Postnatal Expression of Hu-Bcl-2 Gene in Lurcher Mutant Mice Fails to Rescue Purkinje Cells but Protects Inferior Olivary Neurons from Target-Related Cell Death

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The Journal of Neuroscience, January 1, 1998, 18(1):319-327

Postnatal Expression of Hu-Bcl-2 Gene in Lurcher Mutant Mice Fails to Rescue Purkinje Cells but Protects Inferior Olivary Neurons from Target-Related Cell Death
H. S. Zanjani¹^,², M. W. Vogel⁴, J. C. Martinou³, N. Delhaye-Bouchaud¹, and J. Mariani¹
¹ Laboratoire de Neurobiologie du Développement, Institut des Neurosciences et Unité de Recherche Associée, Centre National de la Recherche Scientifique 1488, Université Pierre et Marie Curie, 75005 Paris, France, ² Physiological Science Department, University of California at Los Angeles, Los Angeles, California 90095-1527, ³ Geneva Biomedical Research Institute, Glaxo Wellcome Research and Development SA, 1228 Plan-les-Ouates, Geneva, Switzerland, and ⁴ Maryland Psychiatric Research Center, University of Maryland Medical School, Baltimore, Maryland 21228

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The Lurcher mutant has been extensively studied as a model for cell-autonomous and target-related cell death, yet there arestill many unknowns concerning the mechanisms of neuronal degenerationin this mutant. As a key regulator of apoptosis, a bcl-2 transgenehas been overexpressed in the heterozygous Lurcher mutant to investigatethe effects of BCL-2 on two types of in vivo neuronal cell lossin Lurcher: cell-autonomous Purkinje cell degeneration and target-relatedolivary neuron death. Six adult +/Lc mutants expressing a humanbcl-2 transgene (Hu-bcl-2) were generated by crossing +/Lc mutantswith NSE71 Hu-bcl-2 transgenic mice. Analysis of these brainsshowed that bcl-2 overexpression did not prevent +/Lc Purkinjecell degeneration, but it did rescue most olivary neurons fromtarget-related cell death. Although the number of olivary neuronswas equivalent to wild-type numbers, the inferior olive nucleuswas significantly shorter in its rostrocaudal extent, suggestingthat olivary neurons are atrophied. We propose that Lurcher geneaction causes Purkinje cell degeneration independently of a BCL-2-mediatedpathway. Furthermore, although bcl-2 overexpression rescues olivaryneurons from target-related cell death, it does not prevent theatrophy associated with the loss of target-related trophic support.

Key words: olivary neurons; Purkinje cells; BCL-2; Lurcher mutant; programmed cell death; cerebellar mutants

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Many genes have been identified that promote or inhibit cell death pathways, but their relative functions in various typesof programmed and pathological cell death have yet to be established.The purpose of this study is to determine whether one of the keyregulators of apoptotic cell death, BCL-2, can regulate two distincttypes of cell death: cell-autonomous neuronal degeneration andtarget-related cell death as occurs in the heterozygous Lurcher(+/Lc) mutant. Virtually all cerebellar Purkinje cells, 90% ofthe granule cells, and 60-75% of the olivary neurons degeneratepostnatally in the +/Lc mutant (Phillips, 1960; Caddy and Biscoe,1979). Although +/Lc Purkinje cell loss is attributable to a cell-autonomousgenetic defect involving a gain of function mutation in the $delta$ 2glutamate receptor (Zuo et al., 1997), olivary neuron and granulecell death is secondary to the loss of their primary target, thePurkinje cells (Wetts and Herrup, 1982a,b). Many olivary neuronsand granule cells undergo apoptotic cell death when deprived oftheir target (Chu and Oberdick, 1995; Smeyne et al., 1995), butthe mechanisms of Purkinje cell death in the +/Lc mutant havenot yet been characterized definitively. Both necrotic (Dumesnil-Bousezand Sotelo, 1992) and apoptotic (Norman et al., 1995; Wullneret al., 1995) mechanisms have been hypothesized on the basis ofmorphological and molecular criteria.

The bcl-2 proto-oncogene produces an integral membrane protein that inhibits apoptosis in many cell types, including neuronalcell lines after the withdrawal of growth factors (Hockenberryet al., 1990; Garcia et al., 1992; Allsopp et al., 1993; Batistatouet al., 1993). Overexpression of BCL-2 during embryonic or postnataldevelopment in vivo can significantly reduce the extent of naturallyoccurring cell death in a wide variety of neurons (including Purkinjecells and olivary neurons) and can rescue neurons from externalinjuries (e.g., axotomy or ischemia) or genetic lesions (Dubois-Dauphinet al., 1994; Martinou et al., 1994; Farlie et al., 1995; Sagotet al., 1995; Bonfanti et al., 1996; Chen et al., 1996; De Bilbaoand Dubois-Dauphin, 1996; Lawrence et al., 1996; Zanjani et al.,1996, 1997). The purpose of this investigation is to determinewhether overexpression of a human bcl-2 transgene in the Lurchermutant will rescue +/Lc Purkinje cells from their geneticallyprogrammed cell death and olivary neurons from target-relatedcell death. BCL-2 was overexpressed in the Lurcher mutant by crossing+/Lc mutants with a line of transgenics (NSE71) that overexpressesthe human bcl-2 (Hu-bcl-2) proto-oncogene using a neuron-specificenolase promoter (Dubois-Dauphin et al., 1994; Martinou et al.,1994). Hu-bcl-2 expression in NSE71 transgenics begins aroundbirth, and the transgene is expressed in most neurons throughoutthe nervous system, including Purkinje cells and olivary neurons(Dubois-Dauphin et al., 1994; Martinou et al., 1994; Zanjani etal., 1996, 1997). Analysis of Hu-bcl-2-+/Lc mutants shows thattransgene expression fails to prevent +/Lc Purkinje cell degeneration,but does rescue most olivary neurons.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals. Male heterozygous Lurcher mutants (+/Lc) were crossed with female NSE71 transgenics to create +/Lc mutants (and +/+controls) that overexpress the Hu-bcl-2 transgene. The Lurchermutant mice used in this study (genotype, ++/LcMi^wh) were kindly provided by Dr. K. W. Caddy (University CollegeLondon). In this strain the Lurcher gene (Lc) is on a 129 Sv geneticbackground, and it is closely linked to the gene microphthalmiaand white coat color (Mi^wh), with a 10% frequency of crossover (Doughty et al., 1995). +/Lcmutants were distinguished from their +/+ littermates by the presenceof white spots on their coat and their smaller eyes compared withcontrols. NSE71 transgenic mice were provided by Dr. J. C. Martinou(Biomedical Research Institute, Glaxo Wellcome Research and DevelopmentSA) (Dubois-Dauphin et al., 1994; Martinou et al., 1994). Tailsamples from weanling pups were used to identify mice overexpressingthe Hu-bcl-2 transgene using previously described PCR protocols(Martinou et al., 1994, Zanjani et al., 1996). The crossing experimentswere performed in the animal colonies at the Université Pierreet Marie Curie. Mice were provided food and water ad libitum andmaintained on a 12 hr light/dark cycle.

The crossing experiments produced 22 adult animals. Ten of these mice were identified as +/Lc in genotype by the appearanceof white spots at birth and later by their microphthalmia. Allof these mice later showed the ataxia symptoms characteristicof +/Lc mutants. Of the 10 +/Lc mutants, 6 were genotyped as Hu-bcl-2transgenics by PCR. The 12 remaining mice were identified as wildtype at the Lurcher locus, because they did not show the Mi^wh phenotype, and they displayed normal locomotory behaviors. Fiveof these mice tested positive as Hu-bcl-2 transgenics. In additionto the adult mice, two litters of mice were killed at 18 d ofpostnatal development. Based on the same criteria, four of thepups were identified as +/Lc mutants that also expressed the Hu-bcl-2transgene.

Histology. Adult and postnatal day 18 (P18) mice were killed by cardiac perfusion with 4% paraformaldehyde in phosphate buffer(0.1 M) while deeply anesthetized with Avertin. All of the adultmice were between 5 and 6 months old when they were killed. Brainswere post-fixed overnight in the same fixative and then dehydratedthrough graded alcohol series and embedded in paraffin. The cerebellumwas sectioned sagittally, whereas the brain stem was sectionedcoronally, both at 10 µm. Sections were stained with cresyl violet.

Cell counts. Neurons in the inferior olivary nucleus (ION) were counted using previously described techniques (Shojaeian etal., 1985a,b; Zanjani et al., 1990, 1994). In brief, olivary neuronswere counted in each olivary subnuclei on both sides of the brainin every fifth section at 60× with either a Zeiss or Olympus microscope.Only cells with a clear nucleus and a distinct nucleolus or nucleolarfragment were counted. The correction factor of Floderus (1944)was used for correcting olivary neuron double-counting errors.The area and circular diameter of >300 olivary neurons were measuredin each brain to calculate the correction factor for that brain.We chose to use this traditional correction factor for our cellcounts instead of more recently developed stereological techniques(e.g., Williams and Rakic, 1988; Andersen et al., 1992), so thatour results would be directly comparable with previously publishedolivary neuron counts, including our own (Shojaeian et al., 1985a,b;Zanjani et al., 1990, 1994, 1997; Herrup et al., 1996). In additionto the cell counts, in coronal sections of each brain we measuredthe area of olivary neuron cell body profiles (>90 cells measuredper brain) and the rostrocaudal extent of the ION. The rostrocaudalextent of the ION was determined by multiplying the number ofsections in which olivary neurons were identified by the averagethickness of the sections (10 µm). Quantitative data obtainedfrom the two sides of each animal were averaged, and mean valueswere calculated for each group. Statistical comparisons betweenwild-type mice, Hu-bcl-2 transgenics, and Hu-bcl-2-+/Lc mutantswere made using a one-factor ANOVA. Post hoc comparisons weremade using a Bonferroni-Dunn test (StatView 4.5). Measurementsof nucleolar diameter and size of cell body profiles were madeusing a Macintosh IIci computer and the NIH Image program.

Immunocytochemistry. Immunostaining was used to detect expression of the human BCL-2 protein in olivocerebellar neurons. Animalswere anesthetized and perfused intracardially with 4% paraformaldehydein 0.1 M phosphate buffer, pH 7.4. The brain was removed, post-fixedfor 1 hr in the same fixative, and cryoprotected in a 30% sucrose/PBSsolution at 4°C overnight. Brains were cut at 40 µm on a cryostatand collected in PBS. Sections were incubated for 1 hr in normalhorse serum (3%) diluted in PBS containing 0.3% Triton X-100 andthen incubated overnight at 4°C in mouse monoclonal antibody tohuman Bcl-2 (Cambridge Research Biochemicals) diluted in the samebuffer. The primary antibody was revealed using the avidin-biotin-peroxidasetechnique. Calbindin immunostaining in the cerebellum was performedon paraffin sections using an antiserum to calbindin (calbindin-bindingprotein) from Sigma (St. Louis, MO) and visualized using the avidin-biotin-peroxidasetechnique using standard protocols. Color photomicrographs ofimmunolabeled sections were digitized on an Epson ES-1200C scannerand assembled into color plates in Adobe Photoshop. The imageswere contrast-enhanced but otherwise unretouched.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In this study Hu-bcl-2 transgenic mice (line NSE71; Dubois-Dauphin et al., 1994) were crossed with ++/Lc Mi^wh mutants to overexpress the Hu-bcl-2 transgene in +/Lc Purkinjecells and olivary neurons. In the ++/Lc Mi^wh mutant strain, the Lurcher gene is closely linked to microphthalmic-white.The microphthalmic-white mutation causes a white coat spot inneonates and a microphthalmia that can be recognized within afew weeks. Both phenotypes were used to identify +/Lc mutants.Six adult mice (Hu-bcl-2-+/Lc mutants) were prospectively identifiedas +/Lc mutants that overexpress Hu-bcl-2 on the basis of a whitecoat spot, indicating linkage to Lurcher and by PCR for Hu-bcl-2expression. In retrospect, the +/Lc genotype of the animals wasconfirmed histologically, because virtually all of the Purkinjecells degenerated in these mice.

Qualitative observations

Cerebellum
The foliation and laminar organization of the cerebellum in wild-type and Hu-bcl-2 transgenic cerebella (Fig. 1A) are similarand well preserved, as described previously (Zanjani et al., 1996).In contrast, the degeneration of +/Lc Purkinje cells during thefirst postnatal month development dramatically alters cerebellarcytoarchitecture in the +/Lc mutant, as revealed by Nissl staining(Fig. 1B). The +/Lc cerebellum is visibly atrophied because ofthe prominent loss of granule cells associated with the disappearanceof their Purkinje cell targets. Overexpression of the Hu-bcl-2gene in the +/Lc mutant mice was clearly insufficient to prevent+/Lc Purkinje cells from degenerating; the cerebella of the Hu-bcl-2-+/Lcmutants (Fig. 1C) were similar in size to those of +/Lc mutants(Fig. 1B). Cerebellar atrophy was already apparent in the mutantswhen their brains were removed under a dissecting microscope (resultsnot shown). Examination of serial sections at the light microscopelevel showed that +/Lc Purkinje cell somas had virtually disappearedfrom the Hu-bcl-2-+/Lc cerebellum, and the number of cerebellargranule cells was also dramatically reduced. The Hu-bcl-2 transgeneis not expressed in cerebellar granule cells, so their loss isconsistent with the loss of their Purkinje cell targets.

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Figure 1. Photomicrographs of midsagittal sections of cerebella from a wild-type mouse (A), a +/Lc mutant (B), and an Hu-bcl-2-+/Lcmutant (C) stained with cresyl violet. The low-power photographson the left show the folial organization of each cerebellum, andthe higher-magnification insets on the right illustrate the cytoarchitectureof each type of animal. Both the +/Lc and the Hu-bcl-2-+/Lc mutantsare characterized by a conspicuous reduction in cerebellar sizeattributable to the loss of almost all Purkinje cells and mostgranule cells. Scale bars: low-magnification photographs, 500µm; high-magnification photographs, 20 µm.

To verify the virtually complete degeneration of Purkinje cells in Hu-bcl-2-+/Lc-mutants, cerebellar sections were stainedwith a monoclonal antibody against calbindin. Calbindin is heavilyexpressed in Purkinje cell bodies and dendrites in wild-type animals(Fig. 2A) and NSE71 Hu-bcl-2 transgenic mice (Fig. 2B), makingit easy to identify Purkinje cells. Only a very few Purkinje cellswith small cell bodies and poorly developed dendrites are detectedin the Hu-bcl-2-+/Lc mutant with anti-calbindin antibody labeling(Fig. 2C). The number, abnormal shape, and location (mostly inthe nodulus) of +/Lc Purkinje cells in the Hu-bcl-2-+/Lc mutant(Fig. 2D) were indistinguishable from those of the rare Purkinjecells detected in the +/Lc mutant cerebellum. Immunolabeling forhuman BCL-2 protein was detected in the olivary neurons of bothHu-bcl-2 transgenic mice (Fig. 2E) and Hu-bcl-2-+/Lc mutants (Fig.2F). Human BCL-2 labeling in the Hu-bcl-2-+/Lc mutants is notas robust as in the Hu-bcl-2 transgenics, but immunostained olivaryneurons are apparent throughout the ION in the Hu-bcl-2-+/Lc mutants,as shown in the lower-magnification photomicrograph in Figure2F (arrows indicate individual neurons). Figure 2F, inset, showshuman BCL-2 immunolabeling in Hu-bcl-2-+/Lc mutant olivary neuronsat a higher magnification.

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Figure 2. Immunostaining for calbindin or human BCL-2 antigen in the olivocerebellar system of wild-type, transgenic, and mutant mice.A, B, Photomicrographs show the selective labeling of all Purkinjecell somas and dendrites by anti-calbindin antibodies in wild-type(A) and Hu-bcl-2 transgenic (B) mice. A few Purkinje cells areindicated by arrows. In contrast, only a few Purkinje cells immunopositivefor calbindin (arrows) survive in +/Lc (C) and Hu-bcl-2-+/Lc mutant(D) cerebella, primarily in the nodulus lobule. E, F, Photomicrographsillustrate immunolabeling for the human BCL-2 protein in inferiorolivary neurons in coronal sections at low magnification of anadult Hu-bcl-2 transgenic (E) and an adult Hu-bcl-2-+/Lc mutant(F). Inset in F, Anti-human BCL-2-labeled olivary neurons at ahigher magnification. Immunopositive olivary neurons are indicatedby small arrows.

In addition to looking for calbindin-stained +/Lc Purkinje cells and BCL-2-labeled olivary neurons in Hu-bcl-2-+/Lc adults,four Hu-bcl-2-+/Lc mutants were killed during the period of +/LcPurkinje cell death (P18) to look for human BCL-2 expression in+/Lc Purkinje cells before their degeneration. Selected sectionswere stained with antibodies to human BCL-2, and positive stainingshowed that the Hu-bcl-2 transgene is expressed in +/Lc Purkinjecells before they degenerate (Fig. 3). Human BCL-2 immunoreactivityis concentrated in the molecular layer and Purkinje cell layer,as shown in a low-power photomicrograph of a posterior lobuleof a P18 Hu-bcl-2-+/Lc mutant (Fig. 3A). Human BCL-2 immunoreactivityin the transgenics is not as robust as the Golgi-like calbindinlabeling (compare Figs. 2A,B, 3), but labeled Purkinje cells areapparent. Most +/Lc Purkinje cells at P18 have abnormal dendritictrees, and in the Hu-bcl-2-+/Lc mutants their cell bodies anddendrites are filled with BCL-2 protein, as shown by human BCL-2immunoreactivity in a higher-power photomicrograph from an anteriorlobule (Fig. 3B, arrows). The Purkinje cells shown in Figure 3Bare located in an anterior lobule, so they are destined to die;all Purkinje cells in anterior lobules will have degenerated by5 months postnatally, the age when the adult mutants were analyzed.

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Figure 3. Immunostaining for human BCL-2 antigen in the cerebellum of a P18 +/Lc-Hu-bcl-2 mutant mice. Immunoreactivity is confinedlargely to the molecular and Purkinje cell layers, as shown inthe photomicrograph of a posterior lobule of the +/Lc-Hu-bcl-2mutant (A). At a higher magnification (B), individual +/Lc Purkinjecells can be seen with stunted dendritic trees. B, The photomicrographis taken from an anterior lobule, so these BCL-2-immunostained+/Lc Purkinje cells are destined to die. Scale bars: A, 100 µm;B, 50 µm.

Inferior olive
Overexpression of the Hu-bcl-2 transgene in NSE71 mice increases the number of olivary neurons but does not appreciably alterthe cytoarchitecture of the inferior olive subnuclei (Fig. 4A)(Zanjani et al., 1997). As shown in a coronal section in Figure4A, the four main subnuclei of the inferior olive, medial accessoryolive, the dorsal accessory olive, the principal olive, and thedorsomedial cellular column are clearly delineated in NSE71 transgenics.In contrast, there is relatively poor definition of the subnucleiof the inferior olive in the adult Lurcher mutant (Fig. 4B) comparedwith wild-type or Hu-bcl-2 transgenics. Overexpression of theHu-bcl-2 transgene restores the anatomy and cytoarchitecture ofthe inferior olive subnuclei in Hu-bcl-2-+/Lc transgenic mice(Fig. 4C). The distribution of olivary subnuclei is almost identicalto that in Hu-bcl-2 transgenic (Fig. 4A) or wild-type littermates(data not shown). At a higher magnification, there are no distinctmorphological differences in the appearance of olivary cells inHu-bcl-2 transgenics, +/Lc mutants, and Hu-bcl-2-+/Lc mutants(Fig. 4A-C, insets), although the cell bodies of olivary neuronsin the +/Lc and Hu-bcl-2-+/Lc mutants are slightly smaller comparedwith Hu-bcl-2 transgenics (see next section).

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Figure 4. Coronal sections through the inferior olivary complex of an Hu-bcl-2 transgenic (A), a +/Lc mutant (B), and an Hu-bcl-2-+/Lcmutant (C). Distinct subnuclei are apparent in the organizationof the inferior olivary complex in both the Hu-bcl-2 transgenicand the Hu-bcl-2-+/Lc mutant. In contrast, the inferior olivarynucleus appears atrophic in the +/Lc mutant (B). The insets showthe somas of olivary neurons at higher magnification (arrows);olivary neuron cell bodies appear shrunken in the +/Lc and Hu-bcl-2-+/Lcmutants compared with controls. MAO, Medial accessory olive; DAO,dorsal accessory olive; PO, principal olive; dmcc, dorsomedialcell column. Scale bars: low-power photomicrographs, 200 µm; insets,40 µm.

Quantitative descriptions

Visual inspection of sections from Hu-bcl-2-+/Lc mutants demonstrated that overexpression of the Hu-bcl-2 transgene in +/Lcmutant mice does not prevent Purkinje cell degeneration, but itdoes rescue most olivary neurons from target-related cell death.To quantitate the amount of olivary neuron rescue in Hu-bcl-2-+/Lcmutants compared with NSE71 transgenics, wild-type mice, and +/Lcmutants, we counted the mean number of olivary neurons per hemispherein a subsample of animals from all four groups of mice. To comparethe anatomy of the inferior olive nucleus among the four groups,we calculated the rostrocaudal extent of the inferior olive andmeasured the area of olivary neuron cell body profiles in thesame coronal sections that were used for the cell counts.

Confirming the qualitative observations, the mean number of olivary neurons per hemicerebellum in the Hu-bcl-2-+/Lc mutants(Table 1, Fig. 4) is indistinguishable from the number of olivaryneurons in wild-type controls and increased by 166% relative toolivary neuron numbers in +/Lc mutant mice. Somewhat surprisingly,olivary neuron numbers in the Hu-bcl-2-+/Lc mutants are 20% lowerthan the number of olivary neurons in NSE71 Hu-bcl-2 transgenicmice. The mean differences between olivary neuron cell countsin Hu-bcl-2-+/Lc mutants, Hu-bcl-2 transgenics, and +/Lc mutantsare highly significant (ANOVA, F_(3,10) = 115.012; p < 0.001).Olivary neuron counts are significantly higher in Hu-bcl-2-+/Lcmutants compared with +/Lc mutants (Bonferroni-Dunn post hoc test,p < 0.0001) but significantly lower compared with Hu-bcl-2 transgenics(Bonferroni-Dunn post hoc test, p < 0.0005).


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Table 1. Corrected numbers for inferior olivary neurons per hemicerebellum, the mean rostrocaudal extent of the inferior olive nuclei,and the mean area and long diameter of olivary neuron cell bodyprofiles for wild-type, NSE 71 Hu-bcl-2 transgenic, Hu-bcl-2-+/Lcmutant, and +/Lc mutant mice

Although olivary neurons numbers are comparable in wild-type and Hu-bcl-2-+/Lc mutants, quantitative analysis of the rostrocaudalextent of the inferior olive suggests that the region is atrophiedin Hu-bcl-2-+/Lc mutants. The rostrocaudal length of the olivenucleus is significantly shorter in Hu-bcl-2-+/Lc mutant micecompared with Hu-bcl-2 transgenics and wild-type mice (Table 1,Fig. 4B) (ANOVA, F_(3,10) = 37.074; p < 0.0001). The mean rostrocaudalextent is significantly reduced by >30% in the Hu-bcl-2-+/Lc mutantscompared with both Hu-bcl-2 transgenics and wild-type mice (Bonferroni-Dunnpost hoc test, p < 0.0001). Furthermore, despite the 166% increasein the number of olivary neurons in Hu-bcl-2-+/Lc mutants comparedwith +/Lc mutants, there are no significant differences betweenthe rostrocaudal extent of the inferior olive in the two mutantgroups (Bonferroni-Dunn post hoc test, p > 0.1).

The decrease in the rostrocaudal extent of the inferior olive nucleus in Hu-bcl-2-+/Lc mutants and +/Lc mutants may reflectdecreases in cell body size and/or neuropil volume. As a firstapproximation of cell body size, we measured the area of olivaryneuron cell body profiles in coronal sections and found significantdifferences between Hu-bcl-2 transgenics and Hu-bcl-2-+/Lc mutants,+/Lc mutants, and wild-type mice (Table 1, Fig. 5) (ANOVA, F_(3,9)= 31.5; p < 0.0001). The average area of olivary neuron cell bodyprofiles in Hu-bcl-2-+/Lc and +/Lc mutants is decreased comparedwith wild-type values by 12 and 19%, respectively; however, thedifferences only approach significance for the +/Lc mutant data(p = 0.068). In contrast, average olivary neuron profile areasare >50% higher in Hu-bcl-2 transgenics compared with all othergroups (Bonferroni-Dunn post hoc test, p < 0.001).

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Figure 5. Quantitative analysis of inferior olive numbers and size in wild-type mice (black bars), Hu-bcl-2 transgenics (striped bars),NSe71-+/Lc mutants (gray bars), and +/Lc mutants (cross-hatchedbars). Values are expressed as percentage of wild-type valuesfor the number of olivary neurons, rostrocaudal extent of theinferior olive, and inferior olive cell body profile area. Resultsthat are significantly different from wild-type values are indicatedby asterisks (Bonferroni-Dunn post hoc test, p < 0.0083).

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The results of this study demonstrate that overexpression of BCL-2 in the +/Lc mutant does not prevent Purkinje cell death,but it does rescue most olivary neurons. The simplest explanationfor these results is that +/Lc Purkinje and olivary neuron celldeath is mediated by two distinct BCL-2-independent and BCL-2-dependentpathways. The implications of these results for deciphering themechanisms of +/Lc Purkinje cell death and olivary neuron deathare discussed in turn.

+/Lc Purkinje cell death

Cell-autonomous neuronal degeneration in the Lurcher mutant is apparently caused by a gain of function mutation in the $delta$ 2glutamate receptor (GluR) subunit that results in a large, constitutiveinward current in the cells that express the subunit (Zuo et al.,1997). The GluR $delta$ 2 subunit is preferentially expressed in cerebellarPurkinje cells (Takayama et al., 1996) and perhaps in selectedhindbrain regions, because there is massive cellular degenerationin these regions in homozygous Lurcher mutant embryos (Cheng andHeintz, 1997; Resibois et al., 1997). The timing of +/Lc Purkinjecell death coincides with the translocation of GluR $delta$ 2 immunoreactivityfrom Purkinje cell dendritic shafts to dendritic spines, especiallyto the postsynaptic membrane (Takayama et al., 1996). In the Lurcherheterozygote, Purkinje cells undergo cell-autonomous degeneration,whereas olivary neuron and granule cell death is secondary toPurkinje cell loss (Wetts and Herrup, 1982a,b). Neuronal degenerationcaused directly by the leaky GluR $delta$ 2 subunit is presumably attributableto the induction of excitotoxic mechanisms, and Purkinje cellsmust be especially sensitive to this mutation in the heterozygote(Zuo et al., 1997). The available evidence suggests that +/LcPurkinje cells may die by an excitotoxic mechanism induced bythe accumulation of leaky GluR $delta$ 2 subunits at developing Purkinjecell $right-arrow$ parallel fiber synapses (Zuo et al., 1997). This hypothesisis consistent with previous studies showing that +/Lc Purkinjecells must differentiate before they degenerate (Wuenschell etal., 1990; Messer et al., 1991; Norman et al., 1995). The rescueof +/Lc Purkinje cells in a homozygous staggerer background (Messeret al., 1991), for example, could be attributable to a block inthe developmental expression of the GluR $delta$ 2 receptor.

Although +/Lc Purkinje cells are likely to be dying by a mechanism that is initiated by an excitotoxic lesion, the sequenceof molecular events leading to +/Lc Purkinje cell death stillremains to be determined. Dumesnil-Bousez and Sotelo (1992) argueon morphological criteria that +/Lc Purkinje cells degenerateby a necrotic process; however, fragmented DNA can be detectedin degenerating +/Lc Purkinje cells, suggesting that +/Lc Purkinjecells may degenerate by an apoptotic mechanism (Norman et al.,1995; Wullner et al., 1995). Our results suggest that whatevermechanisms are involved, the overexpression of bcl-2 in the +/LcPurkinje cells is not sufficient to prevent their degeneration.Positive BCL-2 immunolabeling in the P18 +/Lc-Bcl-2 mutant showsthat the human bcl-2 transgene is present in +/Lc Purkinje cellsbefore their death, so their degeneration is not attributableto a failure of transgene expression in the afflicted cells. Ectopicexpression of BCL-2 has been shown to prevent excitotoxic lesionsin other systems (Lawrence et al., 1996). BCL-2 is not normallyexpressed in adult Purkinje cells (Castren et al., 1994), butit appears to be expressed in Purkinje cells during early embryonicand postnatal development, so it may play a role in regulatingPurkinje cell survival early in development (Merry et al., 1994).BCL-2 overexpression, for example, may rescue Purkinje cells fromnaturally occurring cell death (Zanjani et al., 1996). It is notclear why BCL-2 overexpression fails to rescue +/Lc Purkinje cells(Zhong et al., 1993a,b; Jia et al., 1996; Lawrence et al., 1996).A likely explanation is that the aberrant ion current inducedby the mutant GluR $delta$ 2 receptor induces a cell death pathway thatis independent of or downstream from BCL-2 regulation. Both bcl-2-dependentand -independent cell death pathways have been described in otherneurons (Allsopp et al., 1993, 1995; Coulpier et al., 1996). Forexample, in the +/Lc mutant, the ICE-like proteases that executeneuronal cell death programs (Martinou and Sadoul, 1996; Schwartzand Milligan, 1996) may be activated directly in chronically depolarized+/Lc Purkinje cells.

+/Lc olivary neuron cell death

In the olivocerebellar system, surgical and genetic lesions have shown that the survival of olivary neurons and granule cellsis dependent on interactions with their Purkinje cell targets(Harkmark, 1956; Sotelo and Changeux, 1974; Caddy and Biscoe,1979; Wetts and Herrup, 1982a,b; Zanjani et al., 1990; Vogel etal., 1991; Herrup et al., 1996). The hypothesis for target-relatedcell death is well established; if target cells are removed duringa critical period during development, the afferent neurons willundergo retrograde cell death (Oppenheim, 1991). We have shownpreviously that overexpression of the Hu-bcl-2 transgene rescuesolivary neurons from naturally occurring cell death (Zanjani etal., 1997). In this study, we show that overexpression of Hu-bcl-2in the +/Lc mutant rescues most olivary neurons from target-relatedcell death. This result is consistent with previous studies showingin vitro rescue of neurons from trophic factor withdrawal (Garciaet al., 1992; Allsopp et al., 1993; Batistatou et al., 1993) andin vivo rescue of neurons from axotomy or ischemia by bcl-2 overexpression(Dubois-Dauphin et al., 1994; Martinou et al., 1994; Farlie etal., 1995; Bonfanti et al., 1996; De Bilbao and Dubois-Dauphin,1996). A surprising result, however, is that the number of olivaryneurons in the NSE71 line of Hu-bcl-2 transgenics is increasedby 26% compared with Hu-bcl-2-+/Lc mutant mice. This disparityin survival suggests either that the transgene is not expressedequally in all ION neurons or that not all olivary neurons canbe rescued by BCL-2 overexpression. There is indirect evidencethat olivary neurons may die by different mechanisms after targetremoval. Degenerating olivary neurons in the caudal olive canbe detected with terminal deoxynucleotidyl transferase-mediateddUTP-biotin nick end-labeling (TUNEL) labeling at P4 in transgenicmice with neonatal Purkinje cell death (Chu and Oberdick, 1995).However, TUNEL-positive olivary neurons are not detected afterP7, although olivary neuron cell death appears to proceed at leastthrough P15. However, it is not yet apparent why olivary neuronsmay die by different mechanisms after target removal and/or destruction.

Despite the increase in the number of olivary neurons to wild-type levels in Hu-bcl-2-+/Lc mutants, the inferior olive complexappears atrophic. The rostrocaudal extent of the inferior olivein Hu-bcl-2-+/Lc mutants is significantly reduced just as in the+/Lc mutant, and there is a trend toward smaller average cellbody profile areas in coronal sections of Hu-bcl-2-+/Lc and +/Lcmutants. The rostrocaudal extent of the inferior olive and olivaryneuron cell body size are similarly reduced in the staggerer mutant,suggesting that olivary neurons atrophy in the absence of theirPurkinje cell targets (Zanjani et al., 1994). One class of olivaryneurons with large, simple, and unramified dendrites may be predominantlylost in both mutants (Caddy and Biscoe, 1979; Zanjani et al.,1994). Although the loss of this cell type could account for thesmaller olive in the sg/sg and +/Lc mutants, it is likely thatthese cells are rescued in Hu-bcl-2-+/Lc mutants, and there isa general reduction in the size of olivary neurons and the olivaryneuropil in the Hu-bcl-2-+/Lc mutants as a consequence of Purkinjecell loss.

The atrophy of inferior olive neurons rescued by Hu-bcl-2 overexpression supports a hypothesis for BCL-2-mediated rescue ofolivary neurons from trophic factor deprivation after Purkinjecell degeneration. In vitro and in vivo experiments suggest thatthe survival functions of BCL-2 can be separated from growth-promotingactivities. Sympathetic neurons transfected with bcl-2 in vitroand deprived of growth factors will survive, but they suffer thesame decrease in protein synthesis rates after NGF withdrawalas wild-type cells (Greenlund et al., 1995). BAX^/ neurons also survive trophic factor withdrawal in vitro or afterin vivo axotomy, but their cell bodies are atrophied (Deckwerthet al., 1996). In contrast, motoneurons rescued with exogenousglial cell line-derived neurotrophic factor, brain-derived neurotrophicfactor, neurotrophin 3, and insulin-like growth factor 1 appearnormal in size, indicating that the neurotrophic factors can preventthe atrophy associated with axotomy (Li et al., 1994; Oppenheimet al., 1995; Yan et al., 1995) (but see Yan et al., 1993). Theimplication is that although bcl-2 expression (or the lack ofBAX) can block the cell death pathway in models of target-relatedcell death, the lack of appropriate trophic factors prevents therescued cells from growing normally. Conversely, the profilesof inferior olive neurons in the Hu-bcl-2 transgenics are significantlyincreased above wild-type values. It seems unlikely that the increaseis a direct effect of Hu-bcl-2 transgene expression on olivaryneurons, because olivary neurons in the Hu-bcl-2-+/Lc mutantsare not similarly affected. Instead, the increase in olivary cellbody size in Hu-bcl-2 transgenics may reflect a hypertrophy attributableto increased target-derived trophic support from the increasednumbers of Purkinje cells in the transgenics. These results illustratethe key roles neurotrophic factors play in supporting neuronalsurvival and growth.

  FOOTNOTES

Received May 21, 1997; revised Oct. 17, 1997; accepted Oct. 22, 1997.

This work was supported by Grants given to J.M. from Fondation de la Recherche Médicale Grant "vieillissement" to J.M., agrant from Fondation de France AFM to J.M., European CommunityBiotech Grant BIO4CT96 0774 to J.M. and J.C.M., and National Institutesof Health Grants NS 29277 and NS 34309 and a Special ResearchInitiative Support University of Maryland Medical School grantto M.W.V. We thank Ms. P. Bouquet for technical assistance andMs. Sharon Candeloro for editorial assistance.
Correspondence should be addressed to Dr. Michael W. Vogel, Maryland Psychiatric Research Center, University of Maryland MedicalSchool, P.O. Box 21247, Baltimore, MD 21228.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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