RESEARCH ARTICLE
Effects of Cellular Pathway Disturbances on
Misfolded Superoxide Dismutase-1 in
Fibroblasts Derived from ALS Patients
Isil Keskin1, Elin Forsgren1, Dale J. Lange2, Markus Weber3, Anna Birve1,
Matthis Synofzik4,5, Jonathan D. Gilthorpe1, Peter M. Andersen1, Stefan L. Marklund6*
1 Department of Pharmacology and Clinical Neurosciences, Umeå University, Umeå, Sweden,
2 Department of Neurology, Hospital for Special Surgery and Weill Cornell Medical Center, New York, NY,
United States of America, 3 Neuromusucular Diseases Unit/ALS Clinic, Kantonsspital St.Gallen, St. Gallen,
Switzerland, 4 Department of Neurodegenerative Diseases, Hertie Institute for Clinical Brain Research,
Tübingen, Germany, 5 German Research Center for Neurodegenerative Diseases (DZNE), University of
Tübingen, Tübingen, Germany, 6 Department of Medical Biosciences, Clinical Chemistry, Umeå University,
Umeå, Sweden
* stefan.marklund@umu.se
OPEN ACCESS
Citation: Keskin I, Forsgren E, Lange DJ, Weber M,
Birve A, Synofzik M, et al. (2016) Effects of Cellular
Pathway Disturbances on Misfolded Superoxide
Dismutase-1 in Fibroblasts Derived from ALS
Patients. PLoS ONE 11(2): e0150133. doi:10.1371/
journal.pone.0150133
Editor: Gilles J. Guillemin, Macquarie University,
AUSTRALIA
Received: November 5, 2015
Accepted: February 9, 2016
Published: February 26, 2016
Copyright: © 2016 Keskin et al. This is an open
access article distributed under the terms of the
Creative Commons Attribution License, which permits
unrestricted use, distribution, and reproduction in any
medium, provided the original author and source are
credited.
Data Availability Statement: All relevant data are
within the paper and its Supporting Information files.
Funding: The study was supported by the Swedish
Research Council, the Knut and Alice Wallenberg
Foundation, the Bertil Hållsten Foundation, the
Torsten and Ragnar Söderberg Foundation, the
Swedish Brain Foundation, the Stratneuro initiative,
the Västerbotten County Council, the Kempe
Foundation, Neuroförbundet and the Ulla-Carin
Lindquist Foundation. The funders had no role in
study design, data collection and analysis, decision to
publish, or preparation of the manuscript.
Abstract
Mutations in superoxide dismutase-1 (SOD1) are a common known cause of amyotrophic
lateral sclerosis (ALS). The neurotoxicity of mutant SOD1s is most likely caused by misfolded molecular species, but disease pathogenesis is still not understood. Proposed mechanisms include impaired mitochondrial function, induction of endoplasmic reticulum stress,
reduction in the activities of the proteasome and autophagy, and the formation of neurotoxic
aggregates. Here we examined whether perturbations in these cellular pathways in turn
influence levels of misfolded SOD1 species, potentially amplifying neurotoxicity. For the
study we used fibroblasts, which express SOD1 at physiological levels under regulation of
the native promoter. The cells were derived from ALS patients expressing 9 different SOD1
mutants of widely variable molecular characteristics, as well as from patients carrying the
GGGGCC-repeat-expansion in C9orf72 and from non-disease controls. A specific ELISA
was used to quantify soluble, misfolded SOD1, and aggregated SOD1 was analysed by
western blotting. Misfolded SOD1 was detected in all lines. Levels were found to be much
lower in non-disease control and the non-SOD1 C9orf72 ALS lines. This enabled us to validate patient fibroblasts for use in subsequent perturbation studies. Mitochondrial inhibition,
endoplasmic reticulum stress or autophagy inhibition did not affect soluble misfolded SOD1
and in most cases, detergent-resistant SOD1 aggregates were not detected. However, proteasome inhibition led to uniformly large increases in misfolded SOD1 levels in all cell lines
and an increase in SOD1 aggregation in some. Thus the ubiquitin-proteasome pathway is a
principal determinant of misfolded SOD1 levels in cells derived both from patients and controls and a decline in activity with aging could be one of the factors behind the mid-to late-life
onset of inherited ALS.
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Misfolded SOD1 in ALS Fibroblasts
Competing Interests: The authors have declared
that no competing interests exist.
Introduction
Amyotrophic lateral sclerosis (ALS) is characterized by adult-onset degeneration of upper and
lower motor neurons. The disease begins focally and then spreads contiguously, resulting in
progressive paralysis and death from respiratory failure [1]. Mutations in the gene encoding
the ubiquitously expressed free radical scavenging enzyme superoxide dismutase-1 (SOD1) are
known to cause ALS [2], and are found in 1–9% of patients [3]. Since 1993, 188 coding mutations in SOD1 have been associated with ALS as a dominant trait (http://alsod.iop.kcl.ac.uk/),
but disease caused by the most prevalent SOD1 mutation D90A is usually inherited as a recessive trait [4]. While missense mutations are most frequent, some 20 SOD1 mutations result in
insertions, deletions or substitutions resulting in C-terminal truncations or other disruptive
changes, precluding native folding of the mutant protein. Importantly, there are no apparent
clinical (e.g. age of onset, survival time) or post-mortem histological differences between
patients carrying missense mutations and disruptive mutations [5–7]. This suggests that a
common cytotoxic mechanism originates from misfolded SOD1 species. The concentrations of
the most structurally stable SOD1 mutants (e.g. A89V, D90A, and L117V) are, however, similar to wild-type SOD1 in humans [8, 9]. The major proportions of these, which are natively
folded and enzymatically active, are unlikely to contribute significantly to neurotoxicity. In
contrast, the most disrupted truncated mutants are present at 100-fold lower levels [7, 10].
These findings suggest that minute subfractions of misfolded, not total, mutant SOD1 are the
relevant pathogenic species for ALS.
The mechanisms by which misfolded SOD1 species cause the disease are poorly understood.
However, they have been suggested to involve perturbation of mitochondria [11–16], induction
of endoplasmic reticulum (ER)-stress [16–19], reduction of proteasome activity [20–22],
reduction of autophagy [23, 24], and aggregation [25–31]. Another unresolved feature of ALS
is why carriers of SOD1 mutations are apparently healthy until late middle age, and then
undergo rapid neurological decline. Typically, a carrier of a SOD1 A4V or G93A mutation
presents with a sudden focal paresis and wasting that disseminates quickly throughout the
motor system, leading to death in one to two years [5, 32]. Perhaps an age-related decline in
proteostasis and energy metabolism, amplified by a vicious cycle of misfolded SOD1 accumulation, leads to a rapid increase in misfolded SOD1 species in the tissue.
Studies of ALS pathogenesis involving mutant SOD1 are usually conducted in transgenic
animals or transfected cell models, both of which exhibit high levels of overexpression of the
mutant protein. Studies on patient material are typically conducted at end-stage. We have generated dermal fibroblast lines from ALS patients carrying mutations in SOD1 and other ALSlinked genes and from non-disease controls. These cells, in which mutant SOD1 is expressed
under the native promoter, offer opportunities for exploration which are poorly accessible in
most other model systems. We have previously developed methods that enable minute
amounts of misfolded SOD1 species to be determined specifically [33, 34]. We have used these
methods here to gain information on the effects of various ALS-related pathways on the levels
of misfolded SOD1 in patient-specific fibroblasts.
Materials and Methods
Human materials
Blood samples and skin biopsies were collected from patients and non-disease controls with
approval of the Swedish Ethical Review Board for Medical Research and adhering to the principles of the Declaration of Helsinki (WMA, 1964), following written informed consent (Table A
in S1 File).
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Misfolded SOD1 in ALS Fibroblasts
SOD1 and C9orf72 genotyping
Genomic DNA was extracted from whole blood (buffy coat) using the Nucleon BAAC2 kit (GE
Healthcare, Piscataway, NJ, USA) according to the manufacturer's protocol. Amplification of all
5 exons and the corresponding 30–50 bp of flanking intronic regions of the SOD1 gene was performed using the AmpliTaqGold Kit (Applied Biosystems, Foster City, CA, USA) as described by
the manufacturer. Sequencing reactions were performed using BigDye Terminator v3.1 Cycle
Sequencing Kit (Applied Biosystems, Foster City, CA, USA) as recommended and analysed using a
3730xl DNA analyzer with the SeqScape Software v2.5 (Applied Biosystems, Foster City, CA, USA).
The presence of the GGGGCC-hexanucleotide repeat expansion in C9orf72 was screened for by
repeat-primed polymerase chain reaction (RP-PCR) and fragment length-analysis [35]. Fragment
length analysis was performed on a 3730xl DNA analyzer and Peak Scanner Software v1.0 (Applied
Biosystems, Foster City, CA, USA). The presence of an expansion was confirmed by Southern blot
[35]. All individuals tested negative for mutations in a panel of other ALS-linked genes (details
available upon request) and no double mutation carriers were included in the study cohort.
Cell culture
Following screening of blood to identify SOD1 and C9orf72 mutation carriers, a 3 mm punch
skin biopsy (upper arm) was obtained from 9 ALS patients with SOD1 mutations (A4V, H46R,
E78_R79insSI, N86S, D90A, G93A, L117V, D125Tfs 24, and G127X), 1 ALS and 1 FTD
patient with massive intronic GGGGCC repeat-expansions in C9orf72, and 4 non-disease control individuals. The ALS patients were diagnosed according to the EFNS criteria [36]. The
G127X biopsy was obtained from an asymptomatic 31 year old carrier of the mutation belonging to a family where 7 other members have developed ALS [5]. All patients were heterozygous
for their corresponding mutations except the D90A SOD1 patient (homozygous). The control
subjects were relatives of ALS patients. All healthy control subjects tested negative (wt/wt) for a
panel of ALS-associated genes including SOD1, C9orf72, TBK1 and UBQLN2. The study cohort
is summarized in Table A in S1 File.
Adult human dermal fibroblast cell lines were established using standard procedures and
were maintained in RPMI 1640 medium (Gibco, Life Technologies, Carlsbad, CA, USA), with
25 mM HEPES (Gibco, Life Technologies, Carlsbad, CA, USA), and 2 mM L-glutamine
(Gibco, Life Technologies, Carlsbad, CA, USA), 0.1 g/ml penicillin (Meda, Sweden) supplemented with 10% (v/v) foetal bovine serum (Gibco, Life Technologies, Carlsbad, CA, USA)
and incubated at 37°C and 5% (v/v) CO2.
Cell treatments
Fibroblasts were plated at a density of around 8000 cells/cm2 in 60 mm dishes. After reaching
60–70% confluency, the media were replaced with plain culture media (controls) or media containing the proteasome inhibitor bortezomib (0.5, 5 ng/ml; PS-341, Millennium Pharmaceuticals,
USA), 10 mM of the autophagy inhibitor 3-methyladenine (3-MA) (Sigma-Aldrich, St. Louis,
MO, USA), 0.5 μg/ml of the glycosylation inhibitor and ER stress inducer tunicamycin (SigmaAldrich, St. Louis, MO, USA), and 5 μM of the mitochondrial complex 1 inhibitor rotenone
(Sigma-Aldrich, St. Louis, MO, USA). All inhibitor treatments were made in triplicates, with
appropriate triplicates of vehicle only controls and the cells were cultured for 24 h before harvest.
Cell fractionation
Cells were washed with pre-warmed phosphate-buffered saline (PBS; 137 mM NaCl, 2.7 mM
KCl, 4.3 mM Na2HPO4, and 1.4 mM KH2PO4, pH 7.0) containing 40 mM iodoacetamide
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Misfolded SOD1 in ALS Fibroblasts
(IAM, Thermo Scientific, Rockford, IL, USA), which prevents artificial formation of the
C57-C146 disulphide bond in SOD1 by blocking reduced cysteine residues via alkylation [33,
34]. The cells were detached with 0.025% (w/v) trypsin (Gibco, Life Technologies, Carlsbad,
CA, USA) and were then washed with PBS containing 40 mM IAM supplemented with 0.5%
(v/v) foetal bovine serum to inhibit trypsin and were pelleted at 500 x g for 5 min. The cell pellet was resuspended in PBS containing 40 mM IAM and centrifuged at 500 g for 5 min. The
supernatant was removed and the pellet was snap frozen on dry ice and thereafter kept in a
-80°C freezer. For analysis, the cell pellet was rapidly thawed in a 25°C water bath to reduce the
effects of cold denaturation. It was then lysed in 500 μl ice-cold PBS containing the Complete
EDTA-free protease inhibitor cocktail (Roche Diagnostics, Mannheim, Germany), 40 mM
IAM and 0.5% (v/v) NP-40 using a Sonifier Cell Disrupter (Branson, Danbury, CT, USA). The
lysate was centrifuged at 20,000 g for 30 min at 4°C and the supernatant was collected as the
soluble fraction and directly analysed with the misELISA (see below). The resulting pellet was
resuspended in ice-cold lysis buffer containing 0.5% (v/v) NP-40 as described above and recentrifuged twice to remove any contaminating soluble protein. The resulting pellets were used
for determination of detergent-insoluble SOD1 aggregates.
ELISAs for misfolded and total SOD1
The ELISA for misfolded SOD1 (misELISA) was carried out as previously detailed [33, 34]. A
rabbit antibody raised against a peptide corresponding to amino acids (aa) 24–39 in the human
SOD1 sequence was used as primary antibody. This antibody reacts only with disordered
SOD1 species and lacks affinity for the natively folded protein [37–39]. A goat anti-human
SOD1 antibody was used as secondary antibody. It was raised against SOD1 that had been
denatured by incubation with guanidinium chloride and EDTA, and reacts preferentially with
the disordered protein [33]. For calibration of the misELISA, a fresh spinal cord from a transgenic mouse expressing G127X mutant human SOD1 was homogenized in 25 volumes 10 mM
K phosphate, pH 7.0 in 0.15 M NaCl, containing the Complete anti-proteolytic cocktail (Roche
Diagnostics, Mannheim, Germany) and 40 mM IAM. After centrifugation at 20,000 g, the
supernatant was divided into multiple aliquots that were stored at -80°C. In the misELISA
assay, one unit is defined as the amount of “misfolded” SOD1 present in 1 g wet weight of that
particular spinal cord.
For ELISA of native/total SOD1, rabbit and goat anti-native human SOD1 antibodies were
used [40] following partial purification on Protein A- and Protein G-Sepharose (GE Healthcare
Biosciences, Piscataway, NJ, USA), respectively. The rabbit antibody was used as a primary
antibody and the goat antibody as a secondary antibody. The ELISA was standardized with a
human hemolysate, with the SOD1 content calibrated against pure human SOD1, the concentration of which was determined by quantitative amino acid analysis [40]. The ELISA is able to
quantify native SOD1 accurately, but may also respond to some degree to misfolded SOD1 species [33].
Western blot
The protein concentration of lysates was determined using the BCA Protein Assay Kit
(Thermo Scientific, Rockford, IL, USA). Western blots were carried out in Any kD Criterion
TGX precast gels (BioRad Laboratories, Hercules, CA, USA) as previously described [7]. The
primary antibodies used were; rabbit anti-human SOD1 (0.8 μg/ml, raised against a peptide
corresponding to aa 57–72 in the human SOD1) [41], anti-LC3B rabbit (1:1000; SigmaAldrich, St. Louis, MO, USA), anti-GRP78 rabbit (1:5000; Novus Biologicals, Littleton, CO,
USA), anti-β-actin mouse (1:100 000; Milipore, Bedford, MA, USA). The secondary antibodies
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Misfolded SOD1 in ALS Fibroblasts
were horseradish peroxidase (HRP)-conjugated polyclonal anti-mouse or anti-rabbit IgG
(Dako, Glostrup, Denmark). The immunoreaction signal was visualized using an ECL Select
reagent (GE Healthcare Biosciences, Piscataway, NJ, USA) recorded on a ChemiDoc apparatus
(BioRad Laboratories, Hercules, CA, USA) and analysed using Quantity One software (BioRad
Laboratories, Hercules, CA, USA).
Statistical analyses
Statistical analyses were performed with the Prism 6.0 software (GraphPad, San Diego, CA,
USA). For comparison of multiple groups, the one-way ANOVA was used following correction
for multiple testing using Tukey’s post-hoc analyses. F-test was used to test for equal variance
between treatment groups. For p-values 0.05 the Welch test was used. For p-values > 0.05
the two-tailed unpaired t-test was used. For comparison of two groups, the Mann-Whitney U
test was used. The significance level was set to 0.05. All values are given as mean ± SD.
Results
Design of experiments
We used fibroblasts derived from patients carrying different SOD1 mutations and encoding
SOD1 variants with widely variable structural characteristics (Table A in S1 File). This
approach offered several advantages. Since SOD1 is expressed under the control of the endogenous promoter, treatment responses should better reflect the in vivo situation. This also ensures
a native, balanced synthesis rate, which when analysed by western blotting resulted in levels of
mutant SOD1s ranging from those similar to wild-type SOD1 to non-detectable (Fig 1A). The
lysates from fibroblasts expressing the missense mutants D90A, G93A and N86S [9, 42]
showed SOD1/β-actin ratios comparable to controls, whereas the ratios were somewhat
reduced in lysates from fibroblasts expressing L117V, A4V, E78_R79insSI and H46R (Fig 1B).
The disordered, truncated mutants D125Tfs 24 and G127X are rapidly degraded and only
SOD1 derived from the wild-type allele was visible. Addition of the proteasome inhibitor bortezomib resulted in low but detectable amounts of the G127X mutant form of SOD1 (Fig 1A).
We focused primarily on the levels of unfolded/disordered/unstructured/misfolded (in the
following we will use the term misfolded) SOD1, since these are the species that are likely to
provoke the onset of ALS. We utilized an ELISA, which we have developed and detects misfolded SOD1 species specifically (misELISA) but does not detect holoSOD1, or SOD1 that
lacks Cu and/or the C57-C146 disulphide bond, as long as the polypeptide is natively folded
[33, 34]. Fibroblast extracts were incubated for 1 h at 23°C with the capture antibody in the
misELISAs. The physiological 37°C would have been preferable, but at that temperature some
folded SOD1 species have been found to unfold continuously in diluted extracts [34]. Thus, the
levels of misfolded SOD1 at physiological temperature are not mirrored and results are not
directly comparable between cell lines expressing different SOD1 variants. For a certain fibroblast line, however, the effects of perturbations on the levels of misfolded SOD1 can be determined. The misELISA is very sensitive: note for instance the high readings yielded by the
G127X mutant (Figs 2 and 3) which was undetectable by western blot (Fig 1A).
Effect of protein degradation pathways on misfolded SOD1 clearance
Degradation by the proteasome is the primary cellular route of misfolded protein elimination
[43]. Autophagy plays a fundamental role in the degradation of protein aggregates and also
contributes to the elimination of soluble misfolded proteins [43]. Therefore, we determined the
effects of inhibition of both systems on misfolded SOD1 levels.
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Misfolded SOD1 in ALS Fibroblasts
Fig 1. SOD1 protein in lysates of fibroblast cultures. (A) Fibroblast lysates were analysed by western blotting using the anti-SOD1 (57–72 aa) antibody. βactin was used as a loading control. The band of the truncated G127X mutant was not visible except in the presence of the proteasome inhibitor bortezomib
(arrow). The homozygous D90A mutant displays increased mobility. (B) The expression of SOD1 in the fibroblast lines were compared as SOD1/β-actin
ratios. The mean of the 2 control lines was taken as 1. Three replicate sets of fibroblast cultures were analyzed. The data are expressed as means ± SD. (*)
p < 0.05 compared to the results for the controls (Mann-Whitney U test).
doi:10.1371/journal.pone.0150133.g001
Bortezomib acts primarily as a reversible inhibitor on the chymotrypsin-like site of the 20S
proteasome core β5 subunit, but also inhibits the caspase-like site at high concentrations [44].
We first identified a treatment regimen that did not have a significant effect on cell viability,
detected using an assay that reports on plasma membrane integrity (Figure A in S1 File).
Although we cannot exclude activation of earlier stages of cell death before loss of plasma
membrane integrity, under these conditions (5 ng/ml for 24 h) the chymotrypsin-like, caspaselike and trypsin-like activities of the proteasome were inhibited by 96%, 85% and 45%, respectively (Figure B in S1 File). Proteasome inhibition resulted in a marked increase in misfolded
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Misfolded SOD1 in ALS Fibroblasts
Fig 2. Effect of reduction in the activities of the proteasome and autophagy on the levels of misfolded and total SOD1 in fibroblast lines. Misfolded
and total SOD1 in lysates of fibroblasts were analysed with the 24–39 misELISA and ELISA for total SOD1, respectively. Fibroblast cell lines were cultured in
triplicate for 24 h in the absence (blue) or the presence (red) of the proteasome inhibitor bortezomib (A-C; 5 ng/ml), the autophagy inhibitor 3-MA (D-F; 10
mM). Data is expressed as the mean ± SD (n = 3), *p< 0.05, **p< 0.01, ***p< 0.001, ****p< 0.0001 compared to respective non-treated control (Welch test
and two-tailed unpaired t-test).
doi:10.1371/journal.pone.0150133.g002
SOD1 in all lines tested (Fig 2A and 2B). We also analysed total SOD1 levels in bortezomibtreated cultures. The SOD1/total protein ratios were increased in all, by an average of 28% (Fig
2C). However, expressing the results as misSOD1/total SOD1 ratios did not change the conclusion that proteasome inhibition markedly increased the levels of misfolded SOD1 in the fibroblast cultures (Fig 2B).
We investigated the effects of blocking autophagy using the commonly used inhibitor
3-methyladenine (3-MA) [45]. 3-MA is, however, not a specific inhibitor for autophagy and
may affect other cellular processes [46]. Under the current condition -10 mM 3-MA for 24 h- a
moderate inhibition was achieved. The levels of microtubule-associated protein light chain 3-II
(LC3-II) and the ratio of LC3-II/LC3-I were reduced to 78% and 91%, respectively of controls
(Figure C in S1 File). No significant increases in the levels of misfolded SOD1 were detected in
any of the lines and in some cases, moderate reductions were recorded (Fig 2D and 2E). Minor
increases were seen in total SOD1/total protein ratios in the 3-MA-treated fibroblast cultures
(Fig 2F).
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Misfolded SOD1 in ALS Fibroblasts
Endoplasmic reticulum stress
ER stress has been observed in post-mortem spinal cord tissue of humans with sporadic ALS
[47], transgenic mouse models overexpressing mutant human SOD1 [17–19], cell lines overexpressing mutant SOD1s [17] and A4V iPSCs-derived motor neurons [16]. We sought to investigate the role of ER stress on misfolded SOD1 levels in fibroblasts by exposing them to
tunicamycin, an inhibitor of protein glycosylation. Despite strong induction of ER stress measured by the ER chaperone glucose-regulated protein 78 (GRP78) (Figure C in S1 File), no
great differences were found in the levels of misSOD1 in any of the cell lines tested (Fig 3A and
3B). ER stress increased the total SOD1/total protein ratios by an average of 3% (Fig 3C).
Inhibition of mitochondria
Several lines of evidence gathered from studies performed on transgenic mouse and cellular
models overexpressing mutant human SOD1 have shown that mutant SOD1s can interfere
with mitochondria and this has been suggested to be a primary pathogenic mechanism in ALS
Fig 3. Effect of induction of ER stress and perturbation of mitochondria on the levels of misfolded and total SOD1 in fibroblast lines. Misfolded and
total SOD1 in lysates of fibroblasts were analysed with the 24–39 misELISA and ELISA for total SOD1, respectively. Fibroblast cell lines were cultured in
triplicate for 24 h in the absence (blue) and presence (red) of the ER-stress inducer tunicamycin (A-C; 0.5 μg/ml) and the mitochondrial inhibitor rotenone
(D-F; 5 μM). Data is expressed as the mean ± SD (n = 3), *p< 0.05, **p< 0.01, ***p< 0.001 compared to respective non-treated control (Welch test and twotailed unpaired t-test).
doi:10.1371/journal.pone.0150133.g003
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Misfolded SOD1 in ALS Fibroblasts
Fig 4. Inhibition of proteasome causes accumulation of detergent-insoluble SOD1 aggregates. Fibroblast cell lines were cultured in the absence (-)
and presence (+) of bortezomib (5 ng/ml) for 24 h. Detergent insoluble fractions were analysed by western blotting using the anti-SOD1 (57–72 aa) antibody.
No insoluble aggregates were seen in the control and D90A lines. Proteasome inhibition increased the amount of aggregates in G93A, A4V, H46R, G127X
and D125Tfs*24 lines.
doi:10.1371/journal.pone.0150133.g004
[11–14, 16]. Perturbations of mitochondria have also been observed in fibroblasts from a
patient carrying a SOD1 mutation [15] and in A4V iPSCs-derived motor neurons [16]. To
investigate the effect of mitochondrial inhibition on the level of misfolded SOD1 we used rotenone to inhibit Complex I of the mitochondrial respiratory chain. As shown in Fig 3D and 3E,
rotenone treatment caused a moderate reduction in the levels of misfolded SOD1, but no
increases. The SOD1/total proteins ratios were increased in all rotenone-treated fibroblast cultures by an average of 7% (Fig 3F).
Detergent-insoluble aggregates
Accumulation of detergent-insoluble, aggregated forms of mutant SOD1 have been found in
motor neurons of ALS patients [25, 28], transgenic mouse models overexpressing mutant
human SOD1 [26] as well as cells overexpressing human mutant SOD1s [27, 29, 30] and
iPSCs-derived motor neurons [16, 31].
We determined the amount of detergent-insoluble aggregates present following all interventions used in study (Fig 4). Despite a high sensitivity of the assay, no aggregates were found in
the majority of lines (Table 1). The only untreated cultures that showed detectable aggregates
were the cells that expressed H46R, G127X and D125Tfs 24 mutant SOD1s. Moreover, proteasome inhibition was the only intervention that was found to increase aggregate levels. Aggregated species were then also observed in the A4V and G93A lines and there was a remarkable
increase in the D125Tfs 24 line (Fig 4, Table 1).
In the case of aggregates detected in fibroblasts bearing A4V, H46R and G93A mutations,
we were unable to distinguish between the mutant protein and wild-type SOD1. However, we
could confirm aggregation of the truncated G127X and D125Tfs 24 mutants by western blotting using an anti-SOD1 antibody raised against a peptide in the C-terminal end (amino acids
144–153), which is lacking in these mutants. Using this antibody, which only would detect
wild-type SOD1, no aggregates were detectable (Figure D in S1 File).
Fibroblasts from patients carrying C9orf72 expansions
Using antibodies specific for misfolded SOD1 species, we have previously shown that
SOD1-immunoreactive inclusions can occur in motor neurons and glia in patients with
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Table 1. Detergent-resistant SOD1 aggregates in fibroblast cultures.
Proteasome
inhibition
Autophagy inhibition
ER-stress induction
Inhibition of
mitochondria
Bortezomib
3-MA
Tunicamycin
Rotenone
-
+
-
+
-
+
-
+
A4V
<0.03
0.39
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
H46R
<0.03
0.09
0.15
0.14
<0.03
<0.03
0.09
0.23
N86S
<0.03
<0.03
n. t.
n. t.
<0.03
<0.03
n. t.
n. t.
D90A
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
G93A
<0.03
0.04
<0.03
<0.03
n. t.
n. t.
n. t.
n. t.
L117V
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
G127X
0.20
0.75
0.08
0.06
<0.03
<0.03
<0.03
<0.03
E78_R79insSI
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
D125Tfs*24
0.22
25.26
0.49
0.24
0.73
0.41
0.35
0.30
C9orf72exp
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
C9orf72exp
<0.03
<0.03
n. t.
n. t.
<0.03
<0.03
n. t.
n. t.
Control
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
<0.03
The detergent-resistant aggregates were quantified from western blots. Amounts are presented as % of total amounts of SOD1 in the cultures as
measured by ELISA. The detection limit for SOD1 aggregates in the cultures was approximately 0.03% of total SOD1, n. t. = not tested.
doi:10.1371/journal.pone.0150133.t001
sporadic as well as familial ALS without SOD1 mutations [37, 38]. Therefore, we analysed misSOD1 in fibroblasts from patients carrying the GGGGCC-repeat-expansion in C9orf72. The
misSOD1 levels, as well as the changes induced by the various treatments, did not differ
between the non-disease control cultures and the fibroblast cultures derived from patients carrying C9orf72 expansions (Figs 2 and 3).
Discussion
Cellular models of ALS have been used widely to investigate disease-related pathological abnormalities. These have been mostly based on overexpression of mutant human SOD1s in various
cell types [27, 29, 30]. In this study we have performed the first comprehensive analysis of misfolded, aggregated and total SOD1 in a variety of fibroblast cell lines obtained from ALS
patients carrying mutations in SOD1, as well as from patients carrying the GGGGCC-repeatexpansion in C9orf72 and from non-disease controls. The major advantage of patient-derived
fibroblasts is that they express SOD1s under the control of the endogenous promoter ensuring
an appropriately regulated and physiological level of SOD1 expression. We took advantage of
these cells to gain insight into the effects interfering with various ALS-related pathways on the
levels of misfolded SOD1 as analysed by misELISA.
We found elevated levels of misfolded SOD1 in fibroblast lines that expressed mutant SOD1
compared to the non-disease controls. ER stress has been shown to be enhanced in patientderived motor neurons carrying a SOD1 A4V mutation [16]. However, following a 24 h treatment with tunicamycin, ER stress did not result in any significant changes in misfolded SOD1
levels in fibroblasts despite a robust increase in GRP78 levels. We cannot exclude that sustained
ER stress might lead to an increase in misfolded SOD1, or that mitotically active fibroblasts
show a different response to terminally differentiated motor neurons. Inhibition of mitochondria and autophagy in some cases lead to reduced levels of misfolded SOD1, however, we did
not observe a consistent pattern to this and it might be explained by a differential response of
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Misfolded SOD1 in ALS Fibroblasts
cell lines to the treatments and perhaps reduced protein and SOD1 synthesis. The only perturbation that consistently and uniformly increased the levels of misfolded SOD1 was proteasome
inhibition. Clearly these increases can not be explained only by increased levels of total mutant
SOD1s: misfolded D90A SOD1 rose 3-fold, but no significant change in total mutant protein
was observed in fibroblasts from the homozygous D90A patient. It is also notable that,
although the levels were low, we observed increases in misfolded SOD1 in the non-disease control fibroblast cultures (average of 2.1 fold). In this context it is of interest to note that inclusions containing misfolded SOD1 also have been found in motor neurons from ALS patients
lacking SOD1 mutations [37, 38, 48]. Several previous studies have reported that proteasome
inhibition can increase total levels of overexpressed mutant SOD1s, but amounts of misfolded
SOD1 species have not been specifically analysed [29, 49]. Autophagy inhibition has also been
reported to increase levels of total mutant SOD1 in overexpressing cells [29].
Inclusions containing aggregated SOD1 are a hallmark of ALS, both in patients at end stage
and in transgenic animal models overexpressing mutant SOD1 [26, 28]. Therefore, we investigated the appearance of detergent-resistant aggregates in fibroblasts. In most cases none were
found. The only lines that were found to contain aggregates were those expressing the truncated SOD1 variants D125Tfs 24 and G127X, and the missense variant H46R. Proteasome
inhibition increased the levels of soluble misfolded and detergent-resistant aggregates of SOD1
in these, and caused the appearance of SOD1 aggregates in the A4V, H46R and G93A cell lines.
The levels were generally very low; below 1% of the total SOD1 present in the lysates. This is
different from findings in overexpressed cell culture systems where 10-fold larger proportions
are typically found as aggregated species [30]. SOD1 is able to form several different strains of
aggregate in vivo and in vitro [39]. It is not yet known whether or not SOD1 aggregates formed
in cell culture bear any relation to those that arise and propagate in vivo, however, our results
show that patient-derived fibroblasts could be a useful model with which to study the aggregation process.
The D125Tfs 24 mutant form of SOD1 stands out as remarkable among the mutants studied here. This mutation leads to a frameshift and the inclusion of a 23 aa long neopeptide followed by a stop codon (Table A in S1 File) [50]. Under basal conditions, the levels of misfolded
SOD1 detected by the misELISA are low and comparable with those of fibroblast cultures without SOD1 mutations, yet specific aggregates of the mutant protein were detected (Fig 4). Following proteasome inhibition the relative increase in misfolded SOD1 levels were found to be
the greatest among the mutants tested, and copious amounts of mutant SOD1 aggregates were
formed. Apparently, this mutant is efficiently targeted for proteasome degradation, which perhaps compensates for its huge aggregation propensity since this SOD1 mutation is associated
with a very slowly progressing disease phenotype (D. Lange, unpublished data).
We show that patient-derived fibroblasts, with physiological levels of SOD1 expression,
recapitulate some of the aspects of mutant SOD1 that are known to be important for pathophysiology of ALS, namely increased levels of misfolded SOD1 and presence of detergent insoluble aggregates. Despite the fact that these cells are mitotically active and may not accurately
mimic the cellular environment of aged, post-mitotic motor neurons, these properties make
them a useful model to study ALS-related cellular pathway disturbances.
In conclusion, we have found, somewhat surprisingly, that several of the disturbances associated with SOD1-provoked motor neuron disease including mitochondrial dysfunction and
ER stress do not increase SOD1 misfolding or aggregation per se. Nor does autophagy inhibition, however, we hesitate to rule out a role in aggregate degradation since the degree of inhibition achieved was moderate. The ubiquitin-proteasome system has been found to be inhibited
in mutant SOD1-expressing ALS-model mice [21, 22]. Together with autophagy, the activity of
the ubiquitin-proteasome pathway has also been found to decline with aging [51]. Thus,
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Misfolded SOD1 in ALS Fibroblasts
proteasome impairment with age could be one of the key factors behind the age-related
increase in the incidence of ALS and maybe in forming an amplifying vicious circle that leads
to misfolded SOD1 accumulation.
Supporting Information
S1 File. Supporting Materials and Methods, Figures, and Table. Measurement of in vitro cell
cytotoxicity in the fibroblast lines following proteasome inhibition. (Figure A). Inhibition of
chymotrypsin-like (A), caspase-like (B) and trypsin-like (C) proteasome activities in the fibroblast lines following 0.5 and 5 ng/ml bortezomib treatment. (Figure B). Determination of the
efficacy of 3-MA and tunicamycin treatments. Western blots showing the relative amounts of
(A) LC3-I and LC3-II and (B) GRP78. (Figure C). Detection of full length SOD1 in detergentresistant aggregates in fibroblasts. (Figure D). Study cohort. (Table A).
(DOCX)
Acknowledgments
We wish to thank the patients and their relatives who participated in this study by contributing
skin biopsies. We also thank Agneta Öberg, Ann-Charloth Nilsson, Eva Bern and Eva Jonsson
for skilful technical assistance and Dr. Eiichi Tokuda, Dr. Per Zetterström and Dr. Anna Wuolikainen for technical advice.
Author Contributions
Conceived and designed the experiments: SLM PMA JDG. Performed the experiments: IK EF
AB. Analyzed the data: SLM PMA JDG IK. Contributed reagents/materials/analysis tools: DJL
MW MS PMA. Wrote the paper: SLM JDG PMA IK.
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