Abstract
The chief inhibitory neurons of the mammalian brain, GABAergic neurons, are comprised of a myriad of diverse neuronal subtypes. To facilitate the study of these neurons, transgenic mice were generated that express enhanced green fluorescent protein (EGFP) in subpopulations of GABAergic neurons. In one of the resulting transgenic lines, called GIN ( GFP-expressing Inhibitory Neurons), EGFP was found to be expressed in a subpopulation of somatostatin-containing GABAergic interneurons in the hippocampus and neocortex. In both live and fixed brain preparations from these mice, detailed microanatomical features of EGFP-expressing interneurons were readily observed. In stratum oriens of the hippocampus, EGFP-expressing interneurons were comprised almost exclusively of oriens/alveus interneurons with lacunosum-moleculare axon arborization (O-LM cells). In the neocortex, the somata of EGFP-expressing interneurons were largely restricted to layers II-IV and upper layer V.
In hippocampal area CA1, two previously uncharacterized subtypes of interneurons were identified using the GIN mice: stratum pyramidale interneurons with lacunosum-moleculare axon arborization (P-LM cells) and stratum radiatum interneurons with lacunosum-moleculare axon arborization (R-LM cells). These newly identified interneuronal subtypes appeared to be closely related to O-LM cell, as they selectively innervate stratum lacunosum-moleculare. Whole-cell patch-clamp recordings revealed that these cells were fast-spiking and showed virtually no spike frequency accommodation. The microanatomical features of these cells suggest that they function primarily as “input-biasing” neurons, in that synaptic volleys in stratum radiatum would lead to their activation, which in turn would result in selective suppression of excitatory input from the entorhinal cortex onto CA1 pyramidal cells.
- GABAergic neurons
- interneurons
- green fluorescent protein
- GFP
- EGFP
- transgenic mice
- hippocampus
- cortex
- somatostatin
- metabotropic glutamate receptor
- mGluR1
- mGluR1a
- glutamic acid decarboxylase
- GAD67
- Gad1
- GABA
GABAergic neurons, the chief inhibitory neurons of the mammalian brain, are comprised of diverse neuronal subtypes distinguishable on the bases of location in given brain regions, microanatomical features, including dendritic arborizations and axonal projections, expression of specific macromolecules, and neurophysiological properties. Whereas a traditional view of GABAergic interneuronal function has been that of performing feedback inhibition, it has become increasingly evident that these cells perform much more complex functions that are crucial to controlling overall brain activity. In the hippocampus, for example, GABAergic interneurons appear to be critically involved in the initiation and maintenance of theta rhythms, as well as gamma, sharp wave, and fast oscillations (for review, see Freund and Buzsáki, 1996). This is accomplished by intricately interconnected interneuronal networks, composed of various GABAergic subtypes, which strictly regulate pyramidal cell activity.
For every major excitatory pathway of the brain, there appears to be associated inhibitory pathways (Buzsáki and Chrobak, 1995). For example, a subpopulation of hippocampal interneurons, with their somata and dendrites restricted to stratum oriens (SO), selectively innervate stratum lacunosum-moleculare (SLM) (Lacaille et al., 1987; Lacaille and Williams, 1990; Gulyás et al., 1993a,b; McBain et al., 1994;Blasco-Ibáñez and Freund, 1995; Sı́k et al., 1995;Hájos and Mody, 1997; Yanovsky et al., 1997; Alcántara et al., 1998). These cells are thus named O-LM cells (oriens/alveus interneurons with lacunosum-moleculare axon arborization). Since SLM is the input target of the entorhinal cortex via the perforant pathway, O-LM cells have been postulated to control the information flow from the entorhinal cortex into CA1.
To better elucidate how specific interneuronal subtypes contribute to both normal and pathological brain functions, it is essential that specific subtypes be identifiable during experiments and individually manipulated. Whereas patch-clamp recordings using infrared differential interference contrast (IR-DIC) videomicroscopy (Dodt and Zieglgänsberger, 1990, 1994) have greatly expanded our understanding of interneuronal properties, numerous technical limitations nonetheless continue to impede progress toward a thorough understanding of interneurons. In particular is the general inability to visually identify and morphologically characterize specific interneuronal subtypes before electrophysiological recordings.
To facilitate the study of GABAergic neurons, we created transgenic mice that selectively express the “enhanced” derivative of the autofluorescent protein, green fluorescent protein (EGFP) (Morise et al., 1974; Prasher et al., 1992; Cormack et al., 1996) in subpopulations of GABAergic neurons. In one of the derived transgenic lines, EGFP was found to be expressed in a subpopulation of hippocampal and neocortical interneurons that express somatostatin (SOM); this strain has thus been named GIN, for GFP-expressing Inhibitory Neurons. Using these mice, we have characterized two previously unidentified subtypes of SLM-projecting interneurons in hippocampal area CA1.
Portions of this work have previously appeared in abstract form (Oliva et al., 1998).
MATERIALS AND METHODS
Materials. PCR involved in the creation of plasmid vectors used the GeneAmp XL kit (PE Applied Biosystems, Foster City, CA); PCR for screening of transgenic mice used Taq DNA polymerase (Promega, Madison, WI). All other enzymes involved in nucleic acid manipulations were from American Allied Biochemical (Aurora, CO), Ambion (Austin, TX), Epicentre Technologies (Madison, WI), New England Biolabs (Beverly, MA), or Promega. Oligonucleotides were kindly synthesized by Paul Gardner (University of Chicago). QIAEX II (Qiagen, Chatsworth, CA) was used for gel purification of transgene DNA. All chemical reagents were from Sigma (St. Louis, MO), Epicentre Technologies, and Ambion.
Transgene for the creation of transgenic mice. Standard molecular biological techniques were used (Sambrook et al., 1989). Vector pGAD67-EGFP was created as follows. Two identical multiple restriction endonuclease sites were introduced into vector pGFP-1 (Clontech, Palo Alto, CA), one upstream to the GFP open reading frame and the other downstream to the SV40 polyadenylation signals, with the following order: FseI, SfiI, SrfI,NotI, SgfI, and SapI. These sites were introduced via two rounds of PCR with subsequent ligations using the following primer sets: round 1: 5′-CAACACTCAACCCTATCTCGGTCTA-3′; 5′-GGCCGGCCCGGGCGGCCGCGATCGCTCTTCCAGTTTGGAACAAGAGTCCAC-3′; and round 2: 5′-CTCAGATCTCGAGCTCAAGCT-3′; 5′-GGCCGGCCCGGGCGGCCGCGATCGCTCTTCCGGTAGCGCTAGTAATAAC-3′. This resulted in vector pGFP-1/MCS II. A murine Gad1 gene fragment of ∼2.8 kbp was derived via PCR using the following primer set: 5′-ATCCAGTTTGTTTTGCCCCTAAAGG-3′; 5′-TTGGGGTCTCTACGGTTCAAG-3′. The resulting product was subcloned into the SmaI site of vector pGFP-1. The transgene cassette from this resultant vector was gel-isolated after digestion with EcoRI and MluI, and subsequently subcloned intoEcoRI/MluI-digested pGFP-1/MCS II. The resulting vector was then digested with BamHI andHpaI, into which was subcloned the EGFP-bearing fragment from BamHI/HpaI-digested pEGFP-N1 vector (Clontech). This final vector was pGAD67-EGFP.
Creation of transgenic mice. pGAD67-EGFP was digested withSfiI, and the transgene DNA subsequently gel-purified. Pronuclear microinjections of transgene DNA into one-cell stage embryos of the inbred albino mouse strain FVB/N were performed in the laboratory of Dr. Paul Overbeek (Baylor College of Medicine) as described previously (Hogan et al., 1994).
Founder mice were bred to wild-type FVB mice (Harlan Sprague Dawley, Indianapolis, IN), and resultant F1 heterozygotic mice subsequently crossed to each other. F2 and subsequent generations of mice homozygotic for the transgene were crossed to establish colonies.
Screening of transgenic mice. Transgenic mice were screened via PCR similar to the method described by Busler and Li (1996). Briefly, toe clips were placed in a lysis buffer (20 mmTris HCl, pH 8.4, 50 mm KCl, 1 mm EDTA, pH 8.0, 0.1 mg/ml gelatin, 0.1% Triton X-100, and 4 mg/ml proteinase K) at 55°C for 3–5 hr, then 96°C for 10 min, then placed on ice, and 5 μl of the cold lysate used directly for PCR (100 μl reaction volumes). Each PCR reaction used a transgene-specific primer set and a primer set that spanned intron 15 of the murine Gad1 gene (Bu and Tobin, 1994; Szabó et al., 1996; Yanagawa et al., 1997) (used as an internal positive control for each PCR reaction). The transgene-specific primer set was: 5′-ATCCAGTTTGTTTTGCCCCTAAAGG-3′; 5′-CTCTACTGAGCCAGTATGGCTGTACAGG-3′. The Gad1gene-specific primer set was: 5′-CCCCACGCGTGATCACTGAGCGACGAGAAAAGCTAC-3′; 5′-CCCCACGCGTGATCAGAGCTTTGATCTTGGGAGC-3′.
Care and use of animals. Maintenance of all animals and all surgical procedures used were approved by the institutional animal care committee and were in keeping with guidelines established by the National Institutes of Health.
Future availability of animals. The GIN transgenic mice will be made available from The Jackson Laboratory (Bar Harbor, ME).
Immunohistochemistry and cell counting. Adult homozygotic mice were anesthetized with metofane and perfused transcardially with PBS followed by phosphate buffer containing 4% paraformaldehyde/5% sucrose. Brains were removed and immersed overnight in the same fixative at 4°C and subsequently placed overnight at 4°C in PBS containing 30% sucrose. Thirty- and 50-μm-thick coronal brain slices were then prepared using a Microm freezing sliding microtome (model HM 400 R; Carl Zeiss, Thornwood, NY).
Diaminobenzidine (DAB)-based immunohistochemistry was performed on free-floating brain sections using the M.O.M. kit (PK-2200; Vector Laboratories, Burlingame, CA) and Vectastain Elite ABC reagent (included in M.O.M. kit) according to the manufacturer's protocol. Anti-AFP antibody (AFP-5002; Quantum Biotechnologies, Montreal, Quebec, Canada) (specific for green fluorescent protein derivatives) was used at 1:2000 dilution. Sections were ultimately processed 5–15 min with 0.02% 3,3′-diaminobenzidine tetrahydrochloride/0.04% nickle/0.002% H2O2, mounted onto slides, air-dried overnight, and coverslipped using DPX neutral mounting medium (31,761–6; Aldrich, Milwaukee, WI).
Fluorescence immunohistochemistry was performed as follows. Free-floating sections were incubated overnight at room temperature in PBS containing antibody at the appropriate dilution and 0.3% Triton X-100 (except for the anti-GAD67 antibody reactions, in which no detergent was used). Sections were rinsed and incubated with secondary antibody in PBS for 1 hr. Sections were rinsed and wet-mounted using SuperMount permanent aqueous mounting medium (BioGenex Laboratories, San Ramon, CA). Polyclonal anti-GAD67 and anti-SOM, and monoclonal anti-NeuN, antibodies (AB108, AB1752, and MAB377, respectively; Chemicon, Temecula, CA) were used at 1:3000, 1:2000, and 1:400 dilution, respectively. Polyclonal anti-mGluR1a antibodies (06–310; Upstate Biotechnology, Lake Placid, NY) were used at 1:100 dilution. Rhodamine-conjugated secondary antibodies (111-085-144; Jackson ImmunoResearch, West Grove, PA) were used at 1:200 dilution.
Sections were viewed and photographed with a Microphot-FXA upright epifluorescent microscope (Nikon, Dallas, TX) using filter sets from Omega Optical Inc. (Brattleboro, VT; XF100, XF101, XF52, and XF53) and Chroma Technology (Brattleboro, VT; 61000 version 2). Photographic slides were subsequently scanned into a computer using a SprintScan 35 slide scanner (Polaroid, Cambridge, MA). Digital images were also acquired directly with a MicroMax 5 MHz cooled digital camera (Princeton Instruments, Trenton, NJ). Images were rendered using Photoshop 5.0 (Adobe Systems, San Jose, CA) and prints made using a dye sublimation printer (model MD-1300; Alps Electric, San Jose, CA). For Figures 5 and 6, portions of consecutive image planes in thez-axis of DAB-based immunohistochemically processed sections were montaged together to maximize the amount of in focus information; for Figure 9, the scan of the coronal cross-section was directly obtained using a SprintScan 35 slide scanner (Polaroid). Subsequently, the images of Figures 5, 6, and 9 were digitally inverted to enhance contrast. Unless otherwise specified, all images were from 50-μm-thick sections.
Cell counting was performed to determine the colocalization of EGFP with GABAergic cell markers in various hippocampal regions. Coronal sections of mid-dorsal hippocampus were selected 0–0.4 mm caudal to the first appearance of the habenular commissure. Counts of SOM- and mGluR1a-immunoreactive neurons were performed on three sections from each of four mice; counts for GAD67 was performed on four sections from each of two mice. For each mouse, the total number of EGFP-expressing cells and their colocalization with immunoreactive cells was determined by summing the counts for each set of sections for each hippocampal subregion; for the anti-SOM and anti-GAD67 immunoreactions, the total number of immunofluorescent cells was also determined. Data are presented either as straight percentages or as mean percentages ± SDs calculated using population-weighted statistics (Wonnacott and Wonnacott, 1984), for the combined data from all the mice.
Neurolucida reconstructions. DAB-based immunohistochemistry was performed on serial sections of coronal brain sections from adult mice using anti-AFP antibody as described above. Three-dimensional neuronal reconstructions were then performed using the Neurolucida software package in conjunction with the Lucivid display hardware (MicroBrightField, Colchester, VT). For the neurons depicted in Figure 4, the dendritic trees were reconstructed in entirety.
In vitro slices: videomicroscopy and neurophysiological recordings. Postnatal day 10–14 mice were anesthetized with metofane, and transverse brain slices, 250- to 300-μm-thick, were sectioned in ice-cold dissecting solution using a model 752M Vibroslice vibrating slicer (Campden Instruments, Sileby, Loughborough, UK). Slices were transferred to a holding chamber containing an equal mixture of room temperature dissecting and recording solutions for at least 1 hr. For optical imaging and electrophysiological recording, slices were transferred as needed to a recording chamber that was continuously perfused with room temperature recording solution. Dissecting solution consisted of (in mm): 60.0 NaCl, 3.0 KCl, 7.0 MgCl2, 1.25 NaH2PO4, 0.5 CaCl2, 25.0 NaHCO3, 110.0 sucrose, and 7.0 dextrose. Recording solution consisted of (in mm): 125.0 NaCl, 2.5 KCl, 1.0 MgCl2, 1.25 NaH2PO4, 25.0 NaHCO3, 2.0 CaCl2, and 25.0 dextrose. All solutions were continuously bubbled with 95% O2 and 5% CO2.
Whole-cell patch-clamp recordings were performed with fire-polished borosilicate glass electrodes (6–12 MΩ). Electrodes were filled with (in mm): 120 K+d-gluconic acid, 20 KCl, 10 EGTA, 10 HEPES, and 2 MgCl2, pH 7.3–7.4.
An Axioskop upright-microscope (Carl Zeiss) was equipped with a MicroMax 5 MHz cooled digital camera (Princeton Instruments) used for both epifluorescence and IR-DIC videomicroscopy, and an MTI NC-70CX infrared-sensitive camera (Dage-MTI, Michigan City, IN) was used for IR-DIC microscopy. The microscope was also equipped with a model MAC 2000 focus drive (Ludl Electronics Products, Hawthorne, NY), a Lambda 10–2 filter wheel (Sutter Instruments, Novato, CA), and a fiber optic liquid light guide for epifluorescence illumination (Carl Zeiss; 417087). The GFP filter set (XF100) for epifluorescence and infrared band-pass filter (780-DF32) for IR-DIC videomicroscopy were from Omega Optical. EGFP-expressing interneurons were first identified via fluorescence microscopy. Subsequently, IR-DIC videomicroscopy was used to obtain whole-cell patch-clamp recordings. To ensure that each neuron selected via fluorescence microscopy could be readily identified when switching to IR-DIC microscopy, the same digital camera was used for both forms of imaging, which prevented misalignment of the two sets of images. In instances in which selected EGFP-expressing interneurons were in areas densely packed with other neurons [e.g., stratum pyramidale (SP)], this simple alignment between fluorescence and IR-DIC images was insufficient to allow for the unequivocal identification of the appropriate neuron under IR-DIC videomicroscopy. In such circumstances, a filter set consisting of a long-pass dichroic mirror and long-pass emission filter (510DRLP and 510LP, respectively; Omega Optical) were placed in the optical pathway that allowed for visualization of such selected neurons simultaneously on the same camera via both fluorescence and IR-DIC videomicroscopy. After achieving whole-cell recordings, fluorescence microscopy was used to confirm that each patch-clamped neuron was indeed the EGFP-expressing interneuron of interest.
Digital image acquisition was accomplished using the MetaMorph Imaging System (Universal Imaging, West Chester, PA). Before performing patch-clamp recordings, series of consecutive optical sections were taken at 0.5–1.0 μm z-spacing. Subsequent to recording, deconvolution of digital image sets was performed using the AutoDeblur software package (AutoQuant Imaging, Watervliet, NY), with maximum projection images subsequently generated. Iterative deconvolution was performed using a theoretical point-spread function for wide-field epifluorescence microscopy based on the following parameters: the objective's numerical aperture; fluorescence emission wavelength of 510 nm; a refractive index of 1.33; the calculated dx anddy spacing between adjacent pixels as measured with a micrometer; and the calibrated dz spacing between adjacent focal planes. For some neurons, deconvolution was performed on the entire image set as a whole; for other neurons, deconvolution was performed on subsections of each image series from which maximum projection images were made and subsequently montaged to yield a full deconvolved image.
RESULTS
Creation of EGFP-expressing transgenic mice: use ofGad1 gene sequence
EGFP (Cormack et al., 1996) is an “enhanced” version of green fluorescence protein, having ∼35× greater fluorescence than the wild-type protein and a codon bias optimized for mammalian expression. To confer EGFP expression to GABAergic interneurons in transgenic mice, upstream regulatory sequence from the murineGad1 gene (Szabó et al., 1996) was used to control EGFP expression (Fig. 1). Fifty-two pronuclear injections of transgene DNA were performed, resulting in nine founder mice bearing the transgene. Of these, three passed on the transgene in which the mice of each line consistently expressed EGFP in differing distinct subpopulations of GABAergic neurons.
In the line derived from one of these founders, intense EGFP expression was present in interneurons of the hippocampus and cerebral cortex. This line has thus been named GIN, for GFP-expressing Inhibitory Neurons. Mice of the GIN transgenic line showed neither obvious physical nor behavioral abnormalities in either the heterozygotic or homozygotic states. Litter sizes for both heterozygotic and homozygotic crosses ranged from 7 to 13 pups, consistent with that obtained for wild-type crosses. Females were able to have litters every 3.5–4 weeks, and pup mortality was insignificant.
EGFP expression in the GIN transgenic line
EGFP-expressing neurons were found throughout the CNS of GIN mice. Most predominant were those found in the archicortex and neocortex (Fig. 2; see Figs. 8, 9). EGFP-expressing neurons were also found in the midbrain, brainstem, and spinal cord. Most notable among these were the dorsal and ventral cochlear nuclei, the vestibular nuclei, nuclei of the lateral lemniscus, nuclei of the periaqueductal gray, various areas of the reticular nucleus of the thalamus, the inferior salivatory nucleus, the prepositus hypoglossal nucleus, nucleus X, and a dense network of EGFP-expressing neurons throughout the entire length of the dorsal horn of the spinal cord. In general, midbrain and brainstem EGFP-expressing neurons were much less prevalent than their hippocampal, neocortical, and spinal cord counterparts. EGFP expression was also noticeably absent from the cerebellum and striatum, both areas of which are densely populated by GABAergic neurons, as well as the hypothalamus.
EGFP appeared to freely diffuse throughout the cytoplasm of expressing neurons in all brain areas. In both fixed and live preparations, the overwhelming majority of EGFP-expressing neurons were very intensely fluorescent, making the dendrites readily visible and traceable to their terminations. In some instances, axons could also be visualized and followed for hundreds of micrometers from their parent somata. Numerous EGFP-expressing neurons were also found to be sparsely to moderately spiny, particularly those in the neocortex.
The pattern of EGFP expression in line GIN has remained consistent for more than five generations. Little, if any, differences were noticed in either the fluorescence intensity or number of EGFP-expressing neurons of heterozygotic versus homozygotic, as well as male versus female, mice. Induction of hippocampal and cortical EGFP expression was found to begin at approximately postnatal day 5. This developmental onset of EGFP expression temporally coincides with the terminal differentiation of GABAergic interneurons and the onset of expression of many of the macromolecules (e.g., somatostatin) that delineate subpopulations of mature GABAergic neurons (Naus et al., 1988; Bergmann et al., 1991;Jiang and Swann, 1997).
EGFP-expressing neurons of the hippocampus
Figure 2a typifies the pattern of EGFP expression found in the hippocampus of adult GIN mice. This montage was created from overlapping images of a 50-μm-thick coronal brain section from an homozygotic mouse. It should be noted that the EGFP fluorescence shown in this and all other images is intrinsic fluorescence, i.e., it is not the product of a fluorophore-labeled antibody immunoreaction. As was typical for all GIN mice, significantly more EGFP-expressing somata and dendrites were found in area CA3 relative to area CA1 and the dentate gyrus. EGFP-expressing somata and dendrites were generally confined to SO and stratum radiatum (SR) of areas CA1-CA3 and to the hilus of the dentate gyrus. Noticeably, EGFP-expressing somata and dendrites were rarely observed in SLM or in stratum granulosum (SG) or stratum moleculare (SM) of the dentate gyrus. In contrast, a dense plexus of EGFP expression was found in SLM, particularly in area CA3 (Fig.2a, asterisk), as well as noticeable fluorescence in the outer one-third of SM of the dentate gyrus; such fluorescence was not found in wild-type mice and was attributable to dense axonal arborizations in these areas. Based on the relative lack of EGFP-expressing somata in the cell body layers (stratum pyramidale and granulosum), EGFP expression in the hippocampus of GIN mice appeared to be restricted to GABAergic interneurons. EGFP-expressing processes were also found in the fornix, indicating that EGFP-expressing cells had extrahippocampal axonal projections and/or that EGFP-expressing neurons from other brain areas innervated the hippocampus. The former conclusion is indirectly supported by the fact that the medial septum-diagonal band of Broca complex appeared devoid of EGFP-expressing somata and that a dense network of fluorescent fibers were readily visible in the medial septum (Alonso and Köhler, 1982; Tóth and Freund, 1992; Tóth et al., 1993).
Fluorescence visualization of EGFP-expressing somata revealed cellular morphologies that tended to be either oval or pyramidal. In area CA3, for example, many EGFP-expressing somata in SO were pyramidal-shaped (Fig. 2b, arrow), bearing two to four primary dendrites. In general, most of the dendritic ramifications of these cells appeared to be restricted to SO, although dendrites could be found crossing SP to terminate in SR. In SR of area CA3, many of the EGFP-expressing cells had similar morphologies to their SO counterparts. In both SO and SR of area CA3, the diffuse fluorescence was attributed to the high density of EGFP-expressing dendrites in these areas. In SO of area CA1, EGFP-expressing neurons tended to have oval-shaped somata with dendrites restricted to SO that ran parallel to the strata borders (Fig. 2c, arrow). In SR and SP of area CA1, the morphologies of EGFP-expressing neurons were more diverse (Fig. 2d, and see below). In the dentate gyrus, EGFP-expressing somata and dendrites were restricted almost exclusively to the hilus. Somata of these cells often had semicircular shapes with two primary dendrites (Fig. 2e).
Figure 2, f and g, shows area CA3 from a section that was immunohistochemically processed with rhodamine-labeled antibodies directed against the vertebrate neuron-specific nuclear protein NeuN (Neuronal Nuclei) (Mullen et al., 1992). NeuN is a DNA-binding protein that is specifically expressed in neurons of the vertebrate CNS, being restricted primarily to nuclei; thus, immunohistochemistry for this protein serves as a counterstain in EGFP-expressing sections, allowing for the laminar distribution of EGFP-expressing cells to be demonstrated. In f, EGFP expression alone was visualized using an EGFP-selective fluorescence filter set, whereas in g a double filter set was used to show simultaneous expression of both proteins. Every EGFP-expressing cell was found to coexpress NeuN, as indicated by their bright yellow nuclei. As readily seen, very few EGFP-expressing somata and processes were found in the pyramidal cell layer. Stratum lucidum (SL) was also mostly devoid of EGFP expression. The absence of EGFP expression in the vast majority of NeuN-positive neurons in SO, SR, and SLM indicates that only a minority of interneurons expressed EGFP. In SO and SR of area CA1, for instance, the total of NeuN-expressing neurons that coexpressed EGFP was estimated to be ∼10% and <5%, respectively.
Hippocampal EGFP-expressing cells are somatostatin-expressing GABAergic interneurons
To ascertain the identities of the hippocampal EGFP-expressing neurons in GIN mice, fluorescence immunohistochemistry for numerous markers of GABAergic interneurons was performed.
Whereas it was apparent, based on their laminar distributions, that the hippocampal EGFP-expressing cells were interneurons, fluorescence immunohistochemistry against GAD67 was performed to confirm this (Fig.3a–c). Greater than 99% of all hippocampal EGFP-expressing neurons were found to coexpress GAD67 (267 of 268 EGFP-expressing cells). When counts from SO, SP, and SR were combined, ∼7 and 22% of all hippocampal GABAergic neurons were found to express EGFP in areas CA1 and CA3, respectively; in the hilus of the dentate gyrus, ∼10% of all GABAergic interneurons were found to express EGFP. In short, the hippocampal EGFP-expressing cells of the GIN transgenic mice are a subpopulation of GABAergic interneurons.
As mentioned above, a noticeable feature of hippocampal EGFP-expressing interneurons in area CA1 of GIN mice was the localization of their often oval-shaped somata to SO, with dendrites running parallel to the strata borders (Fig. 2a,c, arrow). Such morphology is characteristic of O-LM cells. In area CA3, O-LM cells often have pyramidal-shaped somata with dendrites that span all strata except SLM (Gulyás et al., 1993a,b); thus, the morphologies of EGFP-expressing interneurons in SO of area CA3 (Fig. 2b,arrow) also coincide with those of O-LM cells. Numerous studies have shown that all O-LM cells express the neuropeptide SOM and that SOM expression in the hippocampus defines a subset of GABAergic interneurons (Köhler and Chan-Palay, 1982; Morrison et al., 1982;Johansson et al., 1984; Sloviter and Nilaver, 1987; Kosaka et al., 1988; Kunkel and Schwartzkroin, 1988; Milner and Bacon, 1989; Esclapez and Houser, 1995). As illustrated in Figure 3d–l, fluorescence immunohistochemistry showed a striking overlap between EGFP- and SOM-expressing interneurons of the hippocampus. In the panoramic images of area CA3 (Fig. 3d–f), every EGFP-expressing interneuron was found to coexpress SOM. This coexpression is readily observed in the higher magnification views (Fig. 3g-i) of a cell from SO (Fig. 3d, box). Figure 3j–l shows the clear overlap in EGFP and SOM expression in SO of area CA1. Note the O-LM cell-like morphologies (large arrow); also note the EGFP-expressing interneuron that was very weakly immunopositive for SOM (small arrow). The results of cell counts for the overlap in EGFP and SOM-expressing neurons are detailed in Table 1. On average, 95.13 ± 2.33% (n = 707) of hippocampal EGFP-expressing neurons in GIN mice coexpressed SOM. The total portion of SOM-expressing hippocampal interneurons that coexpressed EGFP ranged from ∼15% (hilus and CA1 SO) to ∼35% (CA3 SO). Thus, the EGFP-expressing hippocampal interneurons in GIN mice define a subset of SOM-expressing interneurons.
Previous studies have shown that every SOM-expressing neuron in the rat hippocampus coexpresses the “a” spliced form of the metabotropic glutamate receptor 1 (mGluR1a) with a 1:1 correlation (Martin et al., 1992; Baude et al., 1993; Görcs et al., 1993;Blasco-Ibáñez and Freund, 1995; Kerner et al., 1997). Fluorescence immunohistochemistry was thus performed for mGluR1a. Results showed that every hippocampal EGFP-expressing interneuron coexpressed this receptor subunit (Table 1). Figure 3m–oexemplifies this coexpression in an O-LM cell from area CA1. In this cell, the somata and dendrites were intensely labeled for mGluR1a; in contrast, the axon that emanated from the center of the somata (Figs.3j, arrow) was negative for mGluR1a expression over its entire length. This axon traversed SO and SP, running primarily perpendicular to the strata borders, and only on reaching SLM did it ramify. Quantification of the total number of EGFP-expressing cells that coexpressed mGluR1a was difficult, since an intense fluorescence immunoreactivity to mGluR1a was not observed in every somata; however, mGluR1a- and EGFP-coexpressing dendrites could be traced back to every EGFP-expressing somata examined. Furthermore, we did not observe any EGFP-expressing dendrites devoid of mGluR1a immunoreactivity. Thus, EGFP-expressing hippocampal interneurons in GIN mice coexpress mGluR1a. This further supports the conclusion that every hippocampal EGFP-expressing cell in GIN mice is an SOM-expressing interneuron.
SOM-expressing interneurons of the hippocampus can be divided into a number of subtypes based on the coexpression of other neurochemical markers. In rat, it has been shown that ∼32% of all SOM-expressing interneurons in SO (i.e., O-LM cells) coexpress the calcium-binding protein calbindin (CB) and that these O-LM cells project extrahippocampally (Tóth and Freund, 1992; Tóth et al., 1993; Katona et al., 1996). Furthermore, it has been shown that ∼40–60% of all neuropeptide Y (NPY)-expressing interneurons in area CA1 correspond to O-LM cells (Köhler et al., 1987). Fluorescence immunohistochemistry showed that the overwhelming majority of EGFP-expressing hippocampal interneurons in GIN mice coexpressed neither CB nor NPY. Although these results would argue against the existence of extrahippocampal-projecting EGFP-expressing O-LM cells in GIN mice, EGFP-expressing axons were nonetheless found in the fornix, whereas the medial septum-diagonal band of Broca complex appeared devoid of EGFP-expressing somata. Together with the fact that CB expression significantly differs between mouse and rat (M. Jiang and J. Swann, personal communication), it is possible that hippocampal EGFP-expressing O-LM cells in GIN mice do project extrahippocampally. Fluorescence immunohistochemistry for two other calcium-binding proteins, parvalbumin (PV) and calretinin (CR), also showed a lack of coexpression with EGFP.
In summary, the EGFP-expressing hippocampal interneurons in mice of the GIN transgenic line were phenotypically characterized to be: SOM (+), mGluR1a (+), GAD67 (+), NPY (−), CB (−), CR (−), and PV (−).
EGFP-expressing interneurons in hippocampal area CA1
To more fully characterize EGFP-expressing hippocampal interneurons, three-dimensional dendritic arborization and axonal innervation patterns of EGFP-expressing interneurons were determined in hippocampal area CA1 of adult GIN mice. For these studies, DAB-based immunohistochemistry was performed on serial brain sections to avoid photobleaching during neuronal reconstructions. Analyses revealed that the vast majority of these EGFP-expressing interneurons fell into one of three categories, two of which have previously been unidentified.
O-LM cells
By far the lamina of CA1 with the largest abundance of EGFP-expressing somata was SO. Furthermore, every EGFP-expressing interneuron with its somata in SO of area CA1 and for which its axon could be discerned (n = 10) was found to be an O-LM cell.
Figure 4a shows a Neurolucida reconstruction of one such interneuron from the dorsal hippocampus, illustrating its complete dendritic structure and partial axonal innervation pattern. As is the case for O-LM cells by definition, this interneuron contained a primary axon that projected to SLM where it ramified significantly. This axon arose from a proximal dendrite, close to the somata, and remained mainly unbifurcated through SP and SR. At the most distal aspect of SR, close to SLM, the axon began to bifurcate, although not very extensively. On entering SLM, the axon ramified significantly; but, as was the case for all EGFP-expressing interneurons, reconstruction of only the most proximal axonal segments was feasible because the more distal processes were obscured by the high density of other EGFP-expressing axonal processes in SLM. This O-LM cell also possessed an axonal collateral in SO, which is a feature common to many O-LM cells. For all EGFP-expressing O-LM cells examined, the axons were found to originate either from the somata (Fig.5b, arrow) or a proximal dendrite (Figs. 4a, 5c, small arrow).
In general, EGFP-expressing O-LM cells of area CA1 had morphologies that fell between one of two extremes. EGFP-expressing O-LM cells whose somata were located close to the alveus tended to be bipolar with horizontally traversing dendrites (Fig. 5a). In contrast, O-LM cells with somata located close, or adjacent, to SP tended to have dendrites that initially projected radially toward the alveus, but on reaching the distal half of SO turned to project horizontally (Fig.5b). By far, the vast majority of EGFP-expressing O-LM cells had their dendrites restricted to the distal half of SO, where they traversed parallel to the laminar borders.
Microanatomically, the dendrites of EGFP-expressing O-LM cells varied from smooth to very varicose in appearance. Generally, the primary dendritic branches of these interneurons were nonvaricose (Fig.5c, large arrow). However, second and higher order dendritic branches often abruptly changed to become quite varicose (Fig. 5c, arrowheads). This latter morphology was generally retained throughout the remainder of the dendritic tree to the terminal arbors. Whereas the dendrites of EGFP-expressing O-LM cells were found to be mostly aspiny, sparsely to moderately spiny dendritic branches were occasionally found (Fig.5d). Such spiny branches tended to be very distal from the somata, most often being terminal branches.
R-LM cells
In general, EGFP-expressing somata were infrequent in SR of area CA1: approximately one cell per 50-μm-thick coronal hippocampal section (n = 92 sections) was observed in mid-dorsal hippocampus of adult mice. Overall, these SR interneurons fell into one of two categories: those with pyramidal-shaped somata, which gave rise to two to five large primary dendrites (Figs. 4b,6a), and those that did not have pyramidal-shaped somata. The latter category of EGFP-expressing interneurons were far less abundant than the former, as well as morphologically more diverse. The former category appeared to be comprised of a relatively homogenous subpopulation of interneurons that sent their axonal projections to SLM: for five such cells in which axonal reconstructions were possible, all five were found to project axons to SLM. These cells thus define a newly identified interneuronal subtype, which we refer to as R-LM cell (interneurons with radiatum-located somata and lacunosum-moleculare axon arborization).
Figure 4b shows a Neurolucida reconstruction of an R-LM cell, illustrating its complete dendritic structure and partial axonal innervation pattern. This cell typified the general morphology of this interneuronal subtype. In contrast to O-LM cells, R-LM cell dendrites were not confined to a single lamina. Instead, the dendritic trees of these interneurons ramified extensively in SR and less so in SO, while selectively avoiding SLM. For those R-LM cells that did have dendrites that penetrated into SLM, the dendrites only entered the most proximal portions of SLM (close to SR), where they tended to either terminate, or turn to run parallel to the SR-SLM border. In numerous instances, these SLM-penetrating dendrites would turn back to reenter SR (Fig.6c, arrow). While the dendrites of the cell depicted in Figure 4b were aspiny, they were quite varicose. Typical of R-LM cells, varicosities (Fig. 6a,arrowheads) became prevalent in second and higher order dendritic branches (Fig. 6a, large arrow). Numerous other R-LM cells were found to be sparsely to moderately spiny, particularly at terminal branches, much like O-LM cells.
As exemplified in Figures 4b and 6a (small arrow), R-LM cells gave rise to a single primary axon that often emanated from a primary dendrite. These axons often bifurcated, although not very extensively, in the distal portion of SR, close to SLM. After reaching SLM, the axons began to ramify extensively.
P-LM cells
In hippocampal area CA1, EGFP-expressing interneurons with somata in SP, and for which axonal reconstructions were possible, fell into one of two categories: those that sent axonal projections to SLM and those which sent axonal projections to the alveus. EGFP-expressing interneurons of the former category thus define a second newly identified interneuronal subtype that we refer to as P-LM cells (interneurons with pyramidale-located somata and lacunosum-moleculare axon arborization).
Figure 4c depicts a Neurolucida reconstruction of a P-LM cell, illustrating its complete dendritic structure and partial axonal innervation pattern. Similar to R-LM cells, and in contrast to O-LM cells, P-LM cells had dendritic trees that spanned from SR to SO. Only rarely did dendrites of P-LM cells enter SLM. Much the same as for R-LM cells, those P-LM cell dendrites that did enter SLM only penetrated the most proximal portion of this lamina; these dendrites would then terminate, turn to run parallel to the laminar borders, or turn back to reenter SR. As was the case for both O-LM and R-LM cells, the second and higher order dendritic branches of P-LM cells were often varicose.
As Figures 4c and 6b (arrow) illustrate, P-LM cells gave rise to a primary axon that often emanated from an apical dendrite. Axons of these neurons traversed through the proximal SR where they rarely branched, but after reaching the distal SR, close to SLM, began to branch. On entering SLM, P-LM cell axons ramified extensively.
Overall, the similarities in dendritic and axonal features, as well as their neurochemical profiles, indicate that R-LM and P-LM cells are very closely related.
Neurophysiological properties of hippocampal EGFP-expressing interneurons
Whole-cell patch-clamp studies were undertaken to determine neurophysiological properties of hippocampal EGFP-expressing interneurons in acutely prepared in vitro brain slices. Figure 7a depicts a maximum projection image of a deconvolved image set of an R-LM cell from which neurophysiological recordings were obtained. In this example, the R-LM cell had two major primary dendritic branches that projected toward SO. One of these primary dendrites bifurcated into two major branches of approximately equal size that continued toward SO without further branching in SR. In contrast, the other primary dendrite gave rise to numerous higher order branches in SR, as well as a largely unbifurcating branch that projected toward SO.
Whole-cell recordings revealed that hippocampal EGFP-expressing R-LM cells had properties typical of fast-spiking interneurons: spontaneous action potentials in EGFP-expressing R-LM cells (n = 5) showed a rapid rate of spike repolarization (spike-width at half-maximum <1.2 msec, recordings performed at room temperature) and a notable large afterhyperpolarization (−5 to −10 mV). In response to square-wave depolarizing current steps, trains of actions potentials were elicited that showed little, if any, spike frequency adaptation (accommodation) (Fig. 7b). These action potential trains increased in frequency as depolarization increased, and they typify the responses observed from other EGFP-expressing cells. In response to hyperpolarizing current steps, all five R-LM cells exhibited a time-dependent inward rectification (depolarizing “sag”) that became more prominent with increasing hyperpolarization (Fig.7c). Occasionally, a rebound action potential would be elicited at the end of an hyperpolarizating step (data not shown).
Recordings from EGFP-expressing O-LM cells revealed neurophysiological properties very similar to those of R-LM cells and in accord with previous observations. Figure 7d shows a deconvolved image of an O-LM cell from area CA1 of the dorsal hippocampus from which recordings were made. As was expected, EGFP-expressing O-LM cells (n = 6) were fast-spiking and exhibited nonaccommodating trains of action potential in response to square wave depolarizing current steps (Fig. 7e). In response to hyperpolarizing square-wave current steps, O-LM cells (four of six) often exhibited a depolarizing sag (Fig. 7f), very similar to those seen for R-LM cells. This type of rectification has been previously reported as a distinguishing neurophysiological feature of O-LM cells (McBain et al., 1994; Sı́k et al., 1995).
In addition to the above properties, we did not note any differences in the rate of spontaneous synaptic potentials recorded in R-LM and O-LM cells. Both cell types also discharged spontaneously at resting membrane potential under our experimental conditions. Overall, we did not observe any electrophysiological properties that made R-LM cells readily distinguishable from O-LM cells.
EGFP-expression in the neocortex: SOM-expressing interneurons in layers II-V
Since EGFP was prominently expressed in other areas of the brain, especially in the neocortex, experiments were undertaken to determine if cortical neurons were similar or different from those of the hippocampus. Numerous EGFP-expressing neurons were found throughout all areas of the neocortex (Fig. 8). Among the different neocortical regions, such as primary somatosensory (Figs.8b,c), including barrel field cortex (Fig. 8a), the distribution of EGFP-expressing neurons appeared to be similar; the uniformity of this distribution can be grasped by Figure9. Interestingly, EGFP-expressing neurons were restricted almost exclusively to layers II-IV and upper layer V, as can be seen after immunohistochemical processing for NeuN (Fig.8b,c). Occasionally, EGFP-expressing neurons were found deep in layer V and layer VI, but these were very rare. The vast majority of EGFP-expressing processes were also restricted to layers II-IV and upper layer V, leading to the increased overall fluorescence of these layers.
Whereas the morphologies of EGFP-expressing neurons of the neocortex were quite diverse, at least a few subtypes could be morphologically classified. One of the most prevalent of these consisted of bipolar neurons with radially oriented dendrites (Fig. 8d,arrow). Neurons of this subtype were found at all levels of layers II-IV and often had a single descending and multiple ascending principal dendrites. A second morphologically identifiable subtype was characterized by pyramidal-shaped somata localized to upper layer II, with two long descending dendrites that draped down into layer III, but no prominent ascending dendrites. Figure 8e shows a high-magnification view of a neuron of this subtype from auditory cortex; another cell of this subtype from barrel cortex is visible in Figure 8a (top left). Other morphologies found included neurons (Fig. 8f, large arrow) with dendrites that appeared to “sweep” around their somata (small arrow) to run primarily parallel to the laminar borders, as if sampling synaptic input from other cortical columns. The piriform cortex contained very morphologically diverse interneurons, including particularly striking multipolar neurons (Fig. 8g).
Immunohistochemistry was performed on neocortical sections from GIN mice (Fig. 8h–j). As was readily apparent from visual inspection, the overwhelming majority of, if not every, neocortical EGFP-expressing cell coexpressed both GAD67 and SOM. Thus, like those of the hippocampus, EGFP-expressing neurons of the neocortex are SOM-expressing GABAergic interneurons.
DISCUSSION
To facilitate the study of GABAergic neurons of the CNS, transgenic mice were generated that selectively and consistently express EGFP in distinct subpopulations of GABAergic neurons. Upstream regulatory region from the murine Gad1 gene, which codes for the 67 kDa form of the GABA-synthesizing protein, glutamic acid decarboxylase (GAD67), was chosen to drive EGFP expression, as this gene appears to be ubiquitously expressed in GABAergic neurons. A relatively small fragment of the Gad1 gene was used, with the expectation that such a small fragment would confer GABAergic specificity to the transgene expression, while allowing the temporal and spatial expression of the transgene to be governed by the site of transgene integration into the mouse genome, i.e., positional effects. In a previous study in which LacZ was used as a reporter, we found that while this portion of the Gad1 gene was sufficient to limit transgene expression to GABAergic interneurons in transgenic mice, LacZ expression did appear to be governed by positional effects (A. Oliva, M. Jiang, P. Overbeek, and J. Swann, unpublished results). In creating the EGFP-expressing mice, we reasoned that since a fusion protein was not created, EGFP should freely diffuse throughout the cytoplasm of expressing neurons, filling not only the somata, but dendrites and axons as well. However, if all interneurons expressed EGFP, then visualizing the microanatomical features of individual cells would likely be impossible, as the processes of interest would be obscured by a plethora of other EGFP-expressing processes. To avoid this potential limitation, the positional dependency of the Gad1 gene fragment was exploited: EGFP expression, we anticipated, would be restricted to differing subsets of GABAergic neurons in each derived transgenic line. The merits of this approach are obvious when area CA3 of GIN mice is inspected: whereas only ∼20% of total interneurons included in SO, SP, and SR expressed EGFP, the density of EGFP-containing processes nearly saturates the neuropil.
By allowing for specific interneuronal subtypes to be readily identified, the GIN and future similar strains of transgenic mice should prove to be powerful tools for the study of GABAergic neurons. For example, the GIN mice should facilitate highly detailed studies of previously characterized interneuronal subtypes, e.g., O-LM cells, as well as less well characterized or previously unstudied interneuronal subtypes, e.g., R-LM and P-LM cells, SOM-expressing interneurons in the upper layers of the neocortex, and EGFP-expressing cells in the midbrain, brainstem, and spinal cord. GIN mice should also prove to be useful in the study of epilepsy (Sloviter, 1987, 1991; Sloviter and Nilaver, 1987, Sloviter and Lowenstein, 1992), traumatic brain injury (Lowenstein et al., 1992), and Alzheimer's disease (Davies et al., 1980; Roberts et al., 1985; Bissette, 1997; Grouselle et al., 1998; Van Uden et al., 1999), disorders in which SOM-expressing interneurons appear to be selectively vulnerable.
GIN transgenic mice: EGFP expression and interneuronal subtypes
Hippocampal EGFP-expressing cells of GIN transgenic line were immunohistochemically characterized to be SOM-expressing GABAergic interneurons. In area CA1, the vast majority of these interneurons were comprised of O-LM cells and two newly identified interneuronal subtypes, R-LM and P-LM cells. In addition to sharing neurochemical profiles, including the ability to drive EGFP expression via the GAD67-EGFP transgene, these three interneuronal subtypes were similar in that their axons projected to SLM. Whole-cell patch-clamp recordings from O-LM and R-LM cells also revealed that these interneuronal subtypes had similar neurophysiological profiles: they exhibited fast-spiking, showed little if any spike frequency accommodation, and exhibited a depolarizing “sag” in response to hyperpolarizing current injection. This last feature is likely produced by activation of an IH current (Maccaferri and McBain, 1996; Parra et al., 1998).
Other interneurons known to express SOM include hilar interneurons with perforant pathway projecting axons (HIPP cells) of the hilus of the dentate gyrus (Morrison et al., 1982; Halasy and Somogyi, 1993;Esclapez and Houser, 1995; Katona et al., 1999). To quote from Freund and Buzsáki (1996), “‘SOM’ cells and ‘HIPP cells’ in the dentate gyrus can be considered as synonymous”. In the GIN mice, it appeared that the EGFP-expressing interneurons in the dentate gyrus are indeed HIPP cells. Other hippocampal interneuronal subtypes suggested to express SOM (Sı́k et al., 1994, 1995, 1997) may also express EGFP.
Other areas of the CNS that showed significant EGFP expression included the neocortex and spinal cord. From our immunohistochemical analyses, EGFP-expressing neurons of the neocortex were found to share neurochemical features of their hippocampal counterparts. Since these EGFP-expressing neurons were almost exclusively restricted to layers II-IV and upper layer V, it is unlikely that they correspond to deep-layer Martinotti cells. These cells, however, may correspond to SOM-expressing regular-spiking nonpyramidal (RSNP) cells (Kawaguchi and Kubota, 1996, 1998; Kawaguchi and Shindou, 1998) and/or to the large, vertically oriented low-threshold spiking (LTS) interneurons described recently (Gibson et al., 1999).
Although a detailed immunohistochemical analysis has yet to be performed for the EGFP-expressing cells of the spinal cord, nearly, if not every, expressing cell was determined to be a neuron, as judged by labeling with anti-NeuN antibodies (data not shown). Furthermore, the vast majority of these dorsal horn neurons appeared to be bipolar, with either round or semicircular somata. As a subpopulation of dorsal horn neurons have previously been shown to express SOM (Dalsgaard et al., 1981; Ho and Berelowitz, 1984; Mizukawa et al., 1988), it is possible that these comprise the EGFP-expressing neurons in the spinal cord of GIN mice.
R-LM and P-LM cells: “input-biasing” interneurons
Based on their shared features, R-LM, P-LM, and O-LM cells may be considered as specialized subtypes of a broader category of SLM-projecting interneurons. As such, the primary function of these interneurons appears to be in the regulation of information flow coming from the entorhinal cortex to area CA1 via the perforant pathway. Since R-LM and P-LM cells have dendrites in SR, these interneurons likely receive excitatory input from CA3 Schaffer collaterals (Fig.10). As this input would be monosynaptic from CA3, the resultant inhibition on CA1 pyramidal cell distal dendrites in SLM may prove to be robust with respect to controlling information flow (see below). The strength of this inhibition may be further amplified by recurrent excitation of their dendrites in SO by CA1 pyramidal cells; but as R-LM and P-LM cell dendritic elaborations are much more prevalent in SR relative to SO, the Schaffer collateral input would appear to dominate the overall activity of these interneurons.
By virtue of the laminar restriction of their dendrites, O-LM cells, in contrast to R-LM and P-LM cells, should receive far less direct Schaffer collateral input. Instead, these cells have been shown to be activated directly by local CA1 pyramidal cells (Lacaille et al., 1987;Blasco-Ibáñez and Freund, 1995). Synaptic excitation, as well as spontaneous discharging, of CA1 pyramidal cells would subsequently excite O-LM cells, which in turn would lead to inhibition of pyramidal cell distal dendrites in SLM. Thus, O-LM cells would dampen entorhinal input via CA1 pyramidal cell activation from a variety of sources. O-LM cells may receive Schaffer collateral input, because a fraction of these fibers penetrate SO. However, the prevalence of input fibers from local CA1 pyramidal cells would appear to dominate the activity of these interneurons. In short, depending on the conditions, R-LM, P-LM, and O-LM cells likely perform parallel functions; however, the weights of the synaptic inputs onto these cells would indicate that the predominant functions of R-LM and P-LM cells versus O-LM cells are different.
So what might be the function of R-LM and P-LM cells in CA1 networks? As suggested by their morphologies, these interneuronal subtypes may function to isolate information flowing from CA3 to CA1 by selectively filtering out incoming information from the entorhinal cortex to CA1. This filtering may be accomplished via one or both of the following mechanisms. Most obvious is that GABAAreceptor-mediated IPSPs generated by these interneurons in CA1 pyramidal cell distal dendrites would lead to shunting, thus attenuating EPSPs derived from perforant pathway input. These interneurons may also limit Ca2+ influx via backpropagating action potentials in CA1 pyramidal cell distal dendrites (Traub et al., 1994; Christie et al., 1995; Magee and Johnston, 1995, 1997; Miles et al., 1996; Markram et al., 1997; Parra et al., 1998). In this scenario, Schaffer collateral excitation of R-LM and P-LM cells would produce IPSPs on CA1 pyramidal cell distal dendrites that may temporally coincide with backpropagating action potentials induced by Schaffer collateral excitation of CA1 pyramidal cells. Activation of these interneuronal subtypes may thus function to prevent Hebbian-like synaptic plasticity from occurring at perforant pathway inputs onto CA1 pyramidal cells, while permitting coincidence detection to occur at Schaffer collateral inputs.
Regardless of the mechanism or mechanisms used, the ability to selectively regulate synaptic efficacy of specific pathways could have significant impact on the information flow in hippocampal networks and possibly on the formation and consolidation of memories. In essence, R-LM and P-LM cells likely act as “input-biasing” interneurons.
Footnotes
This work was supported by National Institutes of Health Grants NS18309, NS34504, and NS37171, Mental Retardation Research Grant HD24064, and Texas Advanced Technology Program Grant 004949–030. We thank Dr. Paul Overbeek and Gabriele Schuster for their assistance in creating the transgenic mice, Paul Gardner for the synthesis of oligonucleotides, Jennifer Kramer at Omega Optical, for her assistance in selecting and custom-making filter sets, and Drs. Richard L. and Mary Y. Hurwitz for the generous use of laboratory space used in performing the molecular biology portions of this work. We also thank Drs. Coleen M. Atkins, Stephen Ginsberg, and Michael C. Crair for their critical comments and helpful suggestions in the preparation of this manuscript.
Correspondence should be addressed to Dr. John W. Swann, The Cain Foundation Laboratories, 6621 Fannin Street, MC 3–6365, Houston, TX 77030. E-mail: jswann{at}bcm.tmc.edu.