Targeted Deletion of a Cyclic Nucleotide-Gated Channel Subunit (OCNC1): Biochemical and Morphological Consequences in Adult Mice

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The Journal of Neuroscience, November 1, 1999, 19(21):9313-9321

Targeted Deletion of a Cyclic Nucleotide-Gated Channel Subunit (OCNC1): Biochemical and Morphological Consequences in Adult Mice
Harriet Baker¹, Diana. M. Cummings², Steven D. Munger³, Joyce W. Margolis², Linda Franzen¹, Randall R. Reed³, and Frank L. Margolis²
¹ Cornell University Medical College at The Burke Medical Research Institute, White Plains, New York 10605, ² University of Maryland School of Medicine, Baltimore, Maryland 21201, and ³ The Howard Hughes Medical Institute and Department of Molecular Biology and Genetics, Johns Hopkins Medical Institutes, Baltimore, Maryland 21205

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The olfactory cyclic nucleotide-gated channel subunit 1 (OCNC1) is required for signal transduction in olfactory receptorcells. To further investigate the role of this channel in theolfactory system, the biochemical and morphological consequencesof targeted disruption of OCNC1 were investigated in adult mice.Null as compared to wild-type mice had smaller olfactory bulbs,suggesting compromised development of the central target of thereceptor cells. Ectopic olfactory marker protein (OMP)-stainedfibers localized to the external plexiform layer reflected therelative immaturity of the olfactory bulb in the null mice. Theolfactory epithelium of the knock-out mouse was thinner and showedlower expression of olfactory marker protein and growth-associatedprotein 43, indicating decreases in both generation and maturationof receptor cells. Tyrosine hydroxylase (TH) expression in theolfactory bulb, examined as a reflection of afferent activity,was reduced in the majority of periglomerular neurons but retainedin atypical or "necklace" glomeruli localized to posterior aspectsof the olfactory bulb. Double label studies demonstrated thatthe remaining TH-immunostained neurons received their innervationfrom a subset of receptor cells previously shown to express aphosphodiesterase that differs from that found in most receptorcells. These data indicate that expression of OCNC1 is requiredfor normal development of the olfactory epithelium and olfactorybulb. The robust expression of TH in some periglomerular cellsin the OCNC1-null mice suggests that receptor cells innervatingthese glomeruli may use an alternate signal transductionpathway.

Key words: tyrosine hydroxylase; phosphodiesterase; olfactory marker protein; PAX6; atypical glomeruli; necklace glomeruli

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The olfactory cyclic nucleotide-gated channel (OCNC), a nonselective cation channel, is an integral component of the signaltransduction pathway in olfactory receptor neurons (Zufall etal., 1994; Zagotta and Siegelbaum, 1996; Wei et al., 1998). Inolfactory transduction, a G-protein couples odorant-activatedreceptors to the elevation of intracellular cAMP levels throughstimulation of adenylyl cyclase, leading to direct gating of theOCNC and initial depolarization of olfactory receptor neurons(Jones and Reed, 1989; Buck and Axel, 1991). Three channel subunitswere shown to be expressed in the olfactory epithelium (OE): therelatively olfactory-specific OCNC1 and OCNC2 subunits, as wellas an olfactory-specific splice variant of the rod photoreceptor $beta$ subunit (Dhallan et al., 1990; Liman and Buck, 1994; Bradleyet al., 1994; Sautter et al., 1998; Bönigk et al., 1999). OCNC1forms functional homodimers in vitro (Dhallan et al., 1990) butin vivo is thought to be associated with either the $beta$ subunitand/or OCNC2, each of which confers greater sensitivity to cyclicnucleotides and changes in single-channel kinetics (Bradley etal., 1994; Liman and Buck, 1994; Sautter et al., 1998; Bönigket al., 1999).

A recent study reported that neonatal mice deficient in OCNC1 were anosmic (Brunet et al., 1996) and died within a few daysafter birth, although methods were recently developed to promotetheir survival (Parent et al., 1998). These mice exhibited noEOG responses to odorants previously shown to increase synthesisof either cAMP or IP3 (Boekhoff et al., 1990; Breer et al., 1990)or to complex odorants such as urine, suggesting a lack of sensitivityto all odors. Because the EOG is a cell population measure, responsesmight not have been detected that are mediated through transductionpathways expressed only in a subpopulation of receptorneurons.

Our laboratories addressed this issue by examining afferent neuron activity-dependent regulation of tyrosine hydroxylase (TH)expression in the olfactory bulb. TH expression in intrinsic periglomerularneurons shows profound downregulation after either deafferentationor naris closure and upregulation after reafferentation (Nadiet al., 1981; Kawano and Margolis, 1982; Baker et al., 1983, 1993;Kosaka et al., 1987; Cho et al., 1996). These observations indicatethat bulbar TH expression reflects afferent stimulation of theolfactorybulb.

Recently, receptor neurons were characterized (Juilfs et al., 1997) that are localized to the posterior recesses of the OEand project to a small group of atypical, modified, or "necklace"glomeruli found in posterior aspects of the olfactory bulb (Greeret al., 1982; Pedersen et al., 1986; Zheng et al., 1987; Shinodaet al., 1989, 1990; Ring et al., 1997). These receptor neuronsexpress both a specific guanylyl cyclase (GC-D) and a cyclic GMP-stimulatedphosphodiesterase, PDE2 (Juilfs et al., 1997). The presence ofPDE2 and GC-D in a specific subset of receptor neurons and theirunique projection patterns suggests that a second cyclic nucleotide-mediatedtransduction pathway may be active in the OE. If this second pathwayis functioning in OCNC1-null mice then its activity should alsobe evidenced by alterations in activity-based measures of geneexpression in the olfactorybulb.

The current studies used a line of OCNC1-null mice generated in our laboratory that survived to adulthood (Parent et al.,1998). All glomeruli in wild-type mice exhibited extensive THimmunoreactivity. In null mice, many TH-immunostained cells werefound in necklace glomeruli, but few in other glomeruli, suggestingthat necklace glomeruli receive input from receptor neurons thatuse an alternate signal transduction pathway, independent of thecAMP-activated OCNC1 channel. Differences in olfactory bulb andepithelial morphology also indicated that loss of OCNC1 and resultantlong-term odor deprivation compromised normal development of theolfactorysystem.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Wild-type (male and female) and hemizygous OCNC1-null (male) mice on a 129/svImJ × C57Bl/6J background (Parent etal., 1998) were raised to adulthood in our laboratories. Thisline, developed in our laboratory, also produces the high levelof neonatal lethality reported by Brunet et al. (1996). This propertycan be overcome by reduction of litter size within the first 24hr after birth. Presumably, by reducing competition between nullpups and their littermates, sufficient time to suckle promotesviability. For immunocytochemical procedures, six mice of similarbody weight and of each genotype at 6-8 weeks of age were deeplyanesthetized with ketamine-xylazine (3:1; 100 mg/kg body weight:33mg/kg body weight). Mice were perfused transcardially with salinecontaining 0.5% sodium nitrite followed by either (1) 4% paraformaldehyde(PFA; pH 7.4) for immunohistochemical processing of olfactorybulbs or (2) PLP fixative (2% paraformaldehyde, 0.75 M lysine,and 0.2% sodium periodate in 50 mM phosphate buffer, pH 7.4) forprocessing of olfactory mucosae. Nasal cavities were post-fixedin PLP fixative overnight at 4°C. Olfactory bulbs from mice perfusedwith 4% PFA were post-fixed at room temperature for 2 hr and storedin 0.1 M phosphate buffer, pH 7.4, at 4°C until immunohistochemicalprocessing. After post-fixation, brains were cryoprotected in30% sucrose, and 40 µm horizontal sections were prepared on asliding microtome. Epithelia were decalcified, embedded in paraffin,and 6-8 µm sections were obtained on a rotarymicrotome.

For measurement of TH activity and olfactory marker protein (OMP) levels, animals were killed by cervical dislocation andthoracotomy. Olfactory bulbs were dissected, frozen on dry ice,weighed, and stored at $-$ 80°C until processed. Mice were genotypedby PCR of tail tip DNA as previously described (Parent et al.,1998). All procedures were performed under protocols approvedby the Institutional Animal Care and Use Committees of Johns Hopkins,Cornell University, and the University of Maryland and conformedto National Institutes of Healthguidelines.

Immunocytochemistry. Floating sections of olfactory bulb were processed by previously published methods (Baker et al., 1993).Briefly, sections were first blocked with 1% bovine serum albumin(BSA) in 0.1 M PBS and incubated with the following antisera:rabbit anti-TH (1:25,000; from T. H. Joh, Cornell University MedicalCollege, White Plains, NY), goat anti-OMP (1:35,000; preparedin our laboratory) (Keller and Margolis, 1975), rabbit anti-Pax6(1:1500; against the 17 C-terminal amino acids of the mouse protein;prepared in our laboratory), and sheep anti-cFos (1: 7000; antipeptide;Genosys, The Woodlands, TX). For olfactory bulb staining, tissuewas washed and incubated with the appropriate biotinylated secondaryantibodies obtained from Vector Laboratories (Burlingame, CA).After incubation with the Vector Elite ABC kit, antigens weredetected with 3,3' diaminobenzidine tetrahydrochloride (DAB) asthe chromogen. For double-labeling, sections previously stainedfor TH (1:25,000) using DAB were incubated overnight with a chickenantiserum specific for phosphodiesterase 2 (1:1500; PDE2, kindlyprovided by Dr. J. Beavo, University of Washington) followed bya biotinylated donkey anti-chicken secondary antiserum (JacksonImmunoResearch Laboratories, West Grove, PA) and the ABC kit usingVector blue as thechromogen.

For the olfactory epithelial staining, the nasal cavities from animals perfused with PLP fixative were dehydrated in gradedethanols, cleared in toluene, embedded in paraffin, and sectionedcoronally at 6-8 µm. Every 100th section was mounted onto SuperfrostPlus slides (Fisher Scientific, Pittsburgh, PA) and incubatedin a 60°C oven for 2 hr. Sections were deparaffinized, rehydratedin graded alcohols, and processed for immunohistochemistry forOMP or growth-associated protein 43 (GAP43). Briefly, sectionswere incubated in Tris phosphate buffer (TBS), pH 7.2, containing0.1% gelatin and 0.2% Triton X-100, rinsed, and transferred toTBS with 3% normal rabbit serum to block nonspecific binding.Afterwards, sections were incubated in either goat anti-OMP (1:5000) or mouse anti-GAP43 (1:100; Boehringer Mannheim, Indianapolis,IN) overnight at room temperature. The next day, slides were rinsed,transferred to the appropriate biotinylated secondary antisera(Vector Laboratories; dilution: 1:200), rinsed, and incubatedin avidin biotin complex (ABC; Vector Laboratories). Reactionproducts were visualized by treating sections with DAB (0.15 mg/ml)in the presence of H₂O₂. Slides were then rinsed, dehydrated throughgraded ethanols, cleared in xylenes, and coverslipped using DPXmounting medium (Aldrich, Milwaukee,WI).

Epithelial thickness. Sections adjacent to those processed for immunohistochemistry were stained with hematoxylin and eosin.Coronal sections of the epithelia of wild-type and knock-out micewere traced at 640× magnification using a Nikon Optiphot microscopefitted with a camera lucida drawing tube. On both the left andright sides of the nasal cavity in three representative sectionsseparated by 600 µm, measurements of epithelial thickness weremade at two points along the nasal septum using a computer-controlleddigitizing tablet and Sigma Scan computer software (Jandel Scientific,Corte Madera, CA). At each point, the thickness of the epitheliumwas measured from the luminal surface to the basal lamina. Thetwo measurements along each side of the septum were not substantiallydifferent; therefore they were averaged. In addition, the meanthickness measurements from the left and right sides of the septumwere averaged for each of the three sections measured per animal(n = 3 pergenotype).

Olfactory bulb size. Using an eyepiece micrometer, the widths of the glomerular, external plexiform, and granule cell layersas well as the length of the olfactory bulb were measured in TH-stainedsections from three wild-type and three knock-out mice. Five sections,spanning the dorsoventral aspects of the olfactory bulb, wereassessed for each mouse (n = 3 pergenotype).

Biochemistry. Individual bulbs were homogenized in 250 µl PBS (in mM: 137 NaCl, 2.7 KCl, 10 NaH₂PO₄, and 1.7 KH₂PO₄, pH 7.4).The substantia nigra and caudate nucleus were homogenized in 450µl PBS. Aliquots of homogenates were taken for determination ofTH activity by the method of Joh et al. (1973). OMP was measuredby an ELISA assay as follows. Aliquots of each homogenate wereadjusted to a final concentration of 0.1%Triton X-100 and 0.1%sodium azide, kept on ice for 10 min, and then centrifuged for15 min at 16,000 × g at 4°C. Protein content of the supernatantswas determined by the Bradford method (Bio-Rad, Hercules, CA)using bovine serum albumin as a standard, and the samples werethen stored at $-$ 80°C. For determination of OMP content, sampleswere thawed on ice, and aliquots were diluted 1:1000 in BBS (17mM NaB₄O₇ · H₂O and 120 mM NaCl, pH 8.5). Assays were performedin freshly purchased, 96 well Immulon 2 HB, U-bottom ELISA plates(Dynex Technologies, Chantilly, VA). To wells containing 200 µlof BBS, 10-20 µl aliquots of diluted extracts were added to contain~250 pg of OMP per well. A standard curve of OMP in the rangeof 50-500 pg was included on each plate. The standard OMP solution(10 pg/µl of OMP) was prepared daily. Samples and standards wereall run in triplicate. Each plate also contained several controls,i.e., OMP with no antibody, OMP with only primary antibody, andOMP with only secondary antibody. After vibration mixing of sampleand buffer, the plates were covered and incubated at 37°C for2 hr. The plates were washed three times with TBS (in mM: 25 Tris,137 NaCl, and 2.7 KCl adjusted to pH 7.4 withHCl).

Unreacted sites on the plates were blocked by incubation with 220 µl/well of 1% normal goat serum in dilution buffer (1% bovineserum albumin, 0.1% sodium azide, and 0.5% Tween-20 in TBS) at37°C for 30 min. The blocking solution was removed and replacedwith 200 µl of rabbit anti-OMP diluted 1:2000 in dilution buffer.The covered plates were incubated at room temperature overnightand then washed five times with TBS. Goat anti-rabbit-alkalinephosphatase (Sigma, St. Louis, MO) diluted 1:5000 in dilutionbuffer was added (200 µl/well) and incubated at 37°C for 2 hrfollowed by five washes with TBS. To quantify the phosphataseactivity, 150 µl of freshly prepared p-nitrophenyl phosphate (Sigma104) at 2 mg/ml in assay buffer (10% diethanolamine, 0.02% sodiumazide, and 1 mM MgCl₂, pH 9.8) was added to each well. The increasein absorption at 405 nm was monitored as a function of time atroom temperature, on a Dynatech (Chantilly, VA) MRX microplatereader. OMP content was determined by comparison to the standardcurve on the sameplate.

Statistical analysis. Data were analyzed by either unpaired or paired Student's t test with significance set at p < 0.05.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Morphology and innervation of the olfactory bulb in OCNC1-null and control mice

The most distinguishing characteristic of the OCNC1-null mice was the smaller size of the olfactory bulb (Fig. 1, compareA, B). In null mice all laminae were narrower with the biggestdifferences observed in the external plexiform layer (Table 1),which was 55% of the thickness of that of wild-type mice. Thethickness of the glomerular and granule cell layers also weresmaller as was the length of the olfactory bulb. The protein contentof bulbs from null mice was 53% of wild-type (mean mg/bulb ± SE;0.67 ± 0.03 vs 1.26 ± 0.05, respectively; p < 0.05; n = 3-10).

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Figure 1. OMP immunostaining in horizontal sections of olfactory bulbs from adult wild-type (A, wt) and OCNC1-null (B, ko) mice illustrated in dark-field photomicrographs. Note the smaller size of the olfactory bulbs in the null mice, but the apparently normal OMP staining of the olfactory nerve (on) and glomerular (gl) layers. Boxes indicate regions shown at higher magnification in Figure 2. Scale bar, 200 µm.


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Table 1. Laminar width and bulb length in wild-type and null OCNC-1 mice

To assess afferent innervation, olfactory bulbs were stained for OMP. Nerve fiber and glomerular staining were normal bothin distribution and intensity in the null mice (Fig. 1). However,aberrant fiber staining, reminiscent of that found during normaldevelopment (Monti Graziadei et al., 1980; Baker and Farbman,1993; Gong and Shipley, 1995), was observed in the external plexiformlayer (Fig. 2). The fibers were more disorganized than in developingcontrol mice. Lower levels of OMP, measured by ELISA (Mean percentagedecrease ± SE, 64 ± 3.0%), paralleled the smaller size of theolfactory bulb in the OCNC-1-null mice. These results suggestedthat fewer olfactory receptor cells are innervating the olfactorybulb (see below).

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Figure 2. Bright-field (A, C) and dark-field (B, D) photomicrographs illustrating the presence of ectopic OMP-immunolabeled fibers in OCNC1-null (C, D; ko) and not in wild-type (A, B, wt) mouse olfactory bulbs. Fibers (arrows) are scattered throughout the external plexiform layer (epl) of the null mice. Scale bar, 40 µm.

Tyrosine hydroxylase staining and activity in the olfactory bulb

TH immunostaining was dramatically less in the majority of glomeruli in the null olfactory bulb (Fig. 3) and was similar tothat previously observed in odor-deprived mice (Baker et al.,1993). In most regions the reduction was uniform with only scatteredcells and few intraglomerular fibers retaining TH immunoreactivity.In contrast, a group of glomeruli in the posterior aspects ofthe olfactory bulb, variously called either necklace or atypicalglomeruli and including the modified glomerular complex, retainedstrong TH staining in both cells and fibers (Fig. 4).

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Figure 3. Bright-field photomicrographs of TH immunostaining in wild-type (A, wt) and OCNC1-null (B, ko) mice. In wild-type mice, TH staining occurs in periglomerular cells surrounding all glomeruli and in fibers within the glomeruli. In the null mice, the majority of glomeruli have only a few TH-labeled neurons and display a dramatic reduction in fiber staining within the glomeruli. However, normal TH staining is found in a group of glomeruli (arrows) on posterior aspects of the olfactory bulb. Double arrows indicate the decrease in width of the external plexiform layer in OCNC1-null mice. ep, External plexiform layer; gl, glomerular layer; gr, granule cell layer; m, mitral cell layer; on, olfactory nerve layer. Boxes indicate regions shown at higher magnification in Figure 4. Scale bar, 200 µm.

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Figure 4. Bright-field (A, C) and dark-field (B, D) photomicrographs of TH immunostaining of olfactory bulb in wild-type (A, B; wt) and OCNC1-null (C, D; ko) mice. In wild-type mice, strong staining is observed in periglomerular cells and glomerular processes of all glomeruli. In the null mice, only scattered periglomerular cells (small arrows) contain TH in most glomeruli and, as illustrated in dark-field (D), labeled processes are absent. In contrast, TH staining is normal in both cells and processes in the atypical or necklace glomeruli (large arrow). Scale bar, 40 µm.

In confirmation of the immunocytochemical findings, TH activity in bulbs of OCNC1-null mice was 10% of wild-type levels (Fig.5A). The effect was specific to the olfactory bulbs since TH activitydid not differ between wild-type and null mice in either the substantianigra or the caudate nucleus, the former containing dopaminergiccell bodies that terminate in the latter brain region (Fig. 5B,C).

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Figure 5. TH activity in the olfactory bulb (OB), substantia nigra (SN), and caudate nucleus (CN) of wild-type (wt) and OCNC1-null (ko) mice. In the null mice, TH activity is normal in SN and CN, but lower only in the olfactory bulb. Student's unpaired t test; *p < 0.01; n = 3-10.

cFos and PAX6 immunoreactivity in the olfactory bulb

Previous studies demonstrated that expression of the immediate early gene cfos and its product, cFos, were reduced in parallelwith TH expression (Guthrie and Gall, 1995; Jin et al., 1996).In the current study, cFos immunostaining was much less intensein null mice (Fig. 6B) compared to wild-type mice (Fig. 6A), exceptin the region of the necklace glomeruli where staining was similarto that seen in controls. PAX6 immunoreactivity was of normalintensity in both the granule cell and glomerular layers in nullmice (Fig. 6C,D), suggesting that migration from the subependymalzone through the rostral migratory stream occurred in these mice(Dellovade et al., 1997).

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Figure 6. Bright-field photomicrographs illustrating cFos (A, B) and Pax6 (C, D) immunostaining in the olfactory bulbs of wild-type (A, C; wt) and OCNC1-null (B, D; ko) mice. In null mice, cFos is absent in most glomeruli but staining is present in the region of the necklace glomeruli (arrow, inset). Pax6 immunostaining is present in the olfactory bulbs of both wt and ko mice. Scale bar: A-D, 120 µm; inset, 60 µm.

OMP and GAP43 staining in the olfactory epithelium

Although the olfactory epithelium appeared structurally normal, the OE was thinner in OCNC1-null mice (Fig. 7). In addition,the number of OMP-labeled cells, assessed by the width of thestained area (Fig. 8), also was smaller. There also appeared tobe fewer GAP43 immunostained immature neurons (Fig. 9). Takentogether, these observations indicate that there are alterationsin the genesis and maturation of olfactory neurons in the OE ofthe OCNC1-null mice, leading to a reduction in maturation anddevelopment of the olfactory bulb.

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Figure 7. OMP immunostaining in the olfactory epithelium of wild-type (A, C; wt) and OCNC1-null (B, D; ko) mice. Low-power micrographs (A, B) illustrate that the receptor epithelium (oe) is thinner (C, D, compare length of double arrows) in all regions of the nasal cavity (nc). The boxed areas in A and B are shown at higher magnification in C and D. lp, Lamina propria; s, nasal septum. Scale bar: A, B, 250 µm; C, D, 30 µm.

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Figure 8. Bar graph illustrating that the septal receptor epithelium is 15% thinner in OCNC1-null mice (ko) as compared to wild-type mice (wt). n = 3 per group. *p < 0.05 by paired Student's t test.

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Figure 9. GAP43 immunostaining in the olfactory epithelium of wild-type (A, wt) and OCNC1-null (B, ko) mice. Fewer neurons (small arrows) are stained with GAP43, indicating that the number of both mature and immature neurons is lower in the null mice. The double arrows indicate the difference in the thickness of the olfactory epithelium (oe). lp, Lamina propria; nc, nasal cavity; s, septum. Scale bar, 30 µm.

Double immunolabeling with TH and PDE in olfactory bulb

To demonstrate that the TH-immunostained cells were necklace glomeruli, double label experiments were performed with a PDEantiserum that recognizes PDE2, the PDE subtype found only inatypical glomeruli (Juilfs et al., 1997). With the exception ofscattered fibers in other regions of the olfactory bulb, PDE immunoreactivityin the null mice was limited to fibers innervating glomeruli heavilystained with TH (Fig. 10).

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Figure 10. Low-power (A) and high-power (B) photomicrographs illustrating that only the necklace glomeruli (ng) that display intense TH immunoreactivity are innervated by PDE fibers. Most glomeruli (g) show no tyrosine hydroxylase immunoreactivity (brown) and are not innervated by PDE2-immunoreactive fibers (purple). The PDE2 fibers (A, arrow) course along the edge of the olfactory nerve layer (on) and innervate only the necklace glomeruli (B, arrow). Scale bar: A, 40 µm; B, 20 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These studies demonstrate that expression of the cyclic nucleotide-gated channel 1 subunit (OCNC1) is required for normaldevelopment of the olfactory epithelium and olfactory bulb. Theability of these null mice to survive to adulthood suggested thateither the olfactory system is not necessary for suckling behavioror that some olfactory neurons express other transduction pathwaysthat process sufficient odor information to allow for nipple attachment(Juilfs et al., 1997; but see Gold, 1999).

Loss of OCNC1 significantly altered several aspects of olfactory system development. Most apparent was the smaller size ofthe olfactory bulb that was evident on visual inspection and confirmedby total protein measurements. All laminae were reduced in width,suggesting loss of processes, especially in the external plexiformlayer, and neurons in the granule and periglomerular layers. Whetherthe number of mitral cells is fewer remains to be assessed. Thesmaller olfactory bulb observed in the OCNC1-null mice is similarto that seen after both neonatal and adult odor deprivation (Frazierand Brunjes, 1988; Baker, 1990; Baker et al., 1993), suggestingthat similar activity-dependent mechanisms may regulate neuronalmaturation and survival in the olfactory bulb of the OCNC1-nulland of odor-deprivedmice.

A reduction in bulb size could result from a change in rate or number of cells destined to be granule and periglomerular cellsmigrating to the olfactory bulb from the subventricular zone (SVZ)through the rostral migratory stream (RMS). Because OCNC1 is alsoexpressed in the CNS, including striatum (Bradley et al., 1997;Parent et al., 1998), and bulb size is reduced in other null phenotypesof the CNS, including nCAM-, dlx- and PAX6-deficient mice (Treloaret al., 1997; Bulfone et al., 1998; Dellovade et al., 1998), thereduced size could result from disruption of migration as a consequenceof either odor-induced activity or altered expression of the channelin the forebrain. However, migration of periglomerular and granulecells did occur in the OCNC1-null mice, as evidenced by the presenceof PAX6 labeling in both the RMS (data not shown) and olfactorybulb. PAX6 was previously shown to be a marker for cells in theSVZ that populate the olfactory bulb including TH-expressing periglomerularcells (Dellovade et al., 1997). Further studies will be requiredto determine if granule cell migration is altered in OCNC1-nullmice and if so by whatmechanism.

Abnormal maturation of receptor cell innervation also occurred in the null mice. OMP, which is found in high concentrationsin olfactory receptor cells (Margolis, 1972), was used to demonstratethe afferent innervation to the olfactory bulb. OMP-immunoreactivefibers occurred not only in their characteristic locations inthe nerve fiber and glomerular layers but also randomly distributedin the external plexiform layer (EPL). Previously, aberrant olfactoryreceptor afferent fibers were described during development butgenerally exhibited more organization with distinct bundles inthe EPL and a laminar profile in the mitral cell layer (MontiGraziadei et al., 1980; Baker and Farbman, 1993; Gong and Shipley,1995). The fact that in animals odor-deprived as neonates aberrantfibers are not observed suggests that mechanisms acting prenatallyare important to axon guidance and targeting in the null mice.OMP levels were reduced by 64% in the olfactory bulbs of the nullmice, which was consistent with the smaller size of the bulbs.The receptor epithelium in the null mice was ~15% thinner comparedto controls reflecting the decreased level of OMP immunoreactivityin the olfactory bulb. This reduction confirms the previouslyobserved decrease in OMP message (Parent et al., 1998). In additionto the decline in the number of mature receptor cells stainedwith OMP, there appeared to be fewer immature neurons as reflectedby GAP43 immunostaining, suggesting altered generation and maturationof receptor cells in OCNC1-null mice (Verhaagen et al., 1989,1990).

Transduction of odorant information in OCNC1-null mice may be restricted to a specific subset of receptor cells in the posteriorrecesses of the olfactory epithelium that innervate glomerulilocalized to posterior aspects of the olfactory bulb (Juilfs etal., 1997). These atypical, modified, or necklace glomeruli werepreviously distinguished by several criteria. Studies using 2-deoxyglucoseas an indicator of activity suggested that they were involvedin suckling behavior (Teicher et al., 1980; Greer et al., 1982).The glomeruli also were characterized on the basis of high expressionof acetyl cholinesterase, choline acetyltransferase (Zheng etal., 1987; Le Jeune and Jourdan, 1991), placental antigen X-P2(Shinoda et al., 1990), and immunoreactivities to monoclonal antibodies2C6 and 213 (Ring et al., 1997). They also receive innervationfrom receptor cells that express a specific guanylyl cyclase (GC-D)and a phosphodiesterase, PDE2 (Juilfs et al., 1997). In contrast,the vast majority of receptor neurons contain a calcium-calmodulin-dependentPDE (PDE1C2) and a high-affinity cAMP-specific PDE (PDE4A) (Juilfset al., 1997).

The current studies support the hypothesis that these unique glomeruli are innervated by a subset of receptor cells that maycontain other channels. Previous studies demonstrated that expressionof the catecholamine biosynthetic enzyme TH, expressed in dopamineneurons in the olfactory bulb, is reduced dramatically by odordeprivation (Baker et al., 1983, 1984, 1993; Kosaka et al., 1987;Guthrie et al., 1990; Baker, 1990). Adult OCNC1-null mice hadfewer TH-immunoreactive periglomerular cells in most glomeruli,consistent with the inability of receptor cells that lack OCNC1to respond to odors. However, the necklace glomeruli, identifiedby their PDE2 innervation, continued to express TH, suggestingthat odor-induced stimulation still occurred in the receptor cellsprojecting to these regions of the olfactory bulb. In view ofthe expression of OCNC1 in other brain regions, including striatum(Bradley et al., 1997; Parent et al., 1998), the lower levelsof TH expression in null mice could be secondary to deficiencyof the channel in the CNS and not the receptor epithelium. However,TH activity levels were normal in the substantia nigra and caudatenucleus, the cell body, and target regions of the major midbraindopaminergic pathway, indicating that the TH loss in the olfactorybulbs of the null mice was likely mediated by odor deprivation.The distribution of cFos expression further supports a relationshipbetween receptor cell activity and the loss of TH immunoreactivity.As previously found in odor deprivation (Jin et al., 1996), parallelcFos and TH expression could be demonstrated, with most glomerulicontaining little or no cFos immunoreactivity, whereas the atypicalglomeruli express normal levels of cFoslabeling.

In summary, these studies demonstrate that OCNC1 is required for normal development of the olfactory bulb, including olfactorybulb size, innervation, and dopamine phenotype. Similarly, theolfactory epithelium does not develop its normal complement ofeither mature or immature neurons. Most intriguing is the findingthat one population of bulbar target neurons, those associatedwith the atypical or necklace glomeruli, does retain normal expressionof the dopamine phenotype, as evidenced by TH staining. The periglomerularneurons in these glomeruli receive their innervation from receptorcells that express a phosphodiesterase and a guanyl cyclase notfound in the majority of receptor cells. Therefore, our observationsargue that the PDE/GC-D-expressing receptor cells transduce odorinformation by a mechanism that is not dependent onOCNC1.

  FOOTNOTES

Received June 1, 1999; revised Aug. 11, 1999; accepted Aug. 16, 1999.

This work was supported by National Institutes of Health Grants AG09686 (H.B.) and DC03112 (F.M.), and by Howard Hughes MedicalInstitute (R.R.).
Correspondence should be addressed to Dr. Harriet Baker, Cornell University Medical College at The Burke Medical ResearchInstitute, 785 Mamaroneck Avenue, White Plains, NY 10605. E-mail:habaker{at}med.cornell.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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