significantly reduced the ACh-potentiation: 30 µM DH ${beta}$ E (n = 4, P < 0.01); 50 nM MLA (n = 5, P < 0.05), and 100 nM ${alpha}$ -BgTx (n = 6, P < 0.05).

The following antagonists that block ${alpha}$ 7- and/or ${alpha}$ 8-containing( ${alpha}$ 7*/ ${alpha}$ 8*) nAChRs were tested: MLA, ${alpha}$ -BgTx, and ${alpha}$ -CTx ImI. At 10nM MLA, a concentration reported to completely block mammalian ${alpha}$ 7* receptors (Mogg et al. 2002

; Wooltorton et al. 2003

), theACh-mediated potentiation of glutamatergic transmission wasnot inhibited (Fig. 6Bc; n = 3; P > 0.05). At 50 nM MLA,the potentiation in response to ACh was completely blocked (Fig.6Cd; n = 5; P < 0.05). At a concentration of 100 nM, ${alpha}$ -BgTxalso completely blocked the ACh-induced potentiation (Fig. 6Dd;n = 6; P < 0.05). Another ${alpha}$ 7*/ ${alpha}$ 8* antagonist, ${alpha}$ -CTx ImI (0.1µM), however, did not inhibit the nicotinic potentiationof evoked responses (n = 4; P > 0.05, data not shown).

The next group of antagonists tested were ${alpha}$ 3* antagonists. Theresults with ${kappa}$ -BgTx (100 nM), which is a potent antagonist of ${alpha}$ 3 ${beta}$ 2 and ${alpha}$ 3 ${alpha}$ 5 ${beta}$ 4 nAChRs (Conroy and Berg 1995; Luetje et al. 1998),were complex. Of six neurons examined, two had a complete blockadeof the nicotinic response, two exhibited a partial block, andtwo were little changed from control (data not shown). ${alpha}$ -CTxMII (100 nM), which blocks both ${alpha}$ 6* and ${alpha}$ 3 ${beta}$ 2 nAChRs (Cartier etal. 1996; Champtiaux et al. 2002; Everhart et al. 2004), and ${alpha}$ -CTx AuIB (1 µM), a blocker of ${alpha}$ 3 ${beta}$ 4* nAChRs (Luo et al.1998), did not inhibit the nicotinic potentiation of glutamatergicPSCs (n = 3 for each toxin, P > 0.05, data not shown).

Conditioning trains potentiate glutamatergic transmission evoked by optic tract stimulation

Because the LGNv is innervated by a dense network of cholinergicfibers (Fig. 1 in this report; Sorenson et al. 1989), we soughtto determine whether endogenous release of ACh from these fiberscould enhance evoked glutamatergic transmission in the LGNv.For these experiments, a second stimulating electrode, termedthe conditioning electrode, was placed in the lateral portionof the LGNv while recording from LGNv neurons in the centralportion of the nucleus. Stimulation of the conditioning electrodeevoked small postsynaptic inward currents recorded from LGNvneurons (Fig. 7). These fast inward currents were blocked by20 µM DNQX, but not by 30 µM DH ${beta}$ E, indicating thatthey were likely caused by direct stimulation of glutamatergicfibers running through the LGNv (n = 3). Trains of conditioningstimuli were given before optic tract stimulation. At low conditioningstimulation intensities, there was no change in the glutamatergicresponse evoked by optic tract stimulation (Fig. 7A). However,when the intensity and/or number of conditioning pulses wereincreased, there was a marked enhancement in glutamatergic transmissionbetween retinal ganglion terminals and LGNv neurons (5.2 ±0.6-fold increase vs. control, n = 25, P < 0.0001 by t-test).The timing of the conditioning train was also critical, withthe enhancement disappearing as the time between the conditioningtrain and optic tract stimulation was extended to between 400and 900 ms (Fig. 7B; n = 4). Conditioning stimulation trainsalso markedly enhanced evoked glutamatergic transmission inthe presence of high divalent cations (12 mM Ca²⁺ and 12 mMMg²⁺; 2.5 ± 0.6-fold increase, n = 3, P < 0.05; datanot shown).

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FIG. 7. Conditioning stimulus train before optic tract stimulation potentiates evoked glutamatergic PSCs. Aa: conditioning train of 5 pulses (200-µs pulse duration, 25 Hz) was delivered 300 ms before optic tract stimulation. At the lowest stimulus intensity shown (20 µA), evoked response was unchanged from control (none). At 30 µA, marked potentiation of evoked response to optic tract stimulation was observed, and this potentiation reached a maximum at 40 and 50 µA stimulus intensity. Optic tract was stimulated at 11 µA (200 µs). Ab: in the same neuron, number of pulses in the train was varied from 3 to 8 while maintaining stimulus intensity at 50 µA. A 3-pulse train did not alter evoked response, whereas 5- and 8-pulse trains produced marked potentiation of the evoked glutamatergic response. Ba: in another neuron, the time between the conditioning train and optic tract stimulation was varied. At 70-µA conditioning stimulus intensity, enhancement of glutamatergic-evoked response persisted to $~$ 400 ms after the end of conditioning pulse, but was no longer present after 494 ms. Bb: in the same neuron with a 100-µA conditioning stimulus intensity, enhancement persisted to 700 ms, but was only slightly larger than control after 895 ms.

Pharmacology of glutamatergic enhancement after conditioning trains

To determine whether the potentiation of glutamatergic transmissionby conditioning stimulation was caused by the release of endogenousACh, the ability of nicotinic antagonists to block the potentiationwas examined. Several nicotinic antagonists completely blockedthe enhancement of glutamatergic transmission produced by conditioningtrains, including 100 nM DH ${beta}$ E (Fig. 8 A; n = 10, P < 0.001)and 100 nM ${alpha}$ -CTx MII (Fig. 8B; n = 3, P < 0.001). MLA significantlyinhibited glutamatergic enhancements produced by conditioningtrains at 100 nM (Fig. 8Cb; 64% inhibition, n = 12, P < 0.05)and completely blocked them at 1 µM (Fig. 8Cc; n = 4,P < 0.05). No significant inhibition of the conditioningtrain glutamatergic enhancement was observed in the presenceof ${alpha}$ -BgTx (100 nM), ${kappa}$ -BgTx (100 nM), ${alpha}$ -CTx ImI (0.5 µM),or ${alpha}$ -CTx AuIB (1 µM) (n = 3–4 for each toxin; P >0.05 for all).

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FIG. 8. Potentiation of optic tract stimulation–evoked glutamatergic responses by conditioning trains was blocked in the presence of 100 nM DH ${beta}$ E and 100 nM ${alpha}$ -CTx MII. In this figure, black traces show response in an LGNv neuron to optic tract stimulation without a preceding conditioning train, whereas red traces show identical optic tract stimulation when preceded by a conditioning train of 5 pulses. Aa: control: without nicotinic antagonists present, conditioning train produces a large potentiation of the evoked response to optic tract stimulation. Ac: 100 nM DH ${beta}$ E completely blocks conditioning train potentiation of optic tract–evoked glutamatergic response. Ad: potentiation partially recovers after washout of DH ${beta}$ E. Ba: control: without nicotinic antagonist present, showing potentiation of evoked response by conditioning train. Bc: ${alpha}$ -CTx MII (100 nM) completely blocks conditioning train–induced potentiation. Bd: potentiation by conditioning train recovers after washout of ${alpha}$ -CTx MII. Ca: control. Cb: 100 nM MLA partially decreases the potentiation produced by conditioning train. Cc: at 1 µM MLA, potentiation is completely blocked. Cd: recovery of potentiation after washout of MLA. Row e: summary data are presented for all neurons with similar antagonist treatment. For each graph, conditioning stimulation significantly potentiated the control PSC by $≥$ 4-fold (data reported as mean ± SE of control; n = 3–12, significance determined by ANOVA; *P < 0.05; ***P < 0.001). Effects of antagonists on the potentiation produced by conditioning stimulation are shown, and only the following concentrations of antagonists significantly reduced the potentiation: 100 nM DH ${beta}$ E (n = 10, P < 0.001); 100 nM ${alpha}$ -CTx MII (n = 3, P < 0.001), 100 nM MLA (n = 12, P < 0.05), and 1 µM MLA (n = 4, P < 0.05).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION GRANTS ACKNOWLEDGMENTS REFERENCES

The results show significant nicotinic modulation of evokedglutamatergic transmission in the chick LGNv. Activation ofnAChRs with exogenously applied ACh during optic tract stimulationcaused an average 3.7-fold potentiation of evoked glutamatergicPSPs recorded in LGNv lamina interna neurons. A similar potentiationwas observed with both exogenous nicotine and choline, and thiseffect appears to be caused primarily by the activation of ${alpha}$ 7-and/or ${alpha}$ 8-containing nAChRs located on the glutamatergic nerveterminals of retinal ganglion cells that synapse directly ontoLGNv neurons. Electrically stimulated release of endogenousACh in the LGNv also markedly potentiated glutamatergic transmission(by 5.2-fold), but pharmacologically different nAChRs mediatedthis nicotinic effect.

Cholinergic fibers and several subtypes of nAChRs are presentin high densities throughout the LGNv (Sorenson and Chiappinelli1992; Sorenson et al. 1989). Some of these receptors are locatedon glutamatergic and GABAergic nerve terminals, because activationof these presynaptic nAChRs enhances the spontaneous releaseof glutamate and GABA in the LGNv in the presence of TTX (Guoand Chiappinelli 2002; Guo et al. 1998). These experiments examinedthe possible modulatory role of nAChRs on evoked excitatorysynaptic transmission at LGNv neurons, and it is clear thatactivation of nAChRs can have a profound effect on glutamatergicsignaling between retinal ganglion nerve terminals and LGNvneurons. The nAChRs involved are located presynaptically, becausethe postsynaptic response to exogenous glutamate was unchangedin the presence of nicotinic agonists.

Exogenously applied ACh potentiated evoked glutamatergic transmissionin a dose-dependent manner, and the response was completelyblocked by 30 µM DH ${beta}$ E, showing that nAChRs were mediatingthe response. Choline, a nicotinic agonist with some selectivityfor ${alpha}$ 7-containing nAChRs (Alkondon et al. 1997, 2000), also producedmarked potentiation of evoked glutamatergic transmission, andthe ${alpha}$ 7*/ ${alpha}$ 8*-selective antagonist ${alpha}$ -BgTx blocked the ACh-inducedpotentiation. Thus it is very likely that the major nAChRs mediatingthis enhancement of evoked glutamatergic transmission contain ${alpha}$ 7 and/or ${alpha}$ 8 subunits. However, these ${alpha}$ -BgT–sensitive nAChRsdiffer from classical ${alpha}$ 7 and ${alpha}$ 8 receptors in that they are notsensitive to ${alpha}$ -CTx ImI (Pereira et al. 1996) and are not blockedat 10 nM MLA (but are blocked at 50 nM). The nicotinic enhancementpersisted during a 5-min exposure to ACh applied by U-tube.Previous work in brain slices (Wooltorton et al. 2003) has shownthat ${alpha}$ 7-containing nAChRs are among the least likely of nAChRsto desensitize at lower concentrations of agonist, and becausewe placed our U-tube 2–3 mm from the recorded neuron,there was a substantial dilution (estimated at 3- to 4-fold)of agonist before it reached the receptor sites. The same persistenceof nicotinic agonist effect and ${alpha}$ -BgTx sensitivity was previouslyobserved for the nAChRs mediating enhanced spontaneous releaseof glutamate in the LGNv by exogenous nicotinic agonists (Guoet al. 1998). In contrast, presynaptic nAChRs mediating enhancedGABA release in the LGNv exhibited a very different pharmacology,including insensitivity to ${alpha}$ -BgTx (Guo and Chiappinelli 2002).

The ${alpha}$ 6 and ${beta}$ 3 nAChR subunits are not widely distributed in neuronaltissue, but both are expressed in the retina of chick and mice(Champtiaux et al. 2002; Vailati et al. 1999, 2000). In thechick, two nAChR subtypes containing ${beta}$ 3 subunits have been immunopurifiedand pharmacologically characterized, one of which also containsat least one ${alpha}$ 6 subunit (Vailati et al. 2000). These nAChR subtypesdo not appear to be major subtypes involved in the present enhancementof glutamatergic evoked responses by exogenous agonists in theLGNv, because they are not sensitive to blockade by ${alpha}$ -BgTx. Furthermore,immunoprecipitation experiments using anti- ${beta}$ 3 antibodies failedto precipitate any ${alpha}$ -BgTx–binding nAChRs in chick brainhomogenates (Vailati et al. 2000), indicating that the receptorsmediating enhanced glutamate release by exogenous agonists inthis study are unlikely to contain ${beta}$ 3 subunits.

The somata of chick retinal ganglion neurons express both ${alpha}$ 8and ${alpha}$ 7 subunits (Keyser et al. 1993). At least three subtypesof ${alpha}$ -BgT–sensitive nAChRs are present in the chick retina,including ${alpha}$ 8*, ${alpha}$ 7 ${alpha}$ 8*, and ${alpha}$ 7*, and there is biochemical evidencethat these receptors contain additional subunits (Gotti et al.1997). After unilateral retinal lesions in the chick, thereis a decrease in the intensity (from intense to moderate) ofneuropil staining for ${alpha}$ 8-like immunoreactivity in the contralateralLGNv, whereas ${alpha}$ 7-like immunoreactivity remains unchanged at intense(Britto et al. 1994), suggesting that nAChRs containing the ${alpha}$ 8 subunit are present on retinal ganglion terminals in the LGNv. ${beta}$ 2-like immunoreactivity decreased even more substantially afterretinal lesion, indicating that some nAChRs located on retinalganglion terminals are likely to contain this subunit. Chick(and rat) ${alpha}$ 7 and ${beta}$ 2 subunits can combine to form functional receptors(Girod et al. 1999; Khiroug et al. 2002), so that combinationsof the ${beta}$ 2 subunit with either ${alpha}$ 7 or ${alpha}$ 8 (or both) might occur inthe retinal ganglion terminals within the LGNv. Because theheteromeric ${alpha}$ 7/ ${beta}$ 2* receptor desensitizes significantly slowerthan the homomeric ${alpha}$ 7 receptor (Khiroug et al. 2002), such acombination could contribute to the prolonged nature of thenicotinic response seen in this study in the LGNv. Slowly desensitizing ${alpha}$ 7* receptors have also been described in rat intracardiac ganglia(Cuevas and Berg 1998). The ${alpha}$ 7* responses observed here are alsodistinguished by a faster recovery during washout of ${alpha}$ -BgT thanis observed for mammalian ${alpha}$ 7* receptors, with substantial recoveryof responses observed after 10–15 min of washing out ${alpha}$ -BgT.

Electrical stimulation in the lateral LGNv (conditioning stimulation)produced marked enhancement of optic tract–evoked glutamatergictransmission in LGNv neurons. The potentiation was dependenton the intensity and number of conditioning pulses. A singleconditioning train at higher intensity could elicit potentiationof optic tract-LGNv neuron–evoked glutamatergic transmissionfor >500 ms. The glutamatergic enhancement after conditioningstimulation was nicotinic in nature, because it was completelyblocked by 100 nM ${alpha}$ -CTx MII and 100 nM DH ${beta}$ E. The conditioningresponse was most likely caused by the release of endogenousACh from cholinergic fibers after electrical stimulation throughthe conditioning electrode. The nAChRs mediating this responseto endogenously released ACh were clearly distinct from thereceptors mediating the enhancement because of exogenously appliednicotinic agonists. The blockade by low concentrations of ${alpha}$ -CTxMII and DH ${beta}$ E, the lack of sensitivity to ${alpha}$ -BgTx, and the requirementfor relatively high concentrations of MLA to produce a completeblock (1.0 µM) all make it unlikely that ${alpha}$ 7* or ${alpha}$ 8* receptorsare the major nAChR subtypes mediating the conditioning response.Instead, the response to endogenously released ACh seems tobe mediated primarily by presynaptic ${alpha}$ 6- and/or ${alpha}$ 3-containingnAChRs based on pharmacological properties (Mogg et al. 2002;Salminen et al. 2004). Immunoimmobilized chick ${alpha}$ 6* receptorsexhibited the following K_is against ³H-epibatidine binding: ${alpha}$ -CTx MII, 66 nM; MLA, 1.35 µM, DH ${beta}$ E, 2.8 µM (Vailatiet al. 1999). In comparison, the concentrations required tocompletely block the functional response to conditioning stimulationin this study were as follows: ${alpha}$ -CTx MII, 100 nM; MLA, 1.0 µM,DH ${beta}$ E, 0.1 µM. It is known that the ${alpha}$ 6-containing receptorsin retinal ganglion cells are heterogeneous, and many also contain ${alpha}$ 3 and/or ${beta}$ 3 subunits (Vailati et al. 1999, 2000, 2003). In bothchick and rodent, these ${alpha}$ 6* receptors migrate down the opticnerve and tract and are present in the optic lobe and LGNv (Champtiauxet al. 2002; Vailati et al. 1999). Thus the most parsimoniousexplanation for the enhancement of glutamatergic transmissionobserved in this study after conditioned stimulation is thatACh released from cholinergic fibers activates ${alpha}$ 6* and/or ${alpha}$ 3*( ${alpha}$ 6*/ ${alpha}$ 3*) nAChRs located on retinal ganglion nerve terminals,causing enhanced glutamate release. It is not yet clear whyexogenous nicotinic agonists enhance glutamatergic transmissionin the LGNv primarily by activating ${alpha}$ 7*/ ${alpha}$ 8* receptors, whereasendogenous ACh acts mainly on ${alpha}$ 6*/ ${alpha}$ 3* receptors. One possibilityis that the ${alpha}$ 6*/ ${alpha}$ 3* receptors are located preferentially at cholinergicsynapses, whereas the ${alpha}$ 7*/ ${alpha}$ 8* receptors are primarily extrasynaptic.Exogenous ACh would readily activate all extrasynaptic ${alpha}$ 7*/ ${alpha}$ 8*receptors but would have more limited access to the likely smallernumber of synaptic ${alpha}$ 6*/ ${alpha}$ 3* receptors, whereas endogenously releasedACh would have ready access to ${alpha}$ 6*/ ${alpha}$ 3* receptors but would notbe released nearby ${alpha}$ 7*/ ${alpha}$ 8* receptors. Such segregation of nAChRsubtypes at cholinergic synapses has been described in chickciliary ganglia neurons, where ${alpha}$ 3* nAChRs are preferentiallylocated at synapses, whereas ${alpha}$ 7* receptors are excluded fromthe synapses but are present in extrasynaptic locations (Shoopet al. 1999). The ${alpha}$ 3 subunit shares substantial sequence homologywith the ${alpha}$ 6 subunit (Champtiaux et al. 2002), and it is has beenshown to be critical in targeting nAChRs to synapses in theciliary ganglion (Temburni et al. 2000).

Nicotinic modulation of glutamatergic transmission in the LGNvmay play an important physiological role. The LGNv communicatesbetween the thalamofugal and tectofugal visual pathways, thetwo primary and parallel visual pathways in birds as well asreptiles and mammals (Shimizu and Karten 1993). In additionto the optic tract fibers, the LGNv receives afferents fromthe visual wulst, the homolog of the visual cortex and partof the thalamofugal system, and fibers from the optic tectum,the homolog of the superior colliculus and part of the tectofugalsystem (Crossland and Uchwat 1979; Ehrlich et al. 1989). TheLGNv has been reported to send projections to the optic tectumand the area pretectalis and lesioning studies support a rolefor the LGNv in communicating between the thalamofugal and tectofugalpathways (Hodos et al. 1982; Reiner et al. 1982). Our electrophysiologicalrecordings were from projection neurons in the lamina interna,and these neurons appear to function as color-opponent unitsin the bird (Maturana and Varela 1982). In our reconstructionsof these neurons, the main axon seen traveling medial to thenu. rotundus is likely on its way to the area pretectalis. Themain axons also had collaterals, some of which were localizedto the area between the nu. rotundus and the LGNv, the nucleusmarginalis tractus optici. These axon collaterals may be involvedin modulating the activity of the optic tectum through neuropeptideY-expressing marginalis tractus optici neurons that also sendefferents to the optic tectum (Gunturkun and Karten 1991). Thedendrites of the visualized neurons descend into the neuropilwhere optic tract fibers terminate (Crossland and Uchwat 1979).The interconnections of the LGNv with the optic fibers and thethalamofugal and tectofugal visual systems suggest that nicotinicmodulation of the LGNv may have important effects on the regulationof the visual processing system as a whole.

In humans, a functional MRI (fMRI) study has shown that nicotinecan markedly enhance activation in human brain areas involvedin visual attention, including the thalamus and posterior cortex,during a rapid visual information-processing task that testsboth vigilance and working memory (Lawrence et al. 2002). Consistentwith this neuronal activation of visual centers by nicotinein humans, we found that nicotine can markedly enhance excitatorytransmission through the chick LGNv at a concentration thatcan be attained after cigarette smoking in humans (500 nM; Henningfieldet al. 1993). In another fMRI study in humans, attention toa task was shown to substantially enhance neural responses toattended stimuli in the thalamic LGN, leading the authors topropose that the LGN acts as a "gatekeeper" in regulating attentionalgain control (O'Conner et al. 2002). Our finding that endogenouslyreleased ACh acts on nicotinic receptors to significantly increaseexcitatory transmission through the chick LGNv provides a mechanismwhereby cholinergic fibers and nicotinic receptors could serveto modulate attentional signaling through the LGNv.

Nicotinic receptors have now been shown to play functional rolesat three separate levels of the visual nervous system. In thevisual cortex, fast evoked nicotinic transmission occurs beforeand during innervation by thalamic afferents (Roerig et al.1997). In the retina, activation of nAChRs initiates spontaneousbursts of wave-like activity during development, and in ${beta}$ 2-nullmice, the normal pattern of innervation of the LGN by retinalganglion cells is disrupted (Rossi et al. 2001). This studyshows for the first time that activation of presynaptic nAChRseither by endogenously released ACh or exogenously applied nicotine,choline, or ACh markedly potentiates neurotransmission at glutamatergicsynapses formed by retinal ganglion cell terminals and LGNvneurons.

GRANTS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

This work was supported by National Institute of NeurologicalDisorders and Stroke Grant NS-17574 to V. A. Chiappinelli andThe Ralph E. Loewy Professor Endowment.

ACKNOWLEDGMENTS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

We thank C. Kang for participation in preliminary experimentsand Dr. J. Michael McIntosh for providing the ${alpha}$ -conotoxins usedin this study.

FOOTNOTES

The costs of publication of this article were defrayed in partby the payment of page charges. The article must therefore behereby marked "advertisement" in accordance with 18 U.S.C. Section1734 solely to indicate this fact.

Address for reprint requests and other correspondence: J.-Z. Guo, Dept. of Pharmacology and Physiology, George Washington Univ., School of Medicine and Health Sciences, Suite 640, 2300 Eye St. NW, Washington, DC 20037 (E-mail: phmjzg{at}gwumc.edu)

REFERENCES

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METHODS
RESULTS
DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

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