Anatomical Distribution and Cellular Basis for High Levels of Aromatase Activity in the Brain of Teleost Fish: Aromatase Enzyme and mRNA Expression Identify Glia as Source

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The Journal of Neuroscience, November 15, 2001, 21(22):8943-8955

Anatomical Distribution and Cellular Basis for High Levels of Aromatase Activity in the Brain of Teleost Fish: Aromatase Enzyme and mRNA Expression Identify Glia as Source
Paul M. Forlano¹, David L. Deitcher¹, Dean A. Myers², and Andrew H. Bass¹
¹ Department of Neurobiology and Behavior, Cornell University, Ithaca, New York 14853, and ² Department of Physiology, College of Medicine, Oklahoma University Health Science Center, Oklahoma City, Oklahoma 73190

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although teleost fish have higher levels of brain aromatase activity than any other vertebrate group, its function remainsspeculative, and no study has identified its cellular basis. Aprevious study determined aromatase activity in a vocal fish,the plainfin midshipman (Porichthys notatus), and found highestlevels in the telencephalon and lower levels in the sonic hindbrain,which was dimorphic between and within (males) sexes. We havenow localized aromatase-containing cells in the midshipman brainboth by immunocytochemistry using teleost-specific aromatase antibodiesand by in situ hybridization using midshipman-specific aromataseprobes. Aromatase-immuno-reactivity and mRNA hybridization signalare consistent with relative levels of aromatase activity in differentbrain regions: concentrated in the dimorphic sonic motor nucleus,in a band just beneath the periaqueductal gray in the midbrain,in ventricular regions in the hypothalamus, and highest levelsin the telencephalon especially in preoptic and ventricular areas.Surprisingly, double-label immunofluorescence does not show aromatase-immunoreactivecolocalization in neurons, but instead in radial glia throughoutthe brain. This is the first study to identify aromatase expressionmostly, if not entirely, in glial cells under normal rather thanbrain injury-dependent conditions. The abundance of aromatasein teleosts may represent an adaptation linked to continual neurogenesisthat is known to occur throughout an individual's lifetime amongfishes. The localization of aromatase within the intersexuallyand intrasexually dimorphic vocal-motor circuit further impliesa function in the expression of alternative male reproductivephenotypes and, more generally, the development of natural, individualvariation of specific brainnuclei.

Key words: aromatase; estrogen; radial glia; telencephalon; teleost fish; vocal-motor system

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The aromatization of circulating androgen to estrogen in the brain is known to be a key mechanism by which testosterone regulatesmany physiological and behavioral processes, such as brain sexualdifferentiation, activation of male sexual behavior, and feedbackof steroid hormones on gonadotropin secretion (for review, seeBalthazart and Ball, 1998). Distribution of aromatase activityin the brain appears to be conserved in vertebrates because highestconcentrations are consistently localized in forebrain areas knownto control reproduction and sex behavior (Balthazart and Ball,1998). Teleost fish express the highest levels of brain aromataseactivity (100-1000 times greater in the preoptic area-hypothalamusthan mammals) (Callard et al., 1990), and high steady-state mRNAlevels of brain homogenates corroborate these levels (Gelinaset al., 1998).

Only one study in goldfish attempted to localize aromatase-containing neurons by immunocytochemistry (ICC) using an antiserumto human placental aromatase (Gelinas and Callard, 1997). However,the numbers of aromatase-immunoreactive (IR) cells was not greaterthan those in rodent and avian studies, which conflicts with knownhigh aromatase activity and aromatase mRNA levels. We have nowused species-specific antibodies and mRNA probes to show the anatomicalbasis for high brain aromatase activity levels in teleosts. Surprisinglymost, if not all, aromatase is localized in glialcells.

The plainfin midshipman, Porichthys notatus, exemplifies one of the most broadly studied neuroethological models for brainmechanisms underlying the performance of reproductive tacticsamong teleosts (for review, see Bass, 1992, 1996; Foran and Bass1999). Midshipman have two male morphs with divergent spawningand vocal behaviors. Only type I "singing" males acousticallycourt females, whereas type II "sneaker" males do not court femalesbut instead steal egg fertilizations from singing males. TypeI males are divergent from type II males and females (which resembleeach other) in a large suite of reproductive-related neuronaltraits (Bass, 1992, 1996; Goodson and Bass, 2000). Brain aromataseactivity levels resemble other teleosts with the addition of intersexualand intrasexual differences in the hindbrain region, which includesan expansive vocal pacemaker-motoneuron circuitry (Schlinger etal., 1999). One objective of this study was to map the distributionof aromatase-IR cells throughout the brain of midshipman by usingan antibody made against a conserved amino acid sequence fromknown teleost aromatases. Also, we sought to determine whetherthis antibody would reveal relative numbers of aromatase-IR cellspredicted by levels of aromatase activity in this species. Tocorroborate immunocytochemical localization of aromatase-containingcells, in situ hybridization (ISH) probes based on cloning ofa partial aromatase cDNA of midshipman were also used to detectaromatase mRNA throughout the midshipman's brain. The localizationof abundant aromatase in glial cells, the only other examplesof which are known in mammalian and avian models under brain injury-dependentconditions in situ (Garcia-Segura et al., 1999a,b; Peterson etal., 2001) or in culture (Schlinger et al., 1994), has importantimplications for neurogenesis and likely neuronal repair, whichcan continue throughout an individual's lifetime among teleosts(Gelinas and Callard, 1997; Zupanc, 1999).

Parts of this work have been published previously in abstract form (Forlano et al., 2000, 2001).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. All fish were collected from field sites in Tomales Bay, CA during the 1999 and 2000 summer reproductive season andwere held at the University of California Bodega Marine Laboratoryin running seawater tanks until shipped to Cornell University.Fish were maintained in artificial seawater tanks until they werekilled. All experimental protocols were approved by the CornellUniversity Institutional Animal Care and UseCommittee.

ICC. Two antibodies were generated for this study. The first antibody, made against the peptide CKLQVLESFINESLRFHPVV, wasdesigned a priori, based on a conserved amino acid sequence ofknown teleost aromatases (see below). A second antibody was madeagainst a peptide sequence deduced from the midshipman aromatasecDNA (see below) and used to confirm the same pattern found withthe originalantibody.

All fish (nine type I males, 13-17.2 cm; five type II males, 10.2-10.8 cm; eight females, 10.5-13.7 cm) were deeply anesthetizedin MS222 (tricaine methanesulfonate; Sigma, St. Louis, MO) andperfused transcardially with teleost Ringer's solution, followedby 4% paraformaldehyde in 0.1 M phosphate buffer (PB). Brainswere removed and post-fixed in the same fixative for 1 hr andstored in PB. Before sectioning in the transverse plane at 30µm on a cryostat, brains were cryoprotected overnight in 30% sucrosein PB and frozen in Cryo-M-bed (Hacker Instruments, Huntington,UK). Sections were collected onto chrom-alum-subbed slides andstored at $-$ 80°C until processed as follows: two times for 10 mineach in 0.1 M PBS, 20 min PBS plus 1.0% bovine serum albumin (BSA)plus 0.3% Triton X-100, overnight (16 hr) in primary antibodysolution (anti-aromatase, 400 µl each slide) [ primary antibodies,made by Bethyl Labs Inc. (Montgomery, TX), were diluted 1:5000(final peptide concentration, 0.2 µg/ml) in PBS plus 0.5% BSAplus 0.3% Triton X-100 plus 0.5% sodium azide], two times for10 min each in PBS plus BSA, 1 hr in secondary anti-rabbit antibody(Vectastain Rabbit IgG kit; Vector Laboratories, Burlingame, CA)in PBS plus BSA, two times 10 min each in PBS plus BSA, 1 hr avidin-biotincomplex (Vectastain Rabbit IgG kit; Vector Laboratories) in PBSplus BSA, two times for 10 min each in PB, 1.5 min diaminobenzidinesolution (DAB) (0.05% DAB in 0.1 M PB with 0.3% hydrogen peroxide),two times for 10 min each in PB, dehydrated in a graded seriesof ethanol, three times for 5 min each in xylene, and coverslippedin Permount (Fisher Scientific, Fair Lawn, NJ). Controls includedabsence of primary antibody and preabsorption of primary antibodyovernight with excess peptide used to generate the antibody. Bothcontrols showed no label in thetissue.

The aromatase antigen was designed based on sequence alignment of known brain [Tilapia (GenBank accession number AF135850),Oreochromis (GenBank accession number AF306786), Danio (GenBankaccession number AF120031), and Carassius (GenBank accessionnumber AB009335)] and ovarian [Oryzias (GenBank accession numberD82969), Danio (GenBank accession number AF004521), Tilapia(GenBank accession number AF135851), and Carassius (GenBankaccession number AB009336)] forms of teleost aromatase locatedin the GenBank database. After alignment, a sequence was selectedthat was both highly conserved between brain and ovarian formsof aromatase, as well as displaying a high antigenic index (MacVectorSequence Analysis Software; Oxford Molecular Group). A secondantibody (mentioned above) made against the peptide CGENQTENVNYQNLEVLEKwas based on the deduced amino acid sequence (residues 39-56)from a partial cDNA of midshipman aromatase (see cloning results).For conjugation to a carrier protein, a Cys residue was introducedat the N terminus of both peptides (shownabove).

Also, several other antisera were used with the above protocol to determine the pattern of aromatase immunoreactivity as neuronalor glial: monoclonal mouse anti-human neuronal (Hu) protein antibody(1:1000, 16A11; Molecular Probes, Eugene, OR) as a specific labelfor neuronal cell bodies (Marusich et al., 1994), monoclonal mouseanti-acetylated tubulin (1:2000, T6793; Sigma) as an axonal marker,rabbit anti-glial fibrillary acidic protein (GFAP) (1:1000, G-9269;Sigma) and monoclonal mouse anti-GFAP (1:1000, MAB360; Chemicon,Temecula, CA) as astrocyte or radial glial markers (mouse anti-GFAPhas been shown to work in goldfish; Kalman, 1998), and monoclonalmouse anti-vimentin (VIM) (1:4, 40E-C; Developmental Studies HybridomaBank, University of Iowa, Iowa City, IA) as a radial glia marker(Alvarez-Buylla et al., 1987). The 40E-C monoclonal antibody developedby A. Alvarez-Buylla was obtained from the Developmental StudiesHybridoma Bank developed under the auspices of the National Instituteof Child Health and Human Development and maintained by the Universityof Iowa (Department of Biological Sciences, Iowa City,IA).

In double-label experiments, both primary antibodies [rabbit anti-aromatase (1:1000) and anti-Hu (1:100) or anti-vimentin(1:1), anti-acetylated tubulin (1:1000), or mouse anti-GFAP (1:100)]and, subsequently, both secondary antibodies were combined andapplied as above. Secondary anti-rabbit antibody conjugated tofluorescein (Vector Laboratories) was used to visualize anti-aromatase,and secondary anti-mouse antibody conjugated to Texas Red (VectorLaboratories) was used to visualize anti-Hu, vimentin, GFAP, andacetylated tubulin. Both secondary fluorescence antibodies wereused at 1:100 dilution in PBS plus 0.5% BSA. Slides were incubatedfor 1.5 hr in a 37°C humidified chamber, washed three times for10 min each in PBS, dipped in ddH₂O, and coverslipped with Vectashield(Vector Laboratories). Fluorescently labeled material was visualizedon a Nikon (Tokyo, Japan) ES800 compound microscope outfittedwith epifluorescence and a double-band pass cube (FITC-Texas Red)to allow for simultaneous visualization of both antibodies. Photographswere taken using Kodak Gold color film (iso 400 for fluorescence,iso 100 for bright field; Eastman Kodak, Rochester, NY) and a35 mm Nikon mounted camera on the above microscope. Photographswere then scanned at 600 dpi, compiled into plates, and labeledin Adobe Photoshop 4.0 (Adobe Systems, San Jose,CA).

Cloning of midshipman aromatase cDNA. Fish were deeply anesthetized, and brains were dissected into hindbrain, midbrain, andforebrain regions (Schlinger et al., 1999) (Fig. 1), rapidly frozenin liquid nitrogen, and stored at $-$ 80°C. Because biochemical analysesindicate the highest levels of aromatase activity in the forebrainof these fish (Schlinger et al., 1999), four forebrains of adultfemales were pooled together for total RNA extraction. Brainswere removed from $-$ 80°C and immediately ground into a fine powderin liquid nitrogen, transferred into 4 ml of Trizol (Life Technologies,Carlsbad, CA), and mixed by a Tissue Tearer probe for 30 sec,and RNA was purified according to the instructions of the manufacturer.Reverse transcription was as follows: 3.3 µg of total RNA wasadded to 1 µl of random primers, heated to 70°C for 10 min, chilledon ice 2-3 min, and was reversed transcribed with SuperScriptII (Life Technologies) according to the directions of the manufacturer.For reverse transcription (RT)-PCR, two degenerate oligo primerswere designed based on conserved regions of goldfish (GenBankaccession number AB009335) and Tilapia (GenBank accession numberAF135850) brain aromatase sequence. Forward primer ATGGTNAT(A/C/T)GCNGCNCCNGA(C/T)ACand reverse primer CATNGC(A/G/T)AT (A/G)TG(C/T)TTNCCNAC(A/G)CAwere predicted to amplify a 426 bp sequence from the midshipmanbrain. For amplification of the predicted 426 bp sequence, PCRwas performed in a final volume of 100 µl containing 1× reactionbuffer, 1.5 mM MgCl₂, 200 µM each dNTP, 1 µM each primer, 1 µlTfl DNA polymerase, and 2 µl of first-strand cDNA reaction. Thecomplete reaction was overlaid with 80 µl of mineral oil and runfor 30 cycles under the following conditions: 30 sec at 94°C,1 min at 50°C, 1 min at 72°C, and 10 min at 72°C. PCR productswere run on a 2% agarose gel to confirm predicted size, purifiedwith a Qiagen (Valencia, CA) PCR purification kit, treated withT4 polynucleotide kinase, and blunted with T4 DNA polymerase.This product was then ligated into Bluescript plasmid, which wasdigested previously with SmaI restriction enzyme and treated withcalf intestinal phosphatase. The ligated plasmid was then transformedinto competent X-LI-Blue cells and plated onto LB-agarose plateswith ampicilin (AMP). Resistant colonies were selected and grownin LB plus AMP (100 µl/ml) overnight, miniprepped, and digestedto confirm presence of insert. Two clones with predicted insertwere sequenced at the Cornell University Biotechnology Sequencingfacility, one of which contained a match to other teleost aromatases.

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Figure 1. Dorsal view of a midshipman brain indicating areas of transverse sections in Figure 2, posterior to anterior (A-K), which demonstrate anatomical locations of aromatase immunoreactivity. Cb, Cerebellum; M, midbrain; OB, olfactory bulb; OC, occipital nerve; OL, olfactory nerve; PLLN, posterior lateral line nerve; PN, pacemaker neurons; SMN, sonic motor nucleus; SP, spinal cord; T, telencephalon; VM, ventral medullary neurons; V, trigeminal nerve; VIII, eighth nerve; IX, glossopharyngeal nerve; X, vagus nerve.

ISH. The procedure for in situ hybridization detection of aromatase mRNA in midshipman brain was adapted from that publishedfor gonadotropin-releasing hormone mRNA (Grober et al., 1995).Adult midshipman fish (five type I males, 11.5-21 cm; five typeII males, 7.5-11.4 cm; five females, 10.9-17.2 cm) were perfused,and brains and gonads (both ovary and testis) were sectioned asabove for ICC or dissected fresh and immediately embedded andfrozen over dry ice, sectioned at 30 µm, collected onto SuperfrostPlus slides (Erie Scientific, Portsmouth, NH), and stored in $-$ 80°C.Before hybridization, slides were equilibrated to room temperaturefor 10 min. Slides with unfixed tissue were immersed in 4% paraformaldehydefor 5 min and rinsed twice in potassium PBS (KPBS), pH 7.2. Bothslides that contained both fixed and unfixed tissue were washedtwo times in KPBS and placed into freshly prepared 0.25% aceticanhydride in 0.1 M triethanolamine two times for 5 min each, dehydratedin a series of ethanol washes and chloroform, and airdried.

Hybridization was performed with a mixture of two probes antisense to nucleotides 121-161 (AACCTCTAGGTTTTGGTAATTAACATTT-TCTGTTTGATTC)and 180-220 (GCATTGTGAAGTCAACCACAG-GATGAAACCTCAAAGACTC) of the426 bp sequence of midshipman aromatase. Oligonucleotides werelabeled with a terminal deoxynucleotidyl transferase reactionusing [ $alpha$ -³³P]d-ATP (specific activity, 1000-3000 Ci/mmol; NEN, Boston, MA).Hybridization solution [4× SSC (1× SSC is 0.15 M sodium chlorideand 0.015 M sodium citrate, pH 7.2), 40% deionized formamide,500 µg/ml denatured calf thymus DNA, 250 µg/ml transfer RNA, 4×Denhardt's solution, 4 mM EDTA, 5 mM sodium phosphate, 10% (w/v)Dextran sulfate, and 1 × 10⁶ cpm total radiolabeled probe (0.5 × 10⁶ cpm each probe)] was placed on each slide (300 µl), coverslippedwith parafilm, and incubated overnight (at least 15 hr) in a humidified37°C chamber. After hybridization, slides were briefly washedtwice at 23°C in 1× SCC, washed twice for 30 min at 55°C in 1×SCC in a shaking water bath, and washed once in 1× SCC in 0.1%Triton X-100 at 23°C, briefly rinsed in distilled water and 70%ethanol, and air dried. Slides were then exposed to X-Omat ARfilm (Eastman Kodak) for 2-3 d at $-$ 20°C to confirm signal, subsequentlydipped in nuclear emulsion (NTB-2; Eastman Kodak), and exposedfor 4 weeks at 4°C. Slides were developed in Kodak D-19 (4 minat 14°C), rinsed in distilled water (10 sec at 14°C), fixed (KodakGBX fixer; 5 min at 14°C), rinsed in running distilled water (5min), counterstained in cresyl violet, dehydrated, and coverslippedwith Permount. Both unfixed and fixed tissue showed similar signal,although tissue integrity was improved with fixed tissue. Dark-fieldoptics were used to best visualize the overall mRNA signal patternthroughout the brain at 40× magnification, whereas bright-fieldoptics were used to best visualize ISH signal at higher magnificationover Nissl-stained tissue. Dark-field photography was performedusing Kodak Gold color film (iso 400), after which color printswere scanned at 600 dpi and converted to grayscale, combined intoplates, and labeled in Adobe Photoshop 4.0. Bright-field photographyfor ISH was identical for bright-field ICC (seeabove).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Distribution of aromatase immunoreactivity

The antibody first used in this study (made against a conserved amino acid sequence of known teleost aromatases) before themidshipman sequence was known labels consistently and specificallywithin the same brain regions between animals, independent ofadult morphotype. The second antibody designed against the midshipmanspecific sequence gave an identical labeling pattern to the firstantibody used. All photomicrographs were taken from tissue labeledwith the first antibody. Differences in immunoreactivity betweenand within sexes will be addressedelsewhere.

Hindbrain
Aromatase-IR cells are concentrated dorsal and dorsolaterally within the sonic motor nucleus (SMN) and the ventral half ofthe fourth ventricle, whereas fewer aromatase-IR cells are foundcentrally in the SMN (Figs. 2A, 3A-C). Fibers from the majorityof these cells project ventrally through the SMN, as well as ventrolaterallyalong the reticular formation (Figs. 2A, 3A,B). Several aromatase-IRcells are also found ventral to the SMN, lateral to and sometimeswithin the medial longitudinal fasciculus (MLF) (Fig. 2A,B). Thereappears to be a denser population of aromatase-IR cells in therostral SMN, and some cells extend dorsally along the periventricularregion at the level of the vagal motor nucleus (Fig. 2B, Xm).In other areas in the hindbrain, more cells are found just lateralto the MLF, with fibers extending along the reticular formation(Fig. 2C,D, RF). Double-label ICC with neural-specific anti-Huantibody indicates no obvious overlap between aromatase-IR cellsand neuronal cell bodies in the SMN (Fig. 3C), as well as otherregions in the hindbrain.

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Figure 2. Distribution of aromatase immunoreactivity in the brain of P. notatus. Left half of each section is a camera lucida drawing that shows aromatase-IR cell and fiber distribution; right half is a photomicrograph of ICC processed tissue with Nissl counterstain. A, B, Aromatase-IR cells are concentrated dorsally and dorsolaterally within the sonic motor nucleus (SMN) and around the ventral half of the fourth ventricle (IV). C, D, Aromatase-IR cells remain prominent just lateral to the medial longitudinal fasciculus (MLF) in the rostral hindbrain. E, F, Large numbers of aromatase-IR cells line the periventricular areas of the fourth ventricle (IV) and cerebral aqueduct (CA) in the caudal (E) and rostral (F) midbrain, respectively; label is absent in the midbrain tectum (Te) and torus semicircularis (TS). G, H, Throughout the diencephalon, the third ventricle (III) is lined with aromatase-IR cells, which project ventrolaterally. I, J, Aromatase-IR cells (2-4 layers thick) line the entire periphery of the telencephalic hemispheres, as well as the medial ventricular surface; fiber projections course ventromedially. Aromatase-IR cells are prominent in preoptic areas (PPa, anterior parvocellular; PM, magnocellular). K, Label extends well into the olfactory bulbs (OB) in which numerous IR cells line the dorsomedial edge and fiber projections course ventrolaterally. CC, Cerebellar crest; Cg, granule cell layer of the corpus of the cerebellum; Cm, molecular layer of the cerebellum; CP c/d, compact/diffuse division of the central posterior nucleus; DD, dorsal division of the dorsal telencephalon; DL, dorsolateral telencephalon; DM, dorsomedial telencephalon; DP, dorsal posterior nucleus of the thalamus; Hv, ventral periventricular hypothalamus; iaf, internal arcuate fibers; ll, lateral lemniscus; OC, occipital nerve; ot, optic tract; PAG, periaqueductal gray; PCo, posterior commissure; Pe, periventricular cell layer of the torus semicircularis; PGl, lateral division of nucleus preglomerulosus; PGm, medial division of nucleus preglomerulosus; RF, reticular formation; SOv, ventral division of secondary octaval nucleus; Vd, dorsal nucleus of area ventralis; Vde, descending tract of the trigeminal nerve; Vl, vagal lobe; VP, posterior nucleus of area ventralis of the telencephalon; Vs, supracommissural nucleus of the ventral telencephalon; Vv, ventral nucleus of area ventralis; Xm, vagal motor nucleus. Scale bar, 1 mm.

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Figure 3. Aromatase immunoreactivity in the hindbrain and midbrain. A, B, Low-magnification photomicrographs of aromatase immunoreactivity visualized by DAB chromogen corresponding to levels near Figure 2, A and B. C, Photomicrograph of the sonic motor nucleus fluorescently double-labeled with anti-aromatase (green) and neuronal specific anti-Hu (red). Note the prominent aromatase-IR fibers throughout the entire sonic motor nucleus. D, Low-magnification photomicrograph of aromatase immunoreactivity visualized by DAB chromogen at level near Figure 2F. E, Photomicrograph of the periventricular region in the midbrain (also near level 2F) fluorescently double-labeled with anti-aromatase (green) and neuronal-specific anti-Hu (red). Scale bars: A, B, D, 500 µm; C, 240 µm; E, 80 µm.

Midbrain and diencephalon
In the caudal midbrain, aromatase-IR cells line the ventral half of the fourth ventricle and fibers course ventrolaterally,just around the MLF (Fig. 2E). Fibers also emerge from the areaat the base of the torus semicircularis (Fig. 2E, TS). More rostrally,aromatase-IR cells lie just beneath the periaqueductal gray (PAG),and fibers cover most of the tegmentum (Teg) (Figs. 2F, 3D,E).Throughout the midbrain, label is consistently absent in the tectum(Te) and torus semicircularis. In the diencephalon, the thirdventricle is completely lined by aromatase-IR cells and fibersmostly project ventrolaterally (Figs. 2G,H, 4A,B). The periventricularareas in the hypothalamus also contain labeled cells that projectradially, as well as cells that line the ventral edge of the hypothalamus(Fig. 2G,H). Double-label ICC with neural-specific anti-Hu antibodyindicates no obvious overlap between aromatase-IR cells and neuronalcell bodies in any regions in the midbrain and diencephalon (Figs.3E, 4B).

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Figure 4. Aromatase immunoreactivity in the diencephalon and telencephalon. A, Low-magnification photomicrograph of aromatase immunoreactivity visualized by DAB chromogen at level near Figure 2G. Scale bar, 500 µm. B, Photomicrograph of the diencephalon (also near level G) fluorescently double-labeled with anti-aromatase (green) and neuronal-specific anti-Hu (red). Scale bar, 160 µm. C, Low-magnification photomicrograph of aromatase immunoreactivity visualized by DAB chromogen at level near Figure 2I. Scale bar, 500 µm. D, Photomicrograph of dorsal telencephalon (also near level 2I) fluorescently double-labeled with anti-aromatase (green) and neuronal-specific anti-Hu (red). Scale bar, 80 µm.

Telencephalon
Compared with other brain regions, the forebrain has by far the greatest numbers of aromatase-IR cells. As seen in the hindbrainand midbrain, aromatase-IR cells are consistently found aroundventricular surfaces, and the forebrain is no exception. Duringdevelopment, the telencephalon of teleost fish is formed by aneversion of the ventricular surface (Nieuwenhuys, 1982). Thus,the entire periphery of the telencephalic hemispheres is ventricularsurface, and therefore the expression of aromatase-IR cells alongthis surface is consistent with other brain regions. Labeled cells(two to four thick) line the outer edge of the dorsal and lateralhemispheres, whereas fewer nonventricular cells are found centrally(Figs. 2I-K, 4C). Aromatase-IR cells are also located along themedian ventricular surface and in the preoptic areas (Fig. 2I,PM). Fibers from most of these cells cover the entire forebrainand appear to converge along the ventrolateral (VL) margin ofthe telencephalon, as well as in the optic tract (Fig. 2I,J, ot,4C). Aromatase-IR cells and fibers extend well into the olfactorybulb (Fig. 2K, OB). Again, as in other brain regions, there appearsto be no overlap between aromatase immunoreactivity and neuronalcell bodies (Fig. 4D), which is additional evidence that the majorityof aromatase in these fish is found in glia and notneurons.

Cloning of partial midshipman aromatase cDNA

A predicted 426 bp sequence was amplified from midshipman brain tissue. Figure 5 shows the midshipman partial cDNA sequencewith translated amino acid sequence below. Sense and antisensedegenerate primers for RT-PCR were designed to the two conservedamino acid regions shown in bold. The amplified region of midshipmanbrain aromatase contains presumptive functional domains that areconserved among cytochrome P450 enzymes (Hickey et al., 1990;Gelinas et al., 1998), including partial helical region, Ozolspeptide region, conserved aromatic region, and partial heme bindingregion (Fig. 5). The presumed membrane-spanning domain, whichis not as conserved as the above functional regions, is likelyupstream to the region that was amplified from midshipman brain(Gelinas et al., 1998).

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Figure 5. Nucleotide and deduced amino acid sequence of aromatase cDNA clone isolated from midshipman brain. Bold amino acids indicate conserved regions of teleost brain aromatase (based on goldfish and Tilapia) to which degenerate primers were made for RT-PCR. Presumed functional domains are underlined and correspond to regions identified in goldfish brain aromatase by Gelinas et al. (1998). I, Helical region (partial); II, Ozols peptide; III, aromatic region; IV, heme binding region (partial).

A comparison of midshipman brain aromatase with other aromatases isolated from other teleost brain and ovarian tissue, aswell as zebra finch (ovarian) and human placental aromatase, isshown in Figure 6. The antibody first used in this study (designedagainst a conserved amino acid sequence of known teleost aromatases;see Materials and Methods) corresponds to residues 50-68 and differsfrom midshipman at positions 50, 52, and 56. A BLAST (NationalCenter for Biotechnical Information) search using the unique midshipmanpartial cDNA translated protein (without flanking primers) revealed79% sequence identity to Tilapia mossambica brain aromatase (GenBankaccession number AF135850), 76% identity to Oreochromis niloticusbrain aromatase (GenBank accession number AF306786), 68% toO. niloticus ovarian aromatase (GenBank accession number AF295761),67% identity to Carassius auratus brain aromatase (GenBank accessionnumber AB009335), 64% identity to Danio rerio brain aromatase(GenBank accession number AF226619), 64% identity to T. mossambicaovarian aromatase (GenBank accession number AF135851), 57%identity to Poephila guttata (zebra finch) (GenBank accessionnumber S75898), and 57% identity to human placental aromatase(GenBank accession number HUMARM). As expected, highest homologiesmatch with other teleost brain aromatases, although the ovarianform from O. niloticus contains more identities than aromataseisolated from brain in goldfish (C. auratus) and zebrafish (D.rerio). Differences of aromatase isoforms within a single speciesis exemplified by the high sequence identity of midshipman brainaromatase to Tilapia brain when compared with the relatively lowidentity to Tilapia ovarian aromatase.

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Figure 6. Alignment of deduced amino acid sequences of midshipman, P. notatus (Pn), brain aromatase to known teleost brain (br) aromatases [T. mossambica (Tm); O. niloticus (On); C. auratus (Ca); D. rerio (Dr), as well as Tm and On ovarian (ov), zebra finch P. guttata (Pg) (ovarian), and human placental (Hum pl)]. Boxed areas, which include P. notatus, indicate identical amino acids to midshipman brain aromatase. Bold amino acids indicate conserved regions of teleost brain aromatase (based on goldfish and Tilapia) to which degenerate primers were made for RT-PCR. The antibody used in this study before the midshipman sequence was known (see Materials and Methods) corresponds to residues 50-68 and differs from midshipman at positions 50, 52, and 56.

In situ hybridization

Dark-field illumination was the most effective method to view the overall distribution pattern of hybridization signal (Fig.7A-J). The pattern of aromatase mRNA signal was consistent withthat found by immunocytochemical localization of the enzyme (compareFigs. 2, 7). Bright-field visualization was also used to identifythe location of silver grains in relation to Nissl-stained brainnuclei (Fig. 7K-O). Because teleost ovarian tissue is known toproduce aromatase, we processed sagittal sections of ovary throughthe ISH protocol along with brain tissue; we also processed testis.Unlike testis, adult female ovaries at various stages of oocytedevelopment showed robust hybridization with the probes made frombrain aromatase (Fig. 7P). This pattern attests to the specificityof the labeling and is entirely consistent with gonadal activityin teleost fish, namely that aromatization occurs in ovarian tissue(Nagahama, 1983).

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Figure 7. Dark-field (A-J) and bright-field with Nissl counterstain (K-O) visualization of in situ hybridization throughout the brain of P. notatus using probes from partial cDNA cloning of midshipman brain aromatase. Pattern of signal in all brain regions is consistent with that found by ICC (Fig. 2-4). A, Aromatase mRNA signal clearly defines the sonic motor nucleus (SMN) boundary near level Figure 2A; heaviest signal is around the dorsal and lateral periphery. B, Aromatase mRNA just below the fourth ventricle (IV) in the rostral medulla near Figure 2E. C, Hybridization signal in the caudal midbrain in between levels at Figure 2, E and F. D, Aromatase mRNA expression in the diencephalon near Figure 2G. E, Aromatase mRNA expression in the diencephalon-telencephalon transition area near Figure 2H. F, The caudal telencephalon between Figure 2, H and I. G, Strong hybridization in the anterior parvocellular division of the preoptic area (PPa), posterior nucleus of area ventralis of the telencephalon (VP), and ventrolateral area (near Fig. 2I). H, Section just caudal to Figure 2J at the level of the anterior commissure (ac), which shows very strong punctate signal within the PPa. I, Anterior telencephalon (rostral to Fig. 2J) has high aromatase mRNA signal, especially within ventrolateral (VL) and ventral nucleus of area ventralis (Vv), as well as within the optic tract (ot). J, Aromatase mRNA expression in olfactory bulb (OB, near Fig. 2K). Scale bars: A, B, 200 µm; C-J, 400 µm. K, Section through the hindbrain just caudal to the level at Figures 2B and 3B, which indicates high silver grain concentration in the dorsal rostral SMN; signal within the central SMN is much greater than in the MLF. Scale bar, 100 µm. L, Hybridization signal in the midbrain just below the periaqueductal gray (PAG) near the level at Figure 2F. Scale bar, 100 µm. M, ISH signal in the diencephalon at levels between Figure 2, G and H. Notice the clusters of strong signal along III, which expand into the dorsal posterior nucleus of the thalamus (DP). Scale bar, 100 µm. N, ISH signal in the lateral forebrain between levels at Figure 2, I and J. The ventral and lateral boundaries between VL and DL telencephalon show a strong signal of hybridization. Scale bar, 250 µm. O, Intense ISH signal in Vv and in PPa between levels at Figure 2, I and J. P, ISH signal in a sagittal section through an ovary. Large, discrete clusters of aromatase mRNA hybridization appear between maturing oocytes (O). Scale bar, 500 µm. Hd, Dorsal periventricular hypothalamus; Hv, ventrolateral nucleus of the hypothalamus; tc, tela choroidea; Vm, molecular layer of the valvula; also see Figure 2A-K.

Hindbrain
When viewed under dark-field illumination, grains that indicate hybridization to brain aromatase mRNA clearly define the boundaryof the SMN (see Fig. 9A). The mRNA signal within the SMN togetherwith that surrounding the SMN and within the reticular formationis concordant with the position of the hindbrain vocal pattern-generatingcircuit (Fig. 1) (Bass et al., 1994). Similar to ICC labeling(Figs. 2A,B, 3A,B), hybridization signal is concentrated in thedorsolateral SMN and is stronger more rostrally where silver grainsextend dorsally along the ventricle (Fig. 7A,K). Signal withinthe SMN is also comparatively higher than other surrounding brainareas, such as the MLF (Fig. 7A,K), and dense silver grains fromthe SMN follow the same ventrolateral pathway into the reticularformation as do aromatase-IR labeled fibers (Figs. 2A,B, 3A-C,7A). In the rostral hindbrain, an intense bilateral band formsjust outside the periventricular area, below the fourth ventricle(Fig. 7B), as seen in Figure 2E. Hybridization in other areasof the hindbrain correspond to aromatase immunoreactivity in Figure2, C and D.

Midbrain and diencephalon
Distribution of aromatase mRNA hybridization signal in the midbrain and diencephalon (Fig. 7C,D) also shows the same overallpattern as found by ICC (Figs. 2E,G, 3D, 4A). Dark-field imageof the caudal midbrain identifies a clear signal concentratedbetween the medial boundary of the torus and the valvula, as wellas a strong bilateral signal just beneath the cerebral aqueductalong the periaqueductal gray (Fig. 7C,L), first seen in the rostralhindbrain (Fig. 7B). The signal is concentrated in a lateral bandthat outlines the torus and is more diffuse in the ventral tegmentum(Fig. 7C). There is a clear absence of hybridization in the optictectum and torus, as seen by ICC (Figs. 2E,F, 3D, 7C). AromatasemRNA is concentrated in the diencephalon along the third ventriclein the thalamus, as well as in the dorsal and ventral periventricularareas of the hypothalamus (Fig. 7D,M), similar to that seen inICC-treated tissue (Fig. 2G, 4A). Aromatase mRNA expression inthe diencephalon-telencephalon transition area (near Fig. 2H)shows high signal along the midline ventricle through thalamicand hypothalamic regions and dorsolaterally just beneath the optictract (Fig. 7E).

Telencephalon
The telencephalon has the most abundant aromatase mRNA signal compared with other brain regions and also shows the same overallpattern as found by ICC. Strongest signal is apparent in preopticareas along the ventricular midline and in the VL area. Dark-fieldvisualization (Fig. 7F,G) indicates a broad distribution of hybridizationthroughout the forebrain, with strongest signal in the preopticareas along the midline ventricle (compare with Fig. 2I) and theVL and dorsolateral (DL) interface (Fig. 7N). Dark-field visualizationshows a concentration of silver grains that follow the same patternas aromatase-IR fibers, which course from the periphery to theVL-DL interface (Fig. 7G-I) that lies near the point of attachmentof the tela choroidea (Fig. 7N, tc). Consistent with ICC, hybridizationis found along the entire periphery of the telencephalic hemispheresand along ventricular surfaces, as well as in the optic tract(Fig. 7G-I). Rostral in the telencephalon, robust signal is foundin the anterior parvocellular division of the preoptic area (Fig.7H,O, PPa), ventral nucleus of area ventralis (Fig. 7I,O, Vv),and in the ventral and medial olfactory bulb (Fig. 7J).

Evidence for aromatase expression in glial cells

Because the pattern of aromatase immunoreactivity in P. notatus brain (especially in the telencephalon) appeared reminiscentof radial glia found in other teleosts (Manso et al., 1997; Kalman,1998) and did not colocalize with neural-specific anti-Hu labeledcells, we used three glial antibodies, rabbit anti-GFAP (G-9269),mouse monoclonal anti-GFAP (MAB360), and mouse monoclonal anti-VIM40E-C (Developmental Studies Hybridoma Bank) to localize radialglia in the midshipman brain. The pattern of label with all antiserain the telencephalon is strikingly similar to that seen with anti-aromatase(compare Fig. 8 with 2I,J, 4C,D), as well as the staining patternseen with anti-GFAP and anti-vimentin in other vertebrates, includingteleosts (Alvarez-Buylla et al., 1987; Manso et al., 1997; Kalman,1998). Anti-GFAP (MAB360) labels fibers robustly (Fig. 8A-C).Anti-VIM labels fiber projections robustly, but labels few cellbodies (Fig. 8D). In contrast, anti-GFAP (G-9269) labels morecell bodies (Fig. 8E), but fibers distal to the cell bodies arenot labeled as heavily. Double-label immunofluorescence with anti-aromataseand mouse anti-GFAP (MAB360) or VIM reveals a colocalization ofaromatase immunoreactivity in glial fibers in the forebrain (Fig.9). Direct fiber projections from aromatase-IR cells that linethe entire peripheral ventricular zone of the telencephalon arealso GFAP and VIM-IR (Fig. 9A,B), and some cell bodies that arefound medial to the majority of aromatase-IR cells at the ventricularedge of the forebrain are also double-labeled. The anterior parvocellulardivision of the preoptic area in the forebrain (Fig. 9C) and areasof the hypothalamus (inferior lobe and periventricular areas)are also clearly doubled-labeled. In other brain regions, colocalizationof aromatase and GFAP and VIM-IR fibers is more limited to lateraland ventrolateral projections. In the midbrain ventricular areaand within the SMN of the hindbrain, GFAP and VIM-IR fibers areplentiful, but only few appear colocalized with aromatase-IR fibers.All antisera label glia in areas in which aromatase immunoreactivitynever occurs (i.e., optic tectum), and therefore it appears thataromatase is expressed in a subset of radial glia, as well otherglial types (found in SMN and along midline ventricles) not labeledby the antisera used in this study.

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Figure 8. Distribution of radial glia in the telencephalon. A, DAB visualization of radial glia using monoclonal anti-GFAP (MAB360) near the level of Figure 2J. Note the long fibers that extend throughout the lateral telencephalon and converge in the ventrolateral area, virtually identical to the pattern seen with anti-aromatase (Figs. 2I,J, 4C). B, Higher magnification of the ventrolateral area fiber pattern in A (arrows indicate same position). C, High magnification of faintly labeled somata (arrows) and darkly labeled fibers in the dorsal telencephalon using MAB360. D, DAB visualization of radial glia in the lateral telencephalon (near the level of Fig. 2I) using monoclonal anti-vimentin. Notice the characteristic pattern of labeled fibers similar to anti-GFAP in A. E, Polyclonal anti-GFAP (G-9269) labels glial cell bodies of the same shape and size as anti-aromatase (compare with Fig. 4D). Scale bar: A, 500 µm; B, 100 µm; C, 40 µm; D, 500 µm; E, 35 µm.

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Figure 9. Colocalization of aromatase and GFAP in the telencephalon of P. notatus by double-label immunofluorescence using anti-aromatase and monoclonal anti-GFAP (MAB360) visualized by secondary fluorescein and Texas Red, respectively. A, Low-magnification photomicrograph that shows aromatase-IR cells (green) along the lateral telencephalic lobe whose projections are double-labeled with anti-GFAP (yellow-orange). Scale bar, 200 µm. B, Single cells with aromatase-IR labeled cell bodies (green) with yellow-orange fiber projections indicating that the same cell is labeled for aromatase and GFAP. Because GFAP immunofluorescence was often more robust in fibers than aromatase, fibers distal to the cell body often appeared more red-orange than yellow when viewed through a double-bandpass filter. Scale bar, 50 µm. C, Abundant colocalization (yellow) of aromatase and GFAP in the anterior parvocellular division of the preoptic area (bottom arrows). Again, fibers from aromatase-IR cells along the midline ventricle are also labeled by MAB360 (top arrow). Scale bar, 200 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although other studies have demonstrated that teleost fishes have the highest levels of aromatase activity compared with anyother vertebrate group, this is the first study to corroboratehigh activity levels with expected relative numbers of aromatase-containingcells throughout the brain of a teleost. This was accomplished,in part, because to our knowledge this is also the first studyto use specific antibodies and mRNA probes to localize aromatase-containingcells in the brain. Also, the numbers of aromatase-IR cells andaromatase mRNA in different brain regions correspond well witharomatase activity levels in the brain of this species (i.e.,greatest number of aromatase-IR cells in the telencephalon comparedwith the midbrain and hindbrain). Localization of aromatase immunoreactivityand mRNA in and around the forebrain preoptic nuclei is consistentwith studies in othervertebrates.

The use of a teleost-specific aromatase antibody likely accounts for the difference in our results from those of a previousstudy in goldfish (Gelinas and Callard, 1997). The aromatase enzymethroughout vertebrates shows remarkable variation; our analysisshows only a 57% sequence identity of midshipman brain aromataseto human placental aromatase compared with identities as highas 79% from other teleosts. Thus, as Gelinas and Callard (1997)recognize, it is not surprising that the antibody made againsthuman placental aromatase used in their study might not accuratelybind to goldfish brain aromatase. Our antibody did not work forgoldfish brain (P. Forlano and A. Bass, unpublished observations),perhaps not surprising given the low sequence identity betweenmidshipman and goldfish brain aromatases and their distant phylogeneticrelationship (although the antibody was made to conserved regionsof teleost aromatases, it corresponds more to tilapia and midshipmanbrain, as well as goldfish ovarian aromatase than to goldfishbrain aromatase). Also, as shown in goldfish (Gelinas et al.,1998), aromatase expression can vary seasonally, depending onreproductive condition. Perhaps the few goldfish we tested hadreduced basal levels of aromatase because of their nonreproductivestate. However, our antibody did work on juvenile tilapia (genusOreochromis; Forlano and Bass, unpublished observations). Becauseof the high sequence identity of midshipman brain aromatase toOreochromis brain aromatase, we tested our specific antibody andISH probes on Oreochromis brain tissue and found a similar patternof label as in midshipman with the antibody and ISH probes inthe preoptic area (Forlano and Bass, unpublished observations).The sequence identities to different forms of aromatase (ovarianvs brain) might point to differences in expression in glia versusneurons and explain why our antibody labeled tilapia, but notgoldfish, brain in a manner similar to that ofmidshipman.

As we report here, our ISH probes label ovarian aromatase in midshipman. Thus, midshipman aromatase expressed in brain orovary may be identical forms, or the probes we designed may hybridizeto conserved regions in both tissues. If a distinct ovarian formof aromatase exists in midshipman brain, it could be found inneurons in small amounts. Evidence for multiple transcripts ofaromatase is seen in goldfish and zebrafish (Callard and Tchoudakova,1997) and so far are the only examples in vertebrates in whichtwo aromatase transcripts appear to be the result of two differentaromatase genes. Neuronal aromatase may exist in midshipman, butthe amount we found in glial cells reflects activity levels, whereasneuronal numbers found in goldfish brain doesnot.

Aromatase localization to glia

An unexpected result of this work is that high levels of aromatase expression are localized in glia and not neurons. Otherstudies in mammals and birds have shown aromatase expression inglia only after brain injury in adult animals in situ (Garcia-Seguraet al., 1999a,b; Peterson et al., 2001) or in culture (Schlingeret al., 1994). This is the first study to provide evidence forbrain aromatase expression to be mostly, if not entirely, in glialcells in any vertebrate in unmanipulated animals. Aromatase-IRcells and fibers are glial in appearance, follow the same patternas radial glia, and are colocalized with vimentin and GFAP-IRfibers in certain brain regions but are never colocalized withHu-IR neuronal cell bodies or axons labeled by anti-acetylatedtubulin. The morphology and staining pattern of radial glia inthe adult avian brain using anti-vimentin (the same antiserumused in this study) is remarkably similar to the pattern of aromatase-IRexpression in the midshipman brain, namely, somata in the ventricularzone contain fibers that penetrate the forebrain parenchyma forup to several millimeters (Alvarez-Buylla et al., 1987). In general,radial glial cells are characterized by long radial processesthat reach the basal surface of the brain and their expressionof GFAP and other markers. Radial glia are best known to functionin the guidance of migrating neurons but are also known to transforminto astrocytes after neurogenesis and migration is completed(for review, see Hartfuss et al., 2001). Moreover, astrocytesare proposed as stem cells in the adult telencephalon (Doetschet al., 1999), and Alvarez-Buylla et al. (2001) have proposedradial glia to be elongated neuroepithelial cells that give riseto both neurons and glia throughout ontogeny. Recent studies recognizeseveral subtypes of radial glia based on differential antigenexpression, and the function of radial glia appears to be dependenton subtype within and between distinct brain regions (Hartfusset al., 2001). Therefore, it is not surprising that we found colocalizationof aromatase immunoreactivity and GFAP and vimentin immunoreactivityin some brain regions and not others, because certain glial subsetsmay not express the markers weused.

Function of high aromatase levels

Although the functional outcomes of high aromatase levels in the brain of teleosts, and more generally vertebrates, is unknown,we discuss a number of possibilities, including a role in sexualmaturation events, as a neurotrophic factor, and as a modulatorof steroid-sensitive, neuralcircuitry.

Although the distribution of estrogen receptors in midshipman brain is unknown, Fine et al. (1990) localized [³H]estradiol-concentrating cells in the closely related toadfish(Opsanus tau, same order and family) to many of the same areasin the forebrain and diencephalon in which we found aromataseexpression (area ventralis of the telencephalon, preoptic area,and hypothalamic ventricular regions). Aromatase is known to affectthe development of sexually dimorphic brain nucleus of the preopticarea (SDN-POA) and dendritic morphology (Burke et al., 1999) inother vertebrates (for review, see Beyer, 1999). The SMN, whichinnervates the sonic swimbladder muscles and is intersexuallyand intrasexually dimorphic in midshipman (Bass and Marchaterre,1989; Bass and Baker, 1990; Bass et al., 1996), is enshroudedwith aromatase-IR cells and fibers, contains high levels of aromatasemRNA, and probably accounts for most of the aromatase activityfound in the hindbrain. Whereas type I male midshipman alone havedetectable levels of 11-ketotestosterone (a non-aromatizable androgenin teleost fish), type II males and females have similarly highertestosterone levels than type I males (Brantley et al., 1993).Preliminary results suggest that, like some other vertebrates(Balthazart and Ball, 1998; Gelinas et al., 1998), testosteronecan upregulate aromatase expression (Forlano and Bass, 2001);testosterone can also masculinize the sonic motor system (Bass,1995). We hypothesize that relative levels of aromatase expressionin and around this nucleus that correspond to other dimorphicnuclei in the vocal-motor circuit may function to prevent itsmasculinization by circulating testosterone and therefore maybe a key mechanism in both generating and maintaining alternativemale phenotypes in this species (Schlinger et al., 1999).

A relationship between relative periods of neurogenesis and aromatase activity in different vertebrate taxa may reflect therole of estrogen as a neurotrophic factor. In mammals, the highestpeak of aromatase activity coincides with a critical organizationalperiod of brain development just before birth, followed by a subsequentdecrease in activity with age (Lephart, 1996). Songbirds havehigh aromatase levels in the telencephalon as adults and showdynamic seasonal changes in the song system areas of the brainin which new neurons appear to be recruited at times when songmodification occurs (Alvarez-Buylla and Kirn, 1997). Teleost fishhave the highest brain aromatase levels of all vertebrates andalso show continuous neurogenesis throughout life. The capacityof neurogenesis and plasticity, and regeneration in adult fishresembles properties seen in embryonic mammalian and avian brain(Levine et al., 1994). Possible functions of continual neurogenesisinclude more efficient replacement of damaged cells in the eventof injury and increases in central neuronal elements linked tocontinual somatic growth (increase in number of peripheral motorand sensory structures). Also, the continual addition of new cellsmay enable structural changes centrally that may be required forlong-term changes in behavior (for review, see Zupanc, 1999).The factors that mediate continual neurogenesis in fish are unknown(Zupanc, 1999). One function of high levels of aromatase in theadult teleost brain may be to provide large quantities of estrogeniccompounds to induce continuous cell proliferation (Gelinas etal., 1998). Perhaps the teleost brain, which can grow continuouslythroughout life, requires the continual production of estrogeniccompounds in amounts relative to that seen in upregulation afterbrain injury in other vertebrategroups.

Estrogen is also known to cause synaptic plasticity and glial activation (Garcia-Segura et al., 1989; Naftolin et al., 1990);recent studies show glia to be steroidogenic and express sex steroidreceptors (for review, see Jordan, 1999). In mammals, estrogenis widely documented to act as a growth-stimulating agent, modulateapoptotic cell death, and affect migration of neuroblasts fromthe subventricular layer and thus their aggregation to form brainnuclei with consequent synapse formation. These trophic effectsare mostly seen in distinct brain nuclei that are estrogen-sensitiveand become sexually dimorphic in adults (for review, see Beyer,1999; Wise et al., 2001). Garcia-Segura et al. (1996) first suggestedthat estrogenic control of insulin-like growth factor may be crucialfor the development of sex-specific neuroendocrine circuits andthe synaptic plasticity of adult neuroendocrine systems. Coexpressionof neurotrophins and estrogen, and their receptors, suggest thatboth factors work together to differentiate target neurons (Beyer,1999). Contreras and Wade (1999) demonstrated recently that anaromatase inhibitor administered to 3-d-old zebra finches (a periodof active neural development) significantly lowered nerve growthfactor (NGF) binding sites in telencephalon brain homogenates,supporting the hypothesis that estrogen influences NGF receptorsand therefore brain development. In addition, Dittrich et al.(1999) found 17 $beta$ -estradiol to prematurely upregulate brain-derivedneurotrophic factor (BDNF) in sexually dimorphic song nuclei injuvenile males, and this upregulation was inhibited by an aromataseinhibitor. Thus, regulation of BDNF or other growth factors isone mechanism by which estrogen may influence neural differentiation.In summary, the well established role of glia in neurogenesis,neuroplasticity and repair, as well as recent findings of an intimateinterplay between glia, gonadal steroids, and growth factors,would make glial cells prime candidates to execute multiple functionsessential for neuronal maturation, plasticity, and repair in allvertebrates.

Midshipman (Brantley et al., 1993; Knapp et al., 1999), as other teleosts (Norris, 1997), have relatively high circulatingandrogens, so that high aromatase levels in the brain may alsofunction to regulate the amount of steroid(s) that reaches steroid-sensitiveneural targets or modify the overall hormonal milieu in circulation.The position of aromatase-IR cells and ISH silver grains are consistentlylocated in ventricular areas throughout the brain, and the locationand pattern of projections appears ideal for the conversion oftestosterone to estradiol from the cerebral spinal fluid or bloodvasculature to bathe the brain in estrogenic compounds. The possiblerole of glia in teleosts as mediators of brain steroid levelsthat, in turn, could modulate multiple neuronal functions is consistentwith teleosts showing the widest range of plasticity in vertebratereproductive function at multiple levels of biologicalorganization.

  FOOTNOTES

Received May 24, 2001; revised Aug. 20, 2001; accepted Sept. 5, 2001.

This research was supported by National Institute of Mental Health Predoctoral Training Grant 5 T32 MH15793 (to P.M.F.) andNational Science Foundation Grant IBN9987341 (to A.H.B.). We thankMargaret Marchaterre, James Goodson, Matthew Weeg, Wen Wu, YukoHara, Ilya Vilinsky, and Cathy Lanning for technical advice, JosephSisneros and Margaret Marchaterre for field assistance, ColinSaldanha, Barney Schlinger, Anthony Tramontin, and Neil Segilfor helpful suggestions, and U. C. Bodega Marine Laboratory forlogisticalsupport.
Correspondence should be addressed to Paul M. Forlano, Department of Neurobiology and Behavior, Seeley G. Mudd Hall, CornellUniversity, Ithaca, NY 14853. E-mail: pmf4{at}cornell.edu.

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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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