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DNA-binding and photocleavage, cytotoxicity, apoptosis and antioxidant activity studies of ruthenium(II) complexes
Neurochem Res (2011) 36:1706–1714
DOI 10.1007/s11064-011-0437-y
ORIGINAL PAPER
Mice Lacking Major Brain Gangliosides Develop Parkinsonism
Gusheng Wu • Zi-Hua Lu • Neil Kulkarni •
Ruchi Amin • Robert W. Ledeen
Accepted: 24 February 2011 / Published online: 12 March 2011
Ó The Author(s) 2011. This article is published with open access at Springerlink.com
Abstract Parkinson’s disease (PD) is the second most
prevalent late-onset neurodegenerative disorder that affects
nearly 1% of the global population aged 65 and older.
Whereas palliative treatments are in use, the goal of
blocking progression of motor and cognitive disability
remains unfulfilled. A better understanding of the basic
pathophysiological mechanisms underlying PD would help
to advance that goal. The present study provides evidence
that brain ganglioside abnormality, in particular GM1, may
be involved. This is based on use of the genetically altered
mice with disrupted gene Galgt1 for GM2/GD2 synthase
which depletes GM2/GD2 and all the gangliotetraose
gangliosides that constitute the major molecular species of
brain. These knockout mice show overt motor disability on
aging and clear indications of motor impairment with
appropriate testing at an earlier age. This disability was
rectified by L-dopa administration. These mice show other
characteristic symptoms of PD, including depletion of
striatal dopamine (DA), loss of DA neurons of the substantia nigra pars compacta, and aggregation of alpha
synuclein. These manifestations of parkinsonism were
largely attenuated by administration of LIGA-20, a membrane permeable analog of GM1 that penetrates the blood
brain barrier and enters living neurons. These results suggest that perturbation of intracellular mechanisms mediated
by intracellular GM1 may be a contributing factor to PD.
Keywords Parkinson’s disease � GM1 ganglioside �
LIGA-20 � Dopaminergic neurons � Alpha synuclein
Abbreviations
Ab
antibody
a-syn
alpha-synuclein
BSS
balanced salt solution
CtxB
B subunit of cholera toxin
DA
dopamine or dopaminergic
DOA
days of age
DOPAC dihydroxyphenyl acetic acid
ER
endoplasmic reticulum
HRP
horseradish peroxidase
5-HT
5-hydroxytryptamine (serotonin)
5-HIAA 5-hydroxyindole acetic acid
IP
intraperitoneally
KO
knockout
MPTP
1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine
PBS
phosphate buffered saline
PD
Parkinson’s disease
SNpc
substantia nigra pars compacta
TH
tyrosine hydroxylase
VTA
ventral tegmental area
WT
wild type
Introduction
Special Issue: In Honor Dr. Robert Yu.
G. Wu (&) � Z.-H. Lu � N. Kulkarni � R. Amin � R. W. Ledeen
Department of Neurology and Neurosciences, New Jersey
Medical School, UMDNJ, 185 So. Orange Ave., MSB-H506,
Newark, NJ 07103, USA
e-mail: ledeenro@umdnj.edu
123
Gangliosides are well recognized mediators of certain
essential signaling pathways in the nervous system and
other organs [1], and a growing number of proteins
involved in such pathways are seen to function in association with one or another ganglioside. Considerable insight
into ganglioside-protein interactions has been gained from
�Neurochem Res (2011) 36:1706–1714
a study of animals with mutated genes required for ganglioside biosynthesis. One of the most studied is a mouse
with disrupted gene Galgt1 which encodes the enzyme
UDP-GalNAc:lactosylceramide/GM3/GD3 b-1,4-N-acetylgalactosaminyltransferase (GM2/GD2 synthase; GalNAcT; EC 2.4.1.92). This mutation results in elimination of
GM2 and GM1 along with other members of the gangliotetraose family which compromise [90% of CNS gangliosides. Such mice suffer a slight reduction in neural
conduction velocity [2] in addition to decreased central
myelination and axonal degeneration [3]. They also show
progressive behavioral neuropathies including deficits in
reflexes, strength coordination and balance [4]. At the
cellular level, cultured neurons from such mice were found
deficient in Ca2? regulation as reflected in vitro by
degeneration in the presence of depolarizing levels of K?
[5] and in vivo by enhanced susceptibility to kainateinduced seizures [6].
The present study has probed further into the movement
disorder and pathophysiological manifestations of such
knockout (KO) mice and found a constellation of symptoms
strongly representative of Parkinson’s disease (PD). A primary neuropathological feature of the sporadic form of PD
is the substantial depletion of dopaminergic (DA) neurons
in the substantia nigra pars compacta (SNpc), although loss
of other neuronal types can also occur prior or subsequent to
that in the SNpc [7]. In addition to accompanying decrease
of dopamine (DA) in SNpc and striatum, a prominent
neuropathological feature is accumulation of alpha-synuclein (a-syn) within cytoplasmic inclusions termed Lewy
bodies. In contrast to the much rarer familial cases, which
show generally similar neuropathology, the etiology of
sporadic PD is not well understood as reflected in the several theories that have been proposed. Most of these are
based on a variety of interactions between environmental
factors and genetic predisposition.
Rodents subjected to neurotoxins have been widely used
to model some of the key features of PD, the most prominent being 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine
(MPTP), 6-hydroxy dopamine, rotenone, and paraquat [8].
The above mentioned GalNAcT-/- KO mouse has the
advantage as a model in its spontaneous acquisition of
parkinsonian symptoms, thus avoiding the potentially
confounding influence of extraneous toxins. The present
study chronicles these parallel symptoms and provides
evidence suggesting GM1 as the crucial missing ganglioside. This idea correlates with the many previous studies
demonstrating GM1 amelioration of parkinsonism in
mouse and primate models of PD [9–13] as well as in PD
patients [14, 15]. In that light such treatment might eventually be viewed as a form of replacement therapy pending
verification of the hypothesis that susceptible DA cells in
PD suffer deficiency of GM1.
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Methods
Animals and Behavioral tests
A breeding pair of heterozygotes with disrupted gene for
GM2/GD2 synthase (C57BL/6 background), created by
Dr. Richard Proia and coworkers [16] was provided as a
gift by Dr. Ronald Schnaar (Johns Hopkins University
School of Medicine). Animals were maintained in the
University of Medicine and Dentistry of New Jersey
Research Animal Facility with 12 h light/dark cycles.
They were genotyped by PCR analysis as described [5].
All animal procedures were in accord with the guidelines
of the UMDNJ Animal Care and Use Committee
(IACUC).
Wild type (WT) and KO mice of both genders at 35 and
200 days of age (DOA) were used. To determine physical
impairment, a grip-hanging test was employed in which the
mouse clings with forepaws to a narrow horizontal rod
positioned 50 cm above a pillow and hang time to fall is
measured [17]; the mouse’s tail is gently held by experimenter to prevent climbing with hind legs. Hang times in
three consecutive trials, with rest intervals of 20 min, were
averaged. The second test, adhesive removal, was used to
determine motor response to sensory stimulus [18]. A small
piece of adhesive is applied to the snout and the time to
removal by forepaw is recorded. Durations longer than
120 s were counted as 120 s. Each animal was measured
five times and the shortest three times were averaged. In
rescue experiments, animals were injected intraperitoneally
(IP) with GM1 (30 mg/kg), LIGA-20 (2.5 mg/kg) or balanced salt solution (BSS; Alcon, Fort Worth, TX) 39/week
over 5 weeks and then subjected to behavioral tests. GM1
and LIGA-20 were gifts from the Fidia Research Laboratories (Abano Terme, Italy). To test the rescue effect of
L-dopa on impairment, KO mice were IP injected with
L-dopa (20 mg/kg) plus carbidopa (3 mg/kg) in BSS and
subjected to behavioral tests 3 h after injection; this was
compared to test results before L-dopa administration.
Statistical analysis was via two-tailed Student’s t test. After
behavior tests, mice were perfused (see below) and the
frozen brains stored prior to histochemical and biochemical
assays.
Histochemical Analyses
Animals were subjected to cardiac perfusion with phosphate buffered saline (PBS) followed by 4% parafomaldehyde in PBS. The brains were fixed overnight or longer
in 4% paraformaldehyde followed by transfer to 30%
sucrose (cryoprotection) in PBS and storage at 4°C.
Coronal frozen sections (25 lm) were cut from the midbrain and stained with CtxB-FITC (1 lg/ml; Sigma;
123
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St. Louis, MO) and anti-tyrosine hydroxylase (TH) antibody (Ab) (Millipore; Billerica, MA; 1:1000) plus 2nd Ab
linked to Texas red. Other sections were stained with above
anti-TH Ab plus Texas red 2nd Ab and anti-a-syn Ab (BD
Science, 1:2000) plus 2nd Ab linked to FITC. Immunofluorescence in the SNpc region was photographed with
40X objective lens. Stereological analysis was carried out
on the SNpc and ventral tegmental area (VTA) of brains
from three KO treated with BSS, three KO mice treated
with LIGA-20 (2.5 mg/kg), and three WT brains; this
was done at the Rutgers University Molecular Histology
Center (Dr. Eric Richfield; http://eohsi.rutgers.edu/mhc/).
In preparation the brains were perfused, fixed and cryoprotected as above. Using the above anti-TH Ab with
Texas red 2nd Ab, the total number of TH? neurons in the
SNpc and VTA were counted using the optical fractionator
and previously described counting criteria [19, 20]. The
right and left sides were counted in each brain. Regions of
interest (ROI) were outlined at low magnification (4X
objective) and sampled at high magnification (100X oil
immersion objective) using StereoInvestigator (MicroBrightField, VT). ROI were selected based on literature
descriptions and their consistent visual identification at 4X.
For the area sampling fraction (asf) a sampling frame of
size of 55 9 55 lm (3,025 lm2) and a grid area of
123 9 123 lm (15,129 lm2) yielding an asf of 20% were
employed. All choices were made to obtain sufficient
precision for TH? neuron counts in the SNpc and VTA.
Immunoblot Assay for Alpha-synuclein
Freshly collected brains from PBS perfused mice were
employed and the midbrain cut into 250 lm coronal
sections with a vibratome sectioning system in cold PBS.
The entire SN region, including compact and reticulum,
was isolated with a dissecting microscope. The pooled
sections were extracted with Cell Lysis Buffer (Cell
Signaling, Danvers, MA) and aliquots containing 20 lg
protein were resolved with SDS–PAGE on a 4–15%
gradient gel (Bio-Rad, Hercules, CA). After transfer to
PVDF membrane, proteins were blotted with anti-a-syn
antibody (1:1000; Santa Cruz Biotec; Sanda Cruz, CA)
followed by 2nd Ab linked to horseradish peroxidase
(HRP). Protein bands were revealed by ECL reagent
(Amersham; Piscataway, NJ) on film. Anti-actin Ab
(Sigma) was run in parallel for loading control. The
optical density of actin and a-syn polymer (ranging from
34 to 170 Kd) blots was scanned and quantified by
AlphaEase FC imaging system (Alpha Innotech, San
Leandro, CA). Three brains in each group were assayed,
the data normalized with respect to actin and statistically
analyzed with the Student’s t-test.
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Neurochem Res (2011) 36:1706–1714
Neurochemistry
For DA assay, striatal samples prepared as above were each
homogenized and sonicated in 0.7 ml cold 0.4 N perchloric
acid containing 70 ng dihydroxybenzylamine as internal
standard for 20 min. This was centrifuged for 20 min at
16,000 g, the supernatant filtered through a Millex-GV
syringe filter (0.22 lm; Millipore) and the filtrate stored at
-20°C prior to analysis. One hundred ll was applied to a
DIONEX ICS-3000 HPLC system with a 5-lm C8
Acclaim 120 column and electrochemical detector (0.7 V).
Concentrations of DA and dihydroxyphenylacetic acid
(DOPAC) were determined from peak areas adjusted to
aliquot size, internal standard, and protein content. Also
assayed by HPLC was serotonin (5-HT) and its metabolite,
5-hydroxyindole acetic acid (5-HIAA). Protein content was
determined by the Lowry method following digestion of
the HClO4 pellet several hrs in NaOH/SDS [21].
Results
The impaired movement of KO mice that became more
evident with age was quantified by the two methods
described above. Such mice at 200 DOA retained their
forepaw grasp on a horizontal bar for 20 s or less in contrast to WT mice which maintained their grasp for 150 s or
more (Fig. 1Ab). Surprisingly, the same was true of relatively young KO mice, 35 DOA (Fig. 1Aa). Grip duration
was fully restored to the latter mice by serial IP injections
(39/week) of LIGA-20 over the 5 week period, while grip
duration was significantly improved by LIGA-20, though
less dramatically, for the older mice. GM1 similarly
administered to the younger KO mice had relatively little
effect. The second impairment test, determining motor
response to sensory stimulus by measuring time for
removal of adhesive irritant from the snout, gave similar
results: older KO mice required 60 s in contrast to WT
time of *5 s (Fig. 1Bb). The younger KO mice effected
removal in *30 s, significantly more than the *2 s
required by the younger WT mice. As before, GM1
administered to the younger KO mice had virtually no
effect. In both tests the ameliorative effect of LIGA-20 rose
gradually over the 5 weeks, reaching a plateau at
*3 weeks (not shown).
Comparison of TH-expressing neurons in SNpc of KO
versus WT brains of *200 day old mice suggested significant deficiency in the mutant (Fig. 2). Tyrosine
hydroxylase (TH), an enzyme that catalyzes the first step in
conversion of tyrosine to DA, is a marker for DA neurons.
This was quantified by unbiased stereology employing antiTH Ab to count DA neurons in the SNpc and VTA.
Decrease in TH-expressing neurons was significant in the
�Neurochem Res (2011) 36:1706–1714
1709
Fig. 1 Movement impairment
in KO mice. Mice at 35 (Aa,
Ba) and 200 (Ab, Bb) days of
age were IP injected with GM1,
LIGA20 or BSS for 5 weeks.
They were subjected to the griphanging (A) and adhesive
removal (B) tests. () = n. Data
are average ± SEM. ** and
*** represent P \ 0.01 and
0.001 compared to BSS-treated
WT with Student’s two-tailed t
test
Fig. 2 Degeneration of TH? neurons in SNpc of KO mice. Brain
sections containing SNpc from 200 day old WT (A) and KO (B) mice
were stained with anti-TH antibody (2nd Ab with Texas red) and
CtxB-FITC for GM1 (green), showing reduced number of
TH? neurons in KO mice. Expression of GM1 in WT TH? neurons
is indicated by arrows (plasma membrane) and arrowheads (nuclear
membrane). Photographed with 40X objective lens
SNpc, and although the VTA showed a decrease this did
not reach significance (Fig. 3). These changes accord with
the significant loss of DA neurons in the SNpc and relative
sparing of DA neurons in the VTA reported for murine
models of PD [22]. Treatment of the KO mice with LIGA20 over the 5 week period elevated TH? neurons in the
SNpc to the point where the TH? count in SNpc of LIGA-
20-treated mice was not significantly different from WT
(P = 0.059), even though the difference between KO and
KO ? LIGA-20 did not reach significance.
Alpha synuclein expression was greatly elevated in
SNpc of KO brain, as revealed by immunocytochemistry;
5 weeks of LIGA-20 treatment attenuated a-syn levels
while restoring much of the depleted TH expression
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Neurochem Res (2011) 36:1706–1714
Fig. 3 Stereological analysis. WT and KO mice (200 days old) were
IP injected with LIGA-20 or BSS for 5 weeks. Brain sections were
immunostained with anti-TH as shown in Fig. 2 and subjected to
stereological analysis. Two regions, SNpc (A) and VTA (B),
containing TH? neurons were counted. The data are average
(±SEM) of 3 animals in each group (n = 3). Significant decrease
in DA neurons of SNpc but not VTA was indicated by Student’s two-
tailed t test. These changes accord with the significant loss of DA
neurons in the SNpc and relative sparing of DA neurons in the VTA
reported for PD and murine models of PD [22]. Although the
difference between KO and KO ? LIGA-20 did not reach significance, the treatment rendered the difference between WT and
KO ? LIGA-20 insignificant
Fig. 4 Accumulation of a-syn in TH? neurons. Brain sections were
co-stained with anti-TH (2nd Ab with Texas red) and anti-a-syn (2nd
Ab with FITC), showing reduced TH? neurons and aggregated a-syn
in remaining TH? neurons in KO mouse. IP injection of KO mouse
with LIGA-20 for 5 weeks attenuated a-syn accumulation while
rescuing TH? neurons
(Fig. 4). Quantitative verification of a-syn elevation was
obtained by Western blot analysis, which also indicated
aggregation by marked increase of higher molecular weight
bands at 34- and 170 kDa as well as less dense bands in
between; this applied to mice 200 DOA (Fig. 5Ab) as well
as younger mice at 35 DOA (Fig. 5Aa). Densitometric
quantification revealed significant reduction of aggregated
forms of a-syn following 5 weeks of LIGA-20 treatment of
both age groups, in contrast to GM1 which produced no
significant reduction (Fig. 5B).
Dopamine levels in the striatum, measured as described
by HPLC, were significantly reduced in KO mice compared
to WT, as was also observed for DOPAC, a principal DA
metabolite (Fig. 6a). Serotonin, another neurotransmitter in
123
�Neurochem Res (2011) 36:1706–1714
1711
Fig. 5 Immunoblot analysis for a-syn accumulation. WT and KO
mice at 35 (Aa, Ba) and 200 (Ab, Bb) days of age were treated with
BSS, GM1 (G), or LIGA-20 (L). Brain tissue of SN regions was
micro-dissected, and subjected to immuno-blotting for a-syn. Housekeeping protein actin was run in parallel for loading control. A Blot
images showing polymerization of a-syn ranging form 34- to 170 kD.
B Densitometry quantification of a-syn polymers. Data are mean ±
SEM from 3 mice in each group (n = 3). Student’s two-tailed t test
was employed. *P \ 0.01 versus BSS-treated WT. The results show
enhanced aggregation of a-syn in KO, which is significantly reduce by
LIGA-20 but not GM1
Fig. 6 Biochemical analyses. Dissected striata were extracted with
0.4 N HClO4, spiked with dihydroxybenzylamine as internal standard
and subjected to HPLC. (A) Striatal DA and DOPAC, that were
significantly reduced in the KO; (B) 5-HT and 5-HIAA, that were not
significantly reduced. Data are averages ± SEM; # of animals
indicated in (). Statistical significance was determined by Student’s
two-tailed t test: * and *** represent P \ 0.05 and 0.001, respectively
the striatum, and 5-HIAA, its metabolite, were moderately
reduced by an amount that did not reach significance
(Fig. 6b). To test whether the movement disorders were due
to depleted DA, KO mice were administered L-dopa as
described. The animals thus treated showed highly significant recuperation from physical impairment as determined
by both tests (Fig. 7). Mice in both age groups showed
approximately equal rescue from physical impairment in
both tests.
deficit and aberrations in the activity of the neural circuits
within the basal ganglia that regulate movement. Cytosolic
accumulation of Lewy bodies that contain aggregated a-syn
is an additional hallmark of the disease [25]. The large
majority of PD cases have been described as sporadic, the
remainder as familial based on a variety of genetic mutations. Symptomatic treatments of the motor features are in
clinical use but no neuroprotective treatment to prevent
progressive loss of DA neurons has yet become available.
This study has provided evidence for the presence of key
features of parkinsonism in genetically modified mice with
disrupted gene for Galgt1 (GalNAcT; GM2/GD2 synthase).
This included behavioral, histopathological, and biochemical parameters that are the defining symptoms of PD.
These findings thus amplify and extend previous observations of behavioral and cellular pathologies of these
mutants, which included progressive behavioral neuropathies involving deficits in reflexes, strength, coordination,
balance, and gait [4]. A morphological study revealed
axonal degeneration and decreased central myelination [3].
These earlier reports thus indicated a variety of
Discussion
Parkinson’s disease is the second most prevalent late-onset
neurodegenerative disorder that affects nearly 1% of the
global population aged 65 and older. It is a progressive
neurodegenerative disease characterized by resting tremor,
postural rigidity, bradykinesia, autonomic instability and in
its later stages by cognitive and emotional disorders [23,
24]. A principal feature is loss of pigmented DA neurons in
the SNpc that project to the striatum, resulting in DA
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Fig. 7 Effect of L-dopa on physical impairment. Mice at 35 (Aa,
Ba) and 200 (Ab, Bb) days of age were IP injected with L-dopa
(20 mg/kg) and carbidopa (3 mg/kg). Behavior tests, grip-hanging
(A) and adhesive removal (B), were performed before and 3 h after
injection. Data are average ± SEM; ( ) = n. Two-tailed Student’s t
test was used for statistical analysis. ** and *** represent P \ 0.01
and 0.001 respectively compared to WT before L-dopa treatment
neuropathies and neuropathologies attendant to these
mutant mice while the present study has elucidated PD-like
symptoms not previously reported. Disruption of this gene
for a key enzyme in synthesis of GM2 results in ablation of
that molelcule and the entire gangliotetraose series [3, 16]
which comprise [90% of the complex gangliosides of
brain; corresponding elevations of GM3 and GD3 have
been observed [5, 26].
We hypothesize that much of the PD-specific symptomatology observed here derives from the GM1 deficit,
based in part on the rescue effects of LIGA-20. This GM1
analog, developed by Costa and coworkers [27], contains
the same oligosaccharide chain as GM1 but a modified
hydrophobic moiety (replacement of ceramide stearoyl by
dichloroacetyl) that induces membrane permeability. The
latter property has been affirmed both in vitro with primary
neurons [28] and in vivo with CNS neurons of ganglioganglioside-deficient mice suffering enhanced kainateinduced seizures [6]. LIGA-20 proved more potent than
GM1 in partially restoring depleted DA levels in MPTPtreated mice [11] and, significantly, was able to accomplish
this via oral administration [29]. These manifestations of
LIGA-20 efficacy, believed to derive from its membrane
permeability, result in enhanced ability to cross the blood
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Neurochem Res (2011) 36:1706–1714
brain barrier and the neuronal plasma membrane. When
applied to cells or mice deficient in GM1 it thus serves as
replacement for the missing ganglioside in both the plasma
membrane and intracellular sites where GM1 has functional roles. Intracellulaar loci include the nuclear Na?/
Ca2? exchanger which is potentiated by GM1 [30, 31], the
autophagy pathway including promotion of lysosomal
integrity [32], and a-syn which requires GM1 association to
prevent fibrillation and maintenance of helical conformation [33]. Long term Ca2? dysregulation in the DA neurons
of the SNpc, associated with their autonomous pacemaker
activity and resultant mitochondrial impairment, has been
suggested as a major contributor to the selective vulnerability of those neurons over time [34]. An additional reason
for ascribing primacy to GM1 is the finding that knockout
mice with disrupted GD3 synthase, resulting in deletion of
all b- and c-series and retention of a-series gangliosides,
showed virtually intact nervous system morphology with
no apparent abnormal behavior despite some aberrations in
pain perception and nerve regeneration [35, 36]. GD1a, the
other prominent ganglioside of the a-series, often functions
as metabolic precursor to GM1 through the action of
membrane-bound sialidase [37, 38]. The complexity of
ganglioside changes that occur in the Galgt1 mutant and
the uncertainty as to which GM1 functions are efficiently
restored by LIGA-20 require caution at this stage in
ascribing a primary role to GM1 deficiency in relation to
parkinsonism. However, the results of this and the other
mentioned studies point to that conclusion.
Additional evidence of a key role for Ca2? dysregulation in PD is the finding that elevated Ca2? promoted a-syn
aggregation in 1321N1 cells expressing an a-syn-GFP
construct [39]. Alpha synuclein in aggregated form, together with ubiquitin, is a prominent component of Lewy
bodies which are pathological hallmarks of PD. Lewy
bodies as such are not usually found in rodent models of
PD, but inclusion bodies staining for a-syn and ubiquitin
have been observed [40]. The present study obtained
Western blot evidence for a-syn aggregation in the prominence of higher molecular weight bands between 34- and
170- kDa in KO striatum compared to WT (Fig. 5). As
shown, the densities of such bands were noticeably
diminished by LIGA-20 treatment of the KO mice. Significantly, a-syn aggregation was inhibited specifically by
GM1 which promoted its alpha-helical structure [33].
A randomized double blind placebo controlled study
reported that GM1-treated PD patients showed significant
improvements on Unified Parkinson’s Disease Rating Scale
(UPDRS) motor scores and performance of timed motor
tasks, compared to baseline performance [14]. Subsequently a 5 year open study revealed that patients using
GM1 had lower UPDRS motor scores than at baseline [15].
These are interesting findings in view of preliminary results
�Neurochem Res (2011) 36:1706–1714
in our lab showing a marked deficiency of GM1 in DA
neurons of the SNpc of PD patients, compared to agematched controls. This suggests that applied GM1 may be
functioning as a form of replacement therapy to the limited
extent it is able to enter the brain of PD patients. This leads
to the further suggestion that membrane permeable derivatives of GM1 may prove more efficacious in preserving
DA neuronal viability and alleviating PD pathology.
Acknowledgments This work was supported by NIH grant 2 RO1
NS33912.
It is a pleasure to contribute to this special issue of Neurochemical
Research honoring Dr. Robert Yu for his many seminal contributions
to the field of Neurochemistry. His studies on the biochemistry, cell
biology, and pathophysiology of glycosphingolipids have been well
recognized and honored over the years. Bob was my first postdoc (and
his first such experience) more than a few years ago, coming from the
lab of Herbert Carter, an iconic sphingolipid pioneer at the University
of Illinois. Herbert responded to my inquiry with the affirmation that
Bob was indeed a promising young neuroscientist who would likely
contribute to my program. That proved quite a good prophecy;
everyone should be so lucky as to have someone like Bob as their first
posdoc. Those years were memorable for the quality and quantity of
the work he produced as well the beginning of a life long friendship.
I’m convinced there are many more miles to go in terms of Bob’s
contributions to neuroscience.
Open Access This article is distributed under the terms of the
Creative Commons Attribution Noncommercial License which permits any noncommercial use, distribution, and reproduction in any
medium, provided the original author(s) and source are credited.
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