BACKGROUND: Serum neurofilament light chain concentration is a proposed biomarker of axonal injury in multiple sclerosis. Mesenchymal stem cells have anti-inflammatory and repair-promoting activities, making them of interest for potential multiple sclerosis treatment. OBJECTIVES: The purpose of this study was to assess correlation of serum neurofilament light chain concentration and measures of multiple sclerosis disease activity/severity, longitudinal stability of serum neurofilament light chain concentration, and treatment effect of mesenchymal stem cell transplantation on serum neurofilament light chain concentration. METHODS: Twenty-four multiple sclerosis patients underwent intravenous infusion of autologous mesenchymal stem cells. Clinical assessments, serum collection, and brain magnetic resonance imaging were performed at months -1, 0 (transplant), 1, 3, and 6. Matched control serum was collected once (n = 10). Serum neurofilament light chain concentration was measured by single-molecule array. Serum neurofilament light chain concentration correlations with disease measures were analyzed by Spearman correlations and linear mixed effect models. Pre-post transplant serum neurofilament light chain concentration was compared by Wilcoxon signed rank testing. RESULTS: There were significant (p<0.01) correlations between serum neurofilament light chain concentration and gadolinium-enhancing lesion number (rho = 0.55) and volume (rho = 0.65), and new/enlarging T2 lesions (rho = 0.65). Patients without disease activity had lower fluctuation in serum neurofilament light chain concentration (p = 0.01). Mean pre- versus post-treatment serum neurofilament light chain concentration values were not significantly different. CONCLUSIONS: Serum neurofilament light chain concentration correlated with magnetic resonance imaging measures of disease activity cross sectionally and longitudinally, and was stable in patients without disease activity. There was no clear treatment effect of mesenchymal stem cell transplantation on serum neurofilament light chain concentration.
BACKGROUND: Serum neurofilament light chain concentration is a proposed biomarker of axonal injury in multiple sclerosis. Mesenchymal stem cells have anti-inflammatory and repair-promoting activities, making them of interest for potential multiple sclerosis treatment. OBJECTIVES: The purpose of this study was to assess correlation of serum neurofilament light chain concentration and measures of multiple sclerosis disease activity/severity, longitudinal stability of serum neurofilament light chain concentration, and treatment effect of mesenchymal stem cell transplantation on serum neurofilament light chain concentration. METHODS: Twenty-four multiple sclerosis patients underwent intravenous infusion of autologous mesenchymal stem cells. Clinical assessments, serum collection, and brain magnetic resonance imaging were performed at months -1, 0 (transplant), 1, 3, and 6. Matched control serum was collected once (n = 10). Serum neurofilament light chain concentration was measured by single-molecule array. Serum neurofilament light chain concentration correlations with disease measures were analyzed by Spearman correlations and linear mixed effect models. Pre-post transplant serum neurofilament light chain concentration was compared by Wilcoxon signed rank testing. RESULTS: There were significant (p<0.01) correlations between serum neurofilament light chain concentration and gadolinium-enhancing lesion number (rho = 0.55) and volume (rho = 0.65), and new/enlarging T2 lesions (rho = 0.65). Patients without disease activity had lower fluctuation in serum neurofilament light chain concentration (p = 0.01). Mean pre- versus post-treatment serum neurofilament light chain concentration values were not significantly different. CONCLUSIONS: Serum neurofilament light chain concentration correlated with magnetic resonance imaging measures of disease activity cross sectionally and longitudinally, and was stable in patients without disease activity. There was no clear treatment effect of mesenchymal stem cell transplantation on serum neurofilament light chain concentration.
Neurofilaments are protein components of the cytoskeleton of myelinated axons.
Neurofilament-light chain concentration (NfL-c) has generated substantial
interest as a putative biomarker of axonal injury and is being investigated
in several neurological diseases, including multiple sclerosis
(MS).[1-11]
However, it has yet to be fully validated for clinical use in these
settings, as the significance and variability at the individual patient
level is not yet known. Development of a biomarker for disease activity and
potentially prognosis in MS is of significant interest and would be of great
utility in clinical trials, observational studies, and patient care.[12]In MS, prior studies demonstrated elevated NfL-c concentrations in
cerebrospinal fluid (CSF) correlate with relapse, gadolinium-enhancing
lesions on magnetic resonance imaging (MRI), and disease severity.[1,11,13,14]
Initiation of disease modifying therapy in MS is associated with decreased
NfL-c levels in the CSF, possibly reflecting reduced axonal
damage.[15-17] Single-molecule array (Simoa) technology allows NfL-c
to be detected in serum,[18] and there is a strong correlation between CSF and serum
NfL-c.[1,14] Given the less invasive nature of a blood draw
compared to lumbar puncture, evaluation of serum rather than CSF NfL-c is of
substantial interest as a biomarker for MS disease activity and treatment
response.Mesenchymal stem cells (MSCs) are pluripotent, non-hematopoietic precursor
cells that can be isolated from various tissues, including bone marrow and
adipose, and culture-expanded to purity. MSCs are postulated to have a range
of anti-inflammatory and repair-promoting activities, making them of
interest in several neuroinflammatory and tissue injury conditions,
including MS.[19-21] Previously published studies regarding MSC
transplantation in MS have been mostly phase I trials to examine safety and
tolerability, and to date, the safety of MSC transplantation has been
largely supported.[20,22-26]In the MSC transplantation study performed at our institution, there was
suggestion of benefit on the Expanded Disability Status Scale (EDSS), as 17
of 24 patients had improved EDSS at three months post-treatment versus baseline.[22] Additionally, there was suggestion of benefit in two MRI measures,
whole brain magnetization transfer ratio and magnetization transfer ratio
peak height, which trended upwards over post-treatment months 1–3 compared
to baseline. NfL-c has not been examined in previous studies of MSC
transplantation.In this study, we sought to compare serum NfL-c (sNfL-c) between MS patients
and healthy controls, evaluate the correlation of sNfL-c and various imaging
and clinical markers of MS disease activity and severity, evaluate the
short-term longitudinal stability of sNfL-c, and examine the treatment
effect of MSC transplantation on sNfL-c in a previously completed phase 1/2
trial of MSC transplantation in MS.
Materials and methods
Study design
A phase 1/2, single-center, single-arm clinical trial of autologous
culture-expanded MSC transplantation enrolled patients between March
2011–April 2013 at the Cleveland Clinic Mellen Center. Methods have
been previously described.[22,27] The study involved laboratory, clinical, and
imaging evaluations over a seven-month period, with MSC
transplantation (considered month 0 (M0)) occurring two months
following screening (month –2 (M–2)). Each patient had five banked
serum samples, collected at month (M) –1, 0 (baseline), 1, 3, and 6,
with concomitant clinical assessments and brain MRI. Cleveland Clinic
Institutional Review Board approval was obtained, and informed consent
was obtained from all patients prior to any study procedures (Study
#10-726, #08-964).
Patient population
Eligible patients had relapsing–remitting MS (RRMS) or secondary
progressive MS (SPMS), based on the 2010 McDonald criteria,[28] were between the ages of 18–55 years, had an EDSS score of
3.0–6.5, and had evidence of disease activity or disability worsening
in the two prior years. Patients were permitted to continue
interferon-beta or glatiramer acetate during the study. Complete
inclusion/exclusion criteria have been previously reported.[22] Age- and sex-matched healthy controls provided a single serum
sample, 10 of which were available for the current study.
Clinical assessment
At each study visit, patients underwent clinical assessment, including
evaluation for relapse, EDSS, and Multiple Sclerosis Functional
Composite (paced auditory serial addition test (PASAT), 9-hole peg
test (9HPT), timed 25-foot walk (T25FW), and high- and low-contrast
(2.5% and 1.25%) letter acuity (LCLA) using Sloan charts).[29-31] PASAT score
was reported as the three-second total correct. For 9HPT, patients
underwent two trials per hand, and the average of the two trials (in
seconds) in the worse hand was used for this analysis. For T25FW,
patients underwent two trials and the average time (in seconds) of the
trials was used for analysis. For LCLA, 2.5% visual acuity was
reported as the number correct in the worse eye.
Imaging assessment
Brain MRIs were obtained on a 3T Siemens Trio MRI scanner (Erlangen,
Germany) according to a standardized protocol at each study visit.[22] Images were analyzed by the MRI Analysis Center in the
Biomedical Engineering Department of Lerner Research Institute
(Cleveland Clinic, Cleveland, Ohio, USA). MRI measurements included in
the original study were gadolinium-enhancing lesion number and volume,
new/enlarging T2-hyperintense lesion number, T2-hyperintense lesion
volume (T2LV), T1-hypointense lesion volume (T1LV), normalized whole
brain volume (brain parenchymal fraction (BPF)), gray matter fraction,
whole brain diffusion tensor imaging (DTI, mean diffusivity (MD),
fractional anisotropy (FA)), and whole brain magnetization transfer
ratio (MTR). Additional MRI metrics analyzed post-hoc included
cortical thickness and further DTI parameters (FA, MD, transverse
diffusivity (TD), and axial diffusivity (AD)) in lesional tissue,
corticospinal tracts (reported as average of left and right), and the
transcallosal motor tract.[32]Optical coherence tomography (OCT) was performed at each study visit
using a Cirrus spectral domain machine (Carl Zeiss Meditec, Dublin,
California, USA). Patients underwent two OCT scans at each visit. OCT
parameters of interest include average and temporal retinal nerve
fiber layer thickness (RNFL), both of which are reported as the mean
of two measurements in the better eye at each visit, in microns.
Visual evoked potentials
Patients underwent visual evoked potentials (VEPs) at each visit, using
an Eclipse Neurological Workstation (Axon Systems, Hauppauge, New
York, USA) at a single center (Cleveland Clinic EEG Laboratory,
Cleveland, Ohio, USA). Mean P100 latency for each eye was determined
from two recordings.
Serum NfL-c measurement
Patient and control serum samples were run in duplicate on the Quanterix
(Cambridge, Massachusetts, USA) Simoa assay (NF-light Advantage Kit)
to quantify sNfL-c.
Statistical analysis
Demographics of MS patients and controls were compared by Student’s
t-tests for continuous and Chi-squared
testing for categorical variables. Given the non-normality of
sNfL-c distributions, analyses employed non-parametric methods.
Matched MS and control sNfL-c were compared at baseline by
Wilcoxon rank sum testing for paired samples. sNfL-c was
compared between patients with RRMS and SPMS via Kruskal-Wallis
testing. Cross-sectional associations between sNfL-c and markers
of MS disease activity and severity at baseline were evaluated
via Spearman rank correlation coefficients. Metrics with a
significant cross-sectional correlation were further
investigated longitudinally using linear mixed effect models,
using patient as a random effect.To assess short-term longitudinal stability of sNfL-c, the mean
absolute difference in sNfL-c compared to the first measurement
(M–1) was calculated for each patient (sNfL-c fluctuation).
Patients were then characterized as having inflammatory disease
activity if they had any relapse, new/enlarging T2 hyperintense
lesion, or gadolinium-enhancing lesion over the course of the
study. Patients were further delineated into each component of
inflammatory activity, and these groups (presence versus absence
of relapse, new/enlarging T2 hyperintense lesion, or
gadolinium-enhancing lesion) were compared as well. The mean
sNfL-c fluctuation was then compared between the active versus
non-active disease groups via an unpaired t-test.To investigate a potential MSC treatment effect, pre- and
post-treatment average sNfL-c values were compared by Wilcoxon
signed rank testing for paired samples. The correlations between
change in sNfL-c and change in selected clinical and MRI
measures of interest in the pre- versus post-treatment periods
(difference calculated between means for the pre- and
post-treatment values) were evaluated using Spearman rank
correlation coefficients. Given the exploratory nature of this
study, we did not adjust for multiple comparisons. Statistical
analyses were conducted in R (version 3.5.3), utilizing the
packages spearmanCI (version 1.0), nlme (version 3.1–140), and
tidyverse (version 1.2.1).
Results
Patient characteristics
Twenty-four patients with MS, 10 with relapsing–remitting and 14 with
secondary progressive disease underwent MSC transplantation between
2011 and 2013.[22] Twenty-two patients consented to accessory studies and had
banked samples available. Sixteen of these 22 patients were female,
and the patient age range was 18–55 years (mean 46.4 ± 5.2 years)
(Table
1). Serum samples were available from 10 age- and
sex-matched controls.
sNfL-c was higher in MS patients at baseline versus matched controls
(n = 10, p = 0.008) (Figure 1). The
median (interquartile range) sNfL-c in MS patients with a matched
control was 14.60 (6.02) pg/ml (versus 6.92 (3.41) pg/ml in controls),
and without a matched control was 14.71 (5.85) pg/ml. The median
sNfL-c difference between paired MS patients and controls was 5.95
pg/ml (95% confidence interval (CI) 1.60–30.66). There was no
difference in sNfL-c between patients with RRMS and SPMS
(p = 0.393).
Figure 1.
Serum neurofilament light chain concentration (sNfL-c) in
multiple sclerosis (MS) patients versus controls.
A boxplot compares sNfL-c in MS patients and matched
controls, with y-axis on log scale.
sNfL-c was higher in MS patients at baseline (median 14.60
pg/ml) versus matched controls (median 6.92 pg/ml)
(n=10,
p=0.008).
Serum neurofilament light chain concentration (sNfL-c) in
multiple sclerosis (MS) patients versus controls.A boxplot compares sNfL-c in MS patients and matched
controls, with y-axis on log scale.
sNfL-c was higher in MS patients at baseline (median 14.60
pg/ml) versus matched controls (median 6.92 pg/ml)
(n=10,
p=0.008).
Clinical disability and sNfL-c
No significant correlations were observed between sNfL-c and clinical
disability measures (EDSS, PASAT, 9HPT, T25FW, and LCLA) at baseline
(n = 22) (Table 2). There were no
relapses documented at the baseline visit, so the correlation between
relapse and sNfL-c was instead investigated via longitudinal analysis,
described below.
Table 2.
Correlations of serum neurofilament light chain concentration
(sNfL-c) and disease activity measures.
Correlations of serum neurofilament light chain concentration
(sNfL-c) and disease activity measures.CI: confidence interval; MRI: magnetic resonance
imaging; RNFL: retinal nerve fiber layer.Bold indicates statistical significance
(p<0.05)
MRI measures and sNfL-c
There were significant (p<0.05) correlations at M0
(baseline) between sNfL-c and gadolinium-enhancing lesion number
(Spearman’s rho = 0.55, 95% CI 0.27–0.83) and volume (rho = 0.59, 95%
CI 0.35–0.94), new/enlarging T2 lesions (rho = 0.65, 95% CI
0.29–0.99), T2LV (rho = 0.49, 95% CI 0.02–0.95) and T1-hypointense
lesion volume (rho = 0.51, 95% CI 0.12–0.90) (n = 21)
(Table
2, Figure 2). However, there was no correlation between
sNfL-c and brain parenchymal fraction, gray matter fraction, or
DTI-derived metrics (Table 2, Supplemental
Material Table
1).
Figure 2.
Serum neurofilament light chain concentration (sNfL-c)
significantly correlated with measures of magnetic
resonance imaging (MRI) disease activity and severity.
Scatterplots demonstrate that at baseline, sNfL-c
significantly correlated with (a) number and (b) volume of
gadolinium-enhancing lesions, (c) number of new/enlarging
T2 hyperintense lesions, (d) T2 hyperintense lesion
volume, and (e) T1 hypointense lesion volume. The blue
line in each figure represents a simple linear regression
line.
Serum neurofilament light chain concentration (sNfL-c)
significantly correlated with measures of magnetic
resonance imaging (MRI) disease activity and severity.Scatterplots demonstrate that at baseline, sNfL-c
significantly correlated with (a) number and (b) volume of
gadolinium-enhancing lesions, (c) number of new/enlarging
T2 hyperintense lesions, (d) T2 hyperintense lesion
volume, and (e) T1 hypointense lesion volume. The blue
line in each figure represents a simple linear regression
line.
Anterior visual system measures and sNfL-c
No significant correlations were observed between sNfL-c and visual
pathway measures at baseline, including RNFL thickness and P100
latency (n = 22) (Table 2).
Longitudinal analyses
We explored clinical and MRI measures of new disease activity and/or
burden longitudinally using linear mixed effects modeling with a
subject random effect (Table 3). For each
gadolinium-enhancing lesion, there was a 2.62 (95% CI 0.79–4.45) pg/ml
significant increase in sNfL-c. An additional 1 ml of
gadolinium-enhancing lesion volume was associated with a 14.61 (95% CI
6.67–22.56) pg/ml significant increase in sNfL-c. Each additional
new/enlarging T2 hyperintense lesion was associated with a 2.41 (95%
CI 1.06–3.76) pg/ml significant increase in sNfL-c. An additional mL
of T2-hyperintense lesion volume was associated with a 0.47 (95% CI
0.15–0.79) pg/ml significant increase in sNfL-c. An additional 1 ml of
T1-hypointense lesion volume was associated with a 2.06 (95% CI
0.89–3.22) pg/ml significant increase in sNfL-c. A 1 mm decrease in
cortical thickness was associated with a 19.28 (95% CI 1.91–36.64)
pg/ml significant increase in sNfL-c. A 1.0% decrease in BPF was
associated with a 1.33 (95% CI 0.33–2.33) pg/ml significant increase
in sNfL-c. A relapse was associated with an 8.37 (95% CI –2.56–19.29)
pg/ml non-significant increase in sNfL-c.
Table 3.
Longitudinal analyses via linear mixed effects models.
Clinical or MRI metric
Beta (95% CI)
p-Value
Gadolinium-enhancing lesion number
2.62 (0.79–4.45)
0.006
Gadolinium-enhancing lesion volume (ml)
14.61 (6.67–22.56)
0.0004
New/enlarging T2 lesions (number)
2.41 (1.06–3.76)
0.0006
T2 hyperintense lesion volume (ml)
0.47 (0.15–0.79)
0.0046
T1 hypointense lesion volume (ml)
2.06 (0.89–3.22)
0.0007
Brain parenchymal fraction (%)
–1.33 (–2.33––0.33)
0.0099
Cortical thickness (mm)
–19.28 (–36.7––1.9)
0.03
Relapse
8.37 (–2.56–19.29)
0.1315
CI: confidence interval; MRI: magnetic resonance
imaging.
Longitudinal analyses via linear mixed effects models.CI: confidence interval; MRI: magnetic resonance
imaging.
Longitudinal stability of sNfL-c
Overall, the mean ( ± standard deviation) fluctuation in sNfL-c over the
course of the study was 5.67 ± 7.2 pg/ml. In patients with
inflammatory disease activity (n = 17), fluctuation
in sNfL-c was 6.93 ± 7.8 pg/ml, which was significantly higher than
those without inflammatory disease activity (n = 5),
1.38 ± 0.7 pg/ml (p = 0.01) (Figure 3). Two patients with
active disease (one with new/enlarging T2 hyperintense lesions at M–1
and M6, and the other with a clinical relapse and new/enlarging T2
hyperintense lesions at M1) had overall low sNfL-c, and no apparent
changes in sNfL-c associated with observed disease activity.
Figure 3.
Longitudinal stability of serum neurofilament light chain
concentration (sNfL-c) in non-active versus active
disease.
sNfL-c fluctuation in patients with (n=17)
and without (n=5) disease activity
(defined by clinical relapses, new/enlarging T2 lesions on
brain magnetic resonance imaging (MRI), or
gadolinium-enhancing lesions on brain MRI) is demonstrated
in a faceted spaghetti plot. On the left, patients without
active disease had lower sNfL-c fluctuation (1.38±0.7
pg/ml). On the right, patients with active disease had
higher degrees of sNfL-c fluctuation (6.93±7.8 pg/ml,
p-value for comparison=0.01).
Longitudinal stability of serum neurofilament light chain
concentration (sNfL-c) in non-active versus active
disease.sNfL-c fluctuation in patients with (n=17)
and without (n=5) disease activity
(defined by clinical relapses, new/enlarging T2 lesions on
brain magnetic resonance imaging (MRI), or
gadolinium-enhancing lesions on brain MRI) is demonstrated
in a faceted spaghetti plot. On the left, patients without
active disease had lower sNfL-c fluctuation (1.38±0.7
pg/ml). On the right, patients with active disease had
higher degrees of sNfL-c fluctuation (6.93±7.8 pg/ml,
p-value for comparison=0.01).Investigation of sNfL-c fluctuation by each component of inflammatory
disease activity demonstrated that patients with new/enlarging T2
lesions (n = 16) had significantly higher fluctuation
versus those without (7.08 ± 8.1 vs 1.89 ± 1.4 pg/ml, respectively,
p = 0.02) (Supplemental Material Figure 1).
Similarly, patients with gadolinium-enhancing lesions
(n = 13) had significantly higher sNfL-c
fluctuation versus those without (8.57 ± 8.3 vs 1.48 ± 1.2 pg/ml,
respectively, p = 0.01) (Supplemental Material Figure 2).
However, patients with and without clinical relapses were not
significantly different in terms of sNfL-c fluctuation (6.30 ± 8.0 vs
3.52 ± 3.4 pg/ml, respectively, p = 0.28)
(Supplemental Material Figure 3).
Treatment effect of MSCs
Post-transplant, sNfL-c decreased at M1 (median difference –0.91 pg/ml),
M3 (–0.11 pg/ml), and M6 (–0.75 pg/ml) compared to baseline, but
differences did not reach statistical significance (Figure 4(a)).
Mean pre- (M–1, M0) versus post-treatment (M1–6) sNfL-c values were
not significantly different (p = 0.82, Figure 4(b)).
At the individual patient level, changes in sNfL-c were heterogeneous:
some patients had decreased, increased, or stable sNfL-c comparing
pre- and post-treatment (Figure 4(c)).
Figure 4.
Pre- vs post-treatment serum neurofilament light chain
concentration (sNfL-c).
(a) Overall, median sNfL-c decreased post-transplant at M1
(median difference –0.91 pg/ml), M3 (–0.11 pg/ml), and M6
(–0.75 pg/ml) compared to baseline, but differences did
not reach statistical significance. (b) Median and mean
pre- versus post-treatment sNfL-c were not significantly
different (p=0.82). (c) Patients had
heterogeneous pre- versus post- treatment trajectories of
sNfL-c concentrations. The spaghetti plot demonstrates
that some patients had decreased, increased, or stable
sNfL-c comparing pre- and post-treatment. MSC: mesenchymal
stem cell.
Pre- vs post-treatment serum neurofilament light chain
concentration (sNfL-c).(a) Overall, median sNfL-c decreased post-transplant at M1
(median difference –0.91 pg/ml), M3 (–0.11 pg/ml), and M6
(–0.75 pg/ml) compared to baseline, but differences did
not reach statistical significance. (b) Median and mean
pre- versus post-treatment sNfL-c were not significantly
different (p=0.82). (c) Patients had
heterogeneous pre- versus post- treatment trajectories of
sNfL-c concentrations. The spaghetti plot demonstrates
that some patients had decreased, increased, or stable
sNfL-c comparing pre- and post-treatment. MSC: mesenchymal
stem cell.We also investigated the correlation of pre- versus post-treatment change
in sNfL-c and in selected other measures. There were significant
correlations between pre-post treatment differences in sNfL-c and T2LV
(rho = 0.41, 95% CI 0.01–0.80) and gadolinium-enhancing lesion number
(rho = 0.51, 95% CI 0.04–0.97). Given the lack of change observed
pre-post treatment in EDSS, whole brain MTR, whole brain MTR peak
height, new/enlarging T2 lesions, gadolinium-enhancing lesion volume,
cortical thickness, brain parenchymal fraction,[22,32] and relapse,
we did not observe significant correlations between pre-post change in
these measures and change in sNfL-c.
Discussion
sNfL-c was higher in MS patients compared to controls and correlated with
markers of disease severity and activity on MRI, both cross-sectionally and
longitudinally. There were significant correlations between change in pre-
versus post-treatment sNfL-c and corresponding change in T2LV and
gadolinium-enhancing lesion number. Additionally, sNfL-c appeared stable
over a relatively short study period (six months) in the absence of disease
activity. These results are consistent with the growing body of evidence
supporting use of sNfL-c as a biomarker in MS.[1,11,13,14] Additionally, this
study is the first to investigate sNfL-c in the context of MSC
transplantation.Our results differ in some ways from the published literature. The study did
not demonstrate association between relapses and sNfL-c elevation, possibly
due to the low incidence of relapse in this cohort (n = 5)
and the overall small sample size. As sNfL-c is thought to be a marker of
acute axonal injury, our findings that sNfL-c was cross-sectionally
associated with T1LV and T2LV were somewhat surprising, as they are
considered indicators of a more chronic disease burden. However, the
cross-sectional association of CSF NfL-c with T1LV in patients with
progressive MS[33] and longitudinal association with T2LV in patients with
relapsing-onset MS[34] have been reported in recent studies. Further studies are needed to
delineate the relative utility and correlates of sNfL-c in relapsing and
progressive forms of MS to better inform clinical trial design in the
future.The longitudinal variability of sNfL-c at the individual patient level is not
clearly established, but our results demonstrated overall stability over a
six-month period in patients without disease activity. The presence of
gadolinium-enhancing lesions was the most substantial contributor to
increased fluctuation in sNfL-c and most reliably delineated patients with
higher versus lower sNfL-c (Supplemental Material Figure 2). Though new/enlarging
T2-hyperintense lesions and clinical relapses are indicative of inflammatory
disease activity, there were two patients in particular who had such events
without concomitant increase in sNfL-c. These findings may be attributed to
the timing of clinical assessments or brain MRI in relation to disease
activity, though we would expect to detect a meaningful change in sNfL-c
with such close clinical and radiographic surveillance in this study.
Further studies are needed to better quantify the sensitivity of sNfL-c
increase in response to clinical and imaging disease biomarkers of interest,
particularly as sNfL-c is becoming incorporated as a biomarker into larger
clinical trials. The degree of fluctuation of sNfL-c from baseline could
also be investigated as a potential predictor of disease activity in future
studies, as interpretation of an sNfL-c value in isolation may be
misleading.There was no clear treatment effect of MSC transplantation on sNfL-c. Though
the original phase 1/2 clinical trial reported potential improvement in a
few exploratory outcomes, namely EDSS, whole brain MTR, and MTR peak height,
change in sNfL-c did not correlate with these potential indicators of
treatment response, either cross-sectionally or longitudinally. This overall
stability in sNfL-c also coincided with lack of clear clinical improvement
observed in the trial, in contrast to the treatment response in sNfL-c seen
with existing MS disease-modifying therapies. The small sample size limited
power to detect such changes, as did variability of sNfL-c change in the
study population (Figure
4(c)). However, we did observe correlations in pre-post
treatment changes of sNfL-c and T2LV and gadolinium-enhancing lesion number
in expected directions; this finding does not necessarily reflect a
treatment effect of MSCs.The main limitation of this study is its small sample size. As NfL-c is
primarily a biomarker of axonal damage, it is thought to primarily reflect
acute inflammatory activity, including new/enlarging MRI lesions and
clinical relapses. The drivers of sNfL-c in patients with relapsing and
progressive forms of MS may therefore be different, which may have limited
our ability to observe consistent effects in this potentially heterogeneous
population.Given the proposed repair mechanism of action for MSCs, future trials should
consider incorporation of sNfL-c as an outcome measure given its overall
consistent correlations with various markers of disease severity and ease of
collection compared to CSF NfL-c. However, patients with progressive MS are
less likely to have inflammatory disease activity that is more readily
captured by sNfL-c, so using sNfL-c as an indirect marker of repair requires
understanding of the biomarker in the patient population of interest when
planning a clinical trial. Additionally, future work is needed to determine
longitudinal stability and the clinical relevance of sNfL-c changes in an
individual patient.Click here for additional data file.Supplemental material, MSO887198 Supplemetal Material for Serum
neurofilament light chain concentration in a phase 1/2 trial of
autologous mesenchymal stem cell transplantation by Laura E
Baldassari, Sarah M Planchon, Robert A Bermel, Kunio Nakamura,
Elizabeth Fisher, Jenny Feng, Ken E Sakaie, Daniel Ontaneda and
Jeffrey A Cohen in Multiple Sclerosis Journal – Experimental,
Translational and Clinical
Authors: Lenka Novakova; Markus Axelsson; Mohsen Khademi; Henrik Zetterberg; Kaj Blennow; Clas Malmeström; Fredrik Piehl; Tomas Olsson; Jan Lycke Journal: J Neurochem Date: 2016-11-29 Impact factor: 5.372
Authors: Julio C Rojas; Jee Bang; Iryna V Lobach; Richard M Tsai; Gil D Rabinovici; Bruce L Miller; Adam L Boxer Journal: Neurology Date: 2017-12-27 Impact factor: 9.910
Authors: Peter Connick; Madhan Kolappan; Charles Crawley; Daniel J Webber; Rickie Patani; Andrew W Michell; Ming-Qing Du; Shi-Lu Luan; Daniel R Altmann; Alan J Thompson; Alastair Compston; Michael A Scott; David H Miller; Siddharthan Chandran Journal: Lancet Neurol Date: 2012-01-10 Impact factor: 44.182
Authors: Sarah M Planchon; Karen T Lingas; Jane Reese Koç; Brittney M Hooper; Basabi Maitra; Robert M Fox; Peter B Imrey; Kylie M Drake; Micheala A Aldred; Hillard M Lazarus; Jeffrey A Cohen Journal: Mult Scler J Exp Transl Clin Date: 2018-03-26
Authors: Jonathan D Rohrer; Ione O C Woollacott; Katrina M Dick; Emilie Brotherhood; Elizabeth Gordon; Alexander Fellows; Jamie Toombs; Ronald Druyeh; M Jorge Cardoso; Sebastien Ourselin; Jennifer M Nicholas; Niklas Norgren; Simon Mead; Ulf Andreasson; Kaj Blennow; Jonathan M Schott; Nick C Fox; Jason D Warren; Henrik Zetterberg Journal: Neurology Date: 2016-08-31 Impact factor: 9.910
Authors: Philip S J Weston; Teresa Poole; Natalie S Ryan; Akshay Nair; Yuying Liang; Kirsty Macpherson; Ronald Druyeh; Ian B Malone; R Laila Ahsan; Hugh Pemberton; Jana Klimova; Simon Mead; Kaj Blennow; Martin N Rossor; Jonathan M Schott; Henrik Zetterberg; Nick C Fox Journal: Neurology Date: 2017-10-25 Impact factor: 9.910
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