Increased Anxiety and Impaired Pain Response in Puromycin-Sensitive Aminopeptidase Gene-Deficient Mice Obtained by a Mouse Gene-Trap Method

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The Journal of Neuroscience, July 15, 1999, 19(14):6068-6078

Increased Anxiety and Impaired Pain Response in Puromycin-Sensitive Aminopeptidase Gene-Deficient Mice Obtained by a Mouse Gene-Trap Method
Tomoharu Osada¹^,², Shiro Ikegami¹, Keiko Takiguchi-Hayashi¹, Yukiko Yamazaki¹, Yuko Katoh-Fukui¹, Toru Higashinakagawa¹, Yoshiyuki Sakaki², and Takashi Takeuchi¹
¹ Mitsubishi Kasei Institute of Life Sciences, Tokyo,194-8511, Japan, and ² Human Genome Center, Institute of Medical Science, University of Tokyo, Tokyo 108-8639, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A mouse mutation, termed goku, was generated by a gene-trap strategy. goku homozygous mice showed dwarfism, a marked increasein anxiety, and an analgesic effect. Molecular analysis indicatedthat the mutated gene encodes a puromycin-sensitive aminopeptidase(Psa; EC 3.4.11.14), whose functions in vivo are unknown. Transcriptionalarrest of the Psa gene and a drastic decrease of aminopeptidaseactivity indicated that the function of Psa is disrupted in homozygousmice. Together with the finding that the Psa gene is stronglyexpressed in the brain, especially in the striatum and hippocampus,these results suggest that the Psa gene is required for normalgrowth and the behavior associated with anxiety andpain.

Key words: puromycin-sensitive aminopeptidase; anxiety; analgesia; dwarfism; gene trap; enkephalins

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In addition to analyses of spontaneous mutant mice, the technology of artificial mutagenesis in the mouse can give us informativeinsights into higher neuronal functions such as emotion or learningand memory. One methodology, called gene trap, enables us to capturethe novel or functionally unknown genes and, at the same time,to generate the corresponding mutant mice (Gossler et al., 1989).In fact, several genes that play crucial roles in mouse embryogenesishave been identified by this method (for review, see Kitajimaand Takeuchi, 1999). Although few studies on mammalian neuronalfunctions using gene-trap methods have been reported, this methodalso has the potential to identify genes involved in thearea.

Here we established a novel mutant mouse line, goku, by a gene-trap method and proceeded more than 14 backcrosses to transferthe trapped allele to a BALB/cA background. goku mutant mice showdwarfism and several behavioral abnormalities involved in anxietyand pain. We also show that the trapped gene, presumed to be responsiblefor the observed phenotypes, encodes a puromycin-sensitive aminopeptidase(Psa; EC 3.4.11.14) and that the Psa gene was disrupted in themutantmice.

Psa was purified as a candidate protein for involvement in the extracellular metabolism of enkephalins (Hersh and McKelvy,1981; McLellan et al., 1988). Other studies suggest that Psa isinvolved in the inactivation of various neuropeptides such asdynorphins, cholecystokinin, and somatostatin (Hui et al., 1995).However, the functions for Psa in the metabolism of these peptidesremain unclear because Psa was found to be a cytoplasmic protein(Dyer et al., 1990; Constam et al., 1995). In addition, the specificityof the sequences recognized by Psa is very low, and no inhibitorsspecific for Psa are known. These facts have made it difficultto elucidate the substrates and functions of Psa in vivo.

Psa-deficient mice may provide a useful model system to characterize the functions of Psa in vivo. Our present studies suggestthat Psa is required in the brain for normalbehavior.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mice
The goku mouse line was generated using the gene-trap method described elsewhere (Takeuchi et al., 1995). Backcross matingsof heterozygous female mice with BALB/cA strain mice were undertaken.goku homozygous mice were generated by intercrossing heterozygousmice with a BALB/cA background. All mice were housed in littersof one to three in cages with sawdust and with free access tofood and water. They were maintained in a 12 hr light/dark cyclewith lights on at 8:00 A.M. at constant temperature (23 ± 1°C).
Experiments involving animals were performed in accordance with standard ethical guidelines for the care and use of laboratoryanimals (NIH Standards for Treatment of Laboratory Animals, 1985)and approved by the local ethicalcommittee.

5' Rapid-amplified cDNA ends (5'-RACE)
To obtain fragments of goku cDNA, we used a 5'-AmpliFinder RACE Kit (Clontech, Palo Alto, CA) described elsewhere (Takeuchiet al., 1995). Amplified products from the cDNA of heterozygousmouse liver were cloned into a pGEM-T plasmid (Promega, Madison,WI). DNA sequencing analysis was performed with an ABI PRISM DyeTerminator Cycle Sequencing Ready Reaction Kit (Perkin-Elmer,Foster City,CA).

Southern and Northern blot analysis and allele-specific genotyping
Northern blot analysis was performed by a conventional method (Maniatis et al., 1989). To isolate mRNA from the brain of eachgenotype, we used a FastTrack 2.0 kit (Invitrogen, San Diego,CA). mRNA (2 µg) was applied to gel electrophoresis. The 5' (psa-1)and 3' (psa-2, -3) probes for the Northern blot analysis correspondedto nucleotide positions 316-519, 645-1399, and 2284-2803, respectively(GenBank Accession No. MMU35646). For genotyping, the purificationof genomic DNA and genomic Southern blot analysis were performedby a conventional method (Maniatis et al., 1989). Genomic DNAfrom the tails of each mouse genotype was digested with EcoRIand hybridized using psa-2 as aprobe.

Aminopeptidase activity assay
Aminopeptidase activity was assayed as described previously (Dyer et al., 1990; Constam et al., 1995). Cytosolic fractionswere prepared as described (Dyer et al., 1990). Protein concentrationof the crude extracts was measured by a DC protein assay kit (Bio-Rad,Hercules, CA). Aliquots of the crude extracts corresponding to100 µg of protein were used in the assay. The extracts were incubatedwith alanyl p-nitroanilide (Sigma, St. Louis, MO) to assess aminopeptidaseactivity. The release of p-nitroaniline was measured spectrophotometricallyat 405nm.

Physiological analysis in plasma
All parameters in plasma were measured by conventional methods, and total triiodothyronine and thyroxine were also measuredby enzyme immunoassay at the Veterinary Medical Center, Universityof Tokyo (Tokyo, Japan). Growth hormone (GH) and insulin-likegrowth factor (IGF-I) were measured at Koto Biken Co. Ltd. (Tokyo,Japan) byradioimmunoassay.

Behavioral tests
Behavioral tests were performed between 1 and 6 P.M. in a soundproof room where external noise was greatly reduced (from $-$ 30dB at 125 Hz to $-$ 45 dB at 500 Hz). Adult male mice (8-15 weeksold) were used. The room had a clean air conditioning system.All of the apparatus touched by the tested mice were cleaned withdeionized water and 70% ethanol after every testtrial.
Rod-walking and wire-hanging tests. To assess motor coordination and traction in mice, rod-walking and wire-hanging tests,respectively, were performed. Briefly, the tested mouse was placedat the center of an elevated wooden rod (diameter, 1.5 × 60 cm).The time spent in moving from the start point, where the mousewas initially placed, to the edge of the rod (length 30 cm) wasmeasured. This test was duplicated. For the wire-hanging test,forepaws of the tested mouse were hung on an elevated piano wire.Traction was determined as the ability not to drop from the wireand to remain stable and hanging for over 20 sec. This test wasalsoduplicated.
Open-field test. To measure general activity in mice, the open-field test was performed as described previously (Ikegami,1994). Each mouse was initially placed at the center of the apparatus,and movement was recorded for 30min.
Elevated plus-maze test. The elevated plus-maze test was conducted basically as described previously (Lister, 1987). For thetest, each mouse was initially placed in the center of the maze.Behavior was videotaped during a 15 min testperiod.
Hot-plate test. The hot-plate test was performed as described elsewhere (Eddy et al., 1950). An electronically controlledstainless steel plate was heated to 55.0 ± 0.5°C. A cylinder (30cm high) made of a transparent plastic plate was placed on thehot plate. A mouse was initially put on the center of the hotplate. During the test period, all behaviors were videotaped.The latencies of responses (licking and jumping) weremeasured.
Tail-flick test. The tail-flick test was performed with an Omnitech Model TF automated tail-flick apparatus (Omnitech, Columbus,OH) following manufacturer's instructions. The latency of a response(tail-flicking) to the thermal stimulus produced by 20 mA wasmeasured. Three repeated trials were conducted for eachindividual.

Histology and immunodetection
For X-gal staining, Nissl staining, and immunofluorescence analysis, mice were anesthetized and perfused transcardially firstwith PBS and then with 0.5% glutaraldehyde; for immunohistochemistry(IHC), they were then perfused with 4% paraformaldehyde and 7%picric acid in PBS. The brains were removed, post-fixed for 4hr in the same buffer used for perfusion, and stored overnightat 4°C in 30% sucrose inPBS.
For X-gal staining, a series of frozen sections (20 µm) was stained for 6.5 hr as described previously (Motoyama et al., 1997).Another series was stained with cresyl violet for Nissl staining.For double-immunofluorescence experiments, we used rabbit polyclonalantibodies against $beta$ -galactosidase (gal) (Cappel, West Chester,PA; dilution, 1:500) and monoclonal antibodies against glial fibrillaryacidic protein (GFAP) (Sigma; dilution, 1:200), cyclic nucleotidephosphohydrolase (CNP) (Promega; dilution, 1:200), and neuronalnuclei (NeuN) (Chemicon, Temecula, CA; dilution, 1:200) as primaryantibodies. Briefly, incubation with FITC-conjugated secondaryantibodies with a specificity for rabbit IgG (Chemicon; 3 hr),primary monoclonal antibodies (overnight), and finally rhodamine-conjugatedsecondary antibodies with a specificity for mouse IgG (Chemicon;3 hr) was followed by incubation of the sections with primaryantibodies against $beta$ -gal (overnight). The IHC analysis was performedas described elsewhere (Motoyama et al., 1997). As primary antibodies,we used antibodies against methionine (met)-enkephalin, leucine(leu)-enkephalin (Chemicon; dilution, 1:5000), and substance P(Takiguchi-Hayashi et al., 1998) (dilution, 1:5000),respectively.

Statistical analyses
Behavioral abnormalities in the open-field test, the elevated plus-maze test, and the hot-plate test in goku homozygous micewere assessed by one-way or two-way ANOVA. Appropriate pairwisecomparisons were performed by the least significant difference(LSD) test. Mean values between the two groups were tested byStudent's ttest.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Establishment of the goku mutant mouse line

To obtain novel genes that are expressed characteristically in the CNS and are involved in neuronal development or functions,we used a mouse gene-trap method described previously (Takeuchiet al., 1995). A trap vector, designated TV2, that has a lacZgene for monitoring the expression of the trapped gene was introducedinto embryonic stem (ES) cells. Chimeric embryos generated byblastocyst injection with a gene-trapped ES cell line, B8, showedstrong lacZ gene expression in the CNS at embryonic day 10.5.We established a mouse line by crossing the B8-derived chimericmale mice with BALB/cA females. Heterozygous mice were fertileand showed no apparent abnormalities. Southern blot analysis showedthat only one copy of the trap vector was integrated into thegenome of the B8 cells (data notshown).

Homozygous mice showed dwarfism and the behavioral abnormalities described below. We named this mouse line goku (after a characterof the Japanese cartoon "Dragon Ball") because of the characteristicbehaviors associated with homozygous mice. To analyze goku mutantmice in a uniform genetic background, the trapped allele was introducedinto BALB/cA background mice by backcrossing heterozygous micewith BALB/cA mice. In the experiments described in this manuscript,we used F14-17 heterozygotes as parents for the intercross toobtain goku homozygous mice. No apparent phenotypic differencesin goku homozygous mice could be observed throughout the testedgenerations.

Dwarfism in goku mutant mice and the measurement of physiological parameters in plasma

We found that goku mutant mice were smaller than their littermates. The body weight at age 7 weeks was <70% of that of controllittermates (Fig. 1). This difference became apparent first at~3 weeks after birth. Interestingly, no appreciable sex differencein body weight could be observed in goku mutant mice (Fig. 1).Because this phenotype could arise from malnutrition or endocrineimbalance, we measured the plasma levels of major physiologicalparameters that are used as reference values (Table 1). In addition,the plasma levels of growth hormone and insulin-like growth factorI were measured (Table 1). No significant differences betweenwild-type and goku mutants could be observed in any of the parameterstested, suggesting that there are no serious abnormalities inkidney, liver, thyroid, or gastric organs.

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Figure 1. Dwarfism in goku mutant mice. Mean body weights of wild-type males (; n = 13), wild-type females ( $open circle$ ; n = 13), homozygous males ( $black-triangle$ ; n = 10), and homozygous females ( $triangle$ ; n = 8) by age (Weeks) are plotted. Vertical bars represent SEM.


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Table 1. Reference values in wild-type and homozygous mutant mice

goku mutant mice display markedly increased anxiety and analgesia

We found that goku mutant mice froze or sometimes squeaked when presented with physical stimuli such as poking with fingersor tail pulling. To evaluate these behavioral abnormalities, sixbehavioral tests were conducted. To exclude the involvement ofestrous cycling on behavior in female mice, only male mice wereused in these tests. In all six tests, wild-type, heterozygous,and goku mutant mice were used, but no significant differenceswere observed between wild-type and heterozygous mutantmice.

Open-field test, wire-hanging test, and rod-walking test
In the open-field test, we evaluated spontaneous locomotor activity and the pattern of each genotype under a novel environment.Male mice 8-15 weeks old were tested at 1-6 P.M. The mean locomotoractivity in goku mutant mice was reduced to 48.7-57.2% of wild-typemice in any block of 5 min throughout the entire 30 min test (Fig.2A). In addition, mean vertical activity, which means rearingbehavior, was markedly decreased to 5.4-18.8% of wild-type micein each block of 5 min (Fig. 2B). Fisher's LSD test indicatedthat locomotion and rearing in goku mutant mice were significantlylower than in heterozygous mice (locomotion, p < 0.01; rearing,p < 0.01) and wild-type mice (locomotion, p < 0.001; rearing,p < 0.001), after obtaining significant differences with two-wayANOVA (locomotion, F_(2,480) = 161.8, p < 0.001; rearing, F_(2,480)= 90.17, p < 0.001). Moreover, goku mutant mice had a tendencyto stay close to the side walls of the open-field box, indicatingthat goku mutant mice show thigmotaxis (preference for the sidewalls) (Fig. 2C), which is thought to be an index of anxiety inmice (Treit and Fundytus, 1989).

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Figure 2. Altered locomotor activity of goku mutant mice as revealed by the open-field test. A, Means (±SEM) of locomotor activity. B, Mean (±SEM) frequency of rearing behavior. Wild-type mice (; n = 26), heterozygotes ( $open circle$ ; n = 27), and homozygotes ( $black-triangle$ ; n = 30). C, Examples of locomotor patterns of wild-type (top) and homozygous (bottom) mice. In the locomotor patterns, the numbers under the bars represent the frequency of photobeam interruption caused by animal movement. One division of the scale on the bars indicates 250 (5 × 50) counts. Each mouse was kept in the novel environment with the photocell for 30 min.

All abnormalities of goku mutant mice observed in the open-field test during the diurnal periods were also observed duringnocturnal periods (data not shown), suggesting that the decreasedactivities observed in this test were not dependent on the circadianrhythm.
To exclude the possibility that goku mutant mice suffered from myogenic dysfunctions, we performed a wire-hanging test fortraction and a rod-walking test for balance coordination. No significantdifferences were observed among genotypes (Table 2), indicatingthat neither significant ataxia nor dysfunctions of motor coordinationcause the behavioral abnormalities in goku mutant mice.


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Table 2. Balance, coordination, and traction in wild-type, heterozygous, and homozygous mutant mice

Elevated plus-maze test
A marked decrease in rearing behavior in general activity and an increase in thigmotaxis suggest that goku mutant mice maybe emotionally abnormal. We investigated the emotionality of mutantmice using an elevated plus-maze task, which is a useful testfor measuring anxiety or fear (Pellow and File, 1986; Lister,1987). The mean time spent by goku mutant mice in exploring theopen arms was significantly less (56.6%) than that of wild-typemice (Fig. 3A) (F_(2,57 = 4.35, p < 0.05, one-way ANOVA; p < 0.05,LSD test). Moreover, the frequency of entry into the open armswas also significantly less in goku mutant mice than in wild-typemice (Fig. 3B) (F_(2,57) = 4.23, p < 0.05, one-way ANOVA; p < 0.05,LSD test). On the other hand, the frequency of entry into theclosed arms, including turnovers into the same arm, was reduced,but this difference was not significant (Fig. 3C) (F_(2,57) = 1.43,p = 0.25, one-way ANOVA), indicating that a reduction in generalactivity did not cause these abnormalities. We observed that gokumutant mice generally trail in the closed area. Interestingly,we also noticed that goku mutant mice sometimes froze once theyenter the closed arms. Taken together with data from the open-fieldtest, these results suggest that goku mutant mice display a highlyincreased anxiety or fear response in novel environments.

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Figure 3. Increased anxiety and nociceptive response to a thermal stimulus in goku mutant mice. A-C, Elevated plus-maze test. A, Mean (±SEM) percentage of time spent in the open arms. B, Means (±SEM) of total number of entries into the open arms. C, Crossings to closed arms (including turnovers into the same arm). Wild-type mice (; n = 26), heterozygotes (; n = 27), and homozygotes ( $black-square$ ; n = 30); mice were tested for 15 min. *p < 0.05, **p < 0.01 (wild-type mice vs homozygotes), # p < 0.05, ## p < 0.01 (heterozygotes vs homozygotes) (LSD test after one-way ANOVA). D, The hot-plate test. Wild-type mice (; n = 12), heterozygotes (; n = 18), and homozygotes ( $black-square$ ; n = 14). Mean latency (±SEM) of jumping is represented. Mice were placed individually on the 55°C hot-plate surrounded by a cylindrical wall. E, The tail-flick test. Wild-type mice (; n = 4), heterozygotes (; n = 13), and homozygotes ( $black-square$ ; n = 5). **p < 0.001 (wild-type mice vs homozygotes), # p < 0.01, ## p < 0.001 (heterozygotes vs homozygotes) (LSD test after one-way ANOVA).

Hot-plate and tail-flick tests
To test more complex organized unlearned behaviors, we performed a hot-plate test because this involves a voluntary purposefulact requiring supraspinal sensory processing (Chapman et al.,1985). The jumping response is the most typical behavior againsta nociceptive stimulus mediated at the supraspinal level (Woolfeand Macdonald, 1943; Köning et al., 1996). In goku mutant mice,the mean latency of the jumping response was significantly extendedto 1.7 times that in wild-type mice (Fig. 3D) (F_(2,
41) = 17.15,p < 0.001, one-way ANOVA; p < 0.001, LSD test). As another parameterof nociceptive response mediated at the supraspinal level, thelatency of the hindpaw licking response in goku mutant mice wasalso extended compared with wild littermates (data notshown).
To assess pain response mediated at the spinal level, we performed the tail-flick test. No significant differences of themean latency of the tail-flick behavior were observed among threegenotypes, indicating that goku mutant mice exhibit a normal painresponse at the spinal level (Fig. 3E).
These data suggest that responses to thermal stimuli mediated at the supraspinal level are hampered in goku mutantmice.

Cloning of the trapped gene

We identified the trapped gene that is presumably responsible for the abnormal phenotypes in goku mice. It was expected thatthe insertion of the trap vector arrests transcription of thetrapped gene because the trap vector was designed to produce afusion mRNA. To identify the trapped gene, we used the 5' rapidamplification of cDNA ends (RACE) procedure. The two cDNA cloneswere isolated from fusion RNA extracted from the liver of a heterozygousmouse. The 74 bp cDNA sequences, which appeared to be derivedfrom the endogenous genomic DNA, were identical in both clones.A comparison with the EMBL and GenBank databases revealed theisolated cDNA to correspond to nucleotide positions 453-526 ofPsa cDNA (GenBank Accession No. MMU35646). The fusion site betweenthe Psa cDNA and the trap vector is between nucleotide positions526 and 527. The region amplified by PCR in the 5' RACE procedurewas not amplified when genomic DNA from heterozygous mice wasused as a template with the same primer set in conventional PCR.This result suggests that the trap vector is inserted in an intronof the Psa gene. To confirm that the trap vector is inserted withinthe Psa gene, genomic Southern blot analysis was performed (Fig.4). Genomic DNA from the tails of wild-type, heterozygous, andhomozygous mice was digested with endonuclease EcoRI. A probecorresponding to sequences downstream of the insert site (psa-2)yielded a band of ~15 kb that was detected in both wild-type andheterozygous mice and a band of ~3.8 kb that was detected in bothheterozygotes and homozygotes (Fig. 4). Using the 3' region ofthe trap vector as a probe, a band of 3.8 kb was again detectedin both heterozygotes and homozygotes (data not shown). Theseresults show that the trap vector is inserted within the Psa geneand that this analysis enables us to identify all three genotypesin the goku mutant mouse strain.

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Figure 4. A trap vector was inserted in the Psa gene. A, The schema for wild and trapped alleles. a, Wild-type allele; b, trapped allele. Bold bar (psa-2) represents the probe for Southern blot analysis that recognizes an EcoRI fragment of ~15 kb from the wild allele and a 3.8 kb fragment from the trapped allele. Open squares represent exons of the Psa gene. B, Examples of Southern blot analyses of the genotypes. Lanes 1-11, Results of individual mice. Genotype and sex are shown at the top of each lane. W, Wild-type mouse; Ht, heterozygote; Hm, homozygote; M, male; F, female.

Transcriptional arrests in goku homozygotes

We also examined the transcriptional status of Psa gene in goku homozygous mice. Figure 5 shows the results of Northern blotanalysis of the mRNA derived from the brains of the three genotypes.With a probe corresponding to sequences upstream of the fusionsite (psa-1), a 1.7 kb band of unknown origin was detected inall three genotypes. In addition, a 4.5 kb band in wild-type mice,4.5 and 6.7 kb bands in heterozygotes, and a single 6.7 kb bandin homozygotes were detected. Because the size of the 4.5 kb bandis the same as that of the Psa mRNA described in Constam et al.(1995), we concluded that the 4.5 kb band is derived from theintact Psa mRNA. With the lacZ gene as a probe, a 6.7 kb bandwas again detected in both heterozygotes and homozygotes (datanot shown). These results indicate that the 6.7 kb band is derivedfrom a fusion mRNA transcribed from the trapped allele. Otherprobes corresponding to sequences downstream of the fusion site(psa-2 and -3) detected a single 4.5 kb band in wild-type andheterozygous mice, but no signal was detected in homozygotes.These data show that the Psa gene is transcriptionally arrestedin goku homozygous mutant mice. Although residues 1-95 of thePsa protein (total 875 amino acids) (Constam et al., 1995; Tobleret al., 1997) could be produced as a fusion protein with neo^r protein by this arrest, the mutated RNA lacks the region encodingthe catalytic domain (HEXXHX₁₈E, residues 353-376). This indicatesthat Psa activity is disrupted in goku homozygous mice. We designatedthe Psa allele trapped in goku mice as Psa^goku and designated wild-type, heterozygous, and homozygous mice asPsa^+/+, Psa^+/goku, and Psa^goku/goku mice, respectively.

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Figure 5. Transcriptional arrest of the Psa gene in goku mutant mice. A, Schema for transcriptional arrest. a, Wild-type transcript; b, trapped transcript. Filled horizontal bar, Coding region of the Psa gene; hatched horizontal bar, region derived from the trapped vector; double-headed arrow, region encoding the catalytic domain containing HEXXHX₁₈E; psa-1, -2, -3, probes for Northern blots analysis. B, Northern blot analysis. Poly(A⁺) RNA (2 µg) from the brains of 8-week-old mice were electrophoresed. Human $beta$ -actin cDNA was used as a control. W, Wild-type mice; Ht, heterozygotes; Hm, homozygotes.

The activities of aminopeptidases sensitive to puromycin in the brain of Psa^goku/goku mice

Because Northern blot analysis indicated that the Psa gene is disrupted in Psa^goku/goku mice, we assessed this evidence at the protein level. Psa activity,however, cannot be measured directly because there are no knownsubstrates or inhibitors specific for Psa. Therefore, we examinedthe activities of aminopeptidases sensitive to puromycin in Psa^goku/goku mice. Soluble extracts from the brains of Psa^+/+ and Psa^goku/goku mice were tested, because Psa activity in the brain is relativelystronger than in other organs (McLellan et al., 1988). We usedalanyl-p-nitroanilide as a substrate because it is efficientlymetabolized by rat Psa and has a relatively high specificity formouse Psa compared with other p-nitroanilides (Constam et al.,1995). The total aminopeptidase activity in the soluble fractionsfrom Psa^goku/goku mice was reduced to 39.5% of that in Psa^+/+ littermates (Fig. 6). After preincubating tissue extracts withpuromycin as a Psa inhibitor (Hersh, 1985), the aminopeptidaseactivity in Psa^+/+ mice was reduced depending on the dose of puromycin and reacheda plateau level at 12.0% of the activity in Psa^+/+ mice without puromycin (Fig. 6). This final activity was supposedto be derived from the aminopeptidases insensitive to puromycin.In Psa^goku/goku mice, the activity was finally reduced to almost the same levelas that of Psa^+/+ littermates after preincubation with puromycin. These resultsindicate that the activity insensitive to puromycin is not affected,whereas the activity sensitive to puromycin is drastically reducedin Psa^goku/goku mice, supporting the notion that Psa activity is disrupted inPsa^goku/goku mice. The decreased aminopeptidase activity dependent on thedose of puromycin in Psa^goku/goku mice was supposed to be derived from the aminopeptidases sensitiveto puromycin other than Psa.

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Figure 6. Puromycin-sensitive aminopeptidase activity is decreased in Psa^goku/goku mice. The aminopeptidase activity in brain extracts from Psa^+/+ (open columns; n = 8) and Psa^goku/goku mice (filled columns; n = 4) was incubated with alanyl-p-nitroanilide as a substrate. The effect of puromycin as an inhibitor for Psa with various concentrations was also measured. The results are shown as the relative absorbance in which the value of Psa^+/+ with no puromycin added is defined as 100.

Expression pattern of the Psa gene in the brain

The reporter gene lacZ was introduced into the Psa gene and expressed as a fusion mRNA with Psa transcripts in Psa^+/goku and Psa^goku/goku mice. In this way, we can monitor the expression of Psa. Expressionin the brain, liver, kidney, spleen, ovary, and testis of adultPsa^+/goku mice was examined by whole-mount X-gal staining. Although expressionof the Psa gene was observed in all tissues examined, strong expressionwas detected in the brain and testis (data not shown). These dataare consistent with the expression pattern shown by Northern blot(Constam et al., 1995) and with the tissue distribution of Psaactivity (McLellan et al., 1988). We examined the distributionof Psa gene expression in the brain in detail, because the phenotypesobserved in mutant mice were suspected to result from defectsin brain functions. The widespread expression of the Psa genewas observed in the brain. We also doubly stained lacZ-positivecells with markers for neurons, astrocytes, and oligodendrocytes(NeuN, GFAP, and CNP, respectively) (Fig. 7E-G). The Psa genewas found to be expressed in all three cell types (Fig. 7E-G).Almost all neurons and glial cells in the brain appeared to expressthe Psa gene. Among neurons, the intensity of expression was notidentical. Strong expression was observed in the hippocampus,and striatum (Fig. 7A-D). Three types of neurons could be observed,especially in the thalamus. The first type was strongly positive,the second moderately positive, and the third considerably weaker(Fig. 7H).

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Figure 7. Expression patterns of the Psa gene in the adult brain of Psa^+/goku mice. A, C, Brain sections (20 µm) stained with X-gal. B, D, Sections, 60 µm anterior to A and C, respectively, stained with cresyl violet. E-G, Dual color immunofluorescence micrograph images of $beta$ -gal (green; E-G) and markers (red) (E, NeuN; F, GFAP; G, CNP). All neurons (E) and glias (arrows in F and G) investigated were double positive (orange). H, High-power views in the thalamus of section in B using differential interference microscopy. Strong (arrows), moderate (arrowheads), and weak (asterisks) positive cells for $beta$ -gal activity. Scale bars: A-D, 1.6 mm; E-G, 10 µm; H, 100 µm.

Morphology and immunolocalization of neuropeptides in the brain of Psa^goku/goku mice

We compared the morphology of the brains of Psa^goku/goku with those of controls by observing sliced sections (1 mm) of the brains fromeach genotype. We could not detect any morphological differences.The brains of the Psa^goku/goku mice were smaller than those of controls, but the relative weightof the brain (per total body weight) was not different (data notshown). Although there is a possibility that minute abnormalitieswere overlooked, these data suggest that Psa does not play a crucialrole in brain morphogenesis and that the behavioral impairmentobserved in Psa^goku/goku mice does not result from morphological defects in thebrain.

To evaluate the status of neuropeptides in the brains of Psa^goku/goku mice, we performed immunohistochemical analysis. Although a numberof neuropeptides are closely involved in anxiolytic behaviorsand pain responses (for review, see Olson et al., 1996; Woolfet al., 1998), we focused on two types of enkephalins, met-enkephalinand leu-enkephalin, because Psa has been purified as a candidateenkephalinase in vivo. Moreover, enkephalins are reported to beinvolved in both anxiety and pain (Köning et al., 1996). In addition,the status of substance P, one of the main modulators of sensitivityto pain, was examined. We tested the immunolocalization of thesepeptides in the cerebrum of Psa^+/+ and Psa^goku/goku mice. No apparent differences in the distribution patterns orintensity could be detected between these genotypes. This immunoreactivitywas apparent in the subcommissural ventral pallidum in which thesepeptides colocalize (Heimer et al., 1995) (Fig. 8). This showsthat the expression of these three neuropeptides is not severelyaffected in Psa^goku/goku mice.

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Figure 8. Immunolocalization of enkephalins and substance P in the subcommissural ventral pallidum (VP). Sections from Psa^+/+ (A, C, E) and Psa^goku/goku mice (B, D, F), stained with antibodies against met-enkephalin (A, B), leu-enkephalin (C, D), and substance P (E, F). ac, Anterior commissure, posterior. Scale bar, 100 µm.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Behavioral and other physiological traits are adequately complex and occasionally variable, and a number of genes probablycontribute to them. Therefore, to understand the mechanisms ofunusual phenotypes observed in the mutant mice, it is importantto consider the effects of background genes (Gerlai, 1996). Wehave proceeded >14 backcrosses to minimize the effects of co-segregatingloci and genetic background on the phenotypes in Psa^goku/goku mice. Although the repeated backcrosses do not completely eliminatethe influence of the background gene on the phenotypes in themutants, Psa^goku/goku mice provide a genetically preferable means for the study ofthe involvement of Psa in mammalian growth andbehavior.

Dwarfism and physiological condition in Psa^goku/goku mice

Psa^goku/goku mice showed apparent dwarfism from 3 weeks after birth (Fig. 1). Because an adequate supply of GH is essential for thecontrol of normal body growth in mammals, and some dwarf mousestrains show defects in GH (Eicher and Beamer, 1976, 1980), weinvestigated the plasma levels of GH and IGF-I, which is a growthfactor regulated by GH. There were no significant differencesin plasma GH and IGF-I levels between Psa^+/+ and Psa^goku/goku mice. No plasma levels of a number of parameters used as referencevalues showed any significant differences between genotypes (Table1), suggesting that the phenotypes observed in Psa^goku/goku mice are not derived from dysfunctions in the digestiveorgans.

A previous study reported that puromycin arrests the cell cycle of COS cells and induces the cells to undergo apoptosis (Constamet al., 1995), and the authors suggested that the inhibition ofthe activity of Psa or other aminopeptidases by puromycin mayarrest the cell cycle and induce apoptosis. From their study,we can speculate a possibility that dwarfism of Psa^goku/goku mice results from the impairment of the cell cycle or from inducedapoptosis. In fact, several knockout mice carrying mutated genesassociated with the cell cycle events show abnormalities in growth(Sicinski et al., 1995; for review, see Raff, 1996)

Although the molecular roles of Psa in growth remain unknown, it is interesting that no sexual dimorphism in body weightswas observed in Psa^goku/goku mice (Fig. 1). This phenotype was distinguished from some otherspontaneous dwarf mouse strains. Taken together with the observationthat the mutants were infertile in both sexes (T. Osada and T.Takeuchi, unpublished data), dwarfism with no sexual differencein Psa^goku/goku mice may arise from imbalance of the endocrine system independentof GH and IGF-I. In fact, pituitary glycoprotein hormone $alpha$ -subunitgene knockout mice, which lack biologically active pituitary thyrotropinand gonadotropins, show dwarfism with no sex difference, in additionto hypogonadism and hypothyroidism (Kendall et al., 1995). AlthoughPsa^goku/goku mice exhibited comparable levels of thyroxine, which is producedin thyroid in response to thyrotropin stimulation, there is apossibility that other hormonal signalings are hampered in themutants.

Behavioral abnormalities in Psa^goku/goku mutant mice

We evaluated behavioral impairments in Psa-deficient mice by six behavioral tests (rod-walking, wire-hanging, open-field,elevated plus-maze, hot-plate, and tail-flick tests). These testsallowed us to characterize two major features of Psa^goku/goku mice: emotional impairment under a novel environment and theincrease of the analgesia. We discuss each feature observed inPsa^goku/goku micebelow.

Emotional impairment under a novel environment
Decreased locomotor activity in the open-field test and increased anxiolytic features in the open-field test and elevatedplus-maze test have been reported previously in knockout mousestrains that have impairments in learning and memory or otherintegrative brain functions such as emotion (for review, see Nelsonand Young, 1998). There is no evidence that the similarities inbehavioral impairments observed in Psa^goku/goku mice and other mutants originate from the same defects. Becausemet-enkephalin and leu-enkephalin have been reported as possiblePsa targets (Hersh and McKelvy, 1981), and a report on enkephalinknockout mice shows that enkephalins are involved in anxiety andpain (Köning et al., 1996), the expression patterns of theseneuropeptides in the brains of Psa^goku/goku mice were examined by the IHC analysis. Comparable levels andexpression patterns were found in both Psa^+/+ and Psa^goku/goku mice (Fig. 8A-D), although a possibility that some differencebetween the genotypes was undetectable by IHC cannot be excluded.Because Psa hydrolyzes N-terminal amino acids of oligopeptideswith a broad spectrum, it is also possible that neuropeptidesother than enkephalins may affect normal behavior inmammals.

Increase in analgesia
Psa is expressed in the brain broadly (Fig. 7A,C), in spinal cord, and in dorsal root ganglion (data not shown). The increasedlatency of the jumping response and normal reflex response tonoxious thermal stimuli suggests that the increase in analgesiain Psa^goku/goku mice derives from abnormalities in the brain. Because substanceP has been studied extensively as a neuropeptide that modulatespain responses (for review, see Woolf et al., 1998), we assessedthe expression of this peptide in the brains of Psa^goku/goku mice by IHC. No apparent alternations could be detected (Fig.8E,F). It is important to analyze the status of substance P afternociceptive stimulus to examine metabolic defects or syntheticabnormalities of substance P in Psa^goku/goku mice. It is also possible that other molecules in the brain affectedby Psa deficiency might be involved in the analgesic effect observedin mutants. Therefore, intensive studies are needed to elucidatethe molecular mechanisms of the altered response to thermal stimuliin Psa^goku/gokumice.
Pain and emotion are believed to be closely connected to one another. Our study suggests that Psa in the brain plays importantroles in the regulation of thesephenomena.

Psa gene expression in the brain

The expression pattern of the Psa gene in the brain is important because the Psa activity in the brain is reported to be higherthan in other organs (McLellan et al., 1988). Moreover, behavioralimpairments of Psa^goku/goku mice are suggested to result from defects in brain functions.A previous study involving in situ hybridization analysis reportedthat the Psa gene in the human brain is expressed preferentiallyin neurons (Tobler et al., 1997). We observed that the Psa geneis also expressed in astrocytes and oligodendrocytes in additionto neurons (Fig. 7E-G). In neurons, the intensity of expressionwas not identical, although almost all neurons appeared to expressthe Psa gene. In particular, intensive Psa gene expression inneurons was detected in the striatum and hippocampus (Fig. 7A,C).These data suggest that Psa may play some basic roles in the cellphysiology of the brain, as well as more specific roles in thosetypes of the cells in which Psa gene expression is strong. Becausepeptides that exist predominantly in the striatum or hippocampusare known to be involved in normal behavior (for review, see Nelsonand Young, 1998), further analysis of the interaction of thesepeptides with Psa should proveinteresting.

Psa status in Psa^goku/goku mice

We found an additional transcript (1.7 kb), possibly an alternatively spliced isoform, in addition to the Psa transcript (4.5kb). However, the molecule from the transcript was suggested tolack aminopeptidase activity because it does not contain the catalyticdomain ofPsa.

Northern blot analyses also showed that transcriptional arrest occurs in the Psa gene of Psa^goku/goku mice. Transcripts encoding the catalytic domain of Psa were notdetectable in Psa^goku/goku mice. To elucidate Psa status in the mutants, aminopeptidaseactivity in the brains of each genotype was measured. The activityusing the alanyl-p-nitroanilide as a substrate showed a drasticdecrease in activity in Psa^goku/goku mice. In contrast, puromycin-insensitive activity (~12% of totalactivity) did not differ from that in Psa^+/+ mice. These results suggest that the decreased activity observedin Psa^goku/goku mice (~60%) corresponds to the Psa activity in Psa^+/+ mice. On the other hand, a decrease in the puromycin dose-dependentactivity (~28%) was also observed in Psa^goku/goku mice. This decreased activity is thought to derive from puromycin-sensitiveaminopeptidases but not from Psa. Thus, we can classify the aminopeptidaseactivity into Psa-dependent, Psa-independent but puromycin-sensitive,and puromycin-insensitive in all tissues using Psa^goku/goku mice. Recently, a novel aminopeptidase, which is located in abundancein the brain synaptosomes and whose activity is inhibited by puromycin,was identified by Hui et al. (1998) as a puromycin-sensitive aminopeptidaseother thanPsa.

Taken together with the molecular and biochemical analyses, we conclude that the Psa gene is functionally disrupted in Psa^goku/goku mice. Therefore, the observed abnormalities in Psa^goku/goku mice were suggested to originate from the inactivation of Psa.Because the molecular functions and substrates of Psa in vivoremain unknown, this mutant would be a useful tool for gainingnew insights into the physiological functions of the Psa geneinmammals.

  FOOTNOTES

Received Jan. 28, 1999; revised April 13, 1999; accepted April 26, 1999.

We thank Ichiro Koshino (Veterinary Medical Center, University of Tokyo, Tokyo, Japan) for technical assistance with the measurementsof the reference values. We also thank Dr. Takeshi Yagi (NationalInstitute for Physiology, Okazaki, Japan) for thoughtful discussionand critical review of thismanuscript.
Correspondence should be addressed to Dr. Takashi Takeuchi, Mitsubishi Kasei Institute of Life Sciences, 11 Minamiooya, Machida,Tokyo 194-8511,Japan.

Dr. Yamazaki's present address: Department of Information Physiology, National Institute for Physiological Sciences, Myodaiji,Okazaki 444-8585,Japan.

Dr. Higashinakagawa's present address: Department of Biology, School of Education, Waseda University, Nishiwaseda Shinjuku,Tokyo 169-8050,Japan.

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