Published online before print January 17, 2008

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(American Journal of Pathology. 2008;172:406-416.)
© 2008 American Society for Investigative Pathology
DOI: 10.2353/ajpath.2008.070823

Disrupted Membrane Homeostasis and Accumulation of Ubiquitinated Proteins in a Mouse Model of Infantile Neuroaxonal Dystrophy Caused by PLA2G6 Mutations

Ibrahim Malik^*, John Turk, David J. Mancuso, Laura Montier^*, Mary Wohltmann, David F. Wozniak^¶, Robert E. Schmidt^¶||, Richard W. Gross^** and Paul T. Kotzbauer^*¶**

From the Department of Neurology,^*the Divisions of Endocrinology, Metabolism, and Lipid Researchand Bioorganic Chemistry and Molecular Pharmacologyin the Department of Medicine, the Departments of Psychiatryand Pathology and Immunology,||Hope Center for Neurological Disorders,^¶and the Department of Molecular Biology and Pharmacology,^**Washington University School of Medicine, St. Louis; and the Department of Chemistry,Washington University, St. Louis, Missouri

	Abstract

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Mutations in the PLA2G6 gene, which encodes group VIA calcium-independent phospholipase A2 (iPLA₂β), were recently identified in patients with infantile neuroaxonal dystrophy (INAD) and neurodegeneration with brain iron accumulation. A pathological hallmark of these childhood neurodegenerative diseases is the presence of distinctive spheroids in distal axons that contain accumulated membranes. We used iPLA₂β-KO mice generated by homologous recombination to investigate neurodegenerative consequences of PLA2G6 mutations. iPLA₂β-KO mice developed age-dependent neurological impairment that was evident in rotarod, balance, and climbing tests by 13 months of age. The primary abnormality underlying this neurological impairment was the formation of spheroids containing tubulovesicular membranes remarkably similar to human INAD. Spheroids were strongly labeled with anti-ubiquitin antibodies. Accumulation of ubiquitinated protein in spheroids was evident in some brain regions as early as 4 months of age, and the onset of motor impairment correlated with a dramatic increase in ubiquitin-positive spheroids throughout the neuropil in nearly all brain regions. Furthermore accumulating ubiquitinated proteins were observed primarily in insoluble fractions of brain tissue, implicating protein aggregation in this pathogenic process. These results indicate that loss of iPLA₂β causes age-dependent impairment of axonal membrane homeostasis and protein degradation pathways, leading to age-dependent neurological impairment. iPLA₂β-KO mice will be useful for further studies of pathogenesis and experimental interventions in INAD and neurodegeneration with brain iron accumulation.

Many cases of INAD are also characterized by iron deposition in the globus pallidus and substantia nigra pars reticulata, indicating significant overlap with the spectrum of diseases classified as neurodegeneration with brain iron accumulation (NBIA). NBIA currently includes the genetic disorder pantothenate kinase-associated neurodegeneration and possibly other genetic and sporadic etiologies that have not yet been identified.

Morgan and colleagues⁸ recently reported genetic mapping in four families with INAD and NBIA and the subsequent identification of a total of 44 unique PLA2G6 mutations in patients with either INAD or NBIA. Mutations were present in both alleles in all but one patient. In a few cases, both alleles were affected by early frame shift and stop codon mutations and predicted to cause complete loss of iPLA₂β function, but there were also 32 missense mutations causing single amino acid substitutions.⁸ PLA2G6 mutations have also been independently identified in two additional INAD families.⁹

PLA2G6 encodes the calcium-independent phospholipase A₂ β (iPLA2β) enzyme, also designated iPLA₂-VIA, which hydrolyzes the sn-2 ester bond in phospholipids to release a free fatty acid and a 2-lysophospholipid.¹⁰ Mice deficient in iPLA₂β were originally generated and described by Bao and colleagues.¹¹ iPLA₂β knockout (iPLA₂β-KO) mice are born with an expected Mendelian distribution and appear to grow and develop normally. Male iPLA₂β-KO mice have greatly reduced fertility because of impaired function of spermatozoa.¹¹ Pancreatic islet β-cell function in iPLA₂β-KO mice is impaired under conditions of metabolic stress, such as administration of multiple low doses of the β-cell toxin streptozotocin or prolonged feeding of a high-fat diet, although blood insulin and glucose levels are appropriately regulated under normal circumstances.¹²

The recent reports of iPLA₂β mutations underlying INAD and NBIA led us to investigate the possibility that iPLA₂β-null mice might recapitulate the neurodegenerative features of human INAD. We report here that iPLA₂β-KO mice develop progressive age-dependent impairment of sensorimotor function that is accompanied by progressive accumulation of tubulovesicular membranes and ubiquitinated protein in spheroids throughout the brain. These findings demonstrate that iPLA₂β-KO mice are a valuable model for the neurodegenerative process underlying human INAD and provide further insight into disease pathogenesis.

	Materials and Methods

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Materials

Chemicals were obtained from Sigma (St. Louis, MO) unless otherwise indicated.

Animals

iPLA₂β-KO mice were previously generated by insertion of the neomycin resistance gene into exon 9 of the mouse iPLA₂β gene by homologous recombination.^11,12 iPLA₂β-KO and wild-type (WT) animals were obtained by mating heterozygote animals and genotyping by either Southern blot or polymerase chain reaction assay for the KO allele. Mice were housed and cared for in animal facilities administered through the Washington University Division of Comparative Medicine. All animal procedures were performed according to protocols approved by the Washington University Animal Studies Committee.

Behavioral Tests

Neurological impairment of iPLA₂β-KO mice was assessed in groups of mice at two different ages using tests (a battery of sensorimotor measures, 1-hour locomotor activity, rotarod) that we have previously described and shown to be sensitive for detecting ataxia and other sensorimotor deficits in mutant mice that are associated with altered functions in the cerebellum, striatum, neocortex, and other brain regions.^13,14 The younger group consisted of nine mice of each genotype at 3.5 to 4 months old during testing, and the older group consisted of five mice of each genotype at age 12.5 to 13 months during testing. WT and KO animals were littermates in the 13-month-old group but not in the 4-month-old group.

Tissue Processing

Animals from different age groups ranging from 4 to 13 months were deeply anesthetized by intraperitoneal injection of ketamine/xylazine cocktail and tissues were fixed by intracardiac perfusion with phosphate-buffered saline (PBS) followed by 4% paraformaldehyde. Brain, spinal cord, skin, and muscle were harvested. Tissues were postfixed overnight in 4% paraformaldehyde. Fixed brains were cut into 2- to 3-mm coronal sections before routine paraffin embedding.

Immunohistochemistry

Six µm sections were stained as previously described¹⁵ with the following primary antibodies: mouse monoclonal antibody (mAb) anti-ubiquitin 1510 (1:10,000; Chemicon, Temecula, CA), rabbit polyclonal anti-ubiquitin (1:2000; DAKO, Carpinteria, CA), and anti--synuclein 303 antibody¹⁶ (1:1000, a gift from Dr. Virginia M.-Y. Lee, University of Pennsylvania, Philadelphia, PA). Species-specific biotinylated secondary antibodies were applied followed by avidin-horseradish peroxidase, and the chromogenic substrate diaminobenzidine tetrahydrochloride (Vector Laboratories, Burlingame, CA) was used for detection of horseradish peroxidase. Sections were counterstained with hematoxylin.

Prussian Blue Staining

Brains sections were deparaffinized and incubated in a solution containing equal parts of 2% potassium ferrocyanide and 2% hydrochloric acid for 1 hour at room temperature. The sections were washed and counterstained with nuclear-fast red for 5 minutes.

Quantitation of Ubiquitin-Positive Spheroids

Coronal brain sections of iPLA₂β-KO and WT mice, from three different age groups (4, 8, and 13 months) were immunostained with rabbit polyclonal anti-ubiquitin antibody as above, omitting the final hematoxylin counterstain. Images of the striatum from eight randomly selected fields from each brain region (four fields on each side) were obtained at x40 magnification. Metamorph image analysis software (Molecular Devices, Sunnyvale, CA) was used to analyze each image separately. The images were subtracted for background staining, and all particles (spheroids) staining above background were counted. Average numbers were obtained for KO mice and multiplied by 25 to obtain the mean number of spheroids in the striatum per mm². Spheroid densities for KO mice were reduced by averages obtained for WT mice to control for background values obtained with the image analysis method. Results were graphically displayed with Prism software (Graphpad, San Diego, CA).

Transmission EM

WT and KO mice, 8 months of age, were anesthetized with ketamine/xylazine and brains were removed after intracardiac perfusion with PBS followed by a chilled solution of 3% glutaraldehyde in cacodylate buffer. The tissues were fixed overnight in the same fixative at room temperature. Tissue from each region of interest was dissected into several 1-mm pieces and postfixed in buffered OsO₄, dehydrated in graded alcohol solutions and propylene oxide, and embedded in Epon. One-µm-thick sections were examined by light microscopy after staining with toluidine blue. Thin sections were cut onto formvar-coated slot grids and stained with uranyl acetate and lead citrate and examined with a JEOL (Tokyo, Japan) 1200 electron microscope.

Biochemical Fractionation of Brain Tissue

Mice, 13 months of age, were deeply anesthetized and brains were removed and dissected to obtain samples of frontal cortex plus striatum or striatum alone. Tissue was frozen and then subsequently fractionated using a sequential biochemical extraction method as previously described.¹⁷ Two extractions were performed for each of five extraction solutions by homogenizing with 25 strokes in a Dounce homogenizer. Composition of solutions used for extraction were as previously described¹⁷ and were used in the following volume/tissue weight ratios: high salt (HS) (3 ml/g), HS with 1% Triton X-100 (3 ml/g), RIPA (3 ml/g), 2% sodium dodecyl sulfate (SDS) (1 ml/g), and 70% formic acid (1 ml/g). All buffers except formic acid contained freshly added protease inhibitor cocktail. Equal volumes of each fraction were analyzed by SDS-polyacrylamide gel electrophoresis and Western blotting using rabbit anti-ubiquitin antibody (1:1000, DAKO).

	Results

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Mice that do not express iPLA₂β were previously generated and described by Bao and colleagues.¹¹ The mutant allele, generated by homologous recombination in embryonic stem cells, contains an inserted neomycin resistance gene in exon 9 of the mouse iPLA₂β gene. In mice homozygous for the mutant allele, iPLA₂β mRNA is undetectable in a variety of tissues examined, and iPLA₂β protein is absent in all tissues examined, including brain.¹²

We observed iPLA₂β-KO mice at a variety of ages for evidence of gait difficulty or motor impairment. Although younger KO mice displayed no clear evidence of impairment, abnormalities in gait and movement were consistently observed in KO mice older than 12 months. The gait of older KO mice appeared uncoordinated with increased body sway from side to side. KO mice also appeared to have mild difficulty when rearing and climbing.

Age-Dependent Development of Neurological Impairment in iPLA₂β-KO Mice

We used a number of quantitative behavioral tests to characterize the age-dependent development of neurological impairment in iPLA₂β-KO mice. iPLA₂β-KO mice and WT control mice were evaluated at age 4 and 13 months in the rotarod test using stationary, constantly rotating, and accelerating rotational speed paradigms. In each test paradigm the length of time that mice were able to stay on the rotarod was determined in three successive trials performed 3 days apart.

In studies of 4-month-old mice, WT and KO mice performed similarly, but in 13-month-old mice there was profound impairment of KO mice relative to WT littermate controls in all three paradigms (Figure 1, A–F) . Although 13-month-old iPLA₂β-KO mice exhibited large deficits on the stationary and constant speed conditions, they still showed improved performance across time, indicating some motor learning capabilities during these easier tasks. The KO mice performed most poorly in the accelerating rotarod and did not improve with subsequent trials (Figure 1F) .

View larger version (16K): [in this window] [in a new window]   Figure 1. Age-dependent progression of neurological impairment in iPLA2β-KO mice. Motor coordination and balance were assessed in groups of iPLA2β-KO and WT mice, 4 and 13 months of age, with the rotarod test. A–C: The performance of 4-month-old KO mice was similar to WT mice on the stationary rod (A), the constant speed rotarod (B), and the accelerating rotarod (C) conditions. Although KO mice performed slightly worse during initial trials, no significant differences between the genotypes were observed at age 4 months. In addition, KO mice demonstrated improved performance across trials and test days suggesting motor learning capabilities, and their performance was equivalent to that of WT controls by the end of testing. D–F: In contrast to the 4-month-old KO mice, the performance of 13-month-old KO animals was profoundly impaired in all three rotarod conditions. Although the KO mice exhibited large and significant performance deficits on the stationary rod (D) and constant speed rotarod (E) conditions, they still showed improvement across trials and test days suggesting some motor learning capabilities. The performance of the KO mice was worst on the more challenging accelerating rotarod condition (F) where they showed no significant improvement during training. Asterisks in D–F indicate P values for pairwise comparisons between WT and KO genotypes.

View larger version (14K): [in this window] [in a new window]   Figure 2. Thirteen-month-old iPLA2β-KO mice are impaired in other sensorimotor tests involving balance, motor co-ordination, and strength, and they exhibited increased general locomotor activity. A and B: KO mice were able to remain on a narrow Plexiglas ledge (A) or a small circular platform (B) for significantly less time than WT littermate controls. C and D: KO mice also took significantly longer to turn and climb to the top of a 90° inclined screen (C) compared to WT littermates and were able to stay upside down on an inverted screen for a significantly shorter period of time compared to WT littermate controls (D). E: Although differences were not statistically significant, KO mice appeared to have greater difficulty in climbing down a vertical pole although their performance was highly variable. F: KO mice displayed significantly increased levels of general locomotor activity when total ambulations (whole body movements) were measured for 1 hour. Bars represent mean values and error bars represent SEM. P values are indicated in parentheses above error bars.

Accumulation of Ubiquitinated Protein throughout the Brain in iPLA₂β-KO Mice

To investigate mechanisms of neurodegeneration underlying the age-dependent decline in motor function of iPLA₂β-KO mice, brain tissue from mice 4 to 13 months old was fixed and processed by paraffin embedding for histochemical and immunohistochemical analyses. Routine hematoxylin and eosin (H&E) staining of 6-µm sections revealed no apparent anatomical differences between KO and WT mice. Cortical thickness and cerebellar granular and molecular layer thickness also appeared to be similar in both groups of mice.

Although infrequent eosinophilic spheroids were identified in some brain regions by H&E staining, immunostaining with anti-ubiquitin revealed a much greater number of spheroids throughout many brain regions. Examples of spheroids identified by anti-ubiquitin immunostaining of striatum in 8-month-old mice are shown in Figure 3 . These round, ubiquitin-positive inclusions were present in many different brain regions, and were most abundant in striatum, cerebellum, and dorsal column nuclei at the youngest ages examined. As in human INAD, they were found primarily in the neuropil and often in a juxtaneuronal location, which suggests involvement of distal axons, although it is possible that dendritic processes are also affected.

View larger version (93K): [in this window] [in a new window]   Figure 3. Spheroid formation in the striatum of iPLA2β-KO mice. A: H&E staining of a striatum section from an iPLA2β-KO mouse shows a round eosinophilic inclusion in the neuropil (arrowhead). B and C: Many more spheroids are visualized by immunohistochemistry using an antibody to ubiquitin compared to H&E staining. Comparison of ubiquitin staining in 8-month-old WT (B) and KO (C) mouse brain demonstrates numerous ubiquitin-positive spheroids in the neuropil of KO mice. Spheroids present in KO mouse brain, indicated by arrowheads, exhibit heterogeneous ubiquitin staining and range in size from 1 to 10 µm. Scale bar = 10 µm.

We used transmission EM to investigate the structure of spheroids found in the striatum of iPLA₂β-KO mice at 8 months of age. As shown in Figure 4, A–F , we found numerous spheroids with structural features remarkably similar to those reported in human INAD. Spheroids in iPLA₂β-KO mice were typically found among small diameter axons and terminals in the neuropil and typically lacked a myelin sheath. The core structural appearance was one of accumulating densely compacted tubulovesicular elements, a term used to describe the appearance of an anastomosing network of delicate membrane structures with lumens. An additional consistent feature was the presence of a cleft that interrupted or bordered the tubulovesicular material. Clefts often contained sheets of membranes, sometimes found in stacked or whorled arrangements. These features are remarkably similar to those in human INAD.^1-7 Mitochondria were occasionally observed admixed within the tubulovesicular membranes. Some spheroids also contained separate regions of accumulated protein, mitochondria, and vesicles.

View larger version (208K): [in this window] [in a new window]   Figure 4. Transmission EM reveals tubulovesicular membranes and other material accumulating within spheroids. A–F: Images from transmission EM, performed on sections from striatum of 8-month-old KO and WT mice, illustrate ultrastructural features of spheroids. B, D, and F are higher magnification images of A, C, and E, respectively. Spheroids (asterisks) were typically surrounded by an intact membrane. Common to all spheroids was the presence of accumulating membranes. Tubulovesicular membranes were abundant and interrupted or bordered by clefts containing sheets of membranes, often in stacked or whorled structures. These structural features of spheroids strongly resemble those reported in human INAD. Transmission EM in the cerebellar granule layer (G) and molecular layer (H) also indicates accumulation of tubulovesicular membranes in spheroids. Magnifications: x6400 (A, C, F), x8400 (B), x12,800 (D), x3200 (E), x4200 (G), x1280 (H).

Age-Dependent Increase in Ubiquitin-Positive Spheroids throughout Multiple Brain Regions

Immunohistochemistry with anti-ubiquitin antibodies identified a consistent pattern of age-dependent increase in spheroids in three brain regions (Figure 5) . At 4 months spheroids were small and relatively infrequent. With increasing age, ubiquitin-positive spheroids became more abundant and larger in these regions. Furthermore the distribution of spheroids became much more widespread with increasing age, and at 13 months, spheroids were numerous in nearly all cortical, subcortical, and brainstem regions. We also observed spheroids in the spinal cord gray matter. With the exception of rare punctate ubiquitin-positive structures in cerebellum, ubiquitin-positive spheroids were not observed in WT animals at any of the ages examined.

View larger version (165K): [in this window] [in a new window]   Figure 5. Age-dependent increase in spheroid density among multiple brain regions of iPLA2β-KO mice as assessed by ubiquitin immunohistochemistry. Representative photographs from striatum (A–C), cerebellum (D–F), and cortex (G–I) are shown at ages 4, 8, and 13 months from left to right. A progressive increase in the density of ubiquitin-positive spheroids (labeled with brown diaminobenzidine tetrahydrochloride chromagen) in the neuropil was observed with increasing age in these regions and in nearly all other regions of the brain. Scale bar = 10 µm.

View larger version (11K): [in this window] [in a new window]   Figure 6. Quantitative assessment of progressive increases in spheroid density in striatum (A), cerebellum (B), and cortex (C) of iPLA2β-KO mice. Brain sections from iPLA2β-KO mice at 4, 8, and 13 months were stained with a rabbit polyclonal ubiquitin antibody, and average spheroid density in each region was determined by image analysis of multiple random fields in each region. Graphs show mean spheroid density at each age. Error bars indicate SD.

To characterize the biochemical properties of accumulating ubiquitinated proteins, we fractionated brain tissue by sequential extraction with buffers of increasing solubilization strength. Western blots of KO brain tissue fractions with anti-ubiquitin antibodies revealed the accumulation of ubiquitinated proteins that required the strong detergent SDS for extraction and solubilization (Figure 7) . The pattern of accumulating high molecular weight protein species was complex, probably because of the presence of multiple polyubiquitinated proteins, and did not allow individual ubiquitinated protein species to be resolved. The localization of ubiquitinated proteins to SDS-soluble fractions suggests that protein misfolding and aggregation are involved in the process of spheroid formation.

View larger version (73K): [in this window] [in a new window]   Figure 7. Ubiquitinated proteins accumulate in insoluble fractions obtained by sequential extraction of iPLA2β-KO mouse brain. A: Anti-ubiquitin Western blot analysis of fractions obtained by sequential biochemical extraction of KO and WT mouse brain tissue samples containing frontal cortex plus striatum. The profiles of ubiquitinated proteins extracted by high salt (HS), high salt with Triton (HS/T), and RIPA buffers are similar, with perhaps a small increase in ubiquitinated proteins extracted from KO brain by HS/T. However there is a clear increase in a complex pattern of high molecular weight ubiquitinated protein species extracted by SDS buffer from KO brain tissue. The pattern of accumulating high molecular weight protein species was complex, indicating the presence of multiple polyubiquitinated proteins. B: Accumulation of ubiquitinated proteins in insoluble fractions was observed in multiple independent fractionation experiments using brain tissue samples containing frontal cortex plus striatum (FC/S) or striatum alone (S) from 13-month-old WT and KO mice.

Because dystrophic changes are frequently observed in the peripheral nervous system in INAD, we examined the superior mesenteric and celiac ganglia of the sympathetic nervous system in iPLA₂β-KO mice by transmission EM. These peripheral sympathetic ganglia contained significant dystrophic changes with the same characteristic ultrastructural features observed in the central nervous system (Figure 8, A and B) . Spheroids were also observed in axon terminals innervating the carotid body (not shown), but were not present in the superior cervical ganglion. The gracile and cuneate nuclei, which contain termini of dorsal root ganglia neurons, also contained prominent dystrophic changes that increased between 4 and 13 months of age (Figure 8, C and D) . In humans and rodents, dystrophic changes in SMG, CG, and gracile nuclei have also been observed with advanced age.^20,21

View larger version (222K): [in this window] [in a new window]   Figure 8. Neuroaxonal dystrophy affects the sympathetic nervous system and sensory axons in the gracile nucleus in iPLA2β-KO mice. A and B: Images from transmission EM illustrate prominent spheroids with accumulating tubulovesicular membranes in axon terminals within the sympathetic superior mesenteric-celiac ganglia. H&E staining revealed large spheroids in the gracile nucleus at 4 months. C: Spheroids increased in size and number at 13 months (D). Scale bars: 6 µm (A); 2 µm (B); 10 µm (C, D).

Analysis of Pathological Iron and -Synuclein Accumulation

A number of other pathological features often accompany spheroids in human INAD and NBIA, including iron accumulation in certain brain regions and the pathological accumulation of -synuclein in Lewy bodies and Lewy neurites. In brain tissue from iPLA₂β-KO mice, Prussian blue staining for pathological iron accumulation did not provide evidence of iron accumulation in globus pallidus and substantia nigra. Pathological accumulation of -synuclein in axonal and cytoplasmic inclusions, a finding that links both INAD and NBIA to Parkinson’s disease and dementia with Lewy bodies,^22-28 was examined by immunohistochemistry. In WT and KO animals, similar diffuse staining of the neuropil was observed with -synuclein antibodies. Although we have observed no evidence of Lewy bodies or dystrophic neurites using an antibody that preferentially recognizes pathological -synuclein, syn303, we did observe accumulation of -synuclein in spheroids, primarily in striatum, that appeared similar to those identified by ubiquitin staining (Figure 9) . Staining of spheroids with syn303 was less frequent than ubiquitin staining but was observed consistently.

View larger version (150K): [in this window] [in a new window]   Figure 9. Accumulation of -synuclein protein in spheroids in the striatum of iPLA2β-KO mice. Immunohistochemistry using monoclonal synuclein antibody syn303 demonstrates staining of spheroids with morphology similar to those labeled with ubiquitin antibodies. Representative photographs (A, B) are shown from the striatum of a 13-month-old iPLA2β-KO mouse. Syn303 staining was primarily observed in striatum of mice aged 13 months or older, with only rare staining of spheroids in other brain regions. Scale bar = 10 µm.

	Discussion

Top Abstract Materials and Methods Results Discussion References

The development of a mouse model for INAD provides significant opportunities for further studies of disease pathogenesis, as well as opportunities for preclinical testing of potential therapeutic interventions. The progressive neurodegenerative process in these mice can be assessed by quantitative behavioral tests of sensorimotor function and by quantitative assessment of ubiquitin-positive spheroids in the brain. Behavioral and pathological measures of disease progression could be used to investigate the effects of other genetic or metabolic factors linking the loss of iPLA₂β function to neurodegeneration.

The widespread distribution of spheroids throughout the central and peripheral nervous system of iPLA₂β-KO mice resembles the widespread distribution observed in INAD. However, iPLA₂β-KO mice develop pathological and behavioral evidence of disease at a relatively later point within their lifespan than patients with human INAD, when disease onset is typically between 1 and 5 years of age. Spheroids are evident at 4 months of age in iPLA₂β-KO mice, and spheroid density progressively increases with age. Dysfunction in proprioceptive, cerebellar, and basal ganglia pathways reaches the threshold for significant impairment in sensorimotor function near the midpoint in the mouse lifespan. The shift in age dependence could be attributable to a number of factors that differ between mouse and human brain, such as axon length, number of synapses, and neuronal firing patterns, which may determine neuronal vulnerability to loss of iPLA₂β. Alternatively, age-dependent compensatory mechanisms may differ in mice and humans.

The primary pathogenic event caused by loss of iPLA₂β function is likely to be altered membrane composition. In addition to phospholipase A2 activity, iPLA₂β also exhibits acyl CoA thioesterase activity.³⁰ Thus loss of this enzyme could lead to the accumulation of phospholipids and acyl CoAs, or to decreased release of free fatty acids, lysophospholipids, and free CoA. It is unclear whether specific molecular species within these classes of lipid molecules would be affected. Altered membrane composition attributable to changes in these classes of lipid molecules could have a number of downstream consequences through changes in membrane properties and could affect the function of membrane proteins including channels, transporters, receptors, and signaling enzymes.

Our results indicate that loss of membrane homeostasis leading to accumulation of membranes in distal axons underlies progressive neurological impairment in iPLA₂β-KO mice. Loss of iPLA₂β function could alter lipid composition of the plasma membrane, vesicles, or endosomes and thereby affect proteins and processes normally involved in regulating the movement of membranes within axons and dendrites. For example, endocytic or secretory pathways could be impaired by disruption of membrane budding, vesicle transport, or membrane fusion.

Ubiquitin immunohistochemistry is an early and sensitive marker of changes in iPLA₂β-KO mice. Furthermore, pathological ubiquitin immunostaining is accompanied by accumulation of ubiquitinated proteins in insoluble fractions prepared from KO brain tissue. Identification of individual protein species that accumulate in KO brain may provide further insight into changes in protein solubility and clearance because of loss of iPLA₂β. Altered protein solubility accompanies histopathological evidence of accumulating protein in many neurodegenerative diseases and reflects protein misfolding and aggregation.^31,32 These intracellular inclusions are frequently labeled with anti-ubiquitin antibodies, suggesting a link between protein degradation pathways and accumulation of misfolded protein.

Accumulation of ubiquitinated proteins may be mechanistically linked to accumulation of membranes. Ubiquitination of membrane proteins initiates protein turnover through targeting to lysosomes.^33-36 Altered membrane composition might result in membrane protein dysfunction and increased ubiquitination. Membrane composition changes could also cause misfolding and aggregation of membrane-associated proteins. Finally, it is possible that iPLA₂β is required for transport of ubiquitinated proteins for degradation by either lysosomes or the ubiquitin-proteasome system. For example, iPLA₂β deficiency might disrupt vesicle transport or sorting within endosomes and lead to accumulation of tubulovesicular membranes and associated ubiquitinated proteins.

The pathological features of neuroaxonal dystrophy are observed in a number of other settings that might provide further insight into mechanisms underlying this pathological process. Spheroids in the gracile nucleus and in the superior mesenteric and celiac ganglia are observed with advanced age in humans and rodents.^20,21 Diabetes mellitus in humans and rodents also leads to neuroaxonal dystrophy in superior mesenteric and celiac ganglia.³⁷ A number of mouse models of neuroaxonal dystrophy attributable to spontaneous mutations have also been reported,^38-42 and they share the features of age-dependent development of motor and sensory impairment, accompanied by the pathological changes of neuroaxonal dystrophy in some neuronal populations, particularly those in the gracile nucleus.

In at least some neuronal populations, there thus may be multiple convergent pathways that ultimately lead to the final common destination of neuroaxonal dystrophy. It is possible that axon terminals in neuronal populations such as sympathetic ganglia and dorsal column nuclei are vulnerable to other environmental and genetic perturbations that converge on similar pathways involved in membrane homeostasis. A mutation in one of these mouse lines has been identified in the Uchl1 gene, which encodes a ubiquitin carboxy-terminal hydrolase that may regulate levels of free monomeric ubiquitin,⁴² providing further support for the hypothesis that dysregulated protein ubiquitination or failed targeting of ubiquitinated proteins might play a central role in neuroaxonal injury and degeneration. Identification of the genetic defects in other mouse models^38,39 might also provide further insight into pathways involved in these pathological processes.

A common feature linking many neurodegenerative disorders is the accumulation of misfolded and ubiquitinated proteins within neurons. The presence of other histopathological lesions in human INAD and NBIA, such as Lewy bodies and neurofibrillary tangles, further suggests that these diseases share mechanisms of pathogenesis with other disorders including Parkinson’s disease and Alzheimer’s disease. Although Lewy bodies and neurofibrillary tangles were not observed in iPLA₂β-KO mice, pathological accumulation of -syn or tau might be further studied via transgenic expression of these proteins in iPLA₂β-KO mouse lines. Thus further studies of iPLA₂β-KO mice may provide significant insight into the role of altered lipid metabolism in a number of common sporadic neurodegenerative diseases in addition to INAD and NBIA.

	Acknowledgements

 
We thank Karen Green for her excellent ultrastructural technical assistance and Sara Conyers for her excellent technical assistance with animal behavior studies.

	Footnotes

 
Address reprint requests to Paul T. Kotzbauer, M.D., Ph.D., Department of Neurology, Washington University School of Medicine, Box 8111, 660 South Euclid Ave., St. Louis, MO 63110. E-mail: kotzbauerp{at}neuro.wustl.edu

Supported by the National Institutes of Health (National Institute of Neurological Disorders and Stroke (grant NS48924-01 to P.T.K. and Neuroscience Blueprint core grant NS057105 to Washington University), the McDonnell Center for Cellular and Molecular Neurobiology (grant to P.T.K.), the United States Public Health Service (grants R37-DK34388, P41-RR00954, P60-DK20579, and P30-DK56341 to J.T., and 5P01HL57278 to R.W.G.), and the Juvenile Diabetes Research Foundation (grant to R.E.S.).

Accepted for publication October 23, 2007.

	References

Top Abstract Materials and Methods Results Discussion References

 

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