Novel and Transient Populations of Corticotropin-Releasing Hormone-Expressing Neurons in Developing Hippocampus Suggest Unique Functional Roles: A Quantitative Spatiotemporal Analysis

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The Journal of Neuroscience, September 15, 2001, 21(18):7171-7181

Novel and Transient Populations of Corticotropin-Releasing Hormone-Expressing Neurons in Developing Hippocampus Suggest Unique Functional Roles: A Quantitative Spatiotemporal Analysis
Yuncai Chen¹, Roland A. Bender¹, Michael Frotscher², and Tallie Z. Baram¹
¹ Departments of Anatomy/Neurobiology and Pediatrics, University of California at Irvine, Irvine, California 92697-4475, and ² Institute of Anatomy, University of Freiburg, D-79104 Freiburg, Germany

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Robust physiological actions of the neuropeptide corticotropin-releasing hormone (CRH) on hippocampal pyramidal neurons havebeen demonstrated, which may contribute to synaptic efficacy andto learning and memory processes. These excitatory actions ofthe peptide, as well as the expression of the CRH receptor typethat mediates them, are particularly prominent during early postnatallife, suggesting that endogenous CRH may contribute to processesinvolved in maturation of hippocampal circuitry. To further elucidatethe function(s) of endogenous CRH in developing hippocampus, weused neurochemical and quantitative stereological methods to characterizein detail CRH-expressing neuronal populations during postnatalhippocampal differentiation. These experiments revealed progressivelyincreasing numbers of CRH-expressing neurons in developing hippocampusthat peaked on postnatal day 11-18 and then declined drasticallyto adult levels. These cells belonged to several discrete populations,distinguished by GAD67 mRNA expression, morphology, and distinctspatiotemporal distribution profiles. Importantly, a novel populationof Cajal-Retzius-like CRH-expressing neurons was characterizedthat exists only transiently in early postnatal hippocampus andis positioned to contribute to the establishment of hippocampalconnectivity. These findings suggest novel, age-specific rolesfor CRH in regulating early developmental events in the hippocampalformation.

Key words: hippocampus; dentate gyrus; Cajal-Retzius cells; GAD; interneurons; neuropeptide; development; corticotropin releasing hormone; CRF

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The neuropeptide corticotropin-releasing hormone (CRH) functions as the primary regulator of the neuroendocrine responsesto stress (Vale et al., 1981). Hypothalamic CRH is released withinseconds of stress onset from terminals of peptidergic neuronsto influence pituitary hormonal secretion (Rivier et al., 1983;Yi and Baram, 1994). It has been increasingly recognized, however,that the actions of CRH are not confined to the neuroendocrine,hypothalamic-pituitary-adrenal system. Studies of the distributionof CRH in both adult and developing CNS have revealed the presenceof significant populations of CRH-expressing neurons in discretelimbic regions, in particular the central nucleus of the amygdala(Swanson et al., 1983; Gray and Bingaman, 1996) and the hippocampus(Swanson et al., 1983; Merchenthaler, 1984; Sakanaka et al., 1987;Yan et al., 1998). In addition, CRH has been shown to act directlyon central neurons (Aldenhoff et al., 1983; Valentino et al.,1983; Fox and Gruol, 1993; Curtis et al., 1995; Hollrigel et al.,1998), suggesting neuromodulatory roles for the peptide withintheCNS.

Whereas evidence from a number of studies indicates that amygdalar CRH may function in its traditional role as a mediatorof central stress responses (Swiergiel et al., 1993; Kalin etal., 1994; Hatalski et al., 1998; Merali et al., 1998), the roleof hippocampal CRH has remained obscure. In adult rat hippocampus,CRH expression has generally been considered to be confined toinhibitory interneurons (Swanson et al., 1983; Merchenthaler,1984; Smith et al., 1997; Yan et al., 1998). However, the physiologicalactions of CRH in hippocampus are excitatory (Aldenhoff et al.,1983; Smith and Dudek, 1994; Hollrigel et al., 1998). Thus, inthe presence of depolarizing input, activation of CRH-receptorsenhances the excitability of a neuron and increases its firingrate (Aldenhoff et al., 1983; Hollrigel et al., 1998).

Several observations indicate an enhanced excitatory potency of CRH during development. Administration of picomolar amountsof the peptide into the cerebral ventricles of immature rats producessevere seizures that last for several hours (Baram et al., 1992;Baram and Hatalski, 1998), whereas much higher doses (200-fold)are required to elicit excitatory discharges in the adult (Ehlerset al., 1983). The basis for this age-dependent effect of CRHis not fully understood (for review, see Baram and Hatalski, 1998)but may relate to the abundance of target receptors. Binding studies,as well as in situ hybridization histochemistry, have shown thatthe receptor mediating the excitatory effects of CRH on neurons,CRF₁ (Chalmers et al., 1995; Baram et al., 1997), is maximallyexpressed in immature hippocampus (400-600% of adult levels) (Pihokeret al., 1992; Avishai-Eliner et al., 1996). This presence of highlevels of CRH receptors during early postnatal development isintriguing and may also indicate specific roles for the peptideduring hippocampaldevelopment.

To further elucidate the function(s) of CRH in developing hippocampus, we set out to delineate and characterize in detailCRH-expressing neuronal populations that are prominent in, orconfined to, early postnatal development of the hippocampal formation.Using neurochemical and quantitative stereological methods, weestablished the increased abundance of CRH-expressing neuronsin developing hippocampus and discovered several distinct CRH-IRpopulations. Importantly, a population of Cajal-Retzius-like CRH-expressingneurons was characterized that exists only transiently in earlypostnatal hippocampus and is positioned to contribute to the establishmentof hippocampal connectivity. These findings suggest novel, age-specificroles for CRH in regulating early developmental events in thehippocampalformation.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals and tissue preparation. Immature Sprague Dawley-derived rats were born and maintained in a quiet, uncrowded, NationalInstitutes of Health approved facility on a 12 hr light/dark cycle,with access to lab chow and water ad libitum (Yi and Baram, 1994).On postnatal day 1 (P1), P5, P11, P18, or P80 (considering dayof birth as day 0), brains were harvested under relatively stress-freeconditions (Yan et al., 1998). Briefly, rats (n = 4 for each group)were left undisturbed for 24 hr before experiments and were thendeeply anesthetized with sodium pentobarbital (100 mg/kg, i.p.)within 45 sec of entry into the animal facility. Anesthetizedrats were removed to the laboratory and perfused using fresh 4%paraformaldehyde in 0.1 M sodium phosphate buffer (PB), pH 7.4(4°C). Brains were cryoprotected and stored as described previously(Chen et al., 2000) and then sectioned coronally into 20-µm-thickslices using a cryostat. To estimate the total number of CRH-IRneurons, consecutive sections throughout the entire hippocampuswere harvested in 0.1 M PB. For neuroanatomic orientation, 1 in8 (P1, P5, and P11), 1 in 10 (P18), or 1 in 12 (P80) sectionswere stained with cresyl violet. Adjacent series were processedfor immunocytochemistry (ICC) for CRH and calretinin, for in situhybridization (ISH) for glutamic acid decarboxylase 67 (GAD67)mRNA and reelin mRNA, or for coanalysis of these neurochemicalmarkers.

Immunocytochemistry. CRH-ICC was performed on free-floating sections using standard avidin-biotin complex methods as describedpreviously (Yan et al., 1998; Chen et al., 2000). Briefly, afterseveral washes with 0.01 M PBS containing 0.3% Triton X-100 (PBS-T),pH 7.4, sections were treated for 30 min in 0.3% H₂O₂-PBS, followedby blockade of nonspecific sites with 2% normal goat serum inPBS for 30 min. After rinsing, sections were incubated for 36hr at 4°C with rabbit anti-CRH antiserum [1:40,000; a gift fromDr. W. W. Vale (Salk Institute, La Jolla, CA)] in PBS containing1% bovine serum albumin and 2% normal goat serum and washed inPBS-T (three times for 5 min each). Sections were incubated inbiotinylated goat anti-rabbit IgG (1:200; Vector Laboratories,Burlingame, CA) in PBS for 1 hr at room temperature. After washing(three times for 5 min each), sections were incubated in the avidin-biotin-peroxidasecomplex solution (1:100; Vector Laboratories) for 2 hr and rinsed(three times for 5 min each), and the reaction product was visualizedby incubating the sections in 0.04% 3,3'-diaminobenzidine (DAB)containing 0.01% H₂O₂.

In situ hybridization. Digoxigenin (DIG)-labeled antisense and sense probes were generated from a pBluescript transcriptionvector containing rat GAD67 cDNA (Erlander et al., 1991) and frommouse reelin cDNA that was synthesized using PCR (Haas et al.,2000). GAD67- and reelin-ISH was performed as described previously(Bender et al., 2000; Haas et al., 2000). Briefly, sections werewashed with 2× SSC (0.3 M NaCl and 0.03 M Na-citrate) for 30 minand then subjected to an additional 30 min incubation in a solutioncomposed of 2× SSC-prehybridization solution (1:1). Prehybridizationtook place for 1 hr at 55°C in a humid chamber. The prehybridizationsolution consisted of 50% formamide, 4× SSC buffer, 5× Denhardt'ssolution, 5% dextran sulfate, 100 µg/ml yeast tRNA, and 100 µg/mlsalmon sperm DNA. For hybridization, DIG-labeled RNA probes wereadded, and sections were incubated at 55°C for at least 12 hr.For all steps, RNase-free solutions, sterile slides, and six-wellplates were used. After hybridization, sections were washed in2× SSC at room temperature (two times for 15 min each), 50% formamide-2×SSC at 65°C for 60 min, 50% formamide-0.1× SSC at 65°C for 60min, and 0.1× SSC at 65°C for 30 min, and hybrid molecules weredetected with an anti-DIG serum tagged with alkaline phosphataseaccording to the protocol of the manufacturer (Roche Products,Indianapolis, IN). Chromogens consisted of 4-nitro blue tetrazoliumchloride and 5-bromo-4-chloro-3-indolyl phosphate (Roche Products).The specificity of the hybridization reaction was verified bysubstituting labeled sense probe for the antisense probe and byomitting either the antisense probe or alkaline phosphatase-conjugatedantibody. No labeling was observed under theseconditions.

Combined ISH-ICC. For double labeling, free-floating sections were first processed for ISH according to the protocol describedabove. Sections were rinsed and then processed for CRH- or calretinin-ICC,as above, with minor modifications. For visualization of CRH orcalretinin immunoreaction, decreased concentrations of DAB (0.02%)and H₂O₂ (0.005%) were used. Sections were mounted on gelatin-coatedslides, air-dried, and coverslipped with Permount. To evaluatethe possibility of altered sensitivity or specificity attributableto combined ISH-ICC, sections processed only for ICC or ISH werecompared with matched sections processed for double labeling.No differences in intensity, distribution, or number of labeledcells wereobserved.

Double-labeling ICC. Free-floating sections were processed for concurrent immunolabeling using a modification of the dual-chromogenprocedure (Levey et al., 1986). Briefly, sections were first immunostainedfor CRH as described above, yielding a diffuse orange DAB reactionproduct. After CRH detection, sections were rinsed, incubatedin 5% normal horse serum for 30 min, and then exposed to calretininantiserum (1:20,000; Chemicon, Temecula, CA) for 36-48 hr at 4°C.Sections were incubated with biotinylated second antibody (1 hr),followed by the avidin-biotin complex solution (2 hr), rinsed,transferred to 0.01 M PB, pH 6.6, for 30-45 min, and then incubatedin a chromogen solution (0.025% Na-nitroprusside and 0.01-0.02%benzidine dihydrochloride in buffer). The blue granular reactionproduct was visualized by incubating sections for 3-5 min in asolution containing 0.003% H₂O₂. The reaction was stopped by rinsing(0.01 M PB with 0.3% Triton X-100, pH 6.6). The control measuresdescribed for the ISH-ICC procedure above to exclude altered sensitivityor specificity caused by the double-labeling procedure wereperformed.

Estimates of CRH-IR neurons. Total numbers of hippocampal CRH-IR neurons were estimated based on unbiased stereological principles(Sterio, 1984). For an unbiased determination of CRH-IR neurons,a systematic random series of sections (one in 8-12) throughoutthe entire anteroposterior extent of the hippocampal formationwas selected, yielding 14-20 sections per animal. The rostralsampling boundary was the first section containing both CA3 anddentate gyrus (DG) (for early postnatal ages, see Paxinos et al.,1991, their Fig. 92; for older ages, see Paxinos and Watson, 1982,their Fig. 18). The caudal boundary consisted of sections no longercontaining hippocampal subdivisions (Paxinos et al., 1991, theirFig. 111; or Paxinos and Watson, 1982, their Fig. 28). The majorhippocampal subdivisions analyzed were CA1, CA3, and the dentategyrus, defined according to Freund and Buzsáki (1996). Cell nucleiwere counted using the "optical dissector" technique (Gundersenet al., 1988; West, 1999) relying on the leading edges of nucleiin each section. After inspection of CRH-IR neurons in each ofthe hippocampal subdivisions under 20× magnification, countingwas performed under a 100× oil immersion objective (numericalaperture, 1.4). The relatively small numbers of CRH-IR cells permittedcounting of all such neurons in all hippocampal subdivisions ofeach sampledsection.

Colocalization analyses. Colocalization of CRH with GAD67 mRNA, reelin mRNA, or calretinin was determined in eight sectionsper animal (two animals per age group). Counting was performedunder 60× magnification, distinguishing the perinuclear blue mRNAlabel from the homogenous, orange-brown cytoplasmic CRHimmunostain.

5'-Bromodeoxyuridine protocol and cell fate analysis. Timed-pregnant females were injected intraperitoneally with two dosesof 5'-bromodeoxyuridine (BrdU) (50 mg/kg body weight; Sigma, St.Louis, MO) on embryonic day 10 (E10), E11, E12, or E13 to encompassthe time of generation of pioneer neurons in strata radiatum (sr)and lacunosum moleculare (Supèr et al., 1998). Offspring wereperfused transcardially with 4% paraformaldehyde at P1, P5, orP11. Brains were harvested and cut as described above. For detectionof BrdU-labeled nuclei, sections were first treated with the followingDNA denaturation steps: 2 hr incubation in 50% formamide-2× SSCat 65°C, 10 min rinse in 2× SSC, 30 min incubation in 2N HCl at37°C, and 10 min rinse in 0.1 M sodium borate, pH 8.5. Sectionswere rinsed in PBS-T and incubated with monoclonal rat anti-BrdU(1:2000; 20-24 hr; Accurate Chemicals, Westbury, NY). After rinsingin PBS-T, sections were incubated with biotinylated goat anti-ratIgG (1:1000; 1 hr; Chemicon), followed by the avidin-biotin complexsolution (1:100; 2 hr; Vector Laboratories). For BrdU single labeling,the reaction product was visualized using DAB as chromogen (yieldingbrown nuclei). For CRH-BrdU double labeling, sections were firstimmunostained with rabbit anti-CRH (yielding a brown DAB reactionproduct), followed by anti-BrdU as described above, using DAB-nickelto yield a black reactionproduct.

Initial evaluations indicated that 18-20% of CRH-positive Cajal-Retzius cells were labeled with BrdU when animals receivedthe BrdU injections at E12, consistent with numbers expected ifthe majority of these cells were born on this date. Thus, progenyof E12 injected rats were used for cell fate analysis. Every eighthsection of the dorsal hippocampus (8-10 sections per rat, threerats per age) was selected. Cells containing BrdU-labeled nucleiand CRH-BrdU cells were counted in the outer molecular layer (ml)of the dentate gyrus and in a two cell body wide zone of stratumlacunosum moleculare (slm) abutting the hippocampal fissure. Dataare expressed as number of cells per section (BrdU) or per eightsections (see Fig. 7F, CRH-BrdU).

Statistical analysis. Results are presented as mean ± SEM. The effect of age was determined using a one-way ANOVA, followedby either Newman-Keuls or Dunnett's multiple comparison post hoctests. In all cases, significance levels were set at p < 0.05.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Spatiotemporal analysis of the distribution of CRH-IR neurons in the developing hippocampus

CRH-IR neurons were found in the hippocampal formation as early as P1 (Figs. 1A, 2A). The total number of CRH-IR neurons inthe hippocampal formation increased progressively during postnataldevelopment, peaking at P18 (Figs. 2A, 3A,B,E,F, 4B), and decliningthereafter to result in substantially fewer CRH-IR neurons inadult hippocampus (P80) (Figs. 1F, 2A, 4C). The spatiotemporalexpression profile of CRH was highly heterogenous, so that individualsubfields and layers of the hippocampal formation contributeddifferentially to the overall quantitative pattern of CRH expression(Figs. 1, 2B--D). In particular, the distribution of CRH-IR neuronsduring the earlier postnatal time points was striking. The tworegions in developing hippocampus that correspond to the marginalzone in neocortex, CA1 slm and the ml of the DG, contained a prominentpopulation of CRH-IR neurons that was concentrated along the hippocampalfissure (Figs. 1A-C, 2B,D, 4D). Indeed, on P1, the number of CRH-IRneurons located near the hippocampal fissure significantly exceededthat in any other hippocampal subfield (Figs. 1A, 2B-D, 4A). ThisCRH-IR neuronal population was still quite robust on P5 (Figs.1B, 2B-D) but declined rapidly by P11 (Figs. 1C, 2B-D, 4E). Inhippocampi from P18 and older animals, relatively few CRH-IR cells(981 ± 157 in the adult compared with 4568 ± 302 on P1, or 21.4%)remained in these former marginal zones (Figs. 2B-D, 4F).

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Figure 1. Distinct populations of CRH-IR neurons in hippocampal CA1 demonstrate a highly age-dependent spatiotemporal distribution pattern. A, As evident in a section from a P1 rat, a dense population of CRH-expressing neurons inhabits slm, abutting the hippocampal fissure (demarcated by asterisks). Rare CRH-IR cells are found in sr and virtually none in sp or so. B, On P5, the morphologically heterogenous CRH-IR neuronal population in slm remains abundant, and more neurons are located also in sr. C, A remarkable decline in the CRH-IR neuronal population residing in slm is evident by P11. In contrast, CRH-expressing neurons occupy the pyramidal cell layer by this age. A more detailed view of this layer from a P11 rat is shown in D, demonstrating CRH-expressing somata, consistent with basket cells (these cells coexpress GAD67 mRNA; see Fig. 3A,B), as well as an axonal plexus outlining the CRH-negative pyramidal cells. E, On P18, the population of CRH-IR interneurons residing in the sp is maximal. Their dense innervation of the pyramidal cells themselves is apparent. F, In adult CA1, few CRH-IR neurons are found in the pyramidal cell layer, consistent with the literature, and the numbers of CRH-expressing neurons is low in other hippocampal layers as well (see Fig. 2 for quantitative analysis). Scale bar, 90 µm.

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Figure 2. Quantitative analysis of total numbers and regional distribution of CRH-expressing neurons in the developing rat hippocampal formation. A, Age-specific estimates, based on stereological analysis (see Materials and Methods), of the total numbers of CRH-IR neurons demonstrate progressive increase from P1 to P18, with a subsequent decline to adult levels. ANOVA indicates a significant effect of age (F = 45.20; p < 0.0001). These overall values represent the sum of several distinct cell populations that occupy specific layers and regions of the developing hippocampus. B, In CA1, the number of CRH-expressing neurons located in the slm peaks on P5 and declines to 16% of P5 values by adulthood. Conversely, the numbers of CRH-expressing neurons in the sp on P18 is >200-fold higher than on P1 and 220% of adult values. C, D, The distinct spatio-developmental profiles of several CRH-IR neuronal populations is reflected also in CA3 (C) and the dentate gyrus (D). Peak numbers of CRH-IR interneurons (see Fig. 3A,B) occupy the principal cell layers on P18; in contrast, the population of CRH-expressing (non-GABAergic) cells near the hippocampal fissure [slm and outer molecular layer (oml)] decline precipitously with age. iml, Inner molecular layer. Values are presented as mean ± SEM for four rats per age group.

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Figure 3. The majority of CRH-expressing neuronal populations in the principal hippocampal cell layers coexpress GAD67 mRNA, indicating their function as interneurons. A, C, and E are sections labeled for CRH-IR; B, D, and F, demonstrate CRH-IR (orange) and GAD67 mRNA (blue). A and B demonstrate that, in the sp of the P18 rat, CRH-IR neurons are abundant, and virtually all coexpress GAD67 mRNA (arrowheads). C, D, In stratum oriens of the P5 rat, most CRH-IR neurons are GABAergic (arrowheads). E, F, In the dentate gyrus hilus of the P18 rat, a mixed population of CRH-IR neurons comprises both GABAergic (arrowheads) and GAD67-negative (arrow) cells. Also seen are numerous GABAergic interneurons bordering the granule cell layer that do not express CRH. Scale bar, 25 µm.

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Figure 4. Populations of CRH-IR neurons in hippocampal CA3 (A-C) and dentate gyrus (D-F) demonstrate a highly age-dependent spatiotemporal distribution pattern. A-C are sections derived from animals on P1, P18, and P80, respectively. A, On P1, most CRH-IR neurons congregate near the hippocampal fissure and rarely occupy the sp. B, Numerous CRH-IR neurons are located in sp on P18. C, By P80, the pyramidal cell layer is depleted of CRH-IR neurons. D-F, A remarkable "migration" of CRH-IR neurons is evident within the dentate gyrus. D, On P1, most are concentrated along the hippocampal fissure (asterisks) in the molecular layers. E, By P11, few CRH-IR neurons are observed in the outer (oml) and inner (iml) molecular layers; instead, these cells reside in the gl and hilus. F, By P18, the majority of CRH-expressing neurons occupy the hilus. Scale bars: A-C, 150 µm; D-F, 160 µm.

The populations of CRH-IR neurons in the principal cell layers [pyramidal and granule cell layer (gl)], as well as in strataoriens (so), sr, and the hilus demonstrated a diametrically oppositetrend compared with that of CRH-IR neuronal populations residingnear the hippocampal fissure. CRH-expressing neurons were virtuallyabsent in stratum pyramidale (sp) and gl on P1 (Figs. 1A, 2B-D,4A,D) and were rare on P5 (Figs. 1B, 2B-D). Their numbers increasedprogressively with age until P18 (Figs. 1E, 2B-D, 3A,B, 4B) anddeclined thereafter. A similar trend was found for CRH-IR neuronalpopulations located in so, sr, and in the hilus (Fig. 2B-D). Thus,the total number of CRH-IR neurons was maximal in the immature(P11 and P18) hippocampal formation, peaking at ~200% of adultvalues. In addition, the overall increase in the total numberof CRH-IR neurons in the hippocampal formation during the first3 postnatal weeks was attributable to an absolute and dramaticrise in the number of CRH-IR neurons in the principal and polymorphlayers (Fig. 2B,C, so, sr, and hilus), which overrode the drasticloss of CRH-IR neurons located in the slm andml.

Neurochemical characterization reveals a transient, non-GABAergic population of CRH-IR neurons in the developing hippocampus

To characterize the functional properties of CRH-IR neurons in the developing hippocampal formation, we combined CRH-ICC withISH for GAD67 mRNA, a marker for GABAergic neurons (Houser andEsclapez, 1994). This analysis revealed that CRH-IR neurons presentin the early postnatal hippocampus represented at least two clearlydistinguishable populations; the large majority of CRH-IR neuronsin the principal cell layers, as well as in so, sr, and hilus,coexpressed GAD67 mRNA, suggesting that they functioned as GABAergiclocal circuit neurons (Figs. 3, 5A,B). In contrast, CRH-IR neuronslocated near the hippocampal fissure rarely coexpressed GAD67mRNA (Figs. 5, 6B,H). Quantitative analysis of CRH-IR neuronscolocalizing GAD67 mRNA at different ages (Fig. 5) better illustratedthe fate of this population during development compared with thatof non-GABAergic CRH-IR cells. Thus, on P5, the proportion oftotal hippocampal CRH-IR neurons coexpressing GAD67 mRNA was only43% as a result of the large contribution of GAD67 mRNA-negativeCRH-IR neurons in slm and ml. By P11, however, 75% of all CRH-IRneurons coexpressed GAD67 mRNA (Fig. 5), indicating a doublingof GABAergic CRH-IR populations compared with P5. Because thetotal number of CRH-IR neurons increased only by 37% (Fig. 2A),this proportional increase of GABAergic CRH-IR neurons must haveresulted from a sum of two independent processes: first, a progressiveincrease in the numbers of GAD67 mRNA-CRH colocalizing neuronsin principal and polymorph cell layers; second, a decline of theGAD67 mRNA-negative-CRH-IR population in slm and ml.

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Figure 5. Quantitative analysis of GAD67 mRNA expression defines separate hippocampal CRH-expressing neuronal populations, with distinct spatial and age-dependent distribution profiles. Plotting GABAergic CRH-immunoreactive neurons as a proportion of total peptide-expressing cells reveals that the former provide the major contribution to the striking increase of CRH-expressing cells in the principal cell layers between P1 and P18. In contrast, the transient populations in the hippocampal marginal zones [slm and outer molecular layer (oml)] are non-GABAergic. Mixed populations reside in the polymorphic layers, sr, and the inner molecular layer (iml). Quantitative data were derived from eight sections per rat (see Materials and Methods) and two animals per age group.

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Figure 6. CRH-expressing Cajal-Retzius-like neurons demonstrate unique neurochemical characteristics. A, CRH-immunoreactive neurons in the outer molecular layer of the dentate gyrus of the P5 rat (arrow) are aligned along the hippocampal fissure (asterisks) and possess a prominent thick dendrite with branches descending to the pial surface, typical of Cajal-Retzius cells. B, These Cajal-Retzius cell-like CRH-IR neurons (straight arrow) do not coexpress GAD67 mRNA (curved arrows). C, D, CRH-IR Cajal-Retzius-like neurons (arrows) do not coexpress neurochemical markers ascribed to subpopulations of rat Cajal-Retzius cells: calretinin (C), shown as granular black deposits (curved arrows) or reelin mRNA (D, curved arrows). E, F, In contrast, neurons colocalizing calretinin and reelin mRNA (arrowheads) are frequently observed near the hippocampal fissure. G, H, CRH-expressing neurons in the inner molecular layer of the dentate gyrus are morphologically distinct from the Cajal-Retzius-like population abutting the hippocampal fissure but demonstrate similar neurochemical characteristics and do not coexpress GAD67 mRNA (blue, curved arrows). Scale bar, 25 µm.

A transient CRH-IR neuronal population near the hippocampal fissure possesses the neuroanatomical features of Cajal-Retzius cells

In addition to their patterns of GAD67 expression, hippocampal CRH-expressing neurons could be characterized as discrete populationsbased also on morphological, neurochemical, and localization criteria.Thus, CRH-IR neurons in slm and ml of the P1 and P5 rat belongedto two morphologically distinct populations. The first populationconsisted of small (8-12 µm) multipolar neurons (Figs. 1A,B, 6G,H),with varied orientation. These neurons, primarily GAD67 mRNA negative,were mainly observed in slm and in the inner ml of DG, usuallyat some distance from the hippocampal fissure. The second populationconsisted of neurons with a typical morphology described for rodentCajal-Retzius cells (Derer and Derer, 1990) (Fig. 6A-D): largebipolar neurons, with one prominent dendrite oriented horizontallyto the pial surface and fine appendages descending from the dendriteand soma toward the hippocampal fissure (and pia). This populationwas located close to the hippocampal fissure in slm and in theouter ml of DG and was virtually always devoid of GAD67 mRNA expression(Fig. 6B). Both populations were robust on P1 and P5 but declineddrastically by P11 and later ages (Figs. 1A-C, 2B-D,5).

Transient Cajal-Retzius-like CRH-IR neurons near the hippocampal fissure demonstrate a unique neurochemical profile

To better characterize the neurochemical identity of these transient CRH-IR neurons, and guided by their morphology, we determinedwhether they coexpressed neuronal markers for Cajal-Retzius cells.The extracellular matrix protein reelin has been proposed recentlyas a typical product of these cells (D'Arcangelo et al., 1995;Hirotsune et al., 1995; Ogawa et al., 1995). In situ hybridizationhistochemistry revealed that reelin mRNA-expressing neurons wereabundant in the developing hippocampus (P5 and P11), both adjacentto the hippocampal fissure as well as in other hippocampal regions.These results, in concordance to other recent studies (Alcántaraet al., 1998; Haas et al., 2000), indicate that reelin is notexclusively produced and secreted by Cajal-Retzius cells. Importantly,although Cajal-Retzius-like cells expressing reelin were intermingledwith those expressing CRH near the hippocampal fissure, no coexpressionof these two molecules by a single neuron was demonstrated (Fig.6D).

As a second neuronal marker for Cajal-Retzius cells, we studied colocalization of CRH in these neurons with the calcium bindingprotein calretinin. Calretinin has been shown to be a specificneuronal marker for Cajal-Retzius cells in mice (Del Río et al.,1995) and is expressed by a subpopulation of Cajal-Retzius cellsin rat hippocampus, where it also labels other neuronal populations(Jiang and Swann, 1997). However, whereas colocalization of calretininand CRH was occasionally observed in multipolar neurons localizedto the inner ml (data not shown), it was never observed in CRH-IRCajal-Retzius cell-like neurons in the outer ml (Fig. 6C). Itshould be noted that coexpression of calretinin and reelin mRNAwas observed frequently in neurons with Cajal-Retzius-like morphologynear the hippocampal fissure (Fig. 6E,F), consistent with theirneurochemical identity and validating the methodology used fordouble labeling of the cells we identified as Cajal-Retzius-like.Together, these findings indicate that the transient populationof CRH-IR neurons with Cajal-Retzius cell-like morphology in themarginal zones (slm and ml) of the early postnatal hippocampalformation constitutes a distinct subclass of Cajal-Retzius cellswith unique neurochemical and consequent functionalproperties.

Disappearance of transient CRH-IR Cajal-Retzius cells is attributable to their death rather than to phenotype change

Several possible mechanisms may account for the disappearance of the CRH-expressing Cajal-Retzius cells. First, these neuronsmay change their phenotype and cease expressing detectable amountsof CRH. Alternatively, these neurons may die, as shown for othersubpopulations of Cajal-Retzius cells (Del Río et al., 1995).To distinguish between these two fates, we performed a birth-datingstudy, using BrdU injection on E10-E13, days overlapping birthof hippocampal Cajal-Retzius cells in mouse (Supèr et al., 1998)and before the birth of most GABAergic neurons in the rat (E14)(Amaral and Kurz, 1985; Dupuy and Houser, 1997). In animals injectedon E12, 18-20% of CRH-expressing cells with Cajal-Retzius cellmorphology were also BrdU labeled. Because BrdU is available onlyfor a limited time (Takahashi et al., 1992), this high proportionof BrdU labeling in CRH-positive neurons indicates that the injectionoccurred during the peak generation time of this neuronal population,which also concurs with the peak generation of Cajal-Retzius cellsin general (Supèr et al., 1998). Numbers of BrdU-CRH-labeledcells were analyzed on P1, P5, and P11 and were compared withthose labeled with BrdU alone. As evident from Figure 7A, manyBrdU-labeled cells resided near the hippocampal fissure in theP1 rat. Their numbers decreased progressively by P5 and P11 (Fig.7B,C). CRH-expressing, BrdU-labeled cells were also abundant inP1 (Fig. 7D), decreased by P5 (Fig. 7E), and were rarely observedby P11. Importantly, as shown in Figure 7F (left) CRH-BrdU double-labeledneurons disappeared from the hippocampal fissure at a rate similarto the disappearance rate of the population labeled with BrdUalone. The latter population, representing Cajal-Retzius cells,was found to undergo cell death (Del Río et al., 1995). It shouldbe noted that the ratio of cells labeled for both CRH and BrdUto cells labeled with CRH alone (CRH-BrdU/CRH) remained quiteconstant (Fig. 7F, right), indicating that the double-labeledcells are representative of the total CRH-expressing Cajal-Retziuspopulation. In addition, hippocampal growth that occurred betweenP1 and P11 (on P5, 110% of P1; on P11, 140% of P1) was insufficientto account for the drastic reduction in the numbers of BrdU (andBrdU-CRH) -labeled cells.

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Figure 7. The Cajal-Retzius-like CRH-expressing population, born on E12, disappears at the same rate and time course of other (CRH-negative) Cajal-Retzius cell populations, likely via death. A-C, Cells born on E12 (labeled by BrdU injected on that day) are abundant in the hippocampal fissure (asterisks) of animals examined on P1 (A) and P5 (B). A striking reduction in BrdU labeling is found by P11 (C). D, E, BrdU-labeled CRH-like Cajal-Retzius neurons (arrowheads) at P1 (D) and P5 (E). F, Left, Quantitative analysis of cells labeled with both CRH and BrdU compared with those labeled by BrdU alone suggests that these populations disappear at the same rate and time course. Numbers of BrdU single-labeled cells are shown as black bars and are expressed per one section; numbers of CRH-BrdU double-labeled cells are shown as white bars and are expressed per eight sections. Right, The ratio of CRH-expressing Cajal-Retzius cells born on E12 to Cajal-Retzius-like CRH neurons [(CRH $-$ BrdU)/CRH] is similar in the three age groups, indicating that Cajal-Retzius-like CRH neurons labeled with BrdU are representative of the total population of CRH-expressing pioneer cells. Put together, these panels indicate that the fate of BrdU-CRH-labeled Cajal-Retzius cells and of the total CRH-expressing Cajal-Retzius cells conforms to the fate (death) of the general population of Cajal-Retzius cells in the hippocampal fissure. Scale bars: A-C, 50 µm; D, E, 40 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The major results of this study are as follows. (1) CRH-IR neurons are significantly (twofold) more abundant in the immaturecompared with the adult rat hippocampus. (2) Based on anatomicaland neurochemical criteria, a minimum of two populations of CRH-expressingneurons can be clearly distinguished in the developing hippocampus:a subclass of GABAergic (GAD67 mRNA-expressing) interneurons andan apparently transient population of non-GABAergic neurons concentratednear the hippocampal fissure. (3) A significant proportion ofthe CRH-IR non-GABAergic neurons possess the characteristic morphologyof hippocampal Cajal-Retzius cells, and, like them, are born earlyin development and most die by the end of the second postnatalweek. However, these cells express a unique neurochemical profile,suggesting distinct functional role(s). Together, these findingssuggest that CRH may be involved in age-specific processes thatcontribute to postnatal hippocampalmaturation.

Abundance of CRH-IR neurons and its potential relationship to the enhanced excitability of the developing hippocampus

Excitability in the immature hippocampus circuit is generally considered to be enhanced compared with that of the adult, andseveral mechanisms have been suggested to account for this phenomenon(Swann, 1995; Ben-Ari et al., 1997; Holmes, 1997; Baram and Hatalski,1998). The results of this study suggest that CRH, released fromabundant CRH-IR hippocampal neurons, could contribute disproportionatelyto excitability in immature versus adult hippocampus (Baram andHatalski, 1998).

An endogenous population of CRH-expressing neurons in the hippocampus has first been described in adult rat (Swanson et al.,1983; Merchenthaler, 1984; Sakanaka et al., 1987) and was recentlyalso identified in immature rat (P10-P13) (Yan et al., 1998).Colocalization studies demonstrated that the large majority ofthese CRH-IR neurons were GABAergic interneurons, primarily basketor chandelier cells (Yan et al., 1998). These interneurons, synapsingon somata or axon initial segments of pyramidal neurons, typicallyplay a key inhibitory role, modulating the output of the pyramidalcells (Soltesz et al., 1995). However, the physiologic actionsof CRH in hippocampus are excitatory (Aldenhoff et al., 1983;Hollrigel et al., 1998): in hippocampal slices, the peptide significantlyincreases firing rates of hippocampal pyramidal cells in the presenceof an excitatory stimulus, essentially "amplifying" this input.In the absence of depolarizing input, CRH has little effect onthe excitability of the network. Thus, although in some brainregions CRH may act directly as an excitatory neurotransmitter(Ehlers et al., 1983; Rainnie et al., 1992; Weiss et al., 1993;Curtis et al., 1995), in hippocampus its function may best bedescribed as that of an excitatory neuromodulator. Therefore,release of the peptide from the relatively large numbers of CRH-IRinterneurons in principal cell layers should contribute significantlyto excitability of immaturehippocampus.

This enhancement of glutamatergic synaptic transmission by CRH may contribute to physiological hippocampal processes of learningand memory (Lee et al., 1992, 1996; Baram and Hatalski, 1998)or stress responses (Hatalski et al., 2000). However, if releasedin excess, CRH may lead to pathological overexcitation of theimmature hippocampus, as evident from the induction of prolongedseizures (involving hippocampus) by picomolar doses of CRH administeredinto the cerebral ventricles of immature rats (Baram et al., 1992;Baram and Hatalski, 1998). This may be attributable to the factthat, in addition to abundant CRH-IR neurons, expression levelsof the CRH-receptor CRF₁ [the receptor mediating excitatory actionsof the peptide (Chalmers et al., 1995; Baram et al., 1997)] arefourfold to sixfold higher in immature compared with mature hippocampus(Pihoker et al., 1992; Avishai-Eliner et al., 1996). Thus, thepresent study demonstrates that the spatiotemporal profile ofneurons providing an endogenous ligand for CRH receptors in hippocampusparallels the expression profile of receptor mRNA. Interestingly,during the second and third postnatal weeks, both endogenous ligandand the CRF₁ receptor are particularly abundant in the CA3 pyramidallayer (Avishai-Eliner et al., 1996) (Figs. 2C, 4B, 5B). CA3 pyramidalneurons have been shown to be particularly excitable at that age(Swann, 1995), at least partially because of dense recurrent innervationby axonal branches that are later pruned (Gomez-Di Cesare et al.,1997). Activation of CRF₁ receptor on the somata of these CA3pyramidal cells (Chen et al., 2000) by CRH that is released frominterneurons, thus provides a molecular machinery that may contributeto heightened excitability and seizure propagation during thisdevelopmental epoch. These effects of CRH may be important incertain age-specific developmental seizure disorders in the human(for review, see Baram and Hatalski, 1998).

Potential developmental roles of GABAergic CRH-IR neurons in hippocampus

The decline of the GABAergic CRH-IR population after the third postnatal week raises the question of the role that CRH mightplay during hippocampal maturation. Interestingly, similar expressionprofiles have also been reported for other neuropeptides; levelsof somatostatin, cholecystokinin, neuropeptide Y, and cortistatinreach a peak in the second and third postnatal weeks and thendecrease to adult values (Cho et al., 1983; Allen et al., 1984;Naus et al., 1988; de Lecea et al., 1997). The second and thirdpostnatal weeks are a period of major maturational transitionsin the hippocampal formation. For example, during the first postnatalweek, hippocampal neuronal activity is mediated primarily by thedepolarizing actions of GABA. GABAergic neurotransmission is thentransformed into hyperpolarizing effects, and functional excitatoryglutamatergic synaptic transmission is established (Ben-Ari etal., 1989; Hosokawa et al., 1994; Durand et al., 1996; Ben-Ariet al., 1997). This "switch" is accompanied by transient hyperexcitabilityof the hippocampal network (Gomez-Di Cesare et al., 1997). Inthese circumstances, alternative means of modulation of excitationand inhibition, provided by neuropeptides (e.g., CRH versus neuropeptideY or somatostatin), might be advantageous. Once hippocampal maturationhas been completed, this mechanism may become less important,resulting in neuropeptide downregulation. These may be reinducedin the adult by extreme neuronal activity (Gall et al., 1990;Schwarzer et al., 1996).

The nature and fate of Cajal-Retzius cell-like CRH-IR neurons in developing hippocampus

An unexpected result of our study was the discovery of a population of CRH-IR neurons in the developing hippocampus that,with respect to location, morphology, and neurochemical phenotype,was clearly distinguishable from the population of GABAergic CRH-IRinterneurons. These neurons were located exclusively in slm ofCA1 and ml of DG and were concentrated near the hippocampal fissure.Many of these cells had the characteristic morphology of Cajal-Retziuscells, and like them, did not express GAD67 mRNA. However, whereasmany (D'Arcangelo et al., 1995; Hirotsune et al., 1995; Ogawaet al., 1995) but not all Cajal-Retzius cells (Meyer et al., 1998)have been shown to express and secrete the glycoprotein reelin,CRH-immunoreactive Cajal-Retzius-like neurons did not coexpressreelin.

Cajal-Retzius cells have been shown to arise and die primarily within a defined developmental epoch (Soriano et al., 1994;Del Río et al., 1995; Drakew et al., 1998). Thus, Cajal-Retziuscells are the first neurons to differentiate in the developingcortex (Edmunds and Parnavelas, 1982; Marín-Padilla, 1984; Dererand Derer, 1990; Del Río et al., 1995; Meyer et al., 1998). Theyreside within the marginal zone of immature neocortex and disappearalmost completely from this zone during its transformation tothe cell-poor layer I, probably by degeneration (Derer and Derer,1990). The hippocampal equivalents of the marginal zones (andneocortical layer I) are slm of hippocampus proper and the outerml of DG. Both are densely populated by Cajal-Retzius cells duringhippocampal formation, but, as in neocortex, most of these cellsdegenerate progressively with maturation (Del Río et al., 1995).The data presented here indicate that CRH-immunoreactive Cajal-Retziuscells demonstrate the same distinctive lifeprofile.

The dates of birth and the fate of CRH-immunoreactive Cajal-Retzius cells support their designation as a distinct transientpopulation of pioneer cells. Whereas the majority of GABAergicinterneurons in the same regions are born at approximately E14in the rat (Amaral and Kurz, 1985; Dupuy and Houser, 1997), CRH-immunoreactiveCajal-Retzius cells are likely born at approximately E12 (Fig.7). A progressive disappearance of cells labeled by BrdU injectionon E12 (born on that day) was evident (Fig. 7F), and the rateof disappearance of CRH-negative and CRH-expressing cells wassimilar. This is not consistent with a phenotypic change of CRH-immunoreactiveCajal-Retzius cells (which would have resulted in a steeper slopeof disappearance of CRH-expressing cells, with a "transformation"of double-labeled into single BrdU-labeled cells) and indicatesthat, similar to other subpopulations (Del Río et al., 1995),CRH-immunoreactive Cajal-Retzius likelydie.

Potential function of CRH-expressing Cajal-Retzius cells

Recent data indicate roles for hippocampal Cajal-Retzius cells in the pathfinding of entorhinal axons (Ceranik et al., 2000a)and as transient postsynaptic targets for these axons (Del Ríoet al., 1997). These actions of Cajal-Retzius cells may involvereelin, as evident from the severe cytoarchitectonic malformationsin reelin-deficient (reeler) mice (for review, see Frotscher,1998). However, our demonstration that a considerable proportionof hippocampal Cajal-Retzius cells does not express reelin indicatesthat this cell class is comprised of several subpopulations, withdistinct neurochemical profiles and likely nonoverlapping functions(Ceranik et al., 2000b). Indeed, two temporally distinct populationsof neocortical Cajal-Retzius cells, one reelin-expressing andthe other reelin-negative, have been described recently (Meyeret al., 1998). The relationship of the CRH-expressing reelin-negativehippocampal Cajal-Retzius cell to these neocortical populationsrequires additionalstudy.

What function could CRH-secreting Cajal-Retzius cells serve during hippocampal differentiation? slm and ml are innervatedprenatally by ingrowing entorhinal cortex axons (Supèr and Soriano,1994; Supèr et al., 1998). In the absence of their definitivepostsynaptic targets (pyramidal and granule cell dendrites), theseaxons form transient synapses on Cajal-Retzius cells that provideguidance and synaptic targets (Del Río et al., 1997). However,at least certain subpopulations of cortical and hippocampal Cajal-Retziuscells have be shown recently to be physiologically active andto fire action potentials (Zhou and Hablitz, 1996; Aguiló etal., 1999, Mienville, 1999; Ceranik et al., 2000b). Indeed, theirintegration into the maturing network may trigger their death,because it is prevented by pharmacological blockade of NMDA receptors(Mienville and Pesold, 1999) or by elimination of entorhinal input(Del Río et al., 1996). Therefore, it was suggested recently(Mienville, 1999) that Cajal-Retzius cells may contribute to twocritical aspects of circuit maturation: an early (perhaps reelin-dependent)(but see Ceranik et al., 2000b) phase of neuronal pathfindingand initial arborization, and a subsequent, activity-dependentphase promoting appropriate synaptogenesis. In this later, reelin-independentphase, the synaptic potentiation actions of CRH could play animportantrole.

In summary, the abundance of CRH-IR neurons in early postnatal hippocampus supports its potent physiological actions on developinghippocampal neurons and is consistent with important functionsof the peptide during the "hyperexcitable" epoch of hippocampalmaturation. In addition, the discovery of a novel, early and transientpopulation of CRH-expressing Cajal-Retzius cells provides evidencefor a much earlier contribution of CRH to processes underlyingthe progressive evolution of the hippocampusformation.

  FOOTNOTES

Received Jan. 17, 2001; revised June 15, 2001; accepted June 27, 2001.

This work was supported in part by National Institutes of Health Grant NS 28912 (T.Z.B.) and the Deutsche Forschungsgemeinschaft(M.F.). We thank Drs. C. A. Haas and A. Tielsch for providingreelin cDNA and Drs. N. J. K. Tillakaratne and A. J. Tobin fortranscription vectors containing GAD67cDNA.
Correspondence should be addressed to Dr. Tallie Z. Baram, Departments of Anatomy/Neurobiology and Pediatrics, Universityof California at Irvine, Irvine, CA 92697-4475. E-mail: tallie{at}uci.edu.

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