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NEUROSCIENCE |
1 Unité Récepteurs et Cognition, CNRS URA 2182, Institut Pasteur, 25–28 Rue du Docteur Roux, 75724 Paris Cedex 15, France
2 Neurobiology Department, International School for Advanced Studies, Via Beirut 2–4, 34014 Trieste, Italy
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Abstract |
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7 and ß2-containing (7* and ß2*) nAChRs to nicotine-elicited modulation of GABAergic and glutamatergic activity at the network and single-cell level in the immature hippocampus of wild-type (WT), 7–/– and ß2–/– mice. We found that 7* and ß2* nAChRs were sufficient to modulate nicotine-induced increase in frequency of spontaneously occurring giant depolarizing potentials (GDPs), which are generated at the network level by the synergistic action of glutamate and depolarizing GABA, and thought to play a crucial role in neuronal wiring. However, 7* but not ß2* receptors were essential in nicotine-induced increase of interictal discharge frequency recorded after postnatal day 3 in the presence of bicuculline, when GABA shifted from the depolarizing to the hyperpolarizing direction. To correlate these observations with nicotine-elicited changes in synaptic transmission, we recorded spontaneous GABAergic and glutamatergic postsynaptic currents in pyramidal cells and interneurons localized in stratum oriens, stratum pyramidale and stratum radiatum, in slices obtained from WT and knock-out animals. We found that early in postnatal life 7* and ß2* nAChRs exert a fine regional modulation of GABAergic and glutamatergic transmission that underlies nicotine-elicited changes in network synchronization.
(Received 21 July 2006;
accepted after revision 7 August 2006;
first published online 10 August 2006)
Corresponding author E. Cherubini: Neurobiology Department, International School for Advanced Studies, Via Beirut 2–4, 34014 Trieste, Italy. Email: cher{at}sissa.it
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Introduction |
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TopAbstractIntroductionMethodsResultsDiscussionReferences |
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The hippocampus, a key structure in learning and memory processes, receives a large cholinergic innervation (Kasa, 1986) and is endowed with a variety of nAChRs (Alkondon & Albuquerque, 2004), which increase the release of several neurotransmitters and modulate synaptic plasticity processes (McGehee, 2002). Of the four classes of nAChRs described in the central nervous system (Zoli et al. 1998), the main receptor subtypes present in the hippocampus are the homomeric 7 and the heteromeric 4ß2-containing receptors (Alkondon & Albuquerque, 2004). Interestingly, in the rat hippocampus during the first postnatal week, 7 nAChR mRNA and bungarotoxin binding sites have been shown to be expressed at high levels (Adams et al. 2002; Tribollet et al. 2004), suggesting that 7 may have a role in the development of the immature hippocampus. Moreover, several studies have demonstrated that perinatal exposure to nicotine in rodents and humans impairs cognitive functions, supporting the idea that an excessive activation of nAChRs by nicotine during brain maturation interferes with the development of brain areas involved in learning and memory (Johns et al. 1982; Levin et al. 1993; Ernst et al. 2001; Linnet et al. 2003). However, the molecular and cellular mechanisms underlying these processes remain largely unknown. In a previous study, nicotine was shown to increase the frequency of synchronous network-driven membrane oscillations present in the hippocampus at early postnatal stages of development, and called ‘giant depolarizing potentials’ (GDPs; Maggi et al. 2001). GDPs are characterized by recurrent membrane depolarization with superimposed fast action potentials. They are generated spontaneously by the synergistic action of glutamate and GABA and, in the perinatal period, this exerts a depolarizing and excitatory action (Ben Ari et al. 1989; Cherubini et al. 1991; Sipila et al. 2005). GDPs are reminiscent of correlated network activity observed in the retina (Wong et al. 1995), the spinal cord (Gu et al. 1994) and the neocortex (Garaschuk et al. 2000) during development, thought to contribute to circuit wiring (Ben Ari, 2002).
In the present study, the whole-cell patch-clamp technique was used to assess the contribution of 7-containing (7*) and ß2-containing (ß2*) nAChRs to nicotine-elicited modulation of network and synaptic activity in immature hippocampal slices obtained from wild-type (WT) mice and mice lacking the gene coding for the 7 or the ß2 subunits of nAChRs. In WT, 7 and ß2 knock-out (KO) mice, nicotine increased the frequency of GDPs. Moreover, in ß2 KO, but not in 7 KO mice, in the absence of GABAA-mediated synaptic transmission, nicotine potentiated interictal-like discharges (Wong et al. 1986), indicating a different regulation of GABAergic and glutamatergic signalling by ß2* and 7* nAChRs. To investigate the changes in synaptic activity underpinning these findings, we studied the effect of nicotine on GABAergic and glutamatergic spontaneous synaptic transmission in pyramidal cells and interneurons of the stratum oriens, stratum pyramidale and stratum radiatum, in neonatal WT and KO mice.
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Methods |
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TopAbstractIntroductionMethodsResultsDiscussionReferences |
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Transverse hippocampal slices (400 µm thick) were prepared from mice that were 2–10 postnatal days old (P2–P10), using a method previously described (Maggi et al. 2003). In Italy, the procedure was in accordance with the regulations of the Italian Animal Welfare Act, and was approved by the local authority veterinary service. In France, the procedure was in accordance with the Centre National de la Recherche Scientifique guidelines for care and use of laboratory animals. Briefly, animals were decapitated and the brain was quickly removed from the skull, then sectioned with a vibratome (DTK 1000; DSK, Kyoto, Japan) using ice-cold artificial cerebrospinal fluid (ACSF) containing (mM): NaCl 130, KCl 3.5, NaH2PO4 1.2, NaHCO3 25, MgCl2 1.3, CaCl2 2, and glucose 11, saturated with 95% O2 and 5% CO2 (pH 7.3–7.4). After 1 h, an individual slice was transferred to the recording chamber where it was continuously superfused with oxygenated ACSF at a rate of 2–3 ml min–1.
KO animals
The generation of ß2–/– and 7–/– mice has been previously described (Picciotto et al. 1995; Orr-Urtreger et al. 1997). KO and matching WT colonies were bred separately. For each colony, at least four couples of homozygous breeders were produced by mating heterozygous mice, obtained after 10–12 (7) or 12–19 (ß2) backcrosses with C57Bl/6J mice. For control experiments, WT C57Bl/6J, 7+/+ and ß2+/+ mice were used. Animal care was in line with institutional guidelines.
Electrophysiology
Neurons were visually identified using an upright microscope and infrared differential interference contrast videomicroscopy (Axioskop; Zeiss, Oberkochen, Germany). CA1 pyramidal neurons were voltage clamped at –70 mV using the whole-cell configuration of the patch-clamp technique. Series resistance was compensated (60–80%) and checked regularly during the experiment. Cells exhibiting more than 20% changes were excluded from the analysis.
Patch electrodes, formed from thin borosilicate glass (Hilgenberg, Malsfeld, Germany) had a resistance of 3–6 M
. Network and synaptic activity were recorded with an intracellular solution containing (mM): KCl 140, Hepes 10, EGTA 1, MgCl2 1, MgATP 4 and NaGTP 0.3. The pH was adjusted to 7.25 with CsOH or KOH, and the osmolarity was 280–290 mosmol l–1.
Spontaneous amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid (AMPA)/kainate (KA) receptor-mediated excitatory postsynaptic currents (EPSCs) were routinely recorded from CA1 principal cells and interneurons at a holding potential of –60 mV in the presence of bicuculline (10 µM) to block GABAA receptors.
Spontaneous 
aminobutyric acid (GABA)A-mediated postsynaptic currents (PSCs) were routinely recorded from CA1 principal cells and interneurons at a holding potential of –60 mV in the presence of DNQX (20 µM) to block AMPA/KA-mediated responses.
Drugs were applied to the bath via a three-way tap system. Drugs used were: tetrodotoxin (TTX), purchased from Latoxan, Valence, France; bicuculline methiodide and 6,7-dinitroquinoxaline-2,3-dione (DNQX), from Tocris, Bristol, UK; nicotine, methyllycaconitine (MLA) and dihydro-ß-erythroidine (DHßE), purchased from Sigma, Milan, Italy. Membrane potentials were corrected for liquid junction potential. Experiments were performed at 32–33°C.
Data acquisition and analysis
Data were acquired using pCLAMP 9 software (Axon Instruments, Union City, CA, USA) and currents recorded using an Axopatch 1D amplifier and a Multiclamp 700A amplifier (Axon Instruments). Current signals were transferred to a computer after digitization with an A/D converter (Digidata 1200 and Digidata 1322; Axon Instruments). Data were sampled at 10 kHz, and filtered with a cut-off frequency of 2 kHz.
Spontaneous EPSCs, GABAA-mediated PSCs, GDPs and interictal bursts were analysed off-line with Clampfit 9 software (Axon Instruments).
The rise time of GDPs and interictal discharges was estimated as the time needed for a 10–90% increase of the peak current responses regardless of unclamped action potentials riding on the top.
To examine whether nicotine affected the frequency of EPSCs/GABAA-mediated PSCs/GDPs/interictal bursts, firstly the mean frequency of all events occurring in 6–10 min pre-drug control periods was calculated. Then, synaptic and network events recorded during or after drug application (3 min for EPSCs/GABAA-mediated PSCs and 5 min for GDPs/interictal bursts, starting 2 min after the onset of drug application) were normalized to control values and expressed as percentage changes (see figures).
Interneurons localized in stratum pyramidale were distinguished from pyramidal cells on the basis of their different morphology (rounded soma for interneurons, spindle-shaped for pyramidal cells), and their different firing patterns in response to a steady depolarizing current applied from –60 mV. Pyramidal neurons were characterized by a slow ramp potential before firing initiation, marked spike-frequency accommodation, and small single-spike after-hyperpolarizations (AHPs) in response to depolarizing current steps. In contrast, stratum pyramidale interneurons showed rapid firing initiation, minor spike-frequency accommodation, and big single-spike AHPs.
Data are expressed as means ± S.E.M. Statistical comparisons were made using Student's two-tailed t test. The Kolmogorov-Smirnov test was applied to compare distributions. P < 0.05 was taken as significant.
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Results |
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TopAbstractIntroductionMethodsResultsDiscussionReferences |
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7* and ß2* nAChRsIn the present study, GDPs were recorded in voltage-clamped CA1 hippocampal neurons in slices obtained from P2–P10 WT mice (n = 30). GDPs were characterized by slow inward currents giving rise to high-frequency unclamped spikes (see insets of Fig. 1A and B). As illustrated in the summary graph of Fig. 1B, while GDP frequency remained constant between P2 and P4, and P5 and P7 (0.68 ± 0.16 and 0.92 ± 0.10 min–1, respectively; P > 0.05), it sharply decreased from P8 onwards (0.11 ± 0.06 at P8–P10; P < 0.05 compared with P2–P7). GDPs were rarely observed after P9. Application of the GABAA receptor antagonist bicuculline (10 µM) blocked GDPs and induced interictal discharges whose frequency significantly increased with age. GDPs were also blocked by the AMPA/KA receptor antagonist DNQX (20 µM) (not shown), indicating that GABAergic and glutamatergic neurons both contribute to their generation (Ben Ari et al. 1989). In comparison with GDPs, interictal discharges were not observed at any time before P3, despite the prolonged exposure of slices to bicuculline (10–15 min, see Khazipov et al. 2004), and were characterized by a faster rising phase (47 ± 5 ms for interictal discharges, n = 13, versus 153 ± 14 ms for GDPs, n = 12 cells, see Methods). They were blocked by DNQX (20 µM), suggesting that they were mediated by AMPA/KA ionotropic glutamate receptors (n = 3, not shown). They were generated in the CA3 area, since cutting the slices between the CA3 and CA1 regions prevented the propagation of discharges (n = 3, not shown; see Wong & Traub, 1983). After P3, the frequency of bicuculline-elicited interictal discharges increased significantly (from 0.50 ± 0.24 min–1 at P2–P4, to 1.49 ± 0.36 min–1 at P8–P10; P < 0.05; Fig. 1). The age-dependent reduction in the frequency of GDPs and increase in the frequency of interictal discharges between P3 and P7 (Fig. 1B) can be attributed to the gradual increase in the expression of KCC2 (Rivera et al. 1999), followed by the progressive shift of GABA from the depolarizing to the hyperpolarizing direction.
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7* nAChRs (230 ± 20% change in the presence of MLA; n
= 6, P < 0.05) or DHßE 1 µM, a selective antagonist of ß2* nAChRs (292 ± 85% change in the presence of DHßE; n
= 7, P < 0.05). In the presence of both MLA and DHßE, nicotine did not elicit any significant increase (120 ± 30% change; n
= 6, P > 0.05; Fig. 2).
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7-subunit gene. In 7–/– mice, nicotine caused a 309 ± 47% increase in the frequency of GDPs (from 0.83 ± 0.16 min–1; n
= 7, P < 0.05), an effect that disappeared when slices were first treated with DHßE (1 µM). In this case, GDP frequency remained unchanged (127 ± 29% change; n
= 9, P > 0.05). In ß2–/– mice, nicotine elicited a 292 ± 66% increase in frequency (from 0.84 ± 0.20 min–1; n
= 8, P < 0.05), which was blocked by 10 nM MLA (112 ± 20% change; n
= 10, P > 0.05). These results suggest that 7* and ß2* nAChRs can independently increase GDP frequency (Fig. 2).
Nicotine did not modify the shape or charge transfer associated with GDPs: the charge transfer measured before and after nicotine application was 60.4 ± 10.3 and 63.8 ± 13.6 pA s in WT mice (P > 0.05, n
= 12), 61.9 ± 21.8 and 63.2 ± 19.9 pA s in 7–/– mice (P > 0.05, n
= 7), 46.1 ± 8.1 and 50.7 ± 11.1 pA s in ß2–/– mice (P > 0.05, n
= 8). Moreover, nicotine (1 µM) did not change the membrane potential or the input conductance of the recorded neurons.
Nicotine increases the frequency of interictal discharges via 7* but not ß2* nAChRs
Figure 3 presents the effect of nicotine on interictal discharges caused by bicuculline in WT, 7–/– and ß2–/– mice at P5–P9. Nicotine (1 µM) reversibly increased the frequency of interictal discharges in WT mice (271 ± 46% of control, from 1.08 ± 0.17 min–1 in control; n
= 13, P < 0.01), an effect that was prevented by MLA 10 nM (111 ± 11% of control; n
= 3). Nicotine did not affect the frequency of interictal bursts in slices from 7–/– (103 ± 14% change, from 1.38 ± 0.29 min–1; n
= 11, P > 0.05), but increased interictal burst frequency in ß2–/– mice (247 ± 54% of control, from 1.02 ± 0.15 min–1; n
= 8, P < 0.01). However, in slices from ß2–/– mice preincubated in MLA, the frequency of interictal bursts was unaltered (106 ± 11% change; n
= 6, P > 0.05). These results demonstrate that 7* nAChRs mediate nicotine-elicited change in interictal burst frequency.
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7–/– mice (n
= 11, P > 0.05). As in the case of GDPs, nicotine did not change the membrane potential or the input conductance of the recorded cells.
To correlate these results with nicotine-elicited changes in early postnatal synaptic transmission in the hippocampus, the effects of nicotine were studied on spontaneous GABAergic and glutamatergic signalling in pyramidal cells and interneurons localized in stratum oriens, stratum pyramidale and stratum radiatum from WT, 7–/– and ß2–/– mice between P4 and P8.
Nicotine transiently increases the frequency of miniature glutamatergic PSCs in pyramidal cells from WT and ß2–/– mice, but not those from 7–/– mice
The lack of nicotine-elicited increases in interictal discharges in 7–/– mice and in ß2–/– mice in the presence of MLA suggests that 7 but not ß2-containing nAChRs are crucial for increasing the frequency of epileptiform bursts observed in the absence of GABAA-mediated inhibition. This may be triggered at the level of recurrent collaterals between principal cells in the CA3 area and propagate to the CA1 region via Schaffer collaterals, which originate from the same axon as recurrent collaterals (Miles & Wong, 1987). Moreover, we have previously shown that activation of presynaptic 7* nAChRs enhance glutamatergic transmission in the immature rat hippocampus (Maggi et al. 2003). Other studies have shown that in the adult rat, nicotine increases the frequency of miniature excitatory postsynaptic currents (mEPSCs) recorded from CA1 and CA3 pyramidal cells in the presence of TTX (1 µM) (Gray et al. 1996). Here, the effect of nicotine was tested on mEPSCs recorded from CA1 pyramidal cells in the presence of TTX (1 µM) and bicuculline (10 µM). mEPSCs were mediated by AMPA/KA receptors since they were blocked by the selective AMPA/KA receptor antagonist DNQX (20 µM, n
= 2, not shown). In six neurons nicotine (1 µM for 3 min) enhanced the frequency of mEPSCs by 360 ± 62% (from 0.31 ± 0.11 Hz in control conditions; P < 0.05, Fig. 4) in the absence of any change in their amplitude (12.05 ± 2.83 and 9.82 ± 1.45 pA before and after nicotine application, respectively). A nicotine-elicited increase in frequency of mEPSCs was prevented by MLA 10 nM (102 ± 3% change in the presence of MLA, n
= 5) and was not associated with changes in holding current or in membrane input conductance. The increase in mEPSC frequency was transient, and reversed to control values a few minutes after nicotine was washed out. Similar effects were produced when nicotine was applied to CA1 pyramidal neurons in slices obtained from ß2–/– mice (n
= 6). Also in this case, nicotine produced a transient increase in the frequency of miniature events by 389 ± 62% (from 0.32 ± 0.08 Hz; P < 0.05), which was blocked by preincubation of the slices with MLA (96 ± 12% of control, n
= 5). No change in the amplitude of miniature events was observed before and after nicotine application (10.05 ± 1.74 and 9.81 ± 1.58 pA in the absence and presence of nicotine, respectively).
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7–/– mice (n
= 8) was unaffected by nicotine (113 ± 31% of control, from 0.40 ± 0.19 Hz; P > 0.05). As in WT and ß2–/– mice, the amplitude of mEPSCs was unaltered by nicotine (the mean amplitude values of mEPSCs recorded before and during nicotine application were 9.67 ± 0.57 and 9.32 ± 0.59 pA, respectively).
In pyramidal cells from WT and ß2–/– mice, but not those from 7–/– mice, nicotine increases the frequency of spontaneous GABAA-mediated PSCs
GABAergic neurons in various brain structures have been shown to express presynaptic, preterminal axonal (Lena et al. 1993) or somato-dendritic nAChRs (Frazier et al. 1998). To discriminate between presynaptic (action-potential independent) or preterminal receptors (action-potential dependent, either axonal or somato-dendritic), the frequency of spontaneous GABAA-mediated PSCs in pyramidal cells was studied in the presence and absence of TTX. These PSCs were mediated by GABAA receptors since they were blocked by bicuculline (10 µM, n = 6, not shown).
In the presence of DNQX, nicotine (1 µM for 3 min) increased the frequency of spontaneous GABAergic PSCs in WT mice (150 ± 12% of control; from 2.86 ± 0.31 Hz during control; n
= 5, P < 0.05; Fig. 5). This effect was prevented by MLA 10 nM (109 ± 13% of control; n
= 13). Similar results were obtained in ß2–/– mice (154 ± 10% of control; from 1.78 ± 0.33 Hz during control; n
= 5, P < 0.05). The effect of nicotine in ß2–/– mice was blocked by MLA or TTX (95 ± 13% change, n
= 5, and 103 ± 4% change, n
= 5, respectively; P > 0.05), suggesting that preterminal 7* receptors were involved. Consistent with these results, in 7–/– mice, spontaneous GABA release onto pyramidal cells was not affected by nicotine (nicotine-elicited change in PSC frequency: 95 ± 5% of control, from 4.20 ± 0.54 Hz; n
= 9, P > 0.05).
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7–/– mice (n
= 9, P > 0.05), 19.36 ± 2.65 pA before and 19.91 ± 2.96 pA after nicotine in ß2–/– mice (n
= 9, P > 0.05). Nicotine does not affect the frequency of spontaneous glutamatergic PSCs in interneurons from WT or KO mice
In contrast with pyramidal cells, nicotine (1 µM for 3 min) did not modify the frequency of spontaneous EPSCs recorded in the presence of bicuculline from stratum oriens, stratum pyramidale and stratum radiatum interneurons (in slices obtained from WT, 7–/– and ß2–/– mice of the same age; data not shown). In stratum oriens interneurons, the frequency of spontaneous EPSCs in the presence of nicotine was 100 ± 2, 106 ± 4 and 117 ± 11% of control in WT, 7–/– mice and ß2–/– mice, respectively (average frequencies during control: 1.04 ± 0.12 Hz, n
= 5, 0.98 ± 0.08 Hz, n
= 7, 1.11 ± 0.59 Hz, n
= 5, respectively; P > 0.05). In stratum pyramidale interneurons, this frequency was 112 ± 8, 103 ± 1 and 102 ± 1% of control in WT, 7–/– mice and ß2–/– mice, respectively (average frequencies in control: 0.99 ± 0.41 Hz, n
= 5, 1.05 ± 0.08 Hz, n
= 5, 0.83 ± 0.09 Hz, n
= 7, respectively; P > 0.05). In stratum radiatum interneurons, the frequency was 103 ± 19, 111 ± 7 and 102 ± 1% of control in WT, 7–/– mice and ß2–/– mice, respectively (average frequencies during control: 0.78 ± 0.23 Hz, n
= 6, 0.96 ± 0.10 Hz, n
= 11, 0.76 ± 0.04 Hz, n
= 5, respectively; P > 0.05).
Moreover, in stratum oriens, stratum pyramidale and stratum radiatum interneurons, nicotine did not modify the amplitude of the EPSCs in WT mice (from 9.00 ± 0.53 pA, n
= 5, 7.94 ± 1.45 pA, n
= 6, and 7.87 ± 1.32 pA, n
= 6, during control, to 8.44 ± 0.92, 7.77 ± 1.21 and 8.14 ± 0.83 pA after nicotine, respectively; P > 0.05), 7–/– mice (from 9.74 ± 0.78 pA, n
= 7, 8.14 ± 0.83 pA, n
= 5, and 13.14 ± 2.43 pA, n
= 5, during control, to 9.42 ± 1.00, 8.97 ± 0.67 and 12.57 ± 0.82 pA after nicotine, respectively; P > 0.05) and ß2–/– mice (from 10.28 ± 1.54, 11.01 ± 1.81 and 12.02 ± 1.41 pA during control to 9.49 ± 1.59, 10.30 ± 1.58 and 12.10 ± 1.45 pA after nicotine, respectively; P > 0.05).
Nicotine affects the frequency of spontaneous GABAergic PSCs differently in interneurons from WT and KO mice
The effect of nicotine on spontaneous GABAergic PSCs (recorded in the presence of DNQX, 20 µM) was compared in interneurons from stratum oriens, stratum pyramidale and stratum radiatum in both WT and KO mice. As shown in the graphs of Fig. 6, in WT mice, nicotine enhanced the frequency of spontaneous PSCs to 289 ± 74% (P < 0.05; n
= 6), to 186 ± 24% (P < 0.01; n
= 11) and to 167 ± 13% (P < 0.001; n
= 6) of controls in stratum oriens, stratum pyramidale and stratum radiatum, respectively. These effects were partially or completely antagonized by MLA 10 nM (207 ± 29% change after nicotine, n
= 5, P < 0.05, in stratum oriens; 153 ± 10%, n
= 5, P < 0.05, in stratum pyramidale; 120 ± 11%, n
= 5, P > 0.05 in stratum radiatum) and DHßE 1 µM (176 ± 22% change after nicotine, n
= 5, in stratum oriens; 157 ± 2%, n
= 6, in stratum pyramidale, P < 0.05), indicating that they were mediated by both 7* and ß2* nAChRs. Preincubating the slices with MLA and DHßE together prevented the effect of nicotine in the stratum oriens and stratum pyramidale (95 ± 6% change after nicotine, n
= 5, and 96 ± 3% change, n
= 4, respectively).
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7* receptors only (changes after nicotine: 105 ± 2%, n
= 5, 99 ± 1%, n
= 5, and 102 ± 2%, n
= 6, respectively). In 7–/– mice, nicotine significantly (P < 0.05) enhanced the frequency of PSCs recorded from stratum oriens and stratum pyramidale interneurons (to 225 ± 32%, n
= 6, and to 144 ± 10%, n
= 5, of controls), respectively, but had no effect on stratum radiatum interneurons (to 98 ± 5%; n
= 9, P > 0.05). The potentiating effects of nicotine on interneurons of stratum oriens and pyramidale were antagonized by DHßE 1 µM, indicating that they were mediated by ß2* nAChRs (to 100 ± 4%, n
= 6, and to 98 ± 7%, n
= 4, of controls, respectively).
Finally, the average amplitude of GABAA-mediated PSCs was not changed by the application of nicotine. In stratum oriens, stratum pyramidale, and stratum radiatum interneurons, the average amplitude of GABAergic PSCs was 26.68 ± 4.63 pA (n
= 6), 16.01 ± 2.57 pA (n
= 11) and 14.44 ± 1.64 pA (n
= 6) during control, and 33.90 ± 8.25, 16.35 ± 2.62 and 13.89 ± 1.97 pA after nicotine, respectively (P > 0.05). In 7–/– mice, it changed from 38.69 ± 6.64 pA (n
= 6), 54.50 ± 8.71 pA (n
= 5) and 54.86 ± 5.65 pA (n
= 9) during control, to 46.91 ± 6.66, 41.92 ± 7.31 and 56.56 ± 5.25 pA after nicotine, respectively (P > 0.05). Also in ß2–/– mice, nicotine did not change the average amplitude, from 24.73 ± 3.83 pA (n
= 6), 36.37 ± 10.55 pA (n
= 9), and 23.56 ± 2.88 pA (n
= 6) during control, to 27.58 ± 3.80, 36.09 ± 9.90 and 21.39 ± 2.85 pA after nicotine, respectively (P > 0.05).
Interestingly, nicotine did not modify the frequency of miniature GABAergic events recorded in the presence of TTX (1 µM) from interneurons localized in stratum oriens (to 110 ± 24%, n
= 5, and to 95 ± 2%, n
= 5, for 7–/– and ß2–/– mice, respectively; P > 0.05), in stratum pyramidale (to 99 ± 2%, n
= 5, and to 97 ± 2%, n
= 5, for 7–/– and ß2–/– mice, respectively; P > 0.05) of 7–/– and ß2–/– mice as well as in stratum radiatum of ß2–/– mice (to 108 ± 3%; n
= 6, P > 0.05; data not shown).
In summary, our results demonstrate that both preterminal 7* and ß2* nAChRs modulate GABA release onto stratum oriens and stratum pyramidale interneurons, and that only preterminal 7* receptors modulate GABA release onto stratum radiatum interneurons.
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Discussion |
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TopAbstractIntroductionMethodsResultsDiscussionReferences |
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7* and ß2* nAChRs, exerts a powerful regulatory action on network-driven oscillatory activity in the hippocampus. Moreover, the results demonstrate that in mice lacking the 7 nAChR subunit, nicotine fails to enhance interictal discharges obtained by blocking GABAA receptors with bicuculline. In agreement with these results, we found that nicotine-elicited regulation of glutamatergic signalling occurred via presynaptic 7* nAChRs, while nicotine-elicited modulation of GABAergic transmission needed the activation of both preterminal 7* and ß2* nAChRs. nAChRs contribute to GDP regulation
In a previous study from the neonatal rat hippocampus, it was reported that nicotine is able to increase the frequency of GDPs in a concentration-dependent manner. However, the nAChR subtypes involved in that effect were not identified (Maggi et al. 2001). In the present work, taking advantage of KO mice, we have clearly demonstrated that the potentiating effects of nicotine on GDPs are mediated by both 7 and ß2-containing receptors. While in 7–/– mice, the potentiating effect of nicotine on GDPs was prevented by a low concentration of DHßE, which selectively blocks ß2* nAChRs (Chavez-Noriega et al. 1997), in ß2–/– mice it was antagonized by MLA, which selectively blocks ß2* nAChRs. Since glutamatergic terminals projecting to pyramidal cells are controlled only by 7* nAChRs, in 7–/– mice the nicotine-elicited increase in GDP frequency could be attributed to (i) the enhancement of GABA release through the activation of ß2* nAChRs present on interneurons, or (ii) the enhancement of glutamate release through the activation of ß2* nAChRs present on glutamatergic nerve terminals innervating GABAergic interneurons. In both cases, the increased release of GABA would exert a powerful excitatory action on principal cells. However, it is likely that an increase of GABA release via the activation of ß2* nAChRs present on interneurons projecting onto stratum oriens and stratum pyramidale interneurons accounted for nicotine-induced potentiation of GDPs, since nicotine failed to affect glutamatergic activity in interneurons.
Nicotine-elicited GDP modulation seen in ß2–/– mice is mediated by 7* nAChRs, as assessed by its disappearance in the presence of MLA. Our results suggest that 7* nAChRs controlling GABA release onto stratum pyramidale, stratum oriens, stratum radiatum interneurons and pyramidal cells, as well as 7* nAChRs controlling glutamate release onto pyramidal cells, participate in this effect.
Regardless of the nAChRs involved in the potentiating effect of nicotine, the present experiments clearly indicate that, within the hippocampal network, different patterns are involved in the generation of GDPs and interictal discharges (Fig. 7A).
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7* but not ß2* nAChRs increases the frequency of interictal bursts elicited by removing GABAA-mediated inhibition with bicuculline
At high concentrations, nicotine is known to cause seizures (Miner et al. 1984; Damaj et al. 1999). Although the mechanisms underlying the convulsant effects of nicotine have not been fully elucidated, this issue is important in view of the observation that several nAChR subunits are candidate genes for idiopathic epilepsies (Gotti & Clementi, 2004). By comparing different strains of mice, a positive correlation has been found between the sensitivity to nicotine-elicited seizures and the number of bungarotoxin-binding sites in the hippocampus, indicating that 7* nAChRs are crucial for nicotine-elicited epileptiform discharges (Miner et al. 1984). Here we found that nicotine increased the frequency of interictal-like discharges caused by blocking GABAA receptors with bicuculline. In agreement with our results, it has recently been shown that nicotine increases epileptiform activity caused by bicuculline or DAP 4 in the hippocampus of adult rats (Roshan-Milani et al. 2003). However, unlike our results, nicotine-elicited increase in interictal bursts was dependent on the activation of both 7 and ß2-containing receptors. Although we can not exclude the involvement of ß2-containing receptors at late developmental stages, the observed differences can be attributed to the fact that, in order to block heteromeric nAChRs, Roshan-Milani et al. (2003) used high (10–30 µM) concentrations of DHßE, known to block not only ß2* but also 7* nAChRs (Bertrand et al. 1992). Therefore, it is likely that presynaptic 7* nAChRs localized on recurrent glutamatergic collaterals, thought to be critical for generating bursting activity (Miles & Wong, 1987), facilitate glutamate release leading to an increase in the frequency of interictal discharges. This is in agreement with the increased sensitivity to nicotine-elicited seizures of mice expressing a gain-of-function mutated form of the 7 receptor (Broide et al. 2002). However, experiments have shown that nicotine-elicited seizures do not disappear in 7–/– mice (Franceschini et al. 2002), and that 3 and ß4 nicotinic subunits, presumably located outside the hippocampus, are necessary for nicotine-elicited seizures (Salas et al. 2004). Moreover, mutations in the 4 and ß2 nicotinic subunits have been shown to cause autosomal dominant nocturnal front lobe epilepsy (Steinlein et al. 1995; De Fusco et al. 2000). These mutations may facilitate the synchronization of spontaneous oscillations in thalamocortical circuits (Raggenbass & Bertrand, 2002). So far, a role of 7* nAChRs in human epilepsies remains elusive.
Our data suggest that, in mice, hippocampal presynaptic 7* nAChRs enhance glutamatergic activity and contribute to the modulation of bicuculline-induced interictal discharges during postnatal development (Fig. 7B).
Nicotine regulates glutamate release onto pyramidal cells via presynaptic 7* nAChRs
Although collaterals of the same axons may have different functional properties according to the targets they innervate (Scanziani et al. 1998), nicotine-elicited enhancement of glutamatergic transmission at Schaffer collateral–CA1 synapses was mediated, as in recurrent collaterals, by presynaptic 7* nAChRs, as suggested by the loss of this effect in 7–/– mice.
7* nAChRs have been shown to be expressed on glutamatergic nerve terminals (Gray et al. 1996), on the soma of GABAergic interneurons (Alkondon et al. 1998) and on the dendrites of CA1 pyramidal cells (Ji et al. 2001; but see Khiroug et al. 2003). The present experiments were routinely performed in the presence of bicuculline, and therefore an indirect effect of nicotine via 7* nAChRs located on GABAergic interneurons could not have been detected. The possibility of a direct effect on the dendrites of CA1 principal cells is unlikely since we failed to detect any change in holding current or input conductance during nicotine application, suggesting that, if present, 7* receptors should be expressed at very low density on dendrites.
Nicotine does not affect the release of glutamate onto GABAergic interneurons
In contrast with the present data, previous results have demonstrated that nicotine can activate presynaptic/preterminal 3ß4* receptors and increase the frequency of spontaneous EPSCs in stratum radiatum interneurons of juvenile rats (Alkondon & Albuquerque, 2002). This apparent discrepancy could be attributed to the different expression of 3ß4* receptors in rats and mice or to the different experimental conditions used (neonatal versus juvenile animals). However, we cannot exclude the possibility that the concentration of nicotine (1 µM) used in the present study was too low to produce a statistically significant effect through 3ß4* receptors, since the EC50 of nicotine for 3ß4* receptors varies between 28 and 80 µM for rat and human receptors heterologously expressed (Chavez-Noriega et al. 1997; Xiao et al. 1998). Numerous studies, including the present one, have reported an effect of nicotine at low concentration mediated by presynaptic or preterminal 7* nAChRs, although the EC50 for mouse 7* nAChRs is also in the same order as for 3ß4* receptors (38 ± 5 µM for mouse 7* nAChRs, Macor et al. 2001). This may be due to the fact that 7* receptors undergo fast concentration-dependent desensitization, whereas 3ß4* receptors do not: as a consequence of the preferential desensitization of fully liganded 7* nAChRs, channels are open only within a limited concentration range, corresponding to what would produce a low fractional occupancy of the binding sites. The application of a low concentration of agonist can sustain that condition and maintain channel activation for several seconds during agonist application. Thus, the EC50 of 7* nAChRs calculated with net charge analysis is one to two orders of magnitude smaller than the ‘classical’ EC50 calculated with peak amplitude, the latter being biased by fast desensitization of the receptor (Papke & Porter Papke, 2002; Papke, 2005).
Nicotine regulates GABA release via preterminal 7* and ß2* nAChRs
Our results are in agreement with previous studies showing that 7* and ß2* receptors are present on interneurons (Frazier et al. 1998; Alkondon et al. 2000). Thus, in ß2–/– mice, preterminal (axonal or somato-dendritic) 7* nAChRs mediate nicotine-induced potentiation of GABA release onto pyramidal cells and interneurons. Moreover, in 7–/– mice, preterminal ß2* nAChRs modulate GABA release onto stratum oriens and stratum pyramidale interneurons, but not pyramidal cells or stratum radiatum interneurons. This is in contrast with previous data from adult rats suggesting that activation of ß2* nAChR in stratum radiatum interneurons increases the frequency of spontaneous IPSCs (Alkondon & Albuquerque, 2001). Developmental differences in the expression of nAChRs or between different species may account for this apparent contradiction.
nAChRs expression during hippocampal development
In the rat hippocampus, mRNAs for the 7 and ß2 subunits are present early during embryogenesis, but the expression patterns of 7* nAChR and ß2* nAChRs differ. The density of [3H]epibatidine-binding sites, an indicator of heteromeric nAChR expression, remains stable (Tribollet et al. 2004) during postnatal development. Conversely, in the CA1 region of the hippocampus, both the expression of 7 mRNA and the density of [125I]--bungarotoxin-binding sites, an indicator of 7* nAChR expression, are particularly high during the first postnatal week and decrease subsequently (Shacka & Robinson, 1998; Tribollet et al. 2004). These data suggest that in the hippocampus, the balance between 7* and ß2* nAChRs changes during postnatal development. This may lead to differences in nicotine-induced modulation of synaptic and network activity in the immature and in the adult hippocampus.
nAChRs and network oscillations during postnatal development
Synchronized oscillatory activity, such as GDPs, constitutes a peculiar feature of developing brain. GDPs have been recorded also in vivo in rat pups where they occur during immobility periods, sleep and feeding (Leinekugel et al. 2002). In this respect GDPs can be seen as a primordial form of synchrony between neurons, which precedes the development of the theta and gamma-rhythm.
Similar to GDPs, ‘waves’ of correlated activity have been found in several brain regions during postnatal development (review in O'Donovan, 1999). These waves are thought to be crucial for establishing neural connectivity. In the immature retina for example, blocking high-affinity nAChRs in the desensitized state with epibatidine leads to disruption of correlated network activity and to changes in the pattern of eye-specific connections from the retina to the lateral geniculate nucleus (Penn et al. 1998). 3–/– mice have altered retinal waves and ß2–/– mice completely lack retinal waves, while both show delayed refinement of individual retinal ganglion cell dendrites (Bansal et al. 2000). In ß2–/– mice, the pattern of retinogeniculate and retinocollicular projections, as well as the visual acuity, were found to be altered (Rossi et al. 2001). These studies demonstrate that nAChRs exert a crucial role in the epigenetic maturation of the visual system.
Interestingly, it has been recently reported that intrinsically bursting starburst cells underline the generation of retinal waves in perinatal rabbit retinas (Zheng et al. 2006). Nicotine, by shortening the duration of the afterhyperpolarization, increased the frequency of retinal waves. Therefore, the possibility exists that a similar mechanism is involved in nicotine-induced increase in frequency of GDPs, which at least in CA3 pyramidal cells can be triggered by intrinsic bursts (Sipila et al. 2005). However, unlike retinal waves, and in agreement with a previous report from the rat hippocampus (Cole & Nicoll, 1984), nicotine was unable to modify the afterhyperpolarization following brief trains of action potentials recorded from CA1 pyramidal cells in the immature hippocampus from WT mice in the presence of DNQX, bicuculline and D aminophosphonovalerate (data not shown).
In the developing hippocampus, GDPs are thought to be instructive in enhancing synaptic efficacy and in ‘unsilencing’ silent connections at emerging synapses (Kasyanov et al. 2004). They may contribute to the selective stabilization of neuronal circuits as in the visual cortex, but this remains to be demonstrated. Although activation of nAChRs powerfully regulates GDP frequency, the observation that GDPs are still present in 7 and ß2 KO mice suggests that activation of 7* and ß2* nAChRs is not essential for GDP generation.
In conclusion, our observations demonstrate that, in the developing hippocampus, a low concentration of nicotine modulates synaptic activity and network synchronization. The potency of these effects and the nAChR subtypes involved were not homogeneous and varied among different hippocampal layers, indicating that, during postnatal development, nAChRs participate in different ways in the fine regional tuning of immature hippocampal neurotransmission, which may play a crucial role in wiring the hippocampal circuitry.
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