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J Biol Chem, Vol. 274, Issue 53, 37507-37510, December 31, 1999
§ and¶
**
From the Howard Hughes Medical Institute and
Departments of ¶ Biochemistry,
Pediatrics, and ** Genetics, Emory University School
of Medicine, Atlanta, Georgia 30322
The association of protein deposits with
neurodegeneration has become a consistent finding in a large group of
etiologically diverse diseases (1, 2) (Table I).
The protein deposits are generally dense
fibrillar structures containing a high percentage of Currently there are eight neurodegenerative disorders known to
be caused by the expansion of a CAG
trinucleotide repeat coding for polyglutamine. Protein aggregates have
been observed in most of these disorders (1,
3). A mechanism of pathogenesis for these
disorders has not been elucidated, although it is likely mediated
through the polyglutamine tract because longer tracts lead to earlier
ages of onset and more severe phenotypes.
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-pleated sheet
secondary structure and can be located in various cellular compartments
as well as extracellularly. Moreover, the deposits are generally
ubiquitinated and may contain numerous cellular proteins.
Neurodegenerative Disorders Caused by Polyglutamine
Expansion
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Neurological disorders with aberrant protein deposition
Spinocerebellar Ataxia Type 1 (SCA1)1
SCA1 is
characterized clinically by gait and limb ataxia, dysarthia, dysmetria,
and variable degrees of muscle wasting (4). SCA1 patients have CAG
repeat tracts ranging in size from 39 to 83 glutamines. The SCA1 gene product, ataxin-1, is normally a nuclear protein
except in Purkinje cells where it is also cytoplasmic.
Ubiquitin-positive nuclear inclusions have been observed in
SCA1 transgenic mice, transfected cells, and in affected
brain regions of SCA1 patients (5) (Fig.
1).
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In both cultured cells and cerebellar tissue of SCA1 transgenic mice, ataxin-1 associates with the nuclear matrix (5). An associated redistribution of the matrix-associated promyelocytic leukemia protein suggests that SCA1 pathogenesis may be due to morphologic changes within the nucleus. Transgenic mice expressing mutant ataxin-1 without a nuclear localization sequence fail to develop disease-related pathology and exhibit no signs of ataxin-1 aggregation (6). Interestingly, other transgenic mice lacking a self-association domain outside of the polyglutamine tract express mutant ataxin-1 in the nucleus and develop ataxia without evidence of ataxin-1 nuclear aggregates. Thus, nuclear localization of mutant ataxin-1 appears to be required for pathogenesis, whereas visible nuclear aggregation may not be required.
Spinocerebellar Ataxia Type 3/Machado-Joseph Disease
(SCA3/MJD)Clinically, SCA3 patients present with progressive
ataxia, external ophthalmoplegia, muscle atrophy, and parkinsonian
signs (4). These patients typically have repeat tract expansions ranging from 55 to 84 glutamines. Ataxin-3 is normally a cytoplasmic protein that accumulates in ubiquitinated aggregates in the nuclei of
affected neurons (7). A necessary event in SCA3 pathogenesis is the
entry of expanded ataxin-3 into the nucleus. Ubiquitinated intranuclear
neuronal inclusions were only seen in neurons and not within glial
cells, even though glial cells are immunoreactive with ataxin-3
antibodies. Cells expressing a truncated ataxin-3 fragment produce
intranuclear inclusions, recruit full-length ataxin-3 into aggregates,
and exhibit an induction of cell death (8). An ataxin-3 fragment may
serve to catalyze the formation of intranuclear aggregates by
translocating into the nucleus and recruiting endogenous ataxin-3 and
other proteins into aggregates, in a dominant-negative manner.
Spinocerebellar Ataxia Type 6 (SCA6)SCA6 is an autosomal
dominant cerebellar ataxia caused by a CAG repeat expansion within the
3'-region of the 
1A voltage-dependent calcium channel
gene (CACNA1A) (9). Unlike the other CAG repeat expansion
disorders, expansions within SCA6 patients are relatively small (21-30
glutamines) and fall within the normal range of other CAG tract
lengths. In SCA6 brains numerous protein aggregates, appearing not to
be ubiquitinated, were observed exclusively in the cytoplasm of
Purkinje cells (3). Unlike this cytoplasmic localization, cells
transfected with expanded SCA6 constructs exhibit perinuclear
aggregates leading to apoptotic cell death.
Spinocerebellar Ataxia Type 7 (SCA7) CAG repeat tract
expansions in SCA7 patients have been shown to range from 34 to greater than 200 glutamines (1). In the brain of an early onset patient, intranuclear neuronal ubiquitinated inclusions occurred most frequently in the inferior olivary complex, a site of severe neuronal loss in SCA7
patients (10). However, inclusions were also observed in regions not
affected by the disease, suggesting some cell specificity regarding the
consequence of aggregation. Generally, inclusions in SCA7 brains were
shown to be ubiquitinated to varying degrees. A critical observation is
that the inclusions that are not ubiquitinated are found in regions
that are not affected, suggesting ubiquitination is required for
neurodegeneration. Similarly, ataxin-7 aggregates in Cos-1 cells that
are localized to the nucleus are not ubiquitinated (11). Hence, some
cell specificity with regard to ubiquitination also occurs.
Huntington Disease (HD) The HD gene product,
huntingtin, is predominantly a cytoplasmic protein (12). HD patients
have CAG repeat tract lengths ranging from 38 to 180 glutamines.
Nuclear inclusions in HD patients and transgenic mice have been found both in non-CNS tissue and neurons (13). Generally, the inclusions are
immunoreactive with anti-N-terminal huntingtin and ubiquitin antibodies
(Fig. 1). The striatum, which is predominantly affected in HD, actually
contains far fewer aggregates compared with the cortex (14). This
suggests that huntingtin aggregates may not be a good indicator of
cells destined to die in HD (15). Interestingly, non-ubiquitinated
aggregates have been found, suggesting that ubiquitination occurs late
in formation.
Because there is no obvious nuclear localization sequence in huntingtin known nuclear import mechanisms are not responsible for translocating huntingtin to the nucleus. However, proteolytic processing may produce a smaller protein fragment that can enter the nucleus by diffusion (16). The activation of caspases appears to be involved in proteolytic cleavage, which leads to apoptotic cell death (17, 18). In addition, numerous reports have shown a correlation between the length of a truncated huntingtin protein and the size of the CAG tract with the frequency and localization of aggregates (19). Interestingly, transfection studies have shown that changing the subcellular localization of the huntingtin does not alter the frequency of aggregation or the level of toxicity (16). In contrast, HD constructs transfected into cultured striatal neurons produce intranuclear inclusions that do not correlate with apoptotic cell death (20).
Dentatorubral-Pallidoluysian Atrophy (DRPLA)The clinical
features of DRPLA are similar to HD (12). The DRPLA gene
product, atrophin-1, is normally a cytoplasmic protein that is found in ubiquitinated neuronal intranuclear inclusions in affected brain regions (1). Expansions of the CAG tract in atrophin-1 range from 49 to
88 glutamines. Caspase cleavage of atrophin-1 has been shown to
modulate cell toxicity and aggregate formation (21). Cleavage is
necessary for cell toxicity because mutation of the caspase cleavage
site within atrophin-1 suppresses aggregate formation. In cells
expressing truncated atrophin-1 with an expanded repeat, perinuclear
ubiquitinated aggregates and apoptotic cell death were observed (22).
Interestingly, the full-length expanded protein did not form aggregates
but was drawn into the aggregates containing the truncated protein.
This interaction could be stabilized by a transglutaminase-catalyzed
reaction (23).
Spinal and Bulbar Muscular Atrophy (SBMA)SBMA is an
X-linked recessive disorder caused by expansions of a polyglutamine
repeat, ranging from 38 to 65 CAGs, in the androgen receptor (4).
Patients typically exhibit slow, progressive weakness and atrophy.
Ubiquitinated inclusions have been observed in motor neurons of SBMA
patients and in transfected cells (1, 24). Cytoplasmic protein
aggregation in transfected cells was not observed unless truncated
SBMA constructs were used. The transfected SBMA
gene product was shown to undergo proteolytic processing in transfected
cells, possibly producing fragments due to cleavage within the CAG
tract (25). The appearance of this cleavage product, formation of
cytoplasmic aggregates, and increased cell toxicity occurred in a
repeat tract length-dependent manner.
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Alzheimer's Disease (AD)--
AD is characterized by the
accumulation of extracellular plaques and cytoplasmic neurofibrillary
tangles (NFTs) (2). The major component of the dense plaques is
-amyloid (A), a 39-43-amino acid peptide derived from the larger
amyloid precursor protein (APP). Accumulation of A is an early event
in development of AD that may precede other brain lesions and symptoms
by years. NFTs are bundles of paired helical filaments containing
highly phosphorylated and ubiquitinated forms of the
microtubule-associated factor tau (26).
Tissue-specific processing results in heterogeneity of the A peptide
at both its N and C termini (27). Both - and 
-secretase have been
shown to cleave APP, but this cleavage is not likely the first
pathological alteration in AD because peptide resulting from this
cleavage is found in deposits and in most other cells (28). The
accumulation of A is considered to be a central part of AD
pathogenesis, which implies that over time preamyloid deposits are
"transformed" into amyloid plaques (29). These lesions are thought
to become compacted over a number of years while taking on the
characteristics of amyloid and are associated with neuronal damage and
tangles in the form of neuritic plaques.
Parkinson's Disease (PD)--
Clinically, Parkinson's disease
patients present with resting tremor, muscular rigidity, bradykinesia,
and postural instability (30). The symptoms are suggested to result
from abnormal dopamine levels or degeneration of dopaminergic neurons
in affected regions of the CNS. In addition to neuronal degeneration
ubiquitinated intracytoplasmic inclusion bodies (Lewy bodies) have been
found in numerous brain regions (31). A major component of Lewy bodies is -synuclein. Lewy bodies have been shown to be immunoreactive for
ubiquitin, -amyloid precursor protein, synaptophysin,
neurofilaments, and ubiquitin C-terminal hydrolyase (32, 33).
Two different -synuclein missense mutations (A30P and A53T) have
been found in dominant cases of PD. In vitro studies have shown that when compared with wild-type -synuclein both of these PD-linked mutations accelerate aggregate formation (34). Because A30P
and A53T accelerate aggregation the proteasome may have difficulty in
clearing the aggregates. Furthermore, a mutation in the ubiquitin C-terminal hydrolyase L1 gene (UCH-L1), a deubiquitinating
protease that is thought to cleave polymeric ubiquitin to monomers, has been found in a family with PD (33). In vitro analysis has
shown that a mutation in this gene results in reduced catalytic
activity, supporting the hypothesis that the aggregates are
inefficiently cleared by the proteasome.
Prion Diseases-- Prion diseases comprise a group of disorders characterized by the accumulation of a conformationally modified form of the prion protein (PrP) (35). The infectious prion is an insoluble proteinaceous particle that lacks nucleic acid and to date has been shown to consist only of a modified isoform of PrP, designated PrPsc. The prion diseases are unique in that the proteinaceous prion particle is itself transmissible (36). Prion diseases include scrapie in sheep and bovine spongiform encephalopathy in cattle. In humans the prion diseases include Creutzfeldt-Jakob disease, Gerstmann-Straussler-Scheinker disease, Kuru, and fatal familial insomnia.
Although mutations in PrP are found throughout the protein,
some mutations in PrP have been shown to occur in regions
adjacent to elements of putative secondary structure (35, 37).
Structural changes may have dramatic effects on the cellular properties
of the mutant protein. A form with decreased -helical content and increased -pleated sheet content is insoluble and relatively resistant to proteases.
Amyotrophic Lateral Sclerosis (ALS)-- Approximately 90% of ALS cases are sporadic in nature, and the remaining 10% represent familial cases (38). Of the familial ALS cases, approximately 20% are due to mutations in the Cu,Zn-superoxide dismutase gene (SOD1). At least 50 mutations, the majority being missense mutations, have been found in the SOD1 gene in familial ALS families.
Transgenic mice have been made with transgenes harboring
SOD1 mutations previously found in ALS patients. Initial
indicators of disease in mice expressing a SOD1 G85R
mutation include cytoplasmic ubiquitinated astrocytic inclusions
reminiscent of Lewy bodies that stain intensely with SOD1 antibodies
(39). The inclusions are 10 times more abundant in astrocytes than in
neurons, and their frequency escalates markedly with disease
progression. Like other SOD1 mutations this mutation occurs
outside of the active site and may alter the stability of the protein
backbone, resulting in conformational changes that ultimately lead to
its abnormal deposition.
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Formation of Inclusion Bodies--
The disorders discussed here
present pathologically with inclusion bodies that are generally
fibrillar in nature and contain a high percentage of -pleated sheet
secondary structure. Conversion from a soluble form to an insoluble
form may involve a change in the three-dimensional structure of the
protein predominantly found in the aggregate. Protein interactions may
occur by the formation of a stable -pleated sheet via a polar zipper
(40). Alternatively, in the CAG triplet repeat disorders covalent bond formation between proteins has been suggested to occur via a
transglutaminase-catalyzed reaction (23).
The formation of these aggregates may be a lengthy process, including
numerous steps that culminate in targeting for degradation by
ubiquitination. Perhaps the initiating event is proteolytic processing
of the aggregate-forming protein. The major component of -amyloid
plaques in Alzheimer's patients is a proteolytic fragment derived from
the amyloid precursor protein (27). Four of the
polyglutamine-containing proteins have been shown to be cleaved by
caspases (41). Furthermore, in vivo cell toxicity in
cultured neurons and fibril formation in vitro was observed with a PrP fragment (42). Together, these data indicate that proteolytic fragments may be toxic, leading to aggregate formation.
Other issues relevant to the formation of inclusions include the expression level of the protein and the amino acid sequence outside the polyglutamine tract. In HD transgenic mice expressing exon 1, inclusions appear earlier in homozygotes than in heterozygotes suggesting that the rate of inclusion formation is related to the level of transgene expression (43). Moreover, protein concentration and time are critical parameters for the formation of huntingtin aggregates in vitro (44). The protein context in which the expanded polyglutamine tract is located does not appear to be essential for aggregate formation. Ectopically expressed CAG repeats placed within the hypoxanthine phosphoribosyltransferase (HPRT) gene in transgenic mice produced a neurological phenotype and aggregates (45). However, ataxin-1 aggregates do not form in transgenic mice in which the ataxin-1 self-association domain has been deleted (6).
Interacting Proteins-- One mechanism to impart a toxic gain of function by the mutant proteins is if they form stronger and/or more stable interactions with other proteins. Proteins that interact more strongly could be drawn into aggregates and prevented from carrying out their normal cellular function. Moreover, the remarkable cell specificity of the neurodegeneration in most of these disorders does not parallel the expression pattern of the primary protein and therefore may mimic the expression of such an interacting protein. Many proteins have been identified that interact with expanded polyglutamine-containing proteins (46, 47). For example, huntingtin interacts with HIP2, a ubiquitin-conjugating enzyme, suggesting a link between aggregate formation and protein disposal via the ubiquitin-dependent protein degradation pathway. Interestingly, in transfected striatal neurons coexpression of a dominant-negative ubiquitin-conjugating mutant prevented huntingtin aggregation but increased cell death (20).
Protein interactions have also been shown to be important for aggregate
formation in AD. 2-Macroglobulin, a proteinase inhibitor released in response to inflammatory stimuli, strongly and specifically associates with the -amyloid peptide and prevents fibril formation (48). These complexes are then cleared by the low density lipoprotein receptor-related protein (LRP), providing a mechanism of A
clearance. This hypothesis suggests that the mechanism(s) for clearing
aggregate complexes, possibly involving LRP, may be dysfunctional in AD patients.
Abnormal Protein Processing and Disease
Pathogenesis--
Molecular chaperones and proteasome components have
been shown to co-localize to androgen receptor and ataxin-1 aggregates (49, 50). Overexpression of the chaperone HDJ-2/HSDJ in HeLa cells
suppressed aggregate formation, suggesting that the affected neurons
are unable to properly fold or degrade the expanded polyglutamine protein. The 26 S proteasome redistributes to ataxin-3 aggregates, and
proteasome inhibition results in a repeat length-dependent increase in aggregation (51). This suggests that the proteasome may
play a protective role by suppressing aggregate formation. The A
peptide binds to the proteasome and has been shown to inhibit its
activity (52). The inhibition of proteasome activity therefore blocks
ubiquitin-mediated degradation of the A peptide and perhaps hampers
the proteasome's ability to degrade other ubiquitinated proteins.
Furthermore, protein deposits in AD have been shown to contain
ubiquitin-B with a +1 frameshift mutation, inhibiting the ability to
polyubiquitinate proteins (53).
The persistence of ubiquitinated structures could be because of
cellular inability to rescue misfolded proteins, failure to properly
shuttle the complexes into degradation pathways, or exceeding the
capacity of the proteasome (Fig. 2).
Sequestering of ubiquitin and other protein degradation factors within
the protein deposit or blocking of the proteasome lumen by the
aggregate could alter the normal cellular role of the
ubiquitin-mediated protein degradation pathway. Moreover, the function
of cellular proteins in these disorders could be altered either by
sequestration within the aggregate itself or by altered regulation due
to sequestration of ubiquitin-proteasome components (Fig. 2). In
support of this stably transfected PC12 cells expressing a huntingtin
fragment with 150 glutamine repeats showed altered expression of
numerous genes compared with a fragment expressing a normal repeat
(54). Further evidence for the direct involvement of the
ubiquitin-proteasome pathway in neurodegenerative disorders comes from
the discovery that an intragenic deletion in ubiquitin C-terminal
hydrolyase (Uchl1) is responsible for gracile axonal
dystrophy in mice (55). These mice exhibit neurodegeneration and
accumulate amyloid B-protein and ubiquitin-positive deposits within the
brain. Dysfunction of Uchl1 inhibits the processing and reusage of free
ubiquitin and thus may allow the accumulation of abnormal proteins.
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Additional disorders substantiate the idea that abnormal protein processing or degradation may play a key role in the pathogenesis of neurological disease. Early onset torsion dystonia is due to a 3-base pair deletion in the torsinA gene (56). TorsinA shows homology in several domains with a class of heat shock/chaperone proteins. Hence, mutation of torsinA may lead to abnormal folding of proteins involved in early onset torsion dystonia. Autosomal recessive juvenile parkinsonism has been associated with mutations in the parkin gene (57). The N-terminal portion of parkin is fairly homologous to ubiquitin. Mutations in the ubiquitin protein ligase E6-AP are responsible for Angelman's syndrome, an inherited form of mental retardation (58).
Whether protein aggregates directly cause neurodegeneration or are the
result of a dying neuron is not yet known. In the CAG repeat disorders,
aggregates precede the onset of neurological symptoms (19).
Interestingly, small aggregates are not ubiquitinated, indicating that
ubiquitination occurs late in the formation process (14). This suggests
that the cell is attempting to clear the aggregated proteins but is
unsuccessful. The inability to degrade the aggregate may impair the
cell's ability to carry out normal protein processing and degradation
pathways, which could lead to altered half-lives of physiologically
important proteins. Indeed, it may be that in the absence of cell
division, the neuron is hypersensitive to changes in the balance of
protein synthesis and degradation, which may ultimately lead to neurodegeneration.
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ACKNOWLEDGEMENTS |
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We thank Keith Wilkinson, Steven Hersch, and Xiao-Jiang Li for critical reading of the manuscript.
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FOOTNOTES |
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* This minireview will be reprinted in the 1999 Minireview Compendium, which will be available in December, 1999.
§ Associate of the Howard Hughes Medical Institute.
Howard Hughes Medical Institute Investigator. To whom
correspondence should be addressed: Howard Hughes Medical Inst., Emory University School of Medicine, 4035 Rollins Research Center, 1510 Clifton Rd., Atlanta, GA 30322. Tel.: 404-727-5979; Fax: 404-727-5408; E-mail: swarren@ bimcore.emory.edu.
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ABBREVIATIONS |
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The abbreviations used are: SCA, spinocerebellar ataxia; CNS, central nervous system; HD, Huntington disease; DRPLA, dentatorubral-pallidoluysian atrophy; SBMA, spinal and bulbar muscular atrophy; AD, Alzheimer's disease; NFT, neurofibrillary tangle; APP, amyloid precursor protein; PD, Parkinson's disease; ALS, amyotrophic lateral sclerosis; PS, presenilin; LRP, low density lipoprotein receptor-related protein.
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|---|
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|
|---|
| 1. | Paulson, H. L. (1999) Am. J. Hum. Genet. 64, 339-345[CrossRef][Medline] [Order article via Infotrieve] |
| 2. | Tolnay, M., and Probst, A. (1999) Neuropathol. Appl. Neurobiol. 25, 171-187[CrossRef][Medline] [Order article via Infotrieve] |
| 3. |
Ishikawa, K.,
Fujigasaki, H.,
Saegusa, H.,
Ohwada, K.,
Fujita, T.,
Iwamoto, H.,
Komatsuzaki, Y.,
Toru, S.,
Toriyama, H.,
Watanabe, M.,
Ohkoshi, N.,
Shoji, S.,
Kanazawa, I.,
Tanabe, T.,
and Mizusawa, H.
(1999)
Hum. Mol. Genet.
8,
1185-1193 |
| 4. | Koshy, B. T., and Zoghbi, H. Y. (1997) Brain Pathol. 7, 927-942[Medline] [Order article via Infotrieve] |
| 5. | Skinner, P. J., Koshy, B. T., Cummings, C. J., Klement, I. A., Helin, K., Servadio, A., Zoghbi, H. Y., and Orr, H. T. (1997) Nature 389, 971-974[CrossRef][Medline] [Order article via Infotrieve] |
| 6. | Klement, I. A., Skinner, P. J., Kaytor, M. D., Yi, H., Hersch, S. M., Clark, H. B., Zoghbi, H. Y., and Orr, H. T. (1998) Cell 95, 41-53[CrossRef][Medline] [Order article via Infotrieve] |
| 7. | Paulson, H. L., Das, S. S., Crino, P. B., Perez, M., Patel, S. C., Gotsdiner, D., Fischbeck, K. H., and Pittman, R. N. (1997) Am. Neur. Assoc. 41, 453-462 |
| 8. |
Perez, M. K.,
Paulson, H. L.,
Pendse, S. J.,
Saionz, S. J.,
Bonini, N. M.,
and Pittman, R. N.
(1998)
J. Cell Biol.
143,
1457-1470 |
| 9. | Zhuchenko, O., Bailey, J., Bonnen, P., Ashizawa, T., Stockton, D. W., Amos, C., Dobyns, W. B., Subramony, S. H., Zoghbi, H. Y., and Lee, C. C. (1997) Nat. Genet. 15, 62-69[CrossRef][Medline] [Order article via Infotrieve] |
| 10. |
Holmberg, M.,
Duyckaerts, C.,
Durr, A.,
Cancel, G.,
Gourfinkel-An, I.,
Damier, P.,
Faucheux, B.,
Trottier, Y.,
Hirsch, E. C.,
Agid, Y.,
and Brice, A.
(1998)
Hum. Mol. Genet.
7,
913-918 |
| 11. |
Kaytor, M. D.,
Duvick, L. A.,
Skinner, P. J.,
Koob, M. D.,
Ranum, L. P. W.,
and Orr, H. T.
(1999)
Hum. Mol. Genet.
8,
1657-1664 |
| 12. | Ross, C. A., Becher, M. W., Colomer, V., Engelender, S., Wood, J. D., and Sharp, A. H. (1997) Brain Pathol. 7, 1003-1016[Medline] [Order article via Infotrieve] |
| 13. |
Sathasivam, K.,
Hobbs, C.,
Turmaine, M.,
Mangiarini, L.,
Mahal, A.,
Bertaux, F.,
Wanker, E. E.,
Doherty, P.,
Davies, S. W.,
and Bates, G. P.
(1999)
Hum. Mol. Genet.
8,
813-822 |
| 14. |
Gutekunst, C.-A.,
Li, S.-H.,
Yi, H.,
Mulroy, J. S.,
Kuemmerle, S.,
Jones, R.,
Rye, D.,
Ferrante, R. J.,
Hersch, S. M.,
and Li, X.-J.
(1999)
J. Neurosci.
19,
2522-2534 |
| 15. | Kuemmerle, S., Gutekunst, C.-A., Klein, A. M., Li, X.-J., Li, S.-H., Beal, M. F., Hersch, S. M., and Ferrante, R. J. (1999) Ann. Neurol., in press |
| 16. |
Hackam, A. S.,
Singaraja, R.,
Zhang, T.,
Gan, L.,
and Hayden, M. R.
(1999)
Hum. Mol. Genet.
8,
25-33 |
| 17. | Sanchez, I., Xu, C.-J., Juo, P., Kakizaka, A., Blenis, J., and Yuan, J. (1999) Neuron 22, 623-633[CrossRef][Medline] [Order article via Infotrieve] |
| 18. | Ona, V. O., Li, M., Vonsattel, J. P. G., Andrews, L. J., Khan, S. Q., Chung, W. M., Frey, A. S., Menon, A. S., Li, X.-J., Stieg, P. E., Yuan, J., Penney, J. B., Young, A. B., Cha, J.-H. J., and Friedlander, R. M. (1999) Nature 399, 263-267[CrossRef][Medline] [Order article via Infotrieve] |
| 19. |
Rubinsztein, D. C.,
Wyttenbach, A.,
and Rankin, J.
(1999)
J. Med. Genet.
36,
265-270 |
| 20. | Saudou, F., Finkbeiner, S., Devys, D., and Greenberg, M. E. (1998) Cell 95, 55-66[CrossRef][Medline] [Order article via Infotrieve] |
| 21. |
Ellerby, L. M.,
Andrusiak, R. L.,
Wellington, C. L.,
Hackam, A. S.,
Propp, S. S.,
Wood, J. D.,
Sharp, A. H.,
Margolis, R. L.,
Ross, C. A.,
Salvesen, G. S.,
Hayden, M. R.,
and Bredesen, D. E.
(1999)
J. Biol. Chem.
274,
8730-8736 |
| 22. | Igarashi, S., Koide, R., Shimohata, T., Yamada, M., Hayashi, Y., Takano, H., Date, H., Oyake, M., Sato, T., Sato, A., Egawa, S., Ikeuchi, T., Tanaka, H., Nakano, R., Tanaka, K., Hozumi, I., Inuzuka, T., Takahashi, H., and Tsuji, S. (1998) Nat. Genet. 18, 111-117[CrossRef][Medline] [Order article via Infotrieve] |
| 23. |
Kahlem, P.,
Terre, C.,
Green, H.,
and Djian, P.
(1996)
Proc. Natl. Acad. Sci. U. S. A.
93,
14580-14585 |
| 24. |
Merry, D. E.,
Kobayashi, Y.,
Bailey, C. K.,
Taye, A. A.,
and Fischbeck, K. H.
(1998)
Hum. Mol. Genet.
7,
693-701 |
| 25. |
Butler, R.,
Leigh, P. N.,
McPhaul, M. J.,
and Gallo, J.-M.
(1998)
Hum. Mol. Genet.
7,
121-127 |
| 26. | Morishima-Kawashima, M., Hasegawa, M., Takio, K., Suzuki, M., Titani, K., and Ihara, Y. (1993) Neuron 10, 1151-1160[CrossRef][Medline] [Order article via Infotrieve] |
| 27. | Wisniewski, T., Ghiso, J., and Frangione, B. (1997) Neurobiol. Dis. 4, 313-328[CrossRef][Medline] [Order article via Infotrieve] |
| 28. | Selkoe, D. J. (1994) Annu. Rev. Cell Biol. 10, 373-403[CrossRef] |
| 29. | Hardy, J. (1996) Ann. Med. 28, 255-258[Medline] [Order article via Infotrieve] |
| 30. |
Nussbaum, R. L.,
and Polymeropoulos, M. H.
(1997)
Hum. Mol. Genet.
6,
1687-1691 |
| 31. | Duvoisin, R. C. (1996) Adv. Neurol. 69, 33-40[Medline] [Order article via Infotrieve] |
| 32. | Takeda, A., Mallory, M., Sundsmo, M., Honer, W., Hansen, L., and Masliah, E. (1998) Am. J. Pathol. 152, 367-372[Abstract] |
| 33. | Leroy, E., Boyer, B., Auburger, G., Leube, B., Ulm, G., Mezey, E., Harta, G., Brownstein, M. J., Jonnalagada, S., Chernova, T., Dehejia, A., Lavedan, C., Gasser, T., Steinbach, P., Wilkinson, K. D., and Polymeropoulos, M. H. (1998) Nature 395, 451-452[CrossRef][Medline] [Order article via Infotrieve] |
| 34. |
Narhi, L.,
Wood, S. J.,
Steavenson, S.,
Jiang, Y.,
Wu, G. M.,
Anafi, D.,
Kaufman, S. A.,
Martin, F.,
Sitney, K.,
Denis, P.,
Louis, J.-C.,
Wypych, J.,
Biere, A. L.,
and Citron, M.
(1999)
J. Biol. Chem.
274,
9843-9846 |
| 35. | Prusiner, S. B., Scott, M. R., DeArmond, S. J., and Cohen, F. E. (1998) Cell 93, 337-348[CrossRef][Medline] [Order article via Infotrieve] |
| 36. | Horwich, A. L., and Weissman, J. S. (1997) Cell 89, 499-510[CrossRef][Medline] [Order article via Infotrieve] |
| 37. | DeArmond, S. J., Sanchez, H., Yehiely, F., Qiu, Y., Ninchak-Casey, A., Daggett, V., Camerino, A. P., Cayetano, J., Rogers, M., Groth, D., Torchia, M., Tremblay, P., Scott, M. R., Cohen, F. E., and Prusiner, S. B. (1997) Neuron 19, 1337-1348[CrossRef][Medline] [Order article via Infotrieve] |
| 38. | Kato, S., Saito, M., Hirano, A., and Ohama, E. (1999) Histol. Histopathol. 14, 973-989[Medline] [Order article via Infotrieve] |
| 39. | Bruijn, L. I., Becher, M. W., Lee, M. K., Anderson, K. L., Jenkins, N. A., Copeland, N. G., Sisodia, S. S., Rothstein, J. D., Borchelt, D. R., Price, D. L., and Cleveland, D. W. (1997) Neuron 18, 327-338[CrossRef][Medline] [Order article via Infotrieve] |
| 40. |
Perutz, M. F.,
Johnson, T.,
Suzuki, M.,
and Finch, J. T.
(1994)
Proc. Natl. Acad. Sci. U. S. A.
91,
5355-5358 |
| 41. |
Wellington, C. L.,
Ellerby, L. M.,
Hackam, A. S.,
Margolis, R. L.,
Trifori, M. A.,
Singaraja, R.,
McCutcheon, K.,
Salvesen, G. S.,
Propp, S. S.,
Bromm, M.,
Rowland, K. J.,
Zhang, T.,
Rasper, D.,
Roy, S.,
Thornberry, N.,
Pinsky, L.,
Kakizuka, A.,
Ross, C. A.,
Nicholson, D. W.,
Bredesen, D. E.,
and Hayden, M. R.
(1998)
J. Biol. Chem.
273,
9158-9167 |
| 42. | Brown, D. R., Schmidt, B., and Kretzschmar, H. A. (1996) Nature 380, 345-347[CrossRef][Medline] [Order article via Infotrieve] |
| 43. | Davies, S. W., Turmaine, M., Cozens, B. A., DiFiglia, M., Sharp, A. H., Ross, C. A., Scherzinger, E., Wanker, E. E., Mangiarini, L., and Bates, G. P. (1997) Cell 90, 537-548[CrossRef][Medline] [Order article via Infotrieve] |
| 44. |
Scherzinger, E.,
Sittler, A.,
Schweiger, K.,
Heiser, V.,
Lurz, R.,
Hasenbank, R.,
Bates, G. P.,
Lehrach, H.,
and Wanker, E. E.
(1999)
Proc. Natl. Acad. Sci. U. S. A.
96,
4604-4609 |
| 45. | Ordway, J. M., Tallaksen-Greene, S., Gutekunst, C.-A., Bernstein, E. M., Cearley, J. A., Wiener, H. W., Dure, L. S. I., Lindsey, R., Hersch, S. M., Jope, R. S., Albin, R. L., and Detloff, P. J. (1997) Cell 91, 753-763[CrossRef][Medline] [Order article via Infotrieve] |
| 46. | Gusella, J. F., and MacDonald, M. E. (1998) Curr. Opin. Neurobiol. 8, 425-430[CrossRef][Medline] [Order article via Infotrieve] |
| 47. | Hackam, A. S., Wellington, C. L., and Hayden, M. R. (1998) Clin. Genet. 53, 233-242[Medline] [Order article via Infotrieve] |
| 48. |
Hughes, S. R.,
Khorkova, O.,
Goyal, S.,
Knaeblein, J.,
Heroux, J.,
Riedel, N. G.,
and Sahasrabudhe, S.
(1998)
Proc. Natl. Acad. Sci. U. S. A.
95,
3275-3280 |
| 49. | Cummings, C. J., Mancini, M. A., Antalffy, B., DeFranco, D. B., Orr, H. T., and Zoghbi, H. Y. (1998) Nat. Genet. 19, 148-154[CrossRef][Medline] [Order article via Infotrieve] |
| 50. |
Stenoien, D. L.,
Cummings, C. J.,
Adams, H. P.,
Mancini, M. G.,
Patel, K.,
DeMartino, G. N.,
Marcelli, M.,
Weigel, N. L.,
and Mancini, M. A.
(1999)
Hum. Mol. Genet.
8,
731-741 |
| 51. |
Chai, Y.,
Koppenhafer, S. L.,
Shoesmith, S. J.,
Perez, M. K.,
and Paulson, H. L.
(1999)
Hum. Mol. Genet.
8,
673-682 |
| 52. |
Gregori, L.,
Hainfeld, J. F.,
Simon, M. N.,
and Goldgaber, D.
(1997)
J. Biol. Chem.
272,
58-62 |
| 53. |
van Leeuwen, F. W.,
de Kleijn, D. P. V.,
van den Hurk, H. H.,
Neubauer, A.,
Sonnemans, M. A. F.,
Sluijs, J. A.,
Koycu, S.,
Ramdjielal, R. D. J.,
Salehi, A.,
Martens, G. J. M.,
Grosveld, F. G.,
Burbach, P. H.,
and Hol, E. M.
(1998)
Science
279,
242-247 |
| 54. |
Li, S.-H.,
Cheng, A. L.,
Li, H.,
and Li, X.-J.
(1999)
J. Neurosci.
19,
5159-5172 |
| 55. | Saigoh, K., Wang, Y.-L., Suh, J.-G., Yamanishi, T., Sakai, Y., Kiyosawa, H., Harada, T., Ichihara, N., Wakana, S., Kikuchi, T., and Wada, K. (1999) Nat. Genet. 23, 47-51[Medline] [Order article via Infotrieve] |
| 56. | Ozelius, L. J., Hewett, J. W., Page, C. E., Bressman, S. B., Kramer, P. L., Shalish, C., de Leon, D., Brin, M. F., Raymond, D., Corey, D. P., Fahn, S., Risch, N. J., Buckler, A. J., Gusella, J. F., and Breakefield, X. O. (1997) Nat. Genet. 17, 40-48[CrossRef][Medline] [Order article via Infotrieve] |
| 57. | Kitada, T., Asakawa, S., Hattori, N., Matsumine, H., Yamamura, Y., Minoshima, S., Yokochi, M., Mizuno, Y., and Shimizu, N. (1998) Nature 392, 605-608[CrossRef][Medline] [Order article via Infotrieve] |
| 58. | Kishino, T., Lalande, M., and Wagstaff, J. (1997) Nat. Genet. 15, 70-73[CrossRef][Medline] [Order article via Infotrieve] |
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