Mutation in Neurofilament Transgene Implicates RNA Processing in the Pathogenesis of Neurodegenerative Disease

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The Journal of Neuroscience, February 15, 1999, 19(4):1273-1283

Mutation in Neurofilament Transgene Implicates RNA Processing in the Pathogenesis of Neurodegenerative Disease
Rafaela Cañete-Soler¹, Debra G. Silberg², Michael D. Gershon³, and William W. Schlaepfer¹
Divisions of ¹ Neuropathology and ² Gastroenterology, University of Pennsylvania Medical School, Philadelphia, Pennsylvania 19104-6079, and the ³ Department of Anatomy and Cell Biology, Columbia University, New York, New York 10032

  ABSTRACT

Top
Abstract
Introduction
References

A mouse neurofilament light subunit (NF-L) transgene with a 36 bp c-myc insert at the end of the coding region was found tohave neuropathic effects on enteric and motor neurons of transgenicmice. The severity of phenotype was related directly to the levelsof transgenic mRNA expression. High levels of transgene expressionwere lethal to newborn pups, causing profound alterations in thedevelopment of the enteric nervous system and extensive vacuolarchanges in motor neurons. Lower levels of transgene expressionled to a transient stunting of growth and focal alterations ofenteric and motor neurons. Because the positioning of the c-mycinsert coincided with the location of the major stability determinantof the NF-L mRNA (Cañete-Soler et al., 1998a,b), additional studieswere undertaken. These studies showed that the c-myc insert altersthe ribonucleoprotein (RNP) complexes that bind to the stabilitydeterminant and disrupts their ability to regulate the stabilityof the transcripts. The findings indicate that expression of anNF-L transgene with a mutant mRNA stability determinant is highlydisruptive to enteric and motor neurons and implicate alterationsin RNA processing in the pathogenesis of a neurodegenerativecondition.

Key words: neurofilament transgene; motor neuron degeneration; transgenic mice; post-transcriptional regulation; ribonucleoprotein complexes; mRNA stability

  INTRODUCTION

Top
Abstract
Introduction
References

The degeneration of motor neurons in mice bearing a neurofilament (NF) transgene indicates a selective susceptibility of motorneurons to an unknown component of NF transgene expression. Anunknown aspect of NF expression also affects the course of motorneuron degeneration in mice bearing a mutant superoxide dismutase-1(SOD-1) transgene (Couillard-Despres et al., 1998; Williamsonet al., 1998). The neuropathic effects of a NF transgene on motorneurons were detected initially on overexpression of a mouse light(NF-L) or human heavy (NF-H) NF transgene (Cote et al., 1993;Xu et al., 1993), but a much more severe form of motor neurondegeneration occurred in mice bearing a mutant NF-L transgenewith a leucine-to-proline point mutation in the rod domain ofthe protein (Lee et al., 1994). The latter mutation was intendedto disassemble NFs, yet expression of the mutant protein did notlead to a granular disintegration of NF profiles, as characteristicof a dominant filament-disassembling subunit (Gill et al., 1990),nor prevent the accumulation of assembled NFs, admixed with mutantprotein, in cell bodies and dystrophic neurites of degeneratingmotor neurons. It is, therefore, unclear whether the accumulationsof NFs are primary or secondary events of motor neuron degenerationor why the accumulations should occur so selectively in motorneurons. The accumulation of NFs in degenerating motor neuronshas led to the view that the disruptive effects of NF transgenesare attributable to altered NF transport (Collard et al., 1995;Bruijn and Cleveland, 1996), although disruption of NF transportrecently has been discounted in the pathogenesis of other neurodegenerativedisorders (Eyer et al., 1998).

An alternative view as to the nature of motor neuron degeneration in mice expressing a NF-L transgene has arisen from studieson NF mRNA stability (Cañete-Soler et al., 1998a,b). These studiesindicate that the mutant NF-L transgene that causes massive motorneuron degeneration (Lee et al., 1994) also contained a secondmutation by virtue of a 36 bp c-myc tag that was inserted inadvertentlyinto the major stability determinant of the transcript. The c-mycinsert separates components in the coding region and the 3'-UTRof NF-L mRNA that are essential for the binding of ribonucleoprotein(RNP) complexes to the stability determinant (Cañete-Soler etal., 1998b). The findings raise the possibility that motor neurondegeneration may be attributable to expression of mutant mRNArather than mutant protein by the NF-L transgene. Expression ofthe mutant NF-L mRNA could alter the RNP components that regulateNF-L expression as well as expression of other gene products,such as those that override apoptosis and maintain neuronal viability(see Easton et al., 1997).

The possibility that the c-myc mutation in the NF-L transgene is responsible for the neurodegenerative effects would haveimportant implications for the pathogenesis of the neurodegenerativestate. Specifically, it would imply that the neuropathic effectsare attributable to expression of NF mRNA rather than NF proteinby the transgene. This conclusion is supported by studies showingthat appending the same c-myc tag to the C terminus of the NF-L,NF-M, or NF-H subunit does not affect that ability of the subunitto assemble into filaments (Gill et al., 1990; Wong and Cleveland,1990; Lee et al., 1993). Moreover, expression of the c-myc tagin a NF-M transgene is incorporated readily into assembled NFswithout altering neuronal viability in transgenic mice (Wong etal., 1995a). Furthermore, because the aforementioned NF-M transgenealso contained the 3'-UTR from the mouse NF-L (Wong et al., 1995a),the neuropathic effects of the c-myc mutation in the NF-L transgenecould be attributed only to the context of the c-myc mutationin relation to the stability determinant of the NF-L transcript(Cañete-Soler et al., 1998b). Finally, the possibility that theneuropathic effects of the mutant NF-L transgene could be explainedby the stabilization of the message and the overexpression ofthe protein must be discounted because the severe neuropathiceffects from the mutant NF-L transgene occur at reduced levelsof NF-L protein expression (Lee et al., 1994; Bruijn and Cleveland,1996), whereas the neuropathic effects of the wild-type NF-L transgenewere observed only when there was a fourfold increase in the expressionof NF-L protein (Xu et al., 1993).

The present study has begun to test our working hypothesis by examining the biological effects of a NF-L transgene with onlythe c-myc mutation, the functional effects of the c-myc mutationon NF-L mRNA stability, and the biochemical effects of a c-mycmutation on the RNP complexes that bind to the stability determinant.We show that expression of the NF-L transgene with the c-myc mutationhas profound disruptive effects on neurons in the peripheral nervoussystem and that the c-myc mutation alters the binding of RNP complexesand their ability to regulate the stability of the NF-L mRNA.The findings implicate alterations in RNA processing in the pathogenesisof a neurodegenerative state and provide novel insights into thenature of neurodegenerativedisease.

  MATERIALS AND METHODS

Construction of mutant NF-L cDNAs. A full-length mouse NF-L cDNA (Cañete-Soler et al., 1998a) in the HindIII/XbaI polylinkersites of pSK⁺ (Stratagene, La Jolla, CA) was used as a PCR template to inserta 36 bp c-myc insert immediately upstream of the stop codon. Overlappingsense and antisense primers to the c-myc insert (upper case),stop codon (underlined), and NF-L sequence (lower case) were synthesizedas follows: CTCATTTCTGAAGAGGACTTGATTtgagccctattcccaactattcc (sense)andTTCAGAAATGAGCTTTTGCTCCATatctttcttcttagccacc (antisense).PCRfragments of upstream (1.7 kb) and downstream (0.5 kb) NF-L sequencewere generated by using primers to pSK⁺ vector sequence flanking the HindIII and XbaI restriction sites.A full-length NF-L cDNA with 36 bp c-myc insert then was generatedby PCR, using the same flanking primers and the 1.7 kb upstreamand the 0.5 kb downstream NF-L PCR fragments as template. The2.2 kb PCR fragment was gel-excised, cut with HindIII and XbaI,and ligated into the HindIII/XbaI sites of a pRC/CMV expressionvector (Invitrogen, San Diego, CA). The integrity of the NF-LcDNA, c-myc insert, and stop codon was confirmed by sequencingboth strands of the finalconstruct.

NF-L cDNAs were constructed with the same c-myc insert inserted into the BglII site (+828) of exon I (NF-L/c-myc/BglII) orinto the EcoRI (+2055) in the distal 3'-UTR (NF-L/c-myc/EcoRI).In each instance, sense and antisense oligonucleotides containingthe 36 bp c-myc sequence flanked by BglII or EcoRI restrictionsites were synthesized, annealed, cut, and ligated into the respectiverestriction sites of the NF-L cDNA and sequenced to determinethe orientation of the c-myc insert. Insertion of the c-myc sequenceinto the BlgII site did not alter the open reading frame of thecDNA. The integrity of all constructs was confirmed bysequencing.

The NF-L/wt and NF-L/c-myc cDNAs were converted into templates for RNA probes by PCR, using primers that bracketed the 23bp of 3'-coding region (3'-CR) and 45 bp of 3'-UTR and with theT7 promoter sequence appended to the sense primer. The same strategywas used to construct a control c-myc probe with the 23 bp ofupstream and 45 bp of downstream sequence that flanked the c-mycsequence of the BglII site (+828) in exon I, using the NF-L/c-myc/BglIIcDNA astemplate.

Determination of mRNA stability. cDNAs with wild-type sequence (NF-L/wt), with the stability determinant deleted (NF-L/del),and with c-myc mutations (NF-L/c-myc, NF-L/c-myc/BlgII, and NF-L/c-myc/EcoRI)were placed into the HindIII/XbaI polylinker sites of a pRC/RSVvector (Invitrogen) in which the RSV promoter had been replacedwith the heptamerized Tn-10 tet operator sequence, as previouslydescribed (Cañete-Soler et al., 1998a). The modified vectors(NF-L/wt/tet, NF-L/del/tet, and NF-L/c-myc/tet) were transfectedinto Neuro 2a cells containing a tTA transactivator cDNA withan autoinducible promoter (Cañete-Soler et al., 1998a). Cellswith transactivator and inducible target transgenes were selectedby growth in Zeomycin and Neomycin, respectively, and the presenceof the transgenes was monitored by PCR. Multiple clones (>100)with both transgenes were pooled. mRNA was assayed by ribonucleaseprotection assay, and levels of NF-L mRNA were normalized to thoseof $beta$ -actin mRNA in transfected cells. Radioactivity was quantitatedbyphosphoimager.

Transient transfections were conducted to compare the effects of the c-myc insert when placed in the stability determinant(NF-L/c-myc/tet), in exon 1 (NF-L/c-myc/BglII/tet), or in the3'-UTR (NF-L/c-myc/EcoRI/tet). These vectors were cotransfectedwith equal amounts of wild-type vector (NF-L/tet) in Neuro 2acells containing the tTA transactivator expression vector. Expressionof the target NF-L cDNAs was activated for 12 hr by growth inthe absence of tetracycline, and NF-L mRNAs were quantitated at24 and 48 hr after the addition oftetracycline.

NF-L mRNAs in transient transfected cells were quantitated by RT-PCR. RNA was extracted from a Qiagen column (Hilden, Germany)and used as a template for reverse transcriptase with random hexanucleotidesas primers. 20-mer PCR primers were chosen that extended the PCRproducts across the sites of the c-myc inserts, i.e., from +790to +925 in exon 1 of NF-L (for NF-L/c-myc/BglII), from +1701 to+1836 (for NF-L/c-myc), and from +2000 to +2135 (for NF-L/c-myc/EcoRI).Antisense primers were admixed at a 1:50 ratio with ³²P end-labeled primers. Samples were run for 15, 20, and 25 cyclesand separated on 5% acrylamide gels; radioactivity in the PCRproducts from the mutant and wild-type transcripts was quantitatedbyphosphoimager.

Gel-shift and cross-linking of RNP components. Full-length RNA probes were labeled uniformly with ³²P-UTP, eluted from acrylamide gels, and diluted to 2.5 × 10⁴ cpm/µl immediately before use, as previously described (Cañete-Soleret al., 1998b). Gel-shift and cross-linking assays were conductedwith 5 × 10⁴ cpm of probe and 160 µg of protein extracted from rat brain cytosolcontaining (in mM) 50 K-acetate, 3 Mg-acetate, 2 dithiothreitol,and 20 HEPES buffer, pH 7.4, with or without homoribopolymer competitors.RNP complexes on RNA probes were cross-linked by 30 min exposureson ice at 3 cm under a UV light (4 × 10⁶ J/cm²), and the radioactive polypeptides were denatured by boilingin SDS sample buffer and fractionated by SDS-PAGE. High-speedcytosolic extracts were obtained from rat brain and were usedfresh or within a 4 month period of storage at $-$ 80°C. Radioactivityin gel-shifted and cross-linked bands was quantitated byphosphoimager.

Transgenic mice. The NF-L cDNA with 36 bp c-myc insert and hCMV promoter was excised with XhoI and XbaI and microinjectedinto fertilized eggs of B6SJF1/J female mice that had been matedwith B6SJF1/J males. Genomic DNA was extracted from tails of 14d pups and used to detect the transgene by PCR and to estimatetransgene copy number by Southern blot. PCR primers spanned thesequence between +1708 and +1815 and generated PCR fragments of108 and 144 bp from the wild-type and mutant sequence. GenomicDNA was cut with SacI (+1350) and HincII (+1814) to generate fragmentsof 464 and 500 bp from the endogenous NF-L gene and NF-L transgene,respectively. These fragments were separated on a 2% agarose geland hybridized with radioactive cDNA probes made by random primedlabeling of the SacI/HincIIfragment.

Tissue analyses. Transgenic and nontransgenic littermates were euthanized with CO₂ and their brains were excised for RNA protectionassay; vertebral columns, abdominal contents, and hindlimb musculaturewere dissected to expose the tissue for optimal fixation. Theintestines were fixed in situ by immersion in 10% neutral bufferedformalin (NBF) for 24 hr at 4°C and washed and stored in PBS;representative sections were dehydrated and embedded in paraffin.Microscopic sections were stained with hematoxylin and eosin (H&E)or immunostained with PGP9.5 to delineate enteric neurons (Karaosmanogluet al., 1996). Antibodies to PGP9.5 (Biogenesis, Sandown, NH)were applied at a 1:1000 dilution for 1 hr at room temperatureand visualized with goat anti-rabbit biotinylated antiserum andthe avidin/biotin detection system (Vector Laboratories, Burlingame,CA). Then the chromophore was developed with 3,3'-diaminobenzidinetetrahydrochloride (Sigma, St. Louis,MO).

After 4 hr of fixation, the vertebral columns of 14 and 28 d and adult mice were dissected further to expose the spinal cordsdirectly to NBF before the washing and storing of tissues in PBS.The spinal cords were separated from the vertebral columns, dehydrated,and embedded in paraffin. Paraffin-embedded spinal cords thenwere cut and positioned in paraffin blocks to obtain serial microscopiccross sections from the cervical to the lumbar cord. Spinal cordswere stained with hematoxylin or H&E or were immunostained withprimary antibodies to NF-L (N5139; Sigma), to the phosphorylatedepitopes on NF-H and NF-M (Ta51; Carden et al., 1987; Lee et al.,1987), and to the human c-myc tag (AB1; Calbiochem, La Jolla,CA). Secondary antibodies were biotinylated anti-rabbit or anti-mouseIgGs.

Expression of transgenic and endogenous NF-L mRNA. Brains from transgenic and nontransgenic littermates were homogenized in4 M guanidinium thiocyanate, and total RNA was extracted and storedat $-$ 80°C in formamide (Chomczynski and Sacchi, 1987). Levels ofmRNA from the endogenous NF-L gene and from the mutant NF-L transgenewere quantitated by RNA protection assay, using radioactive antisenseRNA probes that spanned the 36 bp c-myc insert (+1770). Templatesfor the RNA probes were generated by PCR and spanned NF-L sequencefrom +1525 to +1846, including the 36 bp c-myc insert and T7 promotersequence that was appended to the antisense primer. A full-lengthRNA probe was labeled uniformly with ³²P-UTP by T7 polymerase (Schwartz et al., 1992, 1995), separatedby electrophoresis, excised from acrylamide gels, eluted overnightinto 0.5 M NH₄ acetate, 0.1% SDS, and 1 mM EDTA, and precipitatedwith ethanol (Cañete-Soler et al., 1998b). An RNA protectionassay was undertaken by hybridizing brain RNA (10-20 µg) withthe RNA probe (10⁴ cpm), as previously described (Schwartz et al., 1992). Protectedfragments of 212 and 322 bp from the wild-type and mutant mRNAwere separated by electrophoresis on 7.5% denaturing acrylamidegels, and radioactivity of the protected fragments was detectedby autoradiogram and quantitated byphosphoimager.

  RESULTS

Expression of NF-L transgene with a 36 bp c-myc tag insert leads to a loss of enteric neurons and malformation of the small intestine

To test whether the c-myc mutation in an NF-L transgene might have disruptive effects in transgenic mice, we constructed amouse NF-L transgene with the 36 bp c-myc tag at the end of thecoding region but without the leucine-to-proline mutation in therod domain of the protein (see Lee et al., 1994). The transgenewas placed behind a strong constitutive promoter and microinjectedinto the mouse germ line. Nine founder mice (of 67 pups) wererecovered. Two founder mice (pups A and B) were born in an agonalstate with markedly distended abdomens (Fig. 1a,b). Examinationof the intestines revealed extensive dilatation of the midgutin pup A (Fig. 1c) and, to a lesser extent, in pup B. No specificsites of intestinal perforation were identified. Milk productswere not present, but fecal content was observed throughout theintestines, indicating that the intestinal dilatation was notattributable to complete obstruction of the alimentary canal.

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Figure 1. Newborn founder mice A (a) and B (b) bearing the NF-L transgene with c-myc mutation have markedly distended abdomens. c, The intestine of pup A reveals a dilated and shortened small intestine (SI) between the stomach (S) and ileum (I). The distal end of the esophagus (arrow) and discontinuous ends of ileum (*) and colon (C) are identified also. Immunohistochemistry for PGP9.5 (Karaosmanoglu et al., 1996) delineates brown reactive products in the enteric ganglia in the walls of small intestine from pup A (d) and a nontransgenic littermate (e) that are everted and folded back on themselves and around the abdominal cavity (x). The wall of the control is studded with immunoreactive enteric ganglia in the myenteric plexus immediately below the serosal surface. In contrast, there is a marked reduction of immunoreactive enteric ganglia in the wall of the small intestine of pup A. Scale bars: d, e, 100 µm.

Microscopic examination showed that intestinal dilatation was associated with a marked depletion of neurons from the entericnervous system when the population of enteric neurons was visualizedby their immunoreactivity to PGP9.5 (Karaosmanoglu et al., 1996).Multiple sections of midgut revealed either an absence or paucityof neurons in the dilated and thinned intestinal walls of thetransgenic pups (Fig. 1d) as compared with nontransgenic littermatecontrols (Fig. 1e). The aganglionic and hypoganglionic (loss of>50%) segments of midgut differed only in the extent of neuronalloss. Residual neurons were observed only in the myenteric plexus,although neurons of the myenteric and submucosal plexi were seenin controls. Residual enteric neurons did not display any distinctivepathological features and were difficult to identify with certaintyon H&E-stainedsections.

Transgene expression leads to vacuolar degeneration of motor neurons and alterations of muscle development

The alterations in the enteric nervous system raised questions as to whether the transgene also might affect the developmentof other neurons, specifically motor neurons. Microscopic examinationsat multiple levels of spinal cord revealed a vacuolar degenerationof anterior horn cells in the transgenic pups (Fig. 2a,b). Theperikarya of altered motor neurons were filled with vacuoles ofvariable sizes, irregular shapes, and sharp borders. Vacuolardegeneration was seen in most anterior horn cells at all levelsof spinal cord, more so in pup A than in pup B. Vacuolar changeswere not seen in other neurons of the spinal cord nor in any neuronsin spinal cords of nontransgenic littermates. A loosening of neuropilin the vicinity of the vacuolated perikarya may have obscuredthe presence of vacuolar changes in the neurites of motor neurons.A loosening of neuropil was seen in other regions of spinal cordand in spinal cords of nontransgenic newborn mice. The remarkablepreservation of nuclear detail, however, attested to the structuralpreservation of neuronal cell bodies in immersion-fixed, paraffin-embeddedtissues. The large, round nuclei of vacuolated motor neurons hadsharply defined nuclear borders, displayed a finely granular chromatinpattern, and often contained very prominent nucleoli. The samenuclear details were observed in vacuolated motor neurons of oldertransgenic mice without a loosening of the surrounding neuropil(Fig. 2c).

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Figure 2. a, A cluster of anterior horn cells in the lumbar spinal cord of pup A is enlarged (b) to reveal the cytoplasmic vacuolar degeneration of motor neurons. The nuclei of vacuolated neurons contain prominent nucleoli. c, Similar vacuolated changes are present in a cluster of three motor neurons of founder mouse D. Stained with hemotoxylin alone (a, b) or with eosin (c). Scale bars: a, 75 µm; b, c, 25 µm.

Immunoreactivities to mouse NF-L and to the human c-myc tag in vacuolated and control motor neurons of newborn mice were testedwith increasing concentrations of primary antibodies to mouseNF-L and the c-myc tag. End products were observed only at titersthat produced extensive nonspecific staining of the tissues. Whenthe spinal cords of newborn mice were examined with highly sensitiveantibodies to phosphorylated epitopes on the NF-H and NF-M subunits,immunoreactivity was detected in white matter tracts along thedorsal and ventral surfaces of spinal cord, as previously described(Carden et al., 1987). Focal NF accumulations in cell bodies ornearby neurites of vacuolated motor neurons were not seen in newbornmice or in the spinal cords of older mice. The limited amountsof motor neuron tissue in newborn mice precluded a biochemicalassessment of NF-L protein levels by Westernblot.

The extensive vacuolar degeneration of motor neurons in newborn mice was associated with perturbations in target organ development.Differences in skeletal muscle development were readily apparentin comparative examinations of muscles at the level of the distaltibia from transgenic and nontransgenic newborn pups. Whereasthe muscle of newborn controls was composed of uniform bundlesof muscle fibers with occasional central nuclei (Fig. 3b), themuscle from the transgenic pups A and B contained numerous smallcells without myofibrils interspersed among large fibers withmyofibrils (Fig. 3a). The large fibers had large and hyperchromaticcentral nuclei that often were associated with perinuclear vacuoles.The features resemble those described during muscle developmentlacking neurogenic input and have been attributed to a persistenceand degeneration of primary myotubes and deficiency of secondarymyotube development (Ontell et al., 1988; Condon et al., 1990).Differences between transgenic and nontransgenic muscle were lessapparent in musculature from the proximal limbs and along theaxial skeleton, suggesting that the changes may reflect a preferentialinvolvement of distal musculature or, possibly, a delay in muscledevelopment.

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Figure 3. a, Cross section of skeletal muscle at the level of the distal tibia from transgenic pup A showing large myofibers with hyperchromatic central nuclei and perinuclear vacuoles (arrow) scattered among numerous small cells without myofibrils. b, Cross section of skeletal muscle at the level of the distal tibia of a nontransgenic littermate control showing a uniform population of myofibers with central and peripheral nuclei. H&E stain. Scale bars: a, b, 50 µm.

Transgene expression leads to a stunting of growth during early development

Founder mice and transgenic F1 pups were smaller and less active than their nontransgenic littermates. These traits becameapparent during the initial 2-3 week period of postnatal developmentbut did not progress and became less apparent after weaning. Figure4 shows the stunted growth in an 18 d transgenic F1 pup (fromfounder E) as well as the abnormal reflex of flexing the limbswhen held by the tail, as previously described (Lee et al., 1994).The mouse did not develop further weakness or paralysis and waskilled along with a nontransgenic littermate at 28 d. Microscopicexamination revealed a loss of enteric neurons and vacuolar degenerationof motor neurons in the transgenic pup (data not shown). Stuntedgrowth was also a useful phenotypic marker of some, but not all,transgenic pups. When subsequently examined for transgene expression,pups with stunted growth had the highest levels of transgene expressionin their respective litters (see below).

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Figure 4. a, b, Stunted growth in an 18 d F1 transgenic pup (arrow) as compared with two nontransgenic littermates. c, The transgenic pup (arrow) displays an abnormal reflex of flexing the hind- and forelimbs when held by the tail, as compared with extension of the limbs and writhing movements of a nontransgenic littermate.

Abnormal phenotype correlates with expression of the mutant transgene

The highest levels of transgene expression were found in newborn pups with dilated and malformed intestines. RNA protectionassays showed the highest level of transgene expression in thebrain of pup A and slightly less in the brain of pup B (Fig. 5),corresponding with the more severe alterations in pup A. Transgeneexpression was greater than that of endogenous NF-L expression,although the latter is present at very low levels in neonatalrodent brain (Julien et al., 1986; Schlaepfer and Bruce, 1990).Similar levels of NF-L mRNA were noted in newborn transgenic andnontransgenic littermates, indicating that transgene expressiondid not appear to alter the expression of endogenous NF-L mRNA.Transgene expression was derived from low transgene copy numbersof 2 and 1 in pups A and B, respectively, as estimated by PCRand Southern blot analyses of genomic DNA.

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Figure 5. RNA protection assay showing protected fragments of 322 and 212 nt from transgenic and endogenous NF-L mRNAs, respectively, in the brains of pup A (lane 1), pub B (lane 2), nontransgenic littermates of pups A and B (lanes 3, 4), founder mouse C (lane 7), two of her transgenic pups (lanes 5, 6), and founder mouse D (lane 8).

Expression of the transgene in other founder mice and in transgenic lines was quite variable. A female founder (mouse C) transmittedthe transgene to four of seven F1 pups, but the transgene wasnot expressed (Fig. 5) and the abnormal phenotype was not detectedin this transgenic line. A male founder (mouse D) was unable totransmit the transgene to three litters of F1 pups. When foundermouse D was killed at 3 months, focal vacuolar degeneration wasobserved in anterior horn cells (see Fig. 2c), and a low levelof transgene expression was detected in brain (Fig. 5). Levelsof transgene expression also correlated with the severity of neuropathicchanges of enteric and motor neurons in the F1 and F2 progeny(seebelow).

Alterations of enteric and motor neurons occur in transgenic lines

Neuropathic changes of enteric and motor neurons occurred in three transgenic lines (from founders E, F, and G), includingeight transgenic pups from the F1 or F2 generations. Two transgenicpups from founder F were less active and without visible milkproducts in their stomachs, as customarily seen through the thinabdominal wall of newborn suckling mice. When they were killedon day 2, the absence of milk products was confirmed by directexamination. Instead, the stomachs and small intestines, but notthe abdominal cavities, were distended with air, as if the pupshad attempted to suckle but had ingested air instead of milk.Microscopically, there was extensive depletion of enteric neuronsin the small intestine and vacuolar degeneration of motor neurons,similar to that described in founder mice A andB.

In several instances, either one or two newborn F1 pups died during the initial 24 hr postnatal period and probably were cannibalizedby the mother so that they were not recovered for genomic typingor examination of the tissues. Nonviability of transgenic pupsalso was suggested in cross-breeding experiments. Initial cross-breedingof founder mice produced F1 litters with only one or two viablepups and F1 litters with a higher percentage of nontransgenicpups than anticipated. Subsequent cross-breedings of the samefounder mice yielded larger F1 litters with close to the anticipated75% rate of transgene transmission. Transgenic F1 pups, killedat 14 and 28 d, revealed focal losses of enteric neurons and vacuolarchanges of motor neurons. The extent of neuropathic changes andcorresponding levels of transgene expression were notable lessthan those observed in founders A and B in the newborn transgenicF1 pups of founder F. Examinations of other tissue, includingthe kidneys, from the founder mice and transgenic lines wereunremarkable.

Our overall findings suggest that the phenotype relates to levels of transgene expression. High-level expression leads toprofound neuropathic changes of enteric and motor neurons andis disruptive to perinatal and, possibly, to prenatal viability.Intermediate levels of expression were found in pups with stuntedgrowth. Low-level expression leads to transient dysfunction andlimited alterations of enteric and motorneurons.

Insertion of c-myc tag disrupts the ability of the stability determinant to regulate the stability of the NF-L transcript

Further studies were undertaken to probe the nature of the c-myc mutation on the NF-L transgene. To test the effects of thec-myc insert on NF-L mRNA stability, we constructed a full-lengthNF-L cDNA (NF-L/wt), a cDNA in which 23 bp of distal coding regionand 45 bp of proximal 3'-UTR were deleted (NF-L/del), and a cDNAcontaining a 36 bp c-myc insert between the coding region and3'-UTR (NF-L/c-myc). Then the NF-L cDNAs were placed behind aTn-10 tetracycline-inducible promoter (Gossen and Bujard, 1992)and stably transfected into a neuronal cell line (Neuro 2a) containingthe tTA transactivator cDNA under control of an autoinduciblepromoter (Shockett et al., 1995). The system was shown to be highlyinducible when tested with a luciferase reporter gene, generating1000-fold increases (and decreases) of luciferase activity inthe 48 hr interval after withdrawal (and readdition) of tetracycline(Cañete-Soler et al., 1998a).

Stability of mRNAs from the NF-L/wt, NF-L/del, and NF-L/c-myc cDNAs was compared by inducing transgene expression for 72 hrin the absence of tetracycline and then measuring mRNA levelsat varying time points after the readdition of the ligand. Figure6a shows a representative RNA protection assay of NF-L mRNA (solidarrow) and $beta$ -actin mRNA (open arrow), whereas Figure 6b showsthe average decline of NF-L/ $beta$ -actin mRNA levels from four experiments.The NF-L transcript is stabilized either by deleting the entirebinding site of the stability determinant (NF-L/del) or by insertinga c-myc tag between the 3'-CR and 3'-UTR components of the bindingsite (NF-L/c-myc). The insertion of the c-myc tag is almost aseffective as the full deletion in disrupting the function of thedeterminant.

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Figure 6. Protection assay (a) and quantitation (b) of NF-L and $beta$ -actin mRNA levels in Neuro 2a cells doubly transfected with tTA transactivator expression vector and target gene in which a Tn-10 tetracycline-inducible promoter drives the expression of wild-type (NF-L/wt) or mutant (NF-L/del and NF-L/c-myc) NF-L cDNA. The mutant transgenes either were deleted of 23 bp of distal coding region and 45 bp of proximal 3'-UTR (NF-L/del) or had a 36 bp c-myc insert and stop codon appended to the end of the coding region (NF-L/c-myc). The NF-L target genes were activated for 72 hr by withdrawal of tetracycline and then inactivated by the readdition of 0.5 µg/ml tetracycline (0 time point). An RNA protection assay detected radioactive fragments of 125 nt (filled arrow) and 83 nt (open arrow) from NF-L and $beta$ -actin mRNAs. NF-L/ $beta$ -actin mRNA levels were averaged from three experiments. c, mRNA levels from mutant NF-L cDNAs with 36 bp c-myc mutation in the BglII site of exon 1 (NF-L/c-myc/BglII), in the EcoRI sites of the distal 3'-UTR (NF-L/c-myc/EcoRI), and at the end of the coding region (NF-L/c-myc). Mutant and wild-type NF-L cDNAs with tetracycline-inducible promoters were cotransfected in Neuro 2a cells, and mRNA levels were assayed by RT-PCR at 0, 24, and 48 hr after inactivation of transcription by the addition of tetracycline. Levels of mRNA from the mutant NF-L cDNAs are expressed as the percentage of mRNA level from the cotransfected wild-type NF-L cDNA.

The ability of the c-myc insert to alter mRNA stability is attributable to its placement in the stability determinant

To test whether the effect of the 36 bp c-myc insert was attributable to the c-myc sequence per se or to the context of itsplacement in the stability determinant, we assessed the stabilityof NF-L mRNAs when the c-myc insert was placed in exon 1 (NF-L/c-myc/BglII)or in the distal 3'-UTR (NF-L/c-myc/EcoRI). In both instances,the presence of the c-myc insert did not alter the stability ofthe transcript (Fig. 6c). As expected, the stability of the NF-Ltranscript was enhanced when the c-myc tag was inserted into thestability determinant (NF-L/c-myc).

The findings indicate that insertion of the c-myc tag into the stability determinant of the NF-L mRNA alters the stabilityof the transcript and that the altered function of the stabilitydeterminant is not attributable to the presence of the c-myc sequencebut to the placement of the c-myc tag within the stability determinant.In further support of this interpretation, we find that the 36bp c-myc tag in exon 1 does not gel shift an RNP complex (datanot shown) but that placement of the c-myc tag at the end of thecoding region alters the RNP complexes that form on the majorstability determinant of the transcript (seebelow).

Insertion of the c-myc tag alters the RNP complexes that bind to the major stability determinant at the junction of the coding region and 3'-UTR of the NF-L transcript

To test whether insertion of a 36 nucleotide (nt) c-myc tag at the junction of coding region and 3'-UTR of NF-L alters thebinding of RNP complexes to this site, we undertook gel-shiftand cross-linking assays to compare the complexes that form whenbrain extracts are incubated with probes of wild-type and mutantsequence (Fig. 7). The RNP complexes that assemble on an RNA probecomposed of the 23 nt of 3'-CR and the 45 nt of proximal 3'-UTR(Fig. 7a, lane 2) consist primarily of a set of bands (solid arrows)that is competed away by poly(C) homoribopolymers (lanes 4, 5),enhanced in the presence of poly(U) (lane 3), and is referredto as the C-binding complex (Cañete-Soler et al., 1998b). A similarC-binding complex with a slightly different pattern of electrophoreticmigration forms on the probe with a c-myc tag insert between the3'-CR and 3'-UTR (lane 6). Although the C-binding complex on themutant probe also is competed with poly(C) (lanes 8, 9) and enhancedin the presence of poly(U) (lane 7), a large percentage of thecomplex has a slower rate of electrophoretic migration (uppersolid arrow), as if forming a larger aggregate. The formationof an additional slower-migrating component in the C-binding complexon the mutant probe was observed consistently in six gel-shiftassays by using three different preparations of brain extractthat were either freshly prepared or retrieved from storage at $-$ 80°C. Formation of slower- and faster-migrating components ofthe C-binding complex on the mutant probe was observed when gel-shiftassays were conducted with 160, 80, 40, 20, or 10 µg of protein.In all instances, at least 35% of radioactivity of the C-bindingcomplex was present in the slower-migrating band.

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Figure 7. Gel-shift (a) and cross-linking (b, c) assays of RNP complexes that form when brain extracts are incubated with probe A (23 nt of distal coding region and 45 nt of proximal 3'-UTR of NF-L) and probe A/c-myc (same probe with c-myc tag inserted between the coding region and 3'-UTR). Gel-shift assay (a) shows a faster migrating complex (solid arrows) competed by poly(C), enhanced by poly(U), and referred to as the C-binding complex. Whereas the C-binding complex primarily is composed of a single band (lower solid arrow) on probe A (lanes 2, 3), an additional slower migrating band (upper solid arrow) forms on probe A/c-myc (lanes 6, 7). A slower migrating complex (open arrows), referred to as the U/A-binding complex, also forms preferentially on the mutant probe. Cross-linking assay (b, c) shows that radioactivity from probes A and A/c-myc is cross-linked to a major 39 kDa polypeptide (solid arrow) and to a minor 80 kDa polypeptide (open arrow) and that cross-linkage to the 39 and 80 kDa polypeptides is competed by poly(C) and poly(U), respectively. Cross-linkage of radioactivity from probe A to the 39 kDa polypeptide is enhanced in the presence of poly(U) or poly(A⁺) (compare lanes 5 and 6 with lane 2 in Fig. 1c), but not from probe A/c-myc (compare lanes 12 and 13 with lane 9 in Fig. 1c). Likewise, cross-linkage of radioactivity from probe A to the 80 kDa polypeptide is enhanced in the presence of low (+) or high (++) levels of poly(C) (compare lanes 3 and 4 with lane 2), but not from probe A/c-myc (compare lanes 10 and 11 with lane 9). Incubations were conducted with or without extract (160 µg) and at low (20 ng) or high (1 µg) levels of poly(C), poly(U), or poly(A⁺) homoribopolymer competitors. A 5% nondenaturing acrylamide gel was used for the gel-shift assay; 10% PAGE was used for cross-linking studies. Molecular weights were estimated by comigration with prestained standards. Figure 1c is a briefly exposed autoradiogram of cross-linkage in the 39 kDa polypeptide.

Insertion of a c-myc tag between the coding region and 3'-UTR of the NF-L probe also led to an enrichment of a slow migratingset of bands (open arrows) on the mutant probe (lane 6) that iscompeted with poly(U) (lanes 7, 9) and is referred to as the U/A-bindingcomplex (Cañete-Soler et al., 1998b). The U/A-binding complextends to aggregate into a slow-migrating band (upper open arrow)when assembled in the presence of poly(C) (lane 8). Small amountsof the U/A-binding complex also form on the wild-type probe (lanes2, 4), but always at lower levels than amounts that form on themutantprobe.

When the complexes that form on radioactive probes from brain extracts are cross-linked by UV irradiation, digested, and examinedon denaturing SDS gels (Fig. 7b), radioactivity from the wild-type(lane 2) and mutant (lane 9) probes are present in a major 39kDa polypeptide (solid arrow) and a minor 80 kDa polypeptide (openarrow). Because the cross-linking to the 39 kDa polypeptides iscompeted with poly(C) (lanes 3-4, 10-11) and the cross-linkingto the 80 kDa polypeptide is competed with poly(U) (lanes 5, 12),they are interpreted as core-binding components of the C-bindingand U/A-binding complexes, respectively (Cañete-Soler et al.,1998b). Although radioactivities from the wild-type and mutantprobes are cross-linked to the same core-binding polypeptides,there are small differences in the amounts of cross-linked radioactivity,especially when formations of the C- or U/A-binding complexesare competed with poly(C) or poly(U). For example, cross-linkingto the 80 kDa polypeptide is enhanced in the presence of poly(C)when the wild-type probe is used (compare lane 2 with lanes 3and 4), but not when the mutant probe is used (compare lane 9with lanes 10 and 11). Likewise, the addition of poly(U) or poly(A⁺) enhances the cross-linking to the 39 kDa polypeptide from thewild-type probe (compare lane 2 with lanes 5 and 6, Fig. 7c),but not from the mutant probe (compare lane 9 with lanes 12 and13, Fig. 7c). The enhanced cross-linking to core binding polypeptideswhen formations of C- and U/A-binding complexes are competed isa characteristic feature of wild-type probes (Cañete-Soler etal., 1998b). The lack of a corresponding enhancement in the cross-linkingto core binding components from the mutant probe was observedconsistently.

Cross-linkage of radioactivity to the 39 kDa polypeptide from the mutant probe was also less than that from the wild-typeprobe (compare lane 2 with lane 9, Fig. 7c). To determine whetherthe reduction in cross-linkage was attributable to differencesin probe concentration, we conducted cross-linkage studies withincreasing amounts of probes that were diluted to the same specificradioactivities. The results indicate that the c-myc mutationleads to a twofold reduction in cross-linkage to the 39 kDa polypeptideover a wide range of probe concentrations (data notshown).

In summary, gel-shift and cross-linking studies show that very similar C-binding and U/A-binding complexes form on the wild-typeand mutant sequences but that the relative amounts, electrophoreticmigrational rates, and putative interactions of C-binding andU/A-binding RNP components are altered by insertion of the c-myctag. The biochemical alterations produced by the c-myc mutationare not dramatic but are reproducible. They could reflect unknownfacets of the RNP interactions that regulate NF-L mRNA stabilityand mediate the neuropathic effects of the mutanttransgene.

  DISCUSSION

The c-myc mutation in the NF-L transgene produces a novel phenotype

The results of this study show that a 36 bp c-myc insert at the end of the coding region in a NF-L transgene is sufficientto cause profound alterations of the enteric nervous system aswell as vacuolar degeneration of motor neurons in transgenic mice.The phenotype differs from that previously reported from a NF-Ltransgene with the same c-myc mutation and a leucine-to-prolinemutation in the rod domain of the protein (Lee et al., 1994).The differences in phenotype are not trivial and could be attributableto additional or separate effects from the point mutation in thetransgene. It is also possible that varying phenotypes could reflectthe use of different promoters. For example, use of a murine sarcomavirus promoter (Lee et al., 1994) may have favored transgene expressionin motor neurons at levels or developmental periods in which theneurons are particularly susceptible to the adverse effects ofthe transgene. The use of a human CMV promoter in the presentstudy may have generated a different pattern of transgene expression,enhancing transgene expression in enteric neurons and alteringlevels or time course of transgene expression in motor neurons.Levels of transgene expression that were not disruptive to theviability of transgenic pups may have been insufficient to causemore than a transient dysfunction of motor neurons. Alternatively,there may have been diminishing levels of transgene expressionin motor neurons during postnataldevelopment.

Mice bearing the NF-L transgene with only the c-myc mutation also displayed a stunting of growth, as previously reported inmice bearing the mutant (Lee et al., 1994) and wild-type (Xu etal., 1993) NF-L transgene. The occurrence of stunted growth withtransient motor neuron dysfunction indicates that the phenomenondoes not necessarily occur pari passu with progressive motor weaknessand paralysis but reflects a separate effect of mutant transgeneexpression. The transient appearance of stunted growth duringa period of rapid maturation of intestinal function (Traber andSilberg, 1996) raises the possibility that the phenomenon mayrelate to alterations of the enteric nervous system and a temporarydisruption of intestinalfunction.

The neuropathic effects of a NF transgene on the enteric nervous system have not been reported previously. The findings suggestan inherent susceptibility of developing enteric neurons to expressionof the mutant transgene or a disproportional level of transgeneexpression in the enteric nervous system. Because the c-myc mutationstabilizes the NF-L mRNA, variability in the stabilizing processcould lead to disparate levels of transgene expression in differentneuronal tissues at varying stages of development. Replacementof the 3'-UTR of a Hox-1.4 transgene leads to a marked and selectiveincrease of transgene expression in the embryonic gut and to aprofound developmental malformation of the distal colon in transgenicmice (Wolgemuth et al., 1989). It is also possible that the useof a different promoter favors the expression of the mutant NF-Ltransgene in entericneurons.

Vacuolar degeneration of motor neurons is characteristic of other transgenic models of motor neuron degeneration (DalCantoand Gurney, 1995; Wong et al., 1995b) but has not been describedpreviously in mice bearing a NF transgene. It is unclear, however,whether the nature of pathological changes is a reliable measurefor distinguishing transgenic models of motor neuron degeneration.For example, vacuolar changes (DalCanto and Gurney, 1995; Wonget al., 1995b) as well as NF accumulations (Tu et al., 1996) canoccur in the same transgenic model of motor neuron degenerationand may or may not relate to the immediate cause of neuronal degeneration.Moreover, the massive vacuolar degeneration, because of swollenmitochondria, coincides with the onset of neuronal dysfunctionand precedes the loss of motor neurons or their axons (Kong andXu, 1998). A similar pattern of motor neuron pathology could explainthe extensive vacuolar degeneration without apparent loss of motorneurons in newborn mice expressing high levels of a mutant NF-Ltransgene. In the latter instance an assessment of the naturalsequelae of extensive vacuolar degeneration is precluded by thelethal effects of the transgene. The presence of focal vacuolarchanges in motor neurons of asymptomatic founder mice suggeststhat the changes may even be transient and, possibly, reversible.Changes of mitochondrial membrane permeability represent a veryearly stage of apoptosis as well as cell necrosis (see Kroemeret al., 1998) so that vacuolar changes could reflect a very earlypathological alteration to which motor neurons are highlysusceptible.

Alterations in RNA processing are implicated in the pathogenesis of neuronal degeneration

The neuropathic effects of NF transgene have been attributed to alterations at the level of protein expression rather thanto alterations at other levels of transgene expression. This perspectiveis exemplified by the view that neuronal degeneration is secondaryto the disruption of NF assembly, axonal transport, or other cytoskeletalfunction (Collard et al., 1995; Bruijn and Cleveland, 1996). Fromthis perspective the neuropathic effects of the c-myc insert mightbe attributed to the stabilization of NF-L mRNA and the consequentincreased expression of NF-L protein, because increased levelsof NF-L protein are known to have neuropathic effects (Xu et al.,1993). This explanation would require an increased expressionof NF-L protein and could not account for the enhanced neuropathiceffect of a NF-L transgene with the c-myc mutation that occursat reduced levels of NF-L protein (Lee et al., 1994). We werealso unable to detect any increase of transgene expression atthe protein level in vacuolated motor neurons. Moreover, our findingsshow that the neuropathic effects of the c-myc mutation occurduring a perinatal (or prenatal) period in which there is verylimited expression of endogenous NF subunits (Julien et al., 1986;Schlaepfer and Bruce, 1990) and before the establishment of anyknown NF function. It therefore seems unlikely that aberrant expressionof NF-L protein during early neuronal development would have neuropathiceffects because of the disruption of NF or cytoskeletal function.Very high levels of NF-L protein can accumulate in non-neuronal(e.g., skeletal muscle and kidney) tissues of transgenic micewithout apparent pathological effects (Monteiro et al., 1990).Moreover, complete loss of NF-L expression because of ablationof the gene in mice (Zhu et al., 1997) or because of a spontaneousmutation in quail (Yamasaki et al., 1992) does not affect theviability of motor neurons or any other subset ofneurons.

An alternative mechanism for the neuropathic effects of the c-myc mutation is that they are attributable to expression ofthe mutant NF-L mRNA, but not because of the stabilization ofmRNA and increased expression of NF-L protein. Instead, the disruptiveeffects could be attributable to the presence of mutant NF-L mRNAas a substrate for the binding of RNP complexes that mediate post-transcriptionalprocessing of NF-L and other gene products. According to thisview, the addition of exogenous NF-L mRNA serves to titrate oralter the RNP complexes with which they interact. If the sameRNP complexes mediate post-transcriptional processing of NF-Land other neuronal mRNAs, a titration of the RNP complexes couldaffect the expression of the other neuronal gene products adversely.Moreover, if the c-myc mutation alters the binding of RNP complexesto the NF-L mRNA, this alteration could be important in mediatingthe enhanced neuropathic effects or "gain-of-adverse function"that is conferred by the c-myc mutation to the NF-Ltransgene.

Our working hypothesis is that the NF-L transgene, by titrating RNP complexes, disrupts the expression of gene products thatmaintain neuronal homeostasis, such as those that override apoptosis(see Easton et al., 1997). Pathways that override apoptosis areacquired during the same postnatal interval in which there isa marked upregulation of NF mRNAs (Schwartz et al., 1990) becauseof a stabilization of the NF transcripts (Schwartz et al., 1994).The axotomy-induced destabilization of NF mRNAs (Schwartz et al.,1992) indicates that the pathways regulating the stability ofNF transcripts are responsive to disruption of neuronal homeostasisand remain operational in mature neurons. Furthermore, both thepostnatal stabilization and the axotomy-induced destabilizationof the NF-L mRNA are regulated by determinants in the 3'-UTR ofthe NF-L gene (Schwartz et al., 1995). Studies are currently underwayto identify the components of RNP complexes that regulate thestability of the NF-L transcript and to uncover other gene productswith which theyinteract.

The ability of the c-myc mutation to confer a gain-of-adverse function to the mutant NF-L transgene directs attention to thestability determinant as the likely binding site of RNP compleximplicated in the neuropathic effects of the transgene. Furtherimplications of the C-binding complex in the neuropathic effectsderive from the fact that this complex assembles on transcriptsof each NF transgene that has neuropathic effects in transgenicmice. Indeed, the same C-binding complex binds to the stabilitydeterminant of the mouse NF-L mRNA and to the 3'-UTR of the humanNF-H mRNA, but not to the 3'-UTR of mouse NF-M (R. Cañete-Soler,unpublished data). These results could explain the neuropathiceffects that occur from overexpression of the mouse NF-L (Xu etal., 1993) and human NF-H (Cote et al., 1993) transgenes and theapparent lack of neuropathic effects from overexpression of themouse NF-M (Wong et al., 1995a) or mouse NF-H (Marszalek et al.,1996) transgenes. The gain-of-adverse effects imparted by thec-myc mutation suggest that the neuropathic effects may relateto the titration or alteration of component(s) within the C-bindingcomplex rather than to titration of the entirecomplex.

Post-transcriptional regulation is important in determining and maintaining neuronal phenotype

The complexities of neuronal development take place entirely in postmitotic neurons. It therefore follows that developingneurons are deprived of the global reorganization of chromatinthat occurs at cell division and may be limited in their opportunityto regulate gene activity at the level of transcription. Underthese circumstances there may have evolved a greater relianceon post-transcriptional mechanisms for establishing neuronal identityand maintaining their viability among the vast arrays of neuronalsubsets. Strongly conserved families of neuron-specific RNA-bindingproteins have been identified that (1) are expressed sequentiallyduring neuronal differentiation (Wakamatsu and Weston, 1997),(2) are expressed specifically in subsets of neurons (Okano andDarnell, 1997), (3) are required for the development and maintenanceof neurons (Yao et al., 1993), and (4) are implicated in the selectivedegeneration of different neuronal subsets in paraneoplastic neurologicalsyndromes (Szabo et al., 1991; Manley et al., 1995; Darnell, 1996).Although members of the Hu and Elav families bind to AU-rich sequenceof neuronal transcripts (Gao et al., 1994) and participate inthe regulation of splicing (Koushika et al., 1996), mRNA stability(Tsai et al., 1997; Fan and Steitz, 1998; Levy et al., 1998; Penget al., 1998), and translation (Antic and Keene, 1998), thereis limited information as to their role in maintaining neuronalviability (see Yao et al., 1993).

There is, however, evidence that RNA processing is involved in the pathogenesis of neurodegenerative diseases, including motorneuron disease. The mutations responsible for spinal muscularatrophy (Lefebvre et al., 1995, 1997) as well as Fragile X syndrome(Verkerk et al., 1991) occur in genes of RNA-binding proteins(Siomi et al., 1993; Liu and Dreyfuss, 1996). The SMN gene productis part of a large complex involved in spliceosomal snRNP biogenesisand function (Liu et al., 1997). Aberrant splicing of RNA recentlyhas been implicated in sporadic amyotrophic lateral sclerosis,albeit in glial supporting cells (Lin et al., 1998). In myotonicdystrophy, expression of a mutant mRNA leads to abnormal splicingof a wild-type gene product, termed a trans-dominant effect (Philipset al., 1998). In the latter instance, a CUG expansion in the3'-UTR of the mutant protein kinase mRNA increases the bindingof a CUG-binding protein (CUG-BP) and promotes alternative splicingof troponin T RNA. A similar trans-dominant effect of a mutantRNP-binding site could be responsible for the adverse effectsof the c-myc mutation in the NF-L mRNA, as described in thisreport.

The present study is the first direct causal linkage between an alteration in RNA processing and a neurodegenerative statein transgenic mice. A transgenic model thereby is establishedfor probing the aberrant pathways leading to a neurodegenerativephenotype. At the same time, the findings underscore the importanceof post-transcriptional regulation in the pathogenesis of a neurodegenerativestate. Further insights into the post-transcriptional mechanismsunderlying neurodegeneration in transgenic mice undoubtedly willadvance our understanding of neurodegenerativediseases.

  FOOTNOTES

Received Aug. 26, 1998; revised Nov. 23, 1998; accepted Nov. 25, 1998.

This study was supported primarily by National Institutes of Health Grant NS15722. We thank Drs. Michael Schwartz, Peifu He,Jean Richa, Taube Rothman, and Elizabeth Furth for their assistancein generating transgenic mice and assessing the neuropathic effectsof thetransgene.
Correspondence should be addressed to Dr. William W. Schlaepfer, 435 Johnson Pavilion, Division of Neuropathology, Universityof Pennsylvania Medical School, Philadelphia, PA 19104-6079.

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