Mice Deficient for Tenascin-R Display Alterations of the Extracellular Matrix and Decreased Axonal Conduction Velocities in the CNS

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The Journal of Neuroscience, June 1, 1999, 19(11):4245-4262

Mice Deficient for Tenascin-R Display Alterations of the Extracellular Matrix and Decreased Axonal Conduction Velocities in the CNS
Philipp Weber¹, Udo Bartsch¹^,³, Matthew N. Rasband², Reiner Czaniera³, Yolande Lang⁴, Horst Bluethmann⁴, Richard U. Margolis⁵, S. Rock Levinson⁶, Peter Shrager², Dirk Montag¹, and Melitta Schachner³
¹ Department of Neurobiology, Swiss Federal Institute of Technology, Hönggerberg, CH 8093 Zürich, Switzerland, ² Department of Neurobiology and Anatomy, University of Rochester Medical Center, Rochester, New York 14642, ³ Zentrum für Molekulare Neurobiologie, Universität Hamburg, D 20246 Hamburg, Germany, ⁴ Department Roche Genetics, F. Hoffmann-LaRoche, CH 4070 Basel, Switzerland, ⁵ Department of Pharmacology, New York University Medical Center, New York, New York 10016, and ⁶ Department of Physiology, University of Colorado Medical School, Denver, Colorado 80262

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Tenascin-R (TN-R), an extracellular matrix glycoprotein of the CNS, localizes to nodes of Ranvier and perineuronal nets andinteracts in vitro with other extracellular matrix componentsand recognition molecules of the immunoglobulin superfamily. Tocharacterize the functional roles of TN-R in vivo, we have generatedmice deficient for TN-R by homologous recombination using embryonicstem cells. TN-R-deficient mice are viable and fertile. The anatomyof all major brain areas and the formation and structure of myelinappear normal. However, immunostaining for the chondroitin sulfateproteoglycan phosphacan, a high-affinity ligand for TN-R, is weakand diffuse in the mutant when compared with wild-type mice. Compoundaction potential recordings from optic nerves of mutant mice showa significant decrease in conduction velocity as compared withcontrols. However, at nodes of Ranvier there is no apparent changein expression and distribution of Na⁺ channels, which are thought to bind to TN-R via their $beta$ 2 subunit.The distribution of carbohydrate epitopes of perineuronal netsrecognized by the lectin Wisteria floribunda or antibodies tothe HNK-1 carbohydrate on somata and dendrites of cortical andhippocampal interneurons is abnormal. These observations indicatean essential role for TN-R in the formation of perineuronal netsand in normal conduction velocity of opticnerve.

Key words: extracellular matrix glycoprotein; HNK-1 carbohydrate; inhibitory interneurons; knock-out mutation; node of Ranvier; parvalbumin; phosphacan; sodium channel

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The extracellular matrix (ECM) is a complex network of macromolecules that includes glycoproteins, polysaccharides, and proteoglycans.These provide mechanical strength, scaffolding, and support totissues and organs, and they participate in cellular differentiation.In the nervous system, interactions of neuronal and glial cellswith the ECM regulate cell migration, survival, and differentiation,axonal pathfinding, and synapseformation.

The tenascin family constitutes a group of extracellular matrix proteins displaying a common structure (for review, see Chiquet-Ehrismannet al., 1994; Erickson, 1994). At the amino terminus, a signalsequence is followed by a cysteine-rich stretch, epidermal growthfactor-like (EGF) repeats, fibronectin-type III (FN) homologousrepeats, and a fibrinogen-like (FG) domain at the C terminus.The number of EGF domains is characteristic for each member ofthe family, whereas because of alternative splicing, the numberof FN repeats may vary, and isoforms of tenascin (TN)-C and TN-Rexist, differing in the number of FN repeats. Currently, fivemembers of the tenascin family (TN-C, TN-R, TN-X, TN-Y, TN-W)have been identified in diverse species from zebrafish to humans(for review, see Bristow et al., 1993; Chiquet-Ehrismann et al.,1994; Erickson, 1994; Tongiorgi et al., 1995; Hagios et al., 1996;Weber et al., 1998).

TN-C is by far the most extensively studied member of this family. TN-C has been implicated, for instance, in different morphogeneticprocesses during development, axonal regeneration, tumorigenesis,and wound healing. Surprisingly and disappointingly, the inactivationof the tn-c gene in mice has not provided any insight into TN-C'sfunctional role in vivo (Saga et al., 1992; Forsberg et al., 1996).The complete absence of TN-C immunoreactivity in the mutant createdby Saga and colleagues is a matter of discussion, however (Mitrovicand Schachner, 1995; Settles et al., 1997). Preliminary evidencefor behavioral defects and a disturbed serotonin and dopaminebalance in these TN-C-deficient mice has been reported (Fukamauchiet al., 1996, 1997; Fukamauchi and Kusakabe, 1997). Furthermore,the structure of the neuromuscular junction and peripheral nervesappears to be altered (Cifuentes-Diaz et al., 1998; but also seeMoscoso et al., 1998).

TN-X may exert an essential role in connective-tissue structure and function, and an association of TN-X deficiency with Ehlers-Danlossyndrome has been discovered recently (Burch et al., 1997).

TN-R [previously designated J1-160/180 and janusin in rodents and restrictin in chicken (Nörenberg et al., 1992; Fuss etal., 1993; for review, see Schachner et al., 1994)] appears tobe restricted to the CNS. TN-R is synthesized by oligodendrocyteswith high expression during the period of active myelination (Bartschet al., 1993; Wintergerst et al., 1993). It is detectable at contactsites between unmyelinated axons, at the interface between axonsand myelinating processes of oligodendrocytes, and between myelinsheaths (Bartsch et al., 1993) and is highly accumulated at thenodes of Ranvier (ffrench-Constant et al., 1986; Bartsch et al.,1993). TN-R is also expressed by subpopulations of neurons, suchas horizontal cells in the retina, stellate and basket cells inthe cerebellum, motoneurons in the spinal cord, and some neuronsin the hippocampus (Fuss et al., 1993; Wintergerst et al., 1993).

In vitro, TN-R promotes neurite outgrowth and morphological polarization of differentiating neurons when presented as a uniformsubstrate (Lochter and Schachner, 1993; Lochter et al., 1994).When offered as a substrate boundary with a neurite outgrowth-conducivemolecule, TN-R is repellent for growth cone advance (Pesheva etal., 1993; Taylor et al., 1993). Recently, a role of TN-R as amodulator of fasciculation has been discovered in a cerebellarexplant cell culture system (Xiao et al., 1998). In addition,TN-R as a substrate promotes adhesion and differentiation of oligodendrocytesand astrocytes (Pesheva et al., 1989, 1997; Morganti et al., 1990).These observations indicate that the cellular responses to TN-Rare complex and probably mediated by several neuronal receptorsthat interact with distinct domains of the TN-Rmolecule.

Among these neuronal receptors for TN-R, one has been identified as the F3/F11/contactin (F3 in rodents and F11 or contactinin chicken) immunoglobulin (Ig) superfamily adhesion molecule(Pesheva et al., 1993). F3/F11/contactin is expressed predominantlyby neurons (Brümmendorf et al., 1989; Gennarini et al., 1989;Faivre-Sarrailh et al., 1992) and mediates cell recognition leadingto heterophilic adhesion with neurons (Brümmendorf et al., 1993;Peles et al., 1995). The interaction of TN-R with F3/F11/contactinhas been localized to the Ig-like domains of F3/F11/contactin(Brümmendorf et al., 1993; Xiao et al., 1996, 1998). TN-R-elicitedrepulsion and defasciculation of neurites are both mediated bybinding of the amino-terminal domain of TN-R to the Ig domainsof F3/F11/contactin (Pesheva et al., 1993; Xiao et al., 1996,1998). F3/F11/contactin is present in a complex comprising bothL1 and Fyn tyrosine kinase (Olive et al., 1995; Zisch et al.,1995), and clustering of F3/F11/contactin at the cell surfaceby antibodies induces tyrosine phosphorylation of several intracellularproteins including Fyn (Zisch et al., 1995; Cervello et al., 1996),suggesting that TN-R-elicited signals can be transmitted via F3/F11/contactinto second messenger pathways into the interior of the target cells.Furthermore, it has been suggested, on the basis of the sequencehomology between F3/F11/contactin and the $beta$ 2 subunit of Na⁺ channels (Isom et al., 1995), that tenascin-C and tenascin-Rmay interact with $beta$ 2 and thereby provide a mechanism for Na⁺ channel localization and regulation of functional activity atnodes of Ranvier (Srinivasan et al., 1997).

TN-R also interacts with other molecules of the extracellular matrix that may influence the properties of the intercellularspace. The chondroitin sulfate proteoglycan versican and TN-Rare colocalized in the granular layer of the cerebellum, and thelectin domain of versican binds to TN-R in vitro (Aspberg et al.,1995). In optic nerve, retina, and brain, there is an overlappinglocalization of TN-R and phosphacan (Xiao et al., 1997; Milevet al., 1998), a nervous tissue-specific chondroitin sulfate proteoglycanthat is an mRNA splicing product containing the entire extracellulardomain of a receptor-type protein tyrosine phosphatase (for review,see Margolis et al., 1996). A brain-derived chondroitin sulfateproteoglycan related to phosphacan has been isolated by affinityto a recombinant amino-terminal EGF domain of TN-R (Xiao et al.,1997), and phosphacan binds with high affinity (K_d ~2 nM) to nativeTN-R (Milev et al., 1998). Furthermore, interactions with receptorsfor the HNK-1 carbohydrate epitope expressed by TN-R, such aslaminin (Hall et al., 1993, 1995), may influence the functionsof TN-R.

On the basis of the cell type-specific distribution, time of expression, and functional activities of TN-R assayed in vitro,various potential functions of TN-R have been proposed (for review,see Schachner et al., 1994). To investigate the functions of TN-Rin vivo, we have generated mice deficient in the expression ofTN-R via homologous recombination in embryonic stem cells. Here,we report that TN-R-deficient mice show alterations in the distributionof extracellular matrix molecules associated with perineuronalnets and nodes of Ranvier, along with a marked decrease in conductionvelocity in CNSaxons.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

tn-r Targeting construct. A genomic clone containing the 5' part of the tn-r gene was isolated from a mouse 129Sv genomiclibrary (Müller et al., 1994) by hybridization with a rat 0.48kb cDNA fragment corresponding the EGF coding region of cloneJ1-160/180 (Fuss et al., 1991). The fragment EcoRV intron 1 toHindIII intron 2 was first subcloned into pUC19 (Yanish-Perronet al., 1985) and then into pBluescript KS (Stratagene, La Jolla,CA), yielding the plasmid pTNR3'. The fragment EcoRV intron 0to SacI exon 1 was subcloned into pBluescript KS (Stratagene),and the PGK promotor-neo cassette of pPGKneobpA (Soriano et al.,1991) located on a XhoI-SalI fragment was inserted in oppositeorientation to tn-r gene transcription. The EcoRI fragment ofthis subclone was inserted into pTNR3', and then a HSV-tk cassette(Mansour et al., 1988) was inserted via SalI in opposite orientationto tn-r gene transcription at the 3' end, resulting in the targetingconstruct p5'PGKneo3'TK (see Fig. 1B).

Embryonic stem cell culture. The embryonic stem cell line E14.1 (Hooper et al., 1987) was cultured on irradiated primary mouseembryonic fibroblasts. Embryonic stem cells (2 × 10⁷) were transfected by electroporation (Bio-Rad Gene Pulser; 230V,500 µF) with 20 µg of NotI-linearized targeting construct, culturedon irradiated SNL 76/7 feeder cells (McMahon and Bradley, 1990)and selected with 0.2 µM 1-(2-deoxy,2-fluoro- $beta$ -D-arabinofuranosyl)-5-iodouracil(FIAU; Bristol Meyers) and 300 µg/ml G418 (Life Technologies,Gaithersburg, MD) for 3 and 6 d, respectively. After single colonieswere picked, aliquots of the individual clones were frozen asdescribed (Chan and Evans, 1991) or cultured in medium containing60% buffalo rat liver-conditioned medium without feeder cellsfor DNAisolation.

Screening of recombinant clones and Southern blot analysis. Embryonic stem cells were lysed and DNA was isolated as described(Ramirez-Solis et al., 1992). DNA of individual embryonic stemcell clones was digested with EcoRI and analyzed after Southernblotting as described (Montag et al., 1994) by hybridization withprobe 5'EX [SacI intron 0 to EcoRV intron 0; labeled to 10⁸ cpm/µg by random priming (Feinberg and Vogelstein, 1983)]. GenomicDNA from positive embryonic stem cells was further analyzed afterrestriction with the appropriate enzymes by Southern blot analysisas above using the probes 3'EX (HindIII intron 2 to SphI intron2) and 3'INT (XhoI intron 2 to HindIII intron2).

Blastocyst injection and mating of mice. Blastocysts were collected from B6CBAF1 females at day 4 of pregnancy in CZB medium(Chalot et al., 1989). Microinjection of embryonic stem cellsinto blastocysts was performed essentially as described (Hoganet al., 1986). Male chimeras were mated with C57BL/6J females,and the heterozygous (tn-r^+/) offspring were crossed to obtain homozygous (tn-r^/) mice. The genotype of the mice was characterized by Southernblotting.

RNA preparation and Northern blot analysis. Total RNA from brains of tn-r^+/+, tn-r^+/, and tn-r^/ mice was isolated using the RNeasy Kit (Qiagen, Hilden, Germany).RNA was electrophoresed in a 1.5% agarose gel containing 7% formaldehydeand transferred onto Hybond-N membranes (Amersham, Arlington Heights,IL). Hybridization was performed with the following probes labeledto 10⁸ cpm/µg by random priming (Feinberg and Vogelstein, 1983): 2676bp EcoRI fragment of rat TN-R cDNA (Fuss et al., 1991) encoding4.5 EGF and 7 FN repeats and 409 bp Sma-CelII fragment of ratTN-R cDNA (Fuss et al., 1991) encoding the 4.5 EGFrepeats.

RT-PCR and sequencing of cDNA. Reverse transcription (AMV reverse transcriptase; Boehringer Mannheim, Mannheim, Germany) oftotal RNA from brains of tn-r^+/ mice was performed according to the manufacturer's instructionsand using primer 211 (5'-CCTTAAGTGGGTGAGGACAATGACA-3'). Two cDNAfragments of 2.6 and 2.0 kb were amplified after PCR (annealingtemperature 60°C, 30 cycles) using primers 211 and 5'UT (5'-GAATTCCAAGAGAAACCATCAGAG-3').The fragments were subcloned into pBluescript KS (Stratagene),and sequence analysis was performed with the T7 Sequencing Kit(Pharmacia, Piscataway,NJ).

Protein analysis of brain extracts. For analysis of proteins, total brains of 14-d-old tn-r^+/+ and tn-r^/ mice were homogenized in buffer H (1 mM NaHCO₃, 0.2 mM CaCl₂,0.2 mM MgCl₂, 1 mM spermidine) complemented with protease inhibitors(10 µg/ml soybean trypsin inhibitor, 10 µg/ml turkey egg-whitetrypsin inhibitor, 1 mM phenylmethylsulfonyl fluoride, 0.5 mMiodoacetamide). The homogenate was centrifuged at 4°C and 30,000× g. The protein concentration of the supernatant was determined(BCA assay, Pierce, Rockford, IL). After addition of 2× loadingbuffer and heat denaturation, the samples were analyzed underreducing conditions by SDS-PAGE (Laemmli, 1970) and Western blotting(Towbin et al., 1979). Primary antibodies were visualized by horseradish peroxidase-coupled antibodies to mouse or rabbit IgG (1:10,000diluted, Dianova, Hamburg, Germany) and enhanced chemiluminescence(Amersham).

Antibodies. Polyclonal antibodies to TN-R (Pesheva et al., 1989), phosphacan (Milev et al., 1994), TN-R domain-specific polyclonalantibodies (pFN, pEGF/S) (Xiao et al., 1998), and monoclonal antibodies596 and 619, recognizing epitopes of the protein backbone of TN-R(Xiao et al., 1996), have been described. Monoclonal antibodiesPA-235 (Sigma, St. Louis, MO) and undiluted hybridoma culturesupernatant (Abo and Balch, 1981) were used for detecting parvalbuminand human natural killer cell antigen-1 (HNK-1), respectively.For indirect immunofluorescence, polyclonal and monoclonal antibodieswere visualized by fluorescein isothiocyanate (FITC)-coupled antibodiesto mouse or rabbit IgG (Dako, Carpinteria,CA).

Light and electron microscopy. For light and electron microscopy, mice were deeply anesthetized and perfused through the leftventricle with 4% paraformaldehyde and 2% glutaraldehyde in 0.1M phosphate buffer, pH 7.4. Optic nerves and brains were removedand post-fixed in the same fixative. Optic nerves or vibratomesections of retinae or brains, 200-500 µm in thickness, were incubatedin 2% OsO₄ for 2 hr, dehydrated in an ascending series of methanol,and embedded in Epon resin. For light microscopy, 3-µm-thick sectionswere stained with Toluidine blue and examined with a Zeiss Axiophot.For electron microscopy, ultrathin sections were counterstainedwith lead citrate and examined with a Zeiss EM10C.

In situ hybridization. In situ hybridization analysis was performed as described (Bartsch et al., 1992b). TN-R cRNA probeswere generated by in vitro transcription (Dörries et al., 1993)of pBluescript KS containing a 2.7 kb insert encoding the 4.5EGF and the first seven FN repeats of TN-R. TN-C cRNA probes weregenerated as described (Bartsch et al., 1992b).

Indirect immunofluorescence of extracellular matrix molecules and myelin-associated glycoprotein. Indirect immunofluorescencefor the detection of myelin-associated glycoprotein (MAG), TN-C,and phosphacan was performed on sections of fresh-frozen tissueas described (Poltorak et al., 1987; Bartsch et al., 1992a; Xiaoet al., 1997). Parvalbumin and the sulfated carbohydrate epitopeHNK-1 were detected on fixed sections. For fixation, animals weredeeply anesthetized with Ketanest/Rompun (0.15 ml/10 gm body weight,i.p.) and transcardially perfused with saline followed by PBS,pH 7.4, containing 4% paraformaldehyde. The brains were post-fixedin the same fixative overnight at 4°C. Immunocytochemistry wasperformed on free-floating vibratome sections (30 µm thick) (Härtiget al., 1992; Seeger et al., 1994). Sections were incubated inPBS, pH 7.4, containing 2% BSA for 2 hr, followed by antibodiesto parvalbumin (diluted 1:5000 in PBS/0.1% BSA) and the sulfatedcarbohydrate HNK-1 epitope (undiluted hybridoma culture supernatant)for 48 hr at 4°C under constant agitation. For the staining ofparvalbumin, 0.1% Triton X-100 was added to the incubation buffer.Sections were rinsed with three changes of the same buffer. Cy-2-conjugatedsecondary anti-mouse antibodies (diluted 1:200) were applied for2 hr at room temperature. Sections were mounted in Aqua-Poly/Mount(Polysciences, Warrington,PA).

Detection of perineuronal nets. The detection of the perineuronal nets was performed on fixed vibratome sections (see above)using the biotinylated lectin Wisteria floribunda (Sigma). Thefinal concentration of the lectin was 20 µg/ml. For double-staining,sections were first incubated with the lectin and then with antibodiesto parvalbumin or to the HNK-1 carbohydrate. Cy-3-conjugated streptavidin(diluted 1:600; Dianova) was used for detection of thelectin.

Quantitative analysis of cytological parameters. Twelve sections per animal (n = 5 for wild-type and TN-R-deficient mice)were chosen to determine the number and length of labeled dendritesper neuron for the lectin- and HNK-1-positive cell. The sectionswere selected from bregma $-$ 1.46 (Franklin and Paxinos, 1997).Sections were evaluated by image analysis (KS-400, Kontron/Zeiss)using an Axiovert microscope (Zeiss) equipped with a motorizedstage and a CCD camera (Hamamatsu) connected to a PC monitor.Frames of 150 × 200 µm were randomly chosen from a particularbrain area and monitored at a magnification of 400×. For the lectinstaining, the primary somatosensory, retrosplenial agranular,and granular cortices (50 frames per slice), and the hippocampus(25 frames per slice) were analyzed. The primary somatosensorycortex (25 frames per slice) and the hippocampus (25 frames perslice) were analyzed by staining for the HNK-1 epitope. All positivelystained cell somata and dendrites were counted. Data were evaluatedusing the two-sample t test (Systat 6.0, SPSS Inc.).

Detection of glycan by digoxigenin-labeled lectin. To determine whether TN-R carries N-acetylgalactosamine carbohydrate epitopes,binding of peanut agglutinin (PNA) to TN-R was analyzed. Proteinextracts from brains of 3-month-old wild-type and TN-R-deficientmice were processed as described above. Samples were analyzedby SDS-PAGE (Laemmli, 1970) and Western blotting (Towbin et al.,1979). Detection of glycans was performed by using digoxigenin-labeledPNA (Boehringer Mannheim) followed by visualization with anti-digoxigenin-alkalinephosphatase conjugates (BoehringerMannheim).

Na⁺ channel immunofluorescence. Optic nerves from wild-type (C57BL/6) and TN-R-deficient postnatal mice (P8 to adult) weredissected immediately after animals were killed. Nerves were thenplaced in 4% paraformaldehyde in 0.1 M phosphate buffer (PB),pH 7.2, for 30 min, then transferred to a 20% sucrose solutionin 0.1 M PB for 3 hr. The nerve was then frozen in OCT mountingmedium (Miller) and cut in 10 µm sections. Sections were placedin 0.1 M PB and finally spread on gelatin-coated coverslips andallowed to air dry. Cryosectioned tissue was then permeabilizedfor 2 hr in 0.1 M PB, pH 7.4, containing 0.3% Triton X-100 and10% goat serum (PBTGS). In all steps involving antibodies, thetissue preparations were washed three times for 5 min each withPBTGS between succeeding steps. All antibodies were diluted inPBTGS. Affinity-purified polyclonal Na⁺ channel antibodies (for details, see Rasband et al., 1998b) werediluted 1:50 and incubated with the cryosectioned tissue overnight.The secondary antibodies, goat anti-rabbit Fc-specific Fab2 fragments,conjugated to biotin (1:400, Accurate Chemicals, Westbury, NY),were applied for 1 hr, followed by Extravadin-FITC (1 hr, 1:200,Sigma). In experiments in which the relative Na⁺ channel fluorescence of nodal regions was compared, the secondaryantibody was a goat anti-rabbit IgG conjugated to FITC and incubationwith Extravadin-FITC was omitted. Finally, labeled cryosectionswere rinsed consecutively in PBTGS, 0.1 M PB, and 0.05 M PB for5 min each. The samples were then air-dried and mounted on slideswith an anti-fade mounting medium. The labeled tissue was examinedon a Nikon Microphot fluorescence microscope fitted with a C4742-95cooled CCD camera (Hamamatsu). The camera was connected to a laboratorycomputer that controlled image acquisition and storage. Each fieldof view (FOV) was later analyzed for the number of nodes and fluorescenceintensity using the analysis program Image Pro (MediaCybernetics).

Electrophysiology. Optic nerves were dissected immediately after animals were killed and placed in Locke's solution consistingof (in mM): NaCl 154, KCl 5.6, CaCl₂ 2, D-glucose 5, and HEPES10, pH 7.4. Nerves were then transferred to a recording chamberthat was continuously perfused, oxygenated, and temperature-regulated.For stimulation and recording of action potentials, each end ofthe nerve was drawn into a suction electrode (Stys et al., 1991).The stimulus was adjusted to ~10% above the level that eliciteda maximum response. Compound action potentials (CAPs) were amplified,digitized, recorded, and analyzed on a laboratory computer. Controloptic nerves used in suction electrode recordings came from C57BL/6(n = 6), 129/SvEv (n = 2), and 129/SvEms (n = 2) mice. In controlexperiments in which the sciatic nerve was used instead of theoptic nerve, the procedure was the same, with the single exceptionbeing that the nerve was desheathed before recording. Amplitudeswere typically ~3 mV but were arbitrary in these external electroderecordings and thus are not included in the Figures. The averageamplitude of CAPs in TN-R-deficient nerves was 3.0 ± 1.4 mV, notsignificantly different from that of wild-type (3.3 ± 1.1mV).

For conduction velocity measurements, the time to the peak amplitude of the CAP was measured from the onset of the nerve stimulus.In two cases (one wild type, one TN-R deficient), a smaller, fastercomponent of the CAP was seen, but it was not possible to derivea peak value from these faster components. Instead, the main peakamplitude was used as in all other experiments. Before transferto the recording chamber, nerve length was measured. The conductionvelocity was then calculated as the length of the nerve dividedby the time to peakamplitude.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Generation of TN-R-deficient mice

Using a rat cDNA fragment corresponding to the amino-terminal region of TN-R, a clone carrying the 5'part of the tn-r genewas isolated from a mouse 129Sv genomic library. The partial structureof the tn-r gene is shown in Figure 1A. Exon 1 encodes the twopotential translational start codons followed by the signal sequenceand the cysteine-rich amino-terminal part, and exon 2 codes forall EGF repeats. To inactivate the tn-r gene, a targeting vectorwas constructed (Fig. 1B). This vector contains a 4.2 kb 5' homologoussequence, a PGK-neo cassette (Soriano et al., 1991) in oppositedirection to the tn-r transcription and replacing the coding regionof exon 1 and part of intron 1, 3.9 kb of the 3' homologous regionincluding exon 2, and the herpes simplex virus (HSV) thymidinekinase gene (tk) for selection against random integration (Mansouret al., 1988). Homologous recombination with this targeting vectorresults in an insertional mutation (Fig. 1C) and deletes the regionencoding the ribosomal binding site, the translation initiationcodon(s), and the amino terminus including the signal sequence,which is thus expected to result in a null mutation.

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Figure 1. tn-r gene, tn-r targeting construct, expected and observed structure of the disrupted tn-r gene, tn-r transcript, and aberrant transcript structure. A, Restriction map of the mouse tn-r gene. Translated and nontranslated exons are represented by closed and open boxes, respectively, and are numbered with Roman numerals. E, S, Sp, R, X, and H represent cleavage sites for EcoRI, SacI, SphI, EcoRV, XhoI, and HindIII (not all sites given), respectively. B, Restriction map of the tn-r targeting construct p5'PGKneo3'TK, containing 4.2 and 3.9 kb of homologous sequences on the 5' and 3' sites of the neo insertion, respectively, and deleting the two potential translation initiation codons. PGKneobpA and HSV-tk cassettes and the pBluescript KS (KS-) vector part are indicated by boxes. Arrows indicate the transcriptional orientation of the respective genes. N represents cleavage site for NotI. C, Expected and observed structure of the tn-r gene after homologous recombination and localization of probes. Horizontal bars indicate the localization of hybridization probes 5'EX, 3'EX, and 3'INT. D, Structure of the wild-type tn-r gene transcript. Translated and nontranslated exons are represented by closed and open boxes, respectively, and are numbered with Roman numerals. E, Structure of the aberrant tn-r gene transcript. Exons are represented by open boxes. The aberrant splicing of 200 bp of intronic sequence is indicated by a hatched box.

After electroporation of the linearized targeting vector into E14 embryonic stem cells (Hooper et al., 1987) and double selectionwith FIAU and G418, approximately 1 clone of 100 carried the desiredmutation as determined by Southern blot analysis with the externalprobe 5'EX (Fig. 2A). The presence of a new EcoRI site introducedby insertion of neo into exon 1 of the tn-r gene was detectedby the appearance of a 7.7 kb band in addition to the wild-typeband of 10.7 kb. Further analysis with the 3' external probe 3'EX(Fig. 2A) and the 3' internal probe 3'INT (data not shown) confirmedthe pattern expected after homologous recombination.

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Figure 2. Southern, Northern, and Western blot analysis of wild-type and tn-r targeted embryonic stem cells and tn-r^/, tn-r^+/, and tn-r^+/+ mice. A, Southern blot analysis. DNA from wild-type (lanes 1 and 3) and tn-r targeted embryonic stem cells (lanes 2 and 4) and DNA from tn-r^+/+ (lanes 6 and 9), tn-r^+/ (lanes 5 and 8), and tn-r^/ (lanes 7 and 10) mice digested with EcoRI (lanes 1, 2, 5-10) or SphI (lanes 3 and 4) was hybridized with probes 5'EX (lanes 1, 2, 8-10), 3'EX (lanes 3 and 4), or 3'INT (lanes 5-7). The size of DNA fragments in kilobases is indicated at the left margin. B, Northern blot analysis. RNA from brains of tn-r^+/+, tn-r^+/, and tn-r^/ mice was hybridized with a 400 bp cDNA fragment specific for the EGF encoding part (exon 2; lanes 1-3) or with a 2.7 kb cDNA fragment specific for the 3' part of the tn-r transcript (lanes 4-6). The size of an RNA marker in kilobases is indicated at the left margin. C, Western blot analysis of brain protein extracts using monoclonal antibody 596 against TN-R. Num-bers indicate micrograms of protein loaded per lane of detergent extracts of a crude soluble fraction from 14-d-old tn-r^+/+ and tn-r^/ mice. In tn-r^+/+ mice, TN-R is detectable in 0.5 µg of protein as a broad band at 160-180 kDa, representing the 160 and 180 kDa isoforms. No signal is obtained in 500 µg of protein from TN-R-deficient mice. D, Western blot analysis of brain extracts using monoclonal antibody 619, polyclonal antibodies against TN-R (pTN-R), and TN-R domain-specific polyclonal antibodies (pEGF/S, pFN). Ten micrograms of protein of detergent extracts of a crude soluble fraction from brains of 14-d-old wild-type and TN-R-deficient mice were loaded per lane. The molecular mass of TN-R isoforms in kilodaltons is indicated at the left margin.

Highly chimeric mice were obtained after injection of targeted embryonic stem cells into blastocysts. Chimeric males showedgermline transmission of the disrupted tn-r gene as analyzed bySouthern blot analysis. Crossing of heterozygous (tn-r^+/) offspring yielded homozygous TN-R-deficient (tn-r^/) mice with strictly Mendelian frequencies. Southern blot analysisof these mice with the probes 3'EX (data not shown), 5'EX, and3'INT showed the pattern expected for a single integration byhomologous recombination (Fig. 2A).

To determine whether the mutated tn-r gene is transcribed, total RNA from brains of tn-r^+/+, tn-r^+/, and tn-r^/ mice was subjected to Northern blot analysis. After hybridizationwith a rat cDNA probe specific for the EGF coding sequence inexon 2, no signal was detectable with RNA from TN-R-deficientmice, whereas TN-R mRNA of ~12 kb was easily detectable in tn-r^+/+ and tn-r^+/ mice (Fig. 2B). Hybridization with a rat cDNA probe correspondingto the 4.5 EGF and the first seven FN repeats of TN-R detectedan RNA of ~12 kb in tn-r^+/+, tn-r^+/, and tn-r^/ mice (Fig. 2B), indicating that the mutated tn-r gene is stilltranscribed yielding an mRNA missing the first exons. The nucleotidesequence of the 5' end of this aberrant RNA was determined afterRT-PCR (see Materials and Methods) and revealed that it contains5' nontranslated sequence of the tn-r cDNA (EMBL accession no.AJ005844) followed by intronic sequences and the exon encodingthe second FN-like domain (Fig. 1E). Therefore, the RNA transcribedfrom the mutated tn-r gene is missing the region encoding theribosomal binding site, the translation initiation codon, thesignal sequence, the EGF-like domains, and the first FN-likedomain.

To confirm that the mutation generated a null allele, proteins from brains of 14-d-old tn-r^+/+, tn-r^+/, and tn-r^/ mice were analyzed by immunoblot analysis. TN-R was easily detectedin 0.5 µg of protein from brains of wild-type mice using monoclonalantibody 596, but no signal could be detected in 500 µg of proteinfrom brains of TN-R-deficient mice (Fig. 2C). Furthermore, usingmonoclonal antibody 619 recognizing the fibrinogen-like domainof TN-R (Xiao et al., 1996), polyclonal antibodies against brain-derivedTN-R, and TN-R domain-specific polyclonal antibodies pEGF-S andpFN, TN-R could not be detected in protein extracts from brainsof TN-R-deficient mice (Fig. 2D). Similarly, immunohistochemicalanalysis of sections through the optic nerve, retina, and thecerebellum from adult TN-R-deficient mice with monoclonal antibody619 showed no immunoreactivity for TN-R (Fig. 3b). The antibodiesalso did not reveal any intracellular staining, indicating thatno TN-R-related truncated form is expressed.

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Figure 3. Immunohistological analysis of wild-type and TN-R-deficient mice. Immunohistological localization of TN-R by indirect immunofluorescence on sections of cerebella of 8-week-old wild-type (a) and TN-R-deficient (b) mice using monoclonal antibody 619 (a, b). Intense TN-R immunoreactivity is visible in sections from wild-type mice (a), whereas no immunoreactivity is detectable on sections from TN-R-deficient mice (b) or from wild-type incubated with secondary antibody only (c). mol, Molecular layer; pcl, Purkinje cell layer; igl, internal granular layer. Scale bar, 100 µm.

Neither heterozygous nor homozygous TN-R-deficient mice showed any obvious, grossly abnormal behavioral phenotype up to anage of ~1 year, the latest time point investigated. Furthermore,we have established TN-R-deficient lines by intercrossing homozygousTN-R-deficient mice, proving that both sexes arefertile.

Morphological analysis of the CNS of TN-R-deficient mice.

At the light microscopic level, the general morphology of brains of 2- and 8-week-old and 9-month-old TN-R-deficient miceappeared normal and was not distinguishable from that of wild-typelittermates. In the cerebellum of 4-month-old TN-R-deficient mice,the molecular layer, Purkinje cell layer, and internal granularlayer revealed an apparently normal morphology (Fig. 4, comparea, b). In the retina of adult TN-R-deficient mice, the inner andouter nuclear layer and the plexiform layers were formed normallywith respect to their thickness and cellular organization (Fig.4, compare c, d). In addition, cross sections through the spinalcord of TN-R-deficient mice displayed a normal pattern of myelination(data not shown).

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Figure 4. Light microscopic analysis of cerebella and retinae from wild-type and TN-R-deficient mice. Semithin sections through cerebella (a, b) and retinae (c, d) of 8-week-old wild-type (a, c) and TN-R-deficient (b, d) mice. The overall histology and number and localization of the different cell types in both brain regions appear normal in TN-R-deficient mice. mol, Molecular layer; igl, internal granular layer; 1, outer nuclear layer; 2, outer plexiform layer; 3, inner nuclear layer; 4, inner plexiform layer; 5, ganglion cell layer and nerve fiber layer. Scale bars (shown in b): a, b, 100 µm; (shown in d): c, d, 100 µm.

Using a cRNA probe directed against a region common to the TN-R mRNA and the truncated RNA expressed in the mutant, cellsnormally expressing TN-R could be visualized in TN-R-deficientmice by in situ hybridization. Horizontal cells located at theouter margin of the inner nuclear layer of the retina, and glialcells in the myelinated part of the optic nerve of 14-d-old TN-R-deficientmice expressed the aberrant TN-R mRNA and were present in a densityand distribution similar to that of TN-R-expressing cells in wild-typelittermates (Fig. 5, compare a, b). In the cerebellum of 14-d-oldTN-R-deficient mice, the aberrant TN-R mRNA was expressed by cellslocated in the developing white matter and internal granular layerand by stellate and basket cells in the molecular layer (datanot shown). This staining pattern in TN-R-deficient mice revealedno difference from that in wild-type littermates. Likewise, motoneuronslocated in the spinal cord showed a distribution and density notdifferent between wild-type and TN-R-deficient animals (data notshown).

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Figure 7. Immunohistochemical localization of phosphacan and TN-C in wild-type and TN-R-deficient mice. TN-C was detected in the cerebellar cortex (a, b) and retina and optic nerve (c, d), and phosphacan was detected in the spinal cord (e, f) and retina and optic nerve (g, h) of adult wild-type (a, c, e, g) and TN-R-deficient (b, d, f, h) mice. TN-C immunoreactivity in the cerebellar cortex of adult mice is homogeneously distributed in the molecular layer (a, mol) and is weakly detectable in the internal granular layer (a, igl), with no obvious differences in intensity and distribution between wild-type (a) and TN-R-deficient (b) mice. Intense TN-C immunoreactivity in the retina and optic nerve of wild-type (c) and TN-R-deficient (d) mice is restricted to the retinal end of the nerve. The retina and distal myelinated part of the optic nerve of both genotypes is hardly stained by TN-C antibodies (c, d). Spots of increased phosphacan immunoreactivity are detectable in the white matter of spinal cords of wild-type mice (e), whereas phosphacan is diffusely distributed in white matter of TN-R-deficient mice (f). Incubation of retinae and optic nerves of wild-type mice with anti-phosphacan antibodies reveals particularly strong staining of the outer plexiform layer of the retina (g, arrows) and a punctuate staining of the distal myelinated part of the optic nerve. Phosphacan immunoreactivity in retinae and optic nerves of TN-R-deficient animals (h), in contrast, is weak and diffusely distributed when compared with wild-type mice. Sections incubated with secondary antibodies only are devoid of any labeling (i). Scale bars (shown in b for a and b, in d for c and d, and in i for g-i), 100 µm; (shown in f) e, f, 250 µm.

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Figure 5. In situ hybridization analysis of retinae, optic nerves, and cerebella from wild-type and TN-R-deficient mice. Localization by in situ hybridization of tn-r (a, b) and tn-c (c, d) transcripts in 14-d-old wild-type (a, c) and TN-R-deficient (b, d) mice. a, b, The tn-r cRNA probe detects wild-type (a) and aberrant (b) transcripts in cells located at the outer margin of the inner nuclear layer of retinae and in cells restricted to the myelinated part of optic nerves. c, d, tn-c transcripts are detected in Golgi epithelial cells of cerebella of both genotypes. igl, Internal granular layer; mol, molecular layer. Scale bar (shown in d) a, b, 200 µm; c, d, 250 µm.

Electron microscopic analysis of optic nerves of TN-R-deficient mice

TN-R is expressed by cells of the oligodendrocyte cell lineage during development and in the adult (Pesheva et al., 1989;Bartsch et al., 1993; Wintergerst et al., 1993) and has been hypothesizedto be functionally involved in the formation of nodes of Ranvier(ffrench-Constant et al., 1986; Bartsch et al., 1993). Myelinationand morphology of myelin sheaths were studied in 14-d-old and2- and 9-month-old TN-R mutants at the ultrastructural level.In cross-sectioned optic nerves of 14-d-old mice, the densityof myelin sheaths was comparable between wild-type and TN-R-deficientanimals (data not shown), indicating that myelination is not delayedin the mutant. Moreover, myelin sheaths in the optic nerve of2- and 9-month-old TN-R-deficient mice did not show obvious morphologicaldefects (Fig. 6, compare a, b). The ultrastructure of nodes ofRanvier also did not reveal obvious morphological differencesbetween wild-type (data not shown) and TN-R-deficient mice (Fig.6c). Paranodal loops of myelin sheaths formed normally in TN-R-deficientmice (Fig. 6c), and processes of perinodal astrocytes extendedin a similar pattern into the nodal region of myelinated axonsof wild-type and mutant mice.

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Figure 6. Electron microscopic analysis of optic nerves of wild-type and TN-R-deficient mice. Cross sections through optic nerves of 8-week-old wild-type (a) and TN-R-deficient (b) mice. There are no significant differences in the number of myelinated axons or the ultrastructure of myelin between both genotypes. c, Longitudinal section through a myelinated ganglion cell axon of an 8-week-old TN-R-deficient mouse. Note the normal ultrastructure of paranodal regions of myelin sheaths and the presence of perinodal astrocyte processes (some marked with stars) extending into the nodal regions of the axon. As, Astrocyte; Ax, axon; M, myelin; P, paranodal loops. Scale bar, 0.5 µm.

Expression of extracellular matrix molecules and myelin-associated glycoprotein in TN-R-deficient mice

In situ hybridization analysis of cerebella from wild-type and TN-R-deficient mice revealed no significant differences inthe distribution and density of cells expressing TN-C mRNA (Fig.5, compare c, d). In agreement with this observation, we foundno obvious differences in the intensity and distribution of TN-Cprotein in the cerebellar cortex of adult wild-type and TN-R-deficientmice (Fig. 7, compare a, b). In the adult optic nerve, TN-C isaccumulated in the unmyelinated proximal, i.e., near retina part,but is hardly detectable in the distal, myelinated part [for awild-type, see Fig. 7c (Bartsch et al., 1992a)]. This characteristic,restricted expression of TN-C was also maintained in TN-R-deficientmice (Fig. 7d). MAG is expressed by oligodendrocytes and locatedon myelinating oligodendrocyte processes and in the periaxonalregion of myelinated axons. Immunohistochemical localization ofMAG did not show differences between TN-R-deficient and wild-typeanimals (data notshown).

Using immunohistochemistry, we recently found a striking colocalization of TN-R and the chondroitin sulfate proteoglycan phosphacanin retinae and optic nerves from adult wild-type mice (Xiao etal., 1997; Milev et al., 1998). In the retina, TN-R [data notshown; see Bartsch et al. (1993)] and phosphacan immunoreactivities(Fig. 7g) are intense in the outer plexiform layer and weak inthe inner plexiform layer and nerve fiber layer. In the opticnerve, TN-R and phosphacan were predominantly detectable in thedistal myelinated part of the nerve, and spot-like intense immunoreactivityof both ECM molecules suggests their accumulation at nodes ofRanvier [for TN-R, see Bartsch et al. (1993); for phosphacan,see Fig. 7g; Xiao et al. (1997)]. Spots of increased TN-R- (Wintergerstet al., 1993) and phosphacan (Fig. 7e) immunoreactivity were alsodetectable in the white matter of longitudinally sectioned spinalcords of wild-type mice. This characteristic distribution of phosphacanimmunoreactivity was not detectable, however, in the retina, opticnerve, or spinal cord of TN-R-deficient mice (Fig. 7f,h). In particular,neither prominent phosphacan positivity of the outer plexiformlayer of the retina nor intense spot-like phosphacan immunoreactivityin the optic nerve or white matter of the spinal cord were visiblein TN-R mutants (Fig. 7, compare e, f and g, h). Instead, phosphacanimmunoreactivity was weak and diffuse, indicating an altered distributionof this ECM component in mutantmice.

Analysis of parvalbumin-positive interneurons and perineuronal nets

TN-R is expressed by interneurons in the cerebellar cortex, retina, and hippocampus (Fuss et al., 1993; Wintergerst et al.,1993). We investigated the density of inhibitory interneuronsby immunocytochemistry using antibodies to the Ca²⁺-binding protein parvalbumin as a marker for a subpopulation ofGABAergic cells. The density of parvalbumin-immunoreactive cellswas not different between wild-type and mutant animals in theregions studied (somatosensory cortex, retrosplenial cortex, andthe CA1 field of the hippocampus). Representative aspects of parvalbumin-positiveneurons are shown for the adult somatosensory cortex of wild-typeand TN-R-deficient animals (Fig. 8, compare a, b).

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Figure 8. Immunohistochemical localization of parvalbumin and Wisteria floribunda lectin-binding sites in the somatosensory cortex and hippocampus of wild-type and TN-R-deficient mice. Parvalbumin (a, b) and lectin-binding sites (c-f) in layer IV of the somatosensory cortex (a-d) and CA1 region of the hippocampus (e, f) of wild-type (a, c, e) and TN-R-deficient (b, d, f) mice. There is no significant difference in density, distribution, or cell morphology of parvalbumin-positive neurons in the somatosensory cortex of wild-type and TN-R-deficient mice (compare a, b). Perineuronal nets stained by the lectin are less developed in TN-R-deficient mice when compared with wild-type mice (compare c, d). In wild-type animals the punctuate staining of cell bodies is distinct and well delineates the primary dendritic shafts extending from the neuronal cell body (c). In TN-R-deficient mice the lectin staining of neuronal cell bodies is less punctuate and does not extend well into the primary dendritic shafts (d). Similarly, in the hippocampus, primary dendritic shafts are distinctly labeled by the lectin in wild-type animals (e), whereas only cell bodies but not dendritic shafts are detectably labeled by the lectin in TN-R-deficient mice (f). Scale bars: a, b, e, f, 40 µm; c, d, 20 µm.

The parvalbumin-immunoreactive GABAergic interneurons are surrounded by perineuronal nets (Härtig et al., 1992, 1994; Lüthet al., 1992; Brückner et al., 1994). Perineuronal nets are describedas a lattice-like accumulation of different extracellular moleculesadhering intimately to the surface of cell body and proximal dendrites,excluding the axon initial segment of certain neurons in the adultbrain (for review, see Celio and Blümcke, 1994), and they arecharacteristically stained by Wisteria floribunda lectin and peanutagglutinin. These lectins label the perineuronal nets in a mesh-likepattern that surrounds the perikarya and the first order branchesof dendrites. Sometimes the initial segments of axons of theseparvalbumin-positive interneurons are also labeled (for instance,see Fig. 8c). Such cells are found in layer IV and, in particular,in its upper part of the somatosensory cortex of adult mice (Fig.8c). This staining pattern is also found associated with neuronsof the agranular and granular retrosplenial cortices. In the hippocampus,lectin-labeled neurons are present in the strata oriens and pyramidaleof the CA1-3 fields and in the stratum radiatum of the dorsalhalf of the CA3 field. Only a few lectin-labeled cells are locatedwithin and underneath the stratum granulare of the dentate gyrus(data notshown).

In TN-R-deficient mice, the distribution and shape of perineuronal nets is clearly different from that in wild-type animals(Fig. 8c-f). The abnormal configuration of perineuronal nets inTN-R-deficient mice is characterized by a less regularly shapeddistribution around the neuronal perikarya, and the primary dendriticshafts are less ensheathed by the punctuate appearance of thelectin labeling. It is noteworthy that all parvalbumin-reactiveneurons contain these abnormally shaped perineuronal nets as revealedby double-labeling (data not shown). Antibodies against the HNK-1carbohydrate structure show a labeling pattern similar to thatof the lectin, thus also revealing a less regularly shaped andaltered appearance of perineuronal nets in the mutant (data notshown). Quantitative evaluation of the density of lectin- andHNK-1-positive neurons, number of lectin- and HNK-1-positive dendritesextending from individual neuronal somata, and lengths of primarydendritic shafts labeled by lectin and HNK-1 antibodies showedsignificant differences between wild-type and TN-R-deficient animals(Table 1). Although the numbers of lectin- and HNK-1-positiveneurons were similar for TN-R-deficient and wild-type mice inthe brain areas analyzed, the numbers of dendrites per neuronand the length of the primary shafts that were labeled by lectinand HNK-1 antibodies were reduced in the TN-R-deficient comparedwith wild-type animals.


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Table 1. Quantitative evaluation of density of neuronal cell bodies, dendrites per neuron, and dendritic length per neuron in wild-type and TN-R-deficient mice as visualized by staining with the lectin Wisteria floribunda and immunocytochemical detection of the HNK-1 carbohydrate epitope

To exclude the possibility that the abnormal distribution of HNK-1 carbohydrate and binding sites for the lectin Wisteriafloribunda detected in TN-R-deficient mice is caused simply bythe absence of TN-R as the major carrier of these carbohydratesin perineuronal nets, we determined whether TN-R carries glycansthat are recognized by PNA, a lectin that, like Wisteria floribunda,recognizes N-acetylgalactosamine in perineuronal nets. The patternof proteins labeled by PNA after Western blot analysis of brainextracts from 3-month-old TN-R-deficient and wild-type mice wereindistinguishable (data not shown). Importantly, TN-R immunopurifiedfrom adult brain was also not recognized by PNA. Thus, the absenceof TN-R from perineuronal nets in TN-R-deficient mice cannot explainthe difference in labeling of perineuronalnets.

In summary, the density of parvalbumin-positive interneurons with perineuronal nets labeled by Wisteria floribunda lectinor HNK-1 antibodies does not differ between wild-type and TN-R-deficientanimals. The perineuronal nets around somata and accompanyingthe primary dendritic shafts are clearly less developed, however,in TN-R-deficient mice than in wild-typemice.

Na⁺ channels at nodes of Ranvier in the optic nerve

The presence of TN-R at CNS nodes of Ranvier, along with the partial homology of the Na⁺ channel $beta$ 2 subunit to the TN-R receptor F3/F11/contactin (Isomet al., 1995), suggested that TN-R might play a role in the denseclustering of channels in the nodal axolemma. Thus, we immunolabeledNa⁺ channels in cryosectioned optic nerves from 8-d-old to adultmice. We compared the number of Na⁺ channel aggregates at nodes of Ranvier in TN-R-deficient micewith wild-type mice. This was performed by selecting a randomFOV within the immunolabeled tissue sample and then counting thenumber of stained nodes within that FOV as a function of age.An average of nine FOVs were used per postnatal day. Figure 9A,Bshows portions of representative FOVs of cryosectioned optic nervesfrom adult TN-R-deficient and adult wild-type mice, respectively.On close examination of individual nodes, the Na⁺ channel immunolabeling was highly focal and was expressed onthe surface identically in TN-R-deficient and wild-type mice.Figure 9C summarizes the data obtained from this comparison. Nodifference was seen in the number of Na⁺ channel clusters at nodes of Ranvier at any stage nor in therate at which these specialized structures formed, suggestingthat the TN-R-deficient mouse was able to target correctly andcluster Na⁺ channels in the absence of TN-R and that internodal distanceswere also unaffected.

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Figure 9. Immunohistochemical evaluation of Na⁺ channel distribution in TN-R-deficient and wild-type mice. Representative regions of Na⁺ channel-immunolabeled optic nerve from TN-R-deficient (A) and wild-type C57BL/6 (B) mice. The region shown is ~70% of one field of view (FOV). Arrowheads in both A and B point to large fibers with double lines of Na⁺ channel immunofluorescence characteristic of surface staining at nodes. C, Development of Na⁺ channel aggregates at nodes of Ranvier in wild-type C57BL/6 and TN-R-deficient mouse optic nerves. The numbers of nodal Na⁺ channel clusters per FOV in both wild-type (wt) and TN-R-deficient (tn-r^/) mice matched closely. The number of nodal aggregates reached the final amount at approximately postnatal day 26. Error bars represent ± SD, and curves were drawn by hand to indicate trends. Scale bar, 10 µm.

Optic nerves of TN-R-deficient mice have a reduced conduction velocity

Despite the apparently normal occurrence of focal Na⁺ channel clusters in the optic nerves of TN-R-deficient mice, functionalchanges could result from more subtle alterations in nodal channeldensity, channel gating characteristics, or local electrical cableproperties. To investigate the electrophysiological propertiesof CNS axons in TN-R-deficient mice, we used suction electrodesto measure CAPs from optic nerves. Figure 10A shows representativeCAPs at 24°C and 37°C. The signals from the knock-out animalsappeared to have slower kinetics than those from controls. Thetime-to-peak for each trace was then measured and converted toa conduction velocity. The average velocity in wild-type micewas nearly two times that of the TN-R-deficient mice at all temperaturesmeasured (Fig. 10C). At 24°C, the conduction velocity of controloptic nerves was 3.5 ± 0.28 m/sec (SEM, n = 10) and that of TN-R-deficientoptic nerves was 1.8 ± 0.18 m/sec (n = 5). At 37°C, the correspondingvelocities were 8.2 ± 0.76 m/sec (n = 9) in wild-type mice and4.5 ± 0.30 m/sec (n = 5) in TN-R-deficient mice. Significancelevels were calculated using the Student's t test and were asfollows: 24°C, p < 0.005; 30°C, p < 0.0005; 37°C, p < 0.005. Thelength of the TN-R-deficient nerves was 4.50 ± 0.20 mm, and thelength of wild-type preparations was 4.44 ± 0.06 mm (SEM). Thus,the length did not vary with the deletion of TN-R and is not likelyto be a significant source of error in velocity measurements giventhe large difference that was observed. The short conduction distanceand high velocity, especially at 37°C, made it difficult to separatethe CAP from the stimulus artifact. Several controls were performedto insure that the measurement of time-to-peak was accurate. Onepossible problem is direct stimulation close to the recordingelectrode. As a test, when the stimulus intensity was raised incrementallyfrom 0 to supramaximal values, no change in the location of theCAP was observed (Fig. 10B, top trace). Second, the slowing ofconduction velocities was similar at 24° and 37°C, whereas directstimulation would appear at both temperatures. Finally, recordswere made before and after addition of 200 nM TTX, and the stimulusartifact in the latter was subsequently subtracted. Randomnessof a few microseconds in the timing of the stimulus introducedlimitations, but this procedure allowed removal of most of thelate phase of the artifact (Fig. 10B, bottom trace). In a controlnerve at 37°C (the most stringent condition), the measured velocitywas 6.91 m/sec before subtraction and 6.70 m/sec afterward, achange of just 3%. Thus, despite these experimental limitations,the measured differences in conduction properties between tn-r^+/+ and tn-r^/ preparations are significant. As a further control, we testedsciatic nerves from TN-R-deficient and wild-type mice, becauseTN-R is absent from the PNS (Pesheva et al., 1989). The conductionvelocities at 24°C in nerves from the wild-type mouse averaged14.62 ± 1.77 m/sec (n = 2); in the TN-R-deficient mouse they averaged17.85 ± 2.07 m/sec (n = 2). At 37°C, the velocities were 27.08± 0.76 m/sec (n = 2) in the wild-type mouse and 30.08 ± 3.77 m/sec(n = 2) in the TN-R-deficient mouse. In these experiments theTN-R-deficient mouse consistently had a slightly higher conductionvelocity, but statistical analysis using a two-tailed Student'st test revealed that the difference was not significant (p > 0.1).This result confirms the fact that the decrease in speed of actionpotential propagation seen in the optic nerve was caused by theabsence of the CNS-specific TN-R.

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Figure 10. Determination of conduction velocities of compound action potentials and of nodal Na⁺ channel aggregates in TN-R-deficient and wild-type mice. A, Representative CAPs from TN-R-deficient (tn-r^/) and wild-type (wt) C57BL/6 mouse optic nerve suction electrode recordings. Records were taken at both 24° and 37°C. The TN-R-deficient record is noticeably slower than the wild-type record at each temperature. Because the seal resistance varied from nerve to nerve, amplitudes are arbitrary. B, Control experiments were performed to insure that conduction velocities were calculated correctly. The top trace shows a series of CAPs at 37°C from a wild-type optic nerve stimulated from 0 to above the supramaximal value. The bottom trace shows a CAP at 37°C, after the stimulus artifact was subtracted as described in Results. C, The conduction velocity measured in wild-type mouse optic nerves (wt, n = 10) was consistently higher than that seen in TN-R-deficient mice (tn-r^/, n = 5) at all temperatures measured. Conduction velocity is defined here as the length of the optic nerve used divided by the time to the peak of the action potential from stimulus onset. Significance values were calculated using the Student's t test and were as follows: 24°C, p < 0.005; 30°C, p < 0.0005; and 37°C, p < 0.005. Error bars represent ±SEM. D, The fluorescence of nodal Na⁺ channel aggregates in TN-R-deficient (tn-r^/, n = 94) and wild-type C57BL/6 (wt, n = 103) mouse optic nerves (arbitrary units) as a function of nodal area (µm²). The data were fit using a least-squares algorithm given a y-intercept of 0, i.e., at 0 nodal area there is 0 fluorescence. In the TN-R-deficient mouse, the equation for the line is y = 24773x and in the wild-type mouse y = 24566x. The lines thus virtually overlap.

Na⁺ channel expression in optic nerves of wild-type and TN-R-deficient mice

One possibility for the difference in conduction velocities between wild-type and TN-R-deficient mice is a difference in thenumber of Na⁺ channels at nodes. To investigate this possibility, in side-by-sidesteps and using the same reagents throughout, cryosections ofoptic nerves from wild-type and TN-R-deficient mice were labeledfor Na⁺ channel immunoreactivity. Subsequent to labeling, the relativefluorescence intensity of each node (from random FOVs) was measuredas a function of nodal area. Figure 10D shows the results for aTN-R-deficient optic nerve and a wild-type optic nerve. Linesthrough the data are least-squares fits, and when plotted on thesame axes the lines for each data set overlapped almost precisely(see Figure caption for additional details). The results thusshow that the relative fluorescence intensity was the same, indicatingno difference in the number of Na⁺ channels per unit area at nodes of Ranvier between mutant andwild-type animals. Furthermore, as the data indicate, if the nodalarea is doubled, the total relative fluorescence doubles. Thedecrease in conduction velocity in the TN-R-deficient animalsis thus not attributable to a significant difference in Na⁺ channeldensity.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The TN-R-deficient mice described in this study are surprisingly normal in their gross general behavior and with respect tofertility, body weight, and life span. There is no doubt thatthe mutation that was introduced abolished expression of TN-R.Southern blot analysis with external and internal tn-r probesshowed the hybridization pattern that was expected when homologousrecombination took place in the predicted manner replacing theexon encoding the amino terminus of TN-R. Although the mutationdoes not ablate transcription of the mutated tn-r gene, determinationof the sequence of the translation product revealed that it containsan intronic region and lacks further sequences encoded by exons2 and 3 located downstream of the mutation. A ribosome-bindingsite, a translation initiation codon, and a signal peptide-encodingsequence preceding an open reading frame are absent, excludingtranslation of this aberrant RNA into an exported TN-R-relatedprotein. Thus, the mutation resulted in a nonfunctional mRNA generatedby an unexpected splicing event. Accordingly, although the aberrantRNA is expressed in the mutant in quantities similar to thoseof the TN-R mRNA in wild-type mice, neither TN-R nor a truncatedform thereof could be detected by Western blot analysis usingvarious polyclonal and monoclonal antibodies at a level of sensitivitysufficient to reveal a 1000-fold reduction of TN-Rexpression.

The gross anatomy of the brain and spinal cord and the morphology of the retina and cerebellum are also indistinguishablebetween TN-R-deficient and wild-type mice at the light microscopiclevel. This could be analyzed in some detail because the mutantmice express a nonfunctional TN-R mRNA, and the localization ofcells normally expressing TN-R could thus be studied by in situhybridization. No aberrant location of normally TN-R-positivecells was detected in cerebellum, optic nerve, and retina of TN-R-deficientmice. Therefore, TN-R appears to be dispensable for the migrationof these neural cell types and their anatomically correct localizationin these areas of theCNS.

TN-R is expressed by oligodendrocytes at times of myelination (Bartsch et al., 1993; Wintergerst et al., 1993) and is highlyaccumulated at nodes of Ranvier in the optic nerve (ffrench-Constantet al., 1986; Bartsch et al., 1993). The interaction of TN-R withits neuronal receptor F3/F11/contactin decreases fasciculationof cerebellar granule cell neurites in vitro (Xiao et al., 1998),and it has been hypothesized that this defasciculating activitymay support the initial ensheathment of axons during myelination(Xiao et al., 1998). The morphological analysis at the ultrastructurallevel revealed an apparently normal structure and developmentof myelin sheaths and nodes of Ranvier in the optic nerve of 2-and 8-week-old and 9-month-old TN-R-deficient mice. Furthermore,no morphological indication for degeneration of myelin sheathsor axons was observed. In the optic nerve (Xiao et al., 1997)and white matter of the spinal cord of wild-type mice, TN-R andthe chondroitin sulfate proteoglycan phosphacan are colocalizedand accumulated at nodes of Ranvier. Remarkably, in the opticnerve and spinal cord of TN-R-deficient mice, phosphacan stainingwas weak and diffuse, and spots of intense immunoreactivity wereabsent. Binding of TN-R to a chondroitin sulfate proteoglycanimmunologically related to phosphacan has been demonstrated invitro (Xiao et al., 1997), and phosphacan is a high-affinity ligandto native TN-C and TN-R (Milev et al., 1998). Int