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Familial Dementia With Lewy Bodies
A Clinical and Neuropathological Study of 2 Families
Debby W. Tsuang, MD, MSc;
Aaron M. Dalan, BS;
Charisma J. Eugenio, BS;
Parvonah Poorkaj, PhD;
Pornprot Limprasert, MD, PhD;
Albert R. La Spada, MD, PhD;
Ellen J. Steinbart, RN, MA;
Thomas D. Bird, MD;
James B. Leverenz, MD
Arch Neurol. 2002;59:1622-1630.
ABSTRACT
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Background Dementia with Lewy bodies (DLB) is characterized by early dementia and
associated visual hallucinations, parkinsonism, and fluctuations in cognition.
Few families with DLB have been described with detailed clinical, pathological,
and genetic assessments.
Objective To investigate the clinical, neuropathological, and genetic characteristics
of families with 2 or more autopsy-proven cases of DLB.
Design Consecutive cases with the neuropathological diagnosis of DLB were reviewed
as part of a case series. Families included in this study have 2 or more autopsy-proven
cases of DLB available and a positive family history of dementia. We obtained
clinical and neuropathological data on all first-degree relatives. Neuropathological
evaluations included  -synuclein immunostaining for Lewy body detection.
We conducted apolipoprotein E genotyping and sequenced the -, ß-,  -synuclein,
and parkin genes.
Setting Subjects were selected from the neuropathology core of the University
of Washington's Alzheimer's Disease Research Center.
Patients The study investigated 2 families. Clinical information was obtained
from 10 individuals in family 1 and 7 individuals in family 2. Neuropathological
examinations were conducted in 3 individuals in family 1 and 2 individuals
in family 2.
Main Outcome Measures Each subject was examined for the presence of clinical symptoms and
neuropathological findings consistent with DLB.
Results While all affected individuals presented with dementia in both families,
only individuals in family 1 developed visual hallucinations and delusions.
Parkinsonism, if present, occurred later in the course of illness. Neuropathological
examination revealed Lewy bodies in all patients, while 1 patient from each
family also met the neuropathological criteria for Alzheimer disease. All
affected individuals carried at least 1 APOE (apolipoprotein
E)  4 allele, while there were no nucleotide alterations in the synuclein
or parkin genes.
Conclusions Familial DLB exists, although there is substantial clinical and neuropathological
heterogeneity within and between families. Additional clinicopathologic and
genetic studies are necessary to further our understanding of DLB.
INTRODUCTION
DEMENTIA WITH Lewy bodies (DLB) is characterized clinically by dementia,
visual hallucinations, parkinsonism, and fluctuations in cognition and attention.1 Recent evidence1 suggests
that Lewy body (LB)–associated dementias may constitute the second largest
neuropathological subgroup associated with dementing disorders, after Alzheimer
disease (AD). There is substantial clinical and neuropathological overlap
between DLB and AD and between DLB and Parkinson disease (PD). Patients with
DLB are frequently misdiagnosed as having AD, although they are more likely
to exhibit hallucinations and/or delusions earlier in the course of illness
than patients with AD.2 Similarly, motor signs
and symptoms observed in patients with PD are frequently found in patients
with DLB. However, parkinsonism (if present in patients with DLB) is often
less severe than in patients with PD. If DLB is a pathophysiologically distinct
entity, our ability to distinguish DLB from AD and PD has important clinical
and research implications.
The Consortium on Dementia With Lewy Bodies1
has developed guidelines for the clinical and neuropathological diagnosis
of DLB. The guidelines for the clinical diagnosis of DLB require the presence
of progressive cognitive decline and the presence of at least 2 of the following
core features: (1) spontaneous parkinsonian signs and symptoms, (2) visual
hallucinations, and (3) fluctuations in consciousness early in the course
of illness.1 In addition, the DLB criteria
stipulate that if parkinsonism precedes dementia by more than 1 year, the
disorder is classified as PD with dementia. Although the specificity (correctly
not diagnosing DLB) of these diagnostic criteria is high, the sensitivity
(correctly diagnosing DLB) is modest.3-5
One of the reasons for this finding may be the clinical variability observed
among patients with DLB. While all patients exhibit cognitive decline, the
presence of the other core features is less consistent. In particular, it
is unclear why some individuals develop hallucinations and/or delusions while
others do not.6 One way to address these questions
is to identify kindreds with familial DLB to investigate whether core clinical
symptoms aggregate within these families.
Several studies have described families with inherited parkinsonism
and dementia. However, most of those families are characterized by parkinsonism
preceding dementia by many years.7-8
A few described families have included some individuals who presented with
dementia, some of whom develop comorbid parkinsonism while others never do.8-10 These families may
be examples of familial DLB. Unfortunately, there is a paucity of neuropathological
description in these families, with LB pathological features confirmed at
most in only 1 family member.8 Therefore, it
is difficult to assess whether all affected individuals had the same disorder.
Molecular genetic studies have identified multiple genetic risk factors
in patients with AD11 and PD.12
However, few studies have investigated genetic risk factors in patients with
DLB. The association between the APOE (apolipoprotein
E) 4 allele and DLB has been inconsistent.13-16
In addition, other studies17-18
have reported that genetic risk factors associated with PD (eg, CYP2D6 and -synuclein) are not present in patients with DLB.
Additional linkage analysis and candidate gene studies in patients with DLB
are necessary. Eventual identification of susceptibility genes in patients
with DLB will improve the classification of this disorder and our understanding
of the underlying pathophysiological features.
To investigate clinical and neuropathological variability and the genetic
risk factors in patients with DLB, we identified several families with multiple
affected individuals who presented with dementia and later developed parkinsonism.
Instead of relying on the clinical diagnosis of DLB, we selected families
based on the neuropathological diagnosis of DLB in 2 or more family members.
Herein, we describe the clinical, neuropathological, and genetic characteristics
of 2 families.
METHODS
Eight families at the University of Washington's Alzheimer's Disease
Research Center with at least 1 autopsy-proven case of DLB and multiple other
family members with dementia were initially eligible for this study. Two families
had 2 or more autopsy-proven cases of DLB (according to the neuropathological
criteria of McKeith et al1) and were included
in the present study.
As approved by the University of Washington's Institutional Review Board,
we obtained informed consent from family members who were willing to participate.
Medical records were obtained and systematically reviewed for the presence
of parkinsonian signs and symptoms, behavioral disturbances, and cognitive
decline. Detailed clinical histories were obtained from the next of kin using
a semistructured dementia questionnaire.19
Medical records were obtained for 10 individuals in family 1 and 7 individuals
in family 2. Because of inconsistent documentation and report of fluctuations
in attention and cognition, we could not reliably assess these symptoms. Two
of us (D.W.T. and J.B.L.) conducted in-person detailed neurological and behavioral
assessments with 4 individuals in family 2.
Neuropathological examinations were performed in 3 individuals in family
1 and 2 individuals in family 2. All patients underwent a standard neuropathological
workup, including hematoxylin-eosin (H&E), modified Bielschowsky, and
thioflavine S staining. Of 5 autopsy cases, 4 had postmortem tissue available
for additional immunohistological studies. In these cases, we performed -synuclein
immunostaining (antibody LB509, dilution, 1:400; Zymol, San Francisco, Calif)
and extranigral sampling to fully characterize LB pathological features.20-22 A neuropathological
review for the presence of LBs in the substantia nigra (SN), hippocampus,
parahippocampal gyrus, amygdala, and cingulate gyrus was conducted. We defined
an LB "positive" case as one having either H&E-positive LB inclusions
in the SN or greater than 5 -synuclein–positive LB inclusions
in an extra brainstem region. In addition, in the absence of LB inclusions
in the SN, cases with 6 or more -synuclein–positive cytoplasmic
inclusions in the amygdala would also be considered as positive for LB pathological
features. These latter cases would be classified as "amygdala predominant"
DLB cases consistent with previous reports.22-23
Genomic DNA was extracted from lymphocytes or skin fibroblast culture.
DNA from 11 individuals were available for APOE genotyping
using the restriction digest methods of Hixson and Vernier.24
Genomic DNA from 1 affected individual (randomly selected) in each family
was screened for -, ß-, and -synuclein and parkin mutations.
Polymerase chain reaction (PCR), with the use of primers flanking each exon,
was performed. Primer sequences (including 3 new primers: A5R, A7-2F, and
A7-1R), expected product sizes, and annealing temperature are described in
detail elsewhere.25 The complete genomic sequence
encompassing the -synuclein gene is available through GenBank (accession
numbers AF163864 and NT_006204; NCBI, Bethesda, Md). The -synuclein
complementary DNA (accession number XM_003494) is encoded by 6 exons and 1
alternatively spliced (1') exon that span a genomic distance of greater
than 116 kb. Polymerase chain reaction products were purified using the QIA-quick
purification kit (QIAGEN, Valencia, Calif) before ABI PRISM BigDye Terminator
(ABI, Foster City, Calif) cycle sequencing on an ABI 377 sequencer. Both strands
were sequenced. The ß-synuclein gene, encoded by 5 exons, encompasses
a genomic distance of approximately 12.8 kb (accession numbers AF053134-AF053136
and NT_006725). Previously published primer sets will be used for PCR amplification
from genomic DNA.26 The -synuclein gene
is similarly encoded by 5 exons and spans 46 kb (excluding promoter sequences)
(accession number AF044311). Primer pairs for genomic sequencing have been
published previously.27
The parkin gene is encoded by 12 exons. Mutation screening methods used
primer sets published by Kitada et al,28 as
well as nested primers for sequencing and new primer pairs designed to amplify
genomic fragments containing a minimum of 150 nucleotides of flanking intronic
sequence for each exon. The complete human genomic sequence for parkin is
available through GenBank (http://www.ncbi.nlm.nih.gov), accession
number NT_007122.29-30 Exons and
flanking intronic splice junctions were PCR-amplified, agarose gel–purified
(Gene-clean III; Bio101, Luton, Bedfordshire, England), and directly sequenced
by dye-terminator cycle sequencing (BigDye) using an ABI 377 sequencer. Both
strands were sequenced. Gene dosage analysis using real-time fluorescence-based
PCR quantitation (ABI 7700 Sequence Detector) was performed to determine parkin
exon copy number. Parkin exons were amplified with 5' FAM/3'TAMRA
(ABI) dual-labeled probes and multiplexed with the amplification of an 84
base pair fragment of a single copy human ß-actin gene (chromosome 7;
5'-VIC/TAMRA-3' [ABI] dual label probe) as an internal copy number
control. Standard curves were generated for each parkin exon and for ß-actin
using control human genomic DNA. The number of PCR cycles required before
the ABI 7700 detects the parkin exon product was plotted against the parkin
standard curve, thus calculating a relative copy number for each exon. Parkin
exon copy number was then normalized to the single copy actin gene within
each multiplexed reaction and to a normal reference individual, thus determining
the number of copies per genome. All experiments were performed in triplicate.
REPORT OF CASES
FAMILY 1
In this family, there were 8 affected individuals in 2 generations (Figure 1). Their mean age of onset was 70.9
(SD, 5.4) years, with a mean age at death of 77.2 (SD, 3.9) years. All 8 affected
individuals exhibited cognitive decline as their first neuropsychiatric symptom.
In addition, of the 8 individuals with dementia, 5 developed subsequent parkinsonism
(resting tremor, cogwheel rigidity, and/or bradykinesia) and 4 exhibited psychotic
symptoms (2 of these 4 had visual hallucinations) (Table 1). Brief descriptions of individuals in this family follow.
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Figure 1. Pedigree from family 1. Circles
indicate females; squares, males; and a slash through a symbol, deceased individuals.
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Table 1. Clinical Characteristics, Source of Information, and APOE
Genotypes in Families 1 and 2*
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I:1
This subject read daily and worked in his garden until his death. There
was no evidence of cognitive impairment or parkinsonism.
II:1
This subject developed dementia at the age of 72 years. She was unable
to live on her own because of her forgetfulness. Her judgment was impaired,
and she inadvertently started several stove fires. She did not have resting
tremor, bradykinesia, or gait disturbance.
III:1
This subject had cognitive decline beginning around the age of 67 years.
He could not manage his own finances. A review of medical records indicates
that he was unable to comprehend directions during a physical examination.
No formal cognitive testing was conducted. He did not have resting tremor,
bradykinesia, or gait disturbances.
III:3
This subject was diagnosed as having AD with PD features at the age
of 81 years. He initially had difficulty keeping track of his finances (at
the age of 73 years) and had poor executive function and judgment. Later,
he developed bradykinesia, stooped posture, axial rigidity, and cogwheel rigidity.
He did not have resting tremor. He also developed paranoid ideation and called
the police on at least 1 occasion. When the police came to investigate, he
stated that a neighbor had actually made the telephone call. The neuropathological
report and additional tissue specimens were available for this subject (Table 2).
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Table 2. Clinical and Neuropathological Characteristics in 2 Families With DLB*
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III:5
This subject developed cognitive impairment at the age of 79 years.
He was unable to organize his home or complete multistep tasks. The family
reported an increase in irritability and agitation. He has accused his family
of "trying to make me think I'm crazy." He did not have resting tremor, bradykinesia,
or gait disturbances.
III:6
This subject does not have any evidence of cognitive decline. He continues
to be physically and mentally active. He reads regularly and hikes 4.8 km
at least once a week. He does not have resting tremor, bradykinesia, or gait
disturbances.
III:7
This subject developed cognitive decline around the age of 77 years.
He had difficulty remembering words and got lost while driving in his hometown.
He developed gait instability and fell on several occasions. He also developed
a stooped posture and bradykinesia, but did not have resting tremor. The patient
had visual hallucinations, reported as seeing his deceased relatives. He believed
that they lived with him and routinely conversed with them.
III:8
This subject first showed signs of cognitive decline at the age of 67
years. She became lost in her hometown and was unable to balance her checkbook.
On physical examination, there was evidence of increased muscle tone, mild
bradykinesia, and masked facies. She did not have resting tremor but was diagnosed
as having PD at the age of 74 years. She also developed emotionally intense
visual hallucinations, reported as seeing chickens pecking at her eyes. The
neuropathological report and additional tissue specimens were available for
this subject (Table 2).
III:9
This subject presented with cognitive deficits at the age of 63 years
and was diagnosed as having AD at the age of 69 years. She was unable to maintain
her home and developed problems with word finding. Physical examination findings
were significant for mild cogwheel rigidity. However, there was no evidence
of resting tremor or bradykinesia. She also developed paranoid ideations that
the neighbors across the street were spying on her. She spent an extensive
amount of time sitting by the window, making sure her neighbors would not
bother her. The neuropathological report was available for this patient, but
additional tissue specimens were unavailable for immunohistochemical staining
(Table 2).
III:11
This subject developed cognitive impairment at the age of 69 years and
was diagnosed as having AD at the age of 75 years. He was unable to handle
his finances and got lost while driving in familiar neighborhoods. His wife
reported that he had progressive bradykinesia and developed a stooped posture.
No resting tremor or cogwheel rigidity was reported.
FAMILY 2
This family had 6 affected individuals in 1 generation (Figure 2). Their mean age of onset was 69.8 (SD, 11.1) years. All
affected individuals presented initially with cognitive decline. In addition,
4 of the 6 individuals had parkinsonism that either presented concurrently
with dementia or developed later in the disease. None of the affected individuals
developed hallucinations or delusions (Table 1). Brief descriptions of individuals in this family follow.
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Figure 2. Pedigree from family 2. The pedigree
has been altered to ensure confidentiality. A slash through a symbol indicates
deceased individuals.
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I:1
This subject had evidence of mild cognitive impairment on neurological
examination, with word recall difficulty at the age of 83 years. On physical
examination, there was evidence of a mildly stooped posture, bradykinesia,
and difficulty performing rapid alternating movements. S/he did not have resting
tremor or cogwheel rigidity.
I:2
This subject developed problems managing his/her finances at the age
of 76 years. S/he subsequently became lost in his/her own neighborhood. On
physical examination, s/he had mild bradykinesia, stooped posture, mild postural
instability, masked facies, and hypophonia. S/he did not have resting tremor
or cogwheel rigidity.
I:3
This subject had mild cognitive impairment on neurological examination
at the age of 80 years, difficulty with word recall, and difficulty with sentence
completion. There was also evidence of gait instability, bradykinesia, and
slowing of rapid alternating movements. There was no resting tremor or cogwheel
rigidity.
I:4
This subject developed cognitive disturbances at the age of 63 years
and was diagnosed as having AD at the age of 70 years. Initially, there was
difficulty with word finding, short-term memory, and managing his finances.
On physical examination, there was bradykinesia, a slightly stooped posture,
and loss of facial expression. There was no resting tremor or cogwheel rigidity.
I:5
This subject first developed cognitive disturbance at the age of 58
years with problems managing finances. S/he was diagnosed as having AD at
the age of 65 years and died at a care facility. There was a long history
of alcohol dependence, including withdrawal symptoms such as delirium tremens.
There was no evidence of resting tremor, bradykinesia, or cogwheel rigidity.
The neuropathological report and additional tissue specimens were available
for this subject (Table 2).
I:6
This subject had no evidence of cognitive impairment or functional decline
at the age of 74 years. There was no evidence of resting tremor, bradykinesia,
or cogwheel rigidity.
I:7
This subject had short-term memory loss at the age of 59 years. S/he
subsequently became apraxic, exemplified by his/her inability to use tools
or utensils. The patient had a long history of alcohol abuse. S/he was admitted
for alcohol detoxification several times. The medical history was significant
for delirium tremens, with reports of visual hallucinations of bugs and snakes.
These symptoms resolved once s/he was treated for alcohol withdrawal. There
was mild bradykinesia, but no resting tremor or cogwheel rigidity. The neuropathological
report and additional tissue specimens were available for this subject (Table 2).
NEUROPATHOLOGICAL FEATURES
Autopsies were performed on 3 affected individuals in family 1 and 2
affected individuals in family 2. Neuropathological findings are summarized
in Table 2. Brain tissue from
1 individual (subject III:9 in family 1) was not available for -synuclein
immunohistochemistry. However, this patient had definite LB pathological features
in the SN on H&E staining and was, therefore, classified as positive for
LB pathological features. Two patients from each family had postmortem tissue
available for additional -synuclein immunohistochemical studies.
Overall, 2 individuals in family 1 (subjects III:3 and III:9) and 1
in family 2 (subject I:5) had typical LB inclusions in the SN on H&E staining
(Table 2 and Figure 3A). Two patients with additional tissue available (subject
III:3 in family 1 and subject I:5 in family 2) also had LB pathological features
detected by -synuclein immunohistochemistry in the SN and amygdala
(Table 2 and Figure 3B and C). One subject from each family (subject III:8 in
family 1 and subject I:7 in family 2) did not have SN LBs detected with either
H&E or -synuclein immunostaining. However, both had 6 or more -synuclein–positive
cytoplasmic inclusions in the amygdala (Table 2 and Figure 3D).
These latter 2 patients are similar to the amygdala-predominant patients described
by other investigators.22-23,32
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Figure 3. A, Lewy body (arrow) in a substantia
nigra neuron of a patient with dementia with Lewy bodies (hematoxylin-eosin,
original magnification, x500). B, -Synuclein immunostaining of
Lewy bodies (large arrow) and Lewy neurites (small arrows) in the substantia
nigra (original magnification, x500). C, -Synuclein–immunopositive
inclusions (arrow) in the amygdala of a patient with additional brainstem
Lewy bodies (original magnification, x250). D, -Synuclein–immunopositive
inclusions (large arrow) and neuritic plaques (small arrow) in a patient without
brainstem Lewy bodies (original magnification, x250). Parts A, B, and
C are from subject III:3 in family 1; part D, subject I:7 in family 2.
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Modified Bielschowsky silver staining for AD pathological features showed
that 1 individual from each family (subject III:8 in family 1 and subject
I:7 in family 2) had sufficient senile plaque and neurofibrillary tangle pathological
features (Braak stage V-C and VI-C, respectively) to meet the neuropathological
criteria for high likelihood of AD (per Reagan Institute Working Group on
Diagnostic Criteria for the Neuropathological Assessment of Alzheimer's Disease/National
Institute on Aging criteria).33 The remaining
3 patients (subjects III:3 and III:9 in family 1 and subject I:5 in family
2) had moderate to frequent senile plaques in limbic and cortical regions,
but only mild to moderate neurofibrillary tangle pathological features that
were limited to limbic structures (Braak stage III for all 3). These latter
patients would fulfill National Institute on Aging/Reagan Institute Working
Group on Diagnostic Criteria for the Neuropathological Assessment of Alzheimer's
Disease criteria for intermediate likelihood of AD.
MOLECULAR GENETICS
Seven individuals in family 1 (6 affected and 1 at risk) and 4 individuals
(all affected) in family 2 had DNA available. In family 1, 5 affected individuals
carried the APOE 3/4 genotype, while
the other affected individual had an APOE 4/4
genotype. One at-risk individual also had the APOE 3/4
genotype (Table 1). In family
2, 3 affected individuals had the APOE 4/4
genotype, while 1 affected individual had the APOE 3/4
genotype (Table 1).
Genetic analyses showed that there were no nucleotide alterations in
the -, ß-, or -synuclein or parkin genes in 1 affected
individual selected from each family. There was no deletion or duplication
in the parkin gene in the individuals examined.
COMMENT
To our knowledge, most previously published studies7-8,34-35
of families with parkinsonism and dementia have included individuals who presented
with parkinsonism. Only 2 published reports8-9
included families with individuals who presented with dementia. However, in
one family, only 1 autopsy was reported,8 while
in the other family, none of the individuals who presented with dementia underwent
an autopsy.9 Therefore, we are unable to determine
whether affected individuals had clinical and neuropathological DLB.
The present study describes the clinical, neuropathological, and genetic
characteristics of persons with dementia in 2 families that included 2 or
more autopsy-proven cases of DLB. We found that substantial clinical and neuropathological
variability exists within each family. All affected individuals exhibited
cognitive decline that either preceded or occurred concurrently with parkinsonism.
However, not all affected individuals exhibited hallucinations, delusions,
or parkinsonism.
We observed the aggregation of hallucinations and/or delusions in one
family, but not in the other. These observations are consistent with previous
findings that some families with hereditary neurodegenerative disorders are
more susceptible to develop hallucinations and/or delusions than other families
with the same disorder. Several reports suggest that some families with Huntington
disease,36-37 frontotemporal dementia,38 and AD39-40
have a higher susceptibility to developing hallucinations and/or delusions.
Even though visual hallucinations and systematized delusions are part of the
clinical criteria for the diagnosis of DLB,1
to our knowledge, there are no reports that hallucinations and/or delusions
are more likely to aggregate in some families with DLB. The present case study
provides preliminary evidence that some families with DLB have an increased
susceptibility to developing hallucinations and/or delusions.
The mechanisms underlying the development of hallucinations and delusions
in patients with dementia are not well understood. One previous study41 showed no clear LB regional distribution associated
with psychosis. Others42 have suggested that
selective loss of different neuronal or neurotransmitter populations may be
associated with prominent hallucinations and delusions. Meanwhile, others
postulate that differences in genetic background may be associated with the
development of hallucinations and delusions. Several reports found an association
between a 5-hydroxytryptamine 2A receptor polymorphism,43-44
dopamine D1 and D3 receptor polymorphisms,45
a serotonin transporter polymorphism, and psychotic symptoms in patients with
AD. Interestingly, a different polymorphism close to the dopamine D2 receptor
gene was associated with hallucinations in patients with PD.46
Additional genetic studies are necessary to confirm these associations.
The APOE 4 allele is associated with
familial and sporadic late-onset AD47-48
but not as clearly with PD.49-50
However, one recent study51 showed that the APOE 4 allele may play a role in dementia associated
with PD. The APOE 4 allele is associated with
an increase in the number of neocortical LBs and amyloid plaques in patients
with PD, thus, possibly predisposing to the development of dementia.52 Investigations14-16,53-54
of the APOE 4 allele as a genetic risk factor
for DLB have led to conflicting results. Some investigations55
have attributed the association between the APOE 4
allele and DLB to the presence of concomitant AD pathological features in
patients with DLB. However, in a large sample of autopsy-proven cases of DLB
without substantial neurofibrillary tangle pathological features, Harrington
and colleagues13 still found that the APOE 4 allele frequency was higher (37%) compared
with that of normal control subjects (15%). An earlier case report56 described an APOE 4
homozygous individual with widespread cortical and subcortical LB pathological
features in the absence of severe neuritic plaque and neurofibrillary tangle
pathological features. In the present study, all 10 affected individuals with
DNA available carried an APOE 4 allele. Our
findings support the hypothesis that the APOE 4
allele may be an independent risk factor in the development of LB pathological
features. However, further delineation of the molecular genetics of families
with DLB is necessary.
The discovery of mutations in the -synuclein gene in familial
PD57 led to the development of highly specific
antibodies to this synaptic protein; these antibodies are highly sensitive
for detecting LB pathological features in familial and sporadic PD.58 Investigations20, 59
using -synuclein antibodies and extranigral sampling (specifically
in the amygdala) have found a high frequency of LB pathological features in
familial and sporadic AD. These results suggest that the use of -synuclein
immunostaining in brainstem and extrabrainstem regions, along with traditional
H&E staining of the SN, is necessary to fully evaluate whether LB pathological
features exist.
In our study, the degree of AD pathological features varied within both
families, with some individuals having sufficient pathological features for
a diagnosis of AD and others having only modest AD-related changes. Although
all affected individuals with autopsy results available had LB inclusions,
several had classic LBs in the SN and amygdala while others had LB pathological
features only in the amygdala. The LB pathological features were detected
only with -synuclein immunostaining in the amygdala. By using less
sensitive detection methods, these patients would be classified as not having
LB pathological features. Interestingly, these patients with amygdala-predominant
LB pathological features had severe AD pathological features. The clinical
and pathological significance of these patients with amygdala-predominant
DLB remains unclear. Further clinical and neuropathological examinations in
patients with familial and sporadic DLB are necessary to investigate the significance
of this pattern of LB pathological features.
We identified 2 families who presented with dementia and had evidence
of LB pathological features in all affected members with autopsy results.
These families may represent examples of familial DLB. Additional clinical,
neuropathological, and genetic studies in these and other families are necessary
to further clarify the etiology of familial DLB. Studies in families with
autopsy-proven DLB can provide important insights into the pathophysiological
features of this increasingly recognized disease. In particular, identification
of the susceptibility genes in patients with DLB could increase our understanding
of the pathophysiological features of this disorder. This knowledge will help
to differentiate DLB from AD and PD.
AUTHOR INFORMATION
Accepted for publication May 14, 2002.
Author contributions: Study concept and design (Drs Tsuang, Bird, and Leverenz and Mr Dalan); acquisition
of data (Drs Tsuang and Poorkaj, Mr Dalan, and Mss Eugenio
and Steinbart); analysis and interpretation of data (Drs Tsuang, Poorkaj, Limprasert, and La Spada); drafting of the manuscript (Dr Tsuang, Mr Dalan, and Mss Eugenio and Steinbart); critical
revision of the manuscript for important intellectual content (Drs Tsuang, Poorkaj, Limprasert, La Spada, Bird, and Leverenz); statistical
expertise (Dr Tsuang); obtained funding (Dr Tsuang); administrative, technical, and material support (Drs Tsuang, Poorkaj, Limprasert, and Leverenz, Mr Dalan, and
Mss Eugenio and Steinbart); study supervision (Drs
Tsuang, La Spada, Bird, and Leverenz).
This study was supported by a pilot proposal (1999-2000) from the Alzheimer's
Disease Research Center, University of Washington; and by Veterans Integrated
Service Network 20 from the Veterans Affairs Northwest Network Mental Illness
Research, Education, and Clinical Center.
We thank Gerard Schellenberg, PhD, for APOE
genotyping, and Lynne Greenup for technical assistance.
Corresponding author and reprints: Debby W. Tsuang, MD, MSc, Department
of Veterans Affairs Northwest Network Mental Illness Research, Education,
and Clinical Center, VA Puget Sound Health Care System, 1660 S Columbian Way,
Mailstop 116MIRECC, Seattle, WA 98108 (e-mail: dwt1{at}u.washington.edu).
From the Department of Veterans Affairs Northwest Network Mental Illness
Research, Education, and Clinical Center (Drs Tsuang and Leverenz and Ms Eugenio)
and the Geriatric Research, Education, and Clinical Center, VA Puget Sound
Health Care System (Drs Poorkaj and Bird and Ms Steinbart); the Departments
of Psychiatry and Behavioral Sciences (Drs Tsuang and Leverenz), Neurology
(Drs La Spada, Bird, and Leverenz and Ms Steinbart), Laboratory Medicine (Drs
Limprasert and La Spada), and Internal Medicine (Drs Poorkaj and La Spada),
and the School of Medicine (Mr Dalan), University of Washington; and the Parkinson's
Disease Research, Education, and Clinical Center (Dr Leverenz), Seattle, Wash.
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