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Original research
Neuronal pentraxin 2: a synapse-derived CSF biomarker in genetic frontotemporal dementia
  1. Emma L van der Ende1,
  2. Meifang Xiao2,
  3. Desheng Xu2,
  4. Jackie M Poos1,
  5. Jessica L Panman1,3,
  6. Lize C Jiskoot1,4,
  7. Lieke H Meeter1,
  8. Elise GP Dopper1,
  9. Janne M Papma1,
  10. Carolin Heller5,
  11. Rhian Convery4,
  12. Katrina Moore4,
  13. Martina Bocchetta4,
  14. Mollie Neason4,
  15. Georgia Peakman4,
  16. David M Cash4,
  17. Charlotte E Teunissen6,
  18. Caroline Graff7,8,
  19. Matthis Synofzik9,10,
  20. Fermin Moreno11,
  21. Elizabeth Finger12,
  22. Raquel Sánchez-Valle13,
  23. Rik Vandenberghe14,
  24. Robert Laforce Jr15,
  25. Mario Masellis16,
  26. Maria Carmela Tartaglia17,
  27. James B Rowe18,
  28. Christopher R Butler19,
  29. Simon Ducharme20,
  30. Alex Gerhard21,22,
  31. Adrian Danek23,
  32. Johannes Levin23,24,25,
  33. Yolande AL Pijnenburg26,
  34. Markus Otto27,
  35. Barbara Borroni28,
  36. Fabrizio Tagliavini29,
  37. Alexandre de Mendonca30,
  38. Isabel Santana31,
  39. Daniela Galimberti32,33,
  40. Harro Seelaar1,
  41. Jonathan D Rohrer4,
  42. Paul F Worley2,34,
  43. John C van Swieten1
  44. on behalf of the Genetic Frontotemporal Dementia Initiative (GENFI)
    1. 1 Department of Neurology and Alzheimer Center, Erasmus University Medical Center, Rotterdam, Netherlands
    2. 2 Solomon H Snyder Department of Neuroscience, Johns Hopkins University School of Medicine, Baltimore, Maryland, United States
    3. 3 Department of Radiology, Leiden University Medical Center, Leiden, Netherlands
    4. 4 Dementia Research Centre, UCL Queen Square Institute of Neurology, London, United Kingdom
    5. 5 Dementia Research Institute, Department of Neurodegenerative Disease, University College London, London, United Kingdom
    6. 6 Neurochemistry Laboratory, Department of Clinical Chemistry, Amsterdam Neuroscience, Amsterdam University Medical Center, Amsterdam, Netherlands
    7. 7 Karolinska Institutet, Dept NVS, Division of Neurogeriatrics, Bioclinicum, Stockholm, Sweden
    8. 8 Unit of Hereditary Dementia, Theme Aging, Karolinska University Hospital-Solna, Stockholm, Sweden
    9. 9 German Center for Neurodegenerative Diseases (DZNE), University of Tübingen, Tübingen, Germany
    10. 10 Department of Neurodegenerative Diseases, Hertie Institute for Clinical Brain Research, Tübingen, Germany
    11. 11 Department of Neurology, Donostia University Hospital, San Sebastian, Gipuzkoa, Spain
    12. 12 Department of Clinical Neurological Sciences, University of Western Ontario, London, Ontario, Canada
    13. 13 Alzheimer's Disease and Other Cognitive Disorders Unit, Hospital Clinic de Barcelona, Barcelona, Spain
    14. 14 Laboratory for Cognitive Neurology, Department of Neurosciences, KU Leuven, Leuven, Belgium
    15. 15 Clinique Interdisciplinaire de Mémoire du CHU de Québec, Département des Sciences Neurologiques, Université Laval, Québec, Quebec City, Canada
    16. 16 Sunnybrook Health Sciences Centre, Sunnybrook Research Institute, University of Toronto, Toronto, Ontario, Canada
    17. 17 Tanz Centre for Research in Neurodegenerative Disease, University of Toronto, Toronto, Ontario, Canada
    18. 18 Cambridge University Centre for Frontotemporal Dementia, University of Cambridge, Cambridge, United Kingdom
    19. 19 Department of Clinical Neurology, University of Oxford, Oxford, United Kingdom
    20. 20 Montreal Neurological Institute and McGill University Health Centre, McGill University, Montreal, Québec, Canada
    21. 21 Department of Nuclear Medicine and Geriatric Medicine, University Hospital Essen, Essen, Germany
    22. 22 Divison of Neuroscience and Experimental Psychology, University of Manchester, Manchester, United Kingdom
    23. 23 Neurologische Klinik und Poliklinik, Ludwig-Maximilians-Universität München, Munich, Germany
    24. 24 German Center for Neurodegenerative Diseases, (DZNE), Munich, Germany
    25. 25 Munich Cluster for Systems Neurology, (SyNergy), Munich, Germany
    26. 26 Alzheimer Center Amsterdam, Department of Neurology, Amsterdam Neuroscience, Vrije Universiteit Amsterdam, Amsterdam UMC, Amsterdam, Netherlands
    27. 27 Department of Neurology, Universität Ulm, Ulm, Germany
    28. 28 Centre for Neurodegenerative Disorders, Neurology Unit, Department of Clinical and Experimental Sciences, University of Brescia, Brescia, Italy
    29. 29 Fondazione IRCCS, Istituto Neurologico Carlo Besta, Milan, Italy
    30. 30 Faculty of Medicine, University of Lisbon, Lisbon, Portugal
    31. 31 Center for Neuroscience and Cell Biology, Faculty of Medicine, University of Coimbra, Coimbra, Portugal
    32. 32 Department of Neurological Sciences, Dino Ferrari Center, University of Milan, Milan, Italy
    33. 33 Fondazione IRCCS Ca' Granda, Ospedale Maggiore Policlinico, Milan, Italy
    34. 34 Department of Neurology, Johns Hopkins University School of Medicine, Baltimore, Maryland, United States
    1. Correspondence to Dr John C van Swieten, Department of Neurology, Erasmus MC, Rotterdam, Netherlands; j.c.vanswieten{at}erasmusmc.nl

    Abstract

    Introduction Synapse dysfunction is emerging as an early pathological event in frontotemporal dementia (FTD), however biomarkers are lacking. We aimed to investigate the value of cerebrospinal fluid (CSF) neuronal pentraxins (NPTXs), a family of proteins involved in homeostatic synapse plasticity, as novel biomarkers in genetic FTD.

    Methods We included 106 presymptomatic and 54 symptomatic carriers of a pathogenic mutation in GRN, C9orf72 or MAPT, and 70 healthy non-carriers participating in the Genetic Frontotemporal dementia Initiative (GENFI), all of whom had at least one CSF sample. We measured CSF concentrations of NPTX2 using an in-house ELISA, and NPTX1 and NPTX receptor (NPTXR) by Western blot. We correlated NPTX2 with corresponding clinical and neuroimaging datasets as well as with CSF neurofilament light chain (NfL) using linear regression analyses.

    Results Symptomatic mutation carriers had lower NPTX2 concentrations (median 643 pg/mL, IQR (301–872)) than presymptomatic carriers (1003 pg/mL (624–1358), p<0.001) and non-carriers (990 pg/mL (597–1373), p<0.001) (corrected for age). Similar results were found for NPTX1 and NPTXR. Among mutation carriers, NPTX2 concentration correlated with several clinical disease severity measures, NfL and grey matter volume of the frontal, temporal and parietal lobes, insula and whole brain. NPTX2 predicted subsequent decline in phonemic verbal fluency and Clinical Dementia Rating scale plus FTD modules. In longitudinal CSF samples, available in 13 subjects, NPTX2 decreased around symptom onset and in the symptomatic stage.

    Discussion We conclude that NPTX2 is a promising synapse-derived disease progression biomarker in genetic FTD.

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    Introduction

    Frontotemporal dementia (FTD), a common form of early-onset dementia, has an autosomal dominant inheritance in 20%–30% of patients, most often due to mutations in granulin (GRN), chromosome 9 open reading frame 72 (C9orf72) or microtubule-associated protein tau (MAPT).1 Developing sensitive biomarkers to detect disease onset at an early, even preclinical stage is of utmost importance for upcoming therapeutic interventions. Genetic forms of FTD provide a unique opportunity to study disease progression from presymptomatic to overt FTD and to identify novel biomarkers.

    Our previous proteomics study identified neuronal pentraxin receptor (NPTXR) in cerebrospinal fluid (CSF) as the most promising candidate biomarker in genetic FTD, with markedly reduced levels in the symptomatic stage.2 NPTXR forms complexes with NPTX1 and NPTX2 (also termed neuronal activity related protein, Narp) at excitatory synapses of pyramidal neurons onto parvalbumin interneurons and contributes to synaptic homeostatic plasticity.3 4 Increasing evidence suggests that dysfunction and degeneration of synapses is an early pathological event in FTD,5–7 especially in GRN-associated FTD,8–10 a concept widely recognised in other neurodegenerative diseases.5 11 Fluid biomarkers reflecting synaptic integrity in FTD might therefore contribute to an early diagnosis and monitoring of disease progression in clinical practice and clinical trials. Following studies in Alzheimer’s disease (AD) that identified NPTXs as candidate biomarkers,12–20 we hypothesised that NPTXs could be valuable synapse-derived biomarkers in genetic FTD.

    In the present study, we measured CSF NPTXs in a large cohort of GRN, C9orf72 and MAPT mutation carriers participating in the international Genetic FTD Initiative (GENFI). We focused our attention on NPTX2, as the available ELISA for NPTX2 allowed for more accurate quantitative measurements than the Western blots used for NPTX1 and NPTXR. We explored the relationship between NPTX2 and clinical disease severity, grey matter volume and CSF neurofilament light chain (NfL), a marker of neuroaxonal damage.21

    Methods

    Subjects

    Subjects were included from 16 centres across Europe and Canada participating in GENFI, a longitudinal cohort study of patients with FTD due to a pathogenic mutation in GRN, C9orf72 or MAPT and healthy 50% at-risk relatives (either presymptomatic mutation carriers or non-carriers). Participants underwent an annual assessment as previously described,22 including neurological and neuropsychological examination, MRI of the brain, and collection of blood and CSF. Knowledgeable informants completed questionnaires about potential changes in cognition or behaviour.

    For the present study, we included all participants with at least one CSF sample, amounting to 54 symptomatic mutation carriers (15 GRN, 31 C9orf72, 8 MAPT), 106 presymptomatic mutation carriers (47 GRN, 42 C9orf72, 17 MAPT) and 70 non-carriers. Longitudinal CSF samples were available in 13 subjects.

    Mutation carriers were considered symptomatic if they fulfilled international consensus criteria for FTD.23 24 Furthermore, as C9orf72 mutations are also associated with amyotrophic lateral sclerosis (ALS), which is increasingly considered part of the FTD disease spectrum,1 C9orf72 mutation carriers fulfilling criteria for ALS,25 but not FTD, were also considered symptomatic. We calculated disease duration based on a caregiver’s estimation of the emergence of first symptoms.

    Global cognition was scored using the Mini Mental State Examination (MMSE) and Clinical Dementia Rating scale (CDR) plus FTD modules.26 The Revised Cambridge Behavioural Inventory (CBI-R) was used to measure behavioural changes.27 The Trail Making Test part B (TMT-B) and phonemic verbal fluency were included as measures of executive functioning.28 TMT-B was truncated to 300 s for subjects that exceeded the time limit. All scores were collected within 6 months of CSF collection.

    T1-weighted MRI on three Tesla scanners was obtained within 6 months of CSF collection in 190 participants (35 symptomatic and 91 presymptomatic mutation carriers, 64 non-carriers). All MRI scans were acquired using a standardised GENFI protocol.22 T1-weighted volumetric MRI scans were parcellated into brain regions as previously described,22 using an atlas propagation and fusion strategy29 to generate volumes of the whole brain, frontal, temporal, parietal and occipital lobes, insula and cingulate gyrus. Brain volumes were expressed as a percentage of total intracranial volume (TIV), computed with SPM12 running under Matlab R2014b (Math Works, Natick, Massachusetts, USA).30

    Sample collection and laboratory methods

    CSF was collected in polypropylene tubes, centrifuged and stored at −80°C within 2 hours of withdrawal according to a standardised GENFI protocol.

    NPTX2 concentrations were measured using an in-house ELISA as described previously.12 The intra-assay and interassay coefficients of variation (CV) were <2% and<5%, respectively. The lower limit of quantification (LLOQ) was 5 pg/mL; all NPTX2 measurements were above the LLOQ. NPTX1 and NPTXR were measured by Western blot. Rabbit anti-NPTX1 was described previously3; sheep anti-NPTXR antibody is from R&D systems (Cat. Number: AF4414; RRID: AB_2153869). Immunoreactive bands were visualised by the enhanced chemiluminescent substrate (ECL, Pierce) on X-ray film and quantified using the image software TINA (www.tina-vision.net). Western blot results were expressed as a percentage of abundancy compared with non-carriers, that is, mean abundancy in non-carriers was set at 100%. Detailed methods are reported in online supplementary file 1.

    Supplemental material

    All NPTX measurements were performed in two batches in the Neuroscience Laboratory at Johns Hopkins University, Baltimore, USA. The mean CV of NPTX2 of the two batches was 5.4%. Longitudinal measurements were performed in one batch.

    CSF NfL concentrations were measured in duplicate in one batch using the Simoa NF-Light Advantage Kit from Quanterix on a Simoa HD-1 analyser instrument according to manufacturer’s instructions. The mean CV of duplicate measurements was 3.2% (range 0.1%–15.6%). NfL measurements were missing in four subjects (two symptomatic GRN and two symptomatic C9orf72 mutation carriers) due to insufficient CSF.

    Standard protocol approvals and patient consents

    Clinical researchers were blinded to the genetic status of at-risk individuals unless they had undergone predictive testing. Laboratory technicians were blinded to all clinical and genetic information.

    Statistical analysis

    Statistical analyses were performed in IBM SPSS Statistics V.24 and R. Graphs were drafted in R and GraphPad Prism 8. Statistical significance was set at 0.05 (two-sided). The primary analysis in the study was to investigate whether NPTX2, NPTX1 and NPTXR concentration differ among symptomatic mutation carriers, presymptomatic mutation carriers and non-carriers. We restricted correlative analyses of clinical and neuroimaging parameters to NPTX2 because an ELISA was available, which is more sensitive for quantitative analyses than Western blots used for NPTX1 and NPTXR.

    Demographic and clinical variables were compared between groups using Kruskal-Wallis tests for continuous variables and a χ2 test for sex. Normality of biomarker data was assessed using Kolmogorov-Smirnov tests and visual inspection of Q-Q plots. While raw biomarker values were not normally distributed, normal distributions were achieved after square-root transformation of NPTX2 and log-transformation of NfL. We performed analyses of covariance (ANCOVAs) on transformed biomarker values with age as a covariate to test for group differences. In comparisons between symptomatic mutation carriers, we also included disease duration as a covariate.

    The diagnostic performance of NPTX2 to discriminate between the three clinical groups (symptomatic mutation carriers, presymptomatic mutation carriers, non-carriers) was assessed by the area under the curve (AUC) of receiver operating characteristic analyses, with optimal cut-off levels determined by the highest Youden’s index.31

    Linear regression models were constructed to study the relationship between NPTX2 concentration (dependent variable; square-root transformed to meet model assumptions) and (1) regional grey matter volume, (2) clinical disease severity measures and (3) NfL, with age, gender and study site as covariates. For analyses of cognitive tests (MMSE, TMT-B, phonemic verbal fluency) we also included years of education as a covariate. All analyses were performed for mutation carriers combined and for symptomatic and presymptomatic mutation carriers separately. Correction for multiple comparisons was done with the Bonferroni method.

    Additional linear regression models were constructed to test whether NPTX2 could predict subsequent cognitive decline, as measured by annualised changes in clinical disease severity scores (score at the time of CSF collection subtracted from a later score and divided by time interval), correcting for age, gender and study site and in cognitive tests for years of education.

    Due to the limited sample size, statistical analyses on longitudinal NPTX2 measurements were limited to exploratory correlations between changes in NPTX2 and time interval, to test for an overall trend in NPTX2 concentration over time.

    Data availability

    The raw data of this project is part of GENFI and de-identified patient data can be accessed on reasonable request (j.c.vanswieten@erasmusmc.nl and j.rohrer@ucl.ac.uk).

    Results

    Demographic and clinical data

    Subject characteristics are shown in table 1. Symptomatic mutation carriers were significantly older than presymptomatic carriers and non-carriers, both overall and for each genetic group (GRN, C9orf72 and MAPT) separately. Three presymptomatic mutation carriers converted to the symptomatic stage (‘converters’) during follow-up (2 GRN, 1 MAPT).

    Table 1

    Subject characteristics. The clinical phenotype of symptomatic mutation carriers was behavioural variant FTD (n=37), primary progressive aphasia (n=7), FTD with amyotrophic lateral sclerosis (ALS) (n=4), ALS without FTD (n=3), memory-predominant FTD (n=1), progressive supranuclear palsy (n=1) and dementia not otherwise specified (n=1). Continuous variables are reported as medians±IQR

    NPTX2 concentration

    Overall, NPTX2 levels were lower in symptomatic mutation carriers (median 643 pg/mL, IQR 301–872) than in presymptomatic carriers (1003 pg/mL (624–1358); p<0.001) and non-carriers (990 pg/mL (597–1373); p<0.001) (figure 1A). NPTX2 levels did not differ significantly between presymptomatic mutation carriers and non-carriers (p=0.859).

    Figure 1

    NPTX2 levels (A) in presymptomatic (n=106) and symptomatic mutation carriers (n=54) and non-carriers (n=70) and (B) separated by genetic group. Whiskers indicate minimum and maximum values. Orange squares indicate subjects who converted to the symptomatic stage during follow-up (n=3); grey asterisks indicate subjects with amyotrophic lateral sclerosis (ALS) without frontotemporal dementia (FTD) (n=3); grey crosses indicate subjects with both FTD and ALS (n=4). P values are from analyses of covariance (ANCOVAs) with age as a covariate and Bonferroni correction for multiple comparisons. *p<0.05; **p<0.01; ***p<0.001. CSF, cerebrospinal fluid; NPTX, neuronal pentraxin; PRE, presymptomatic mutation carrier; SYM: symptomatic mutation carrier.

    When analysed per genetic group, symptomatic GRN and C9orf72 mutation carriers had significantly lower NPTX2 levels than their presymptomatic counterparts (GRN: 741 pg/mL vs 1072 pg/mL; p=0.003; C9orf72: 609 pg/mL vs 901 pg/mL; p=0.023) and non-carriers (GRN: p=0.007; C9orf72: p=0.004) (table 1, figure 1B). Symptomatic MAPT mutation carriers had lower NPTX2 levels than non-carriers (561 pg/mL; p=0.027) but not compared with presymptomatic MAPT mutation carriers (1079 pg/mL; p=0.213). NPTX2 levels did not differ between symptomatic carriers of different genetic groups (p=0.709). Similar results were obtained after excluding mutation carriers with ALS without FTD (n=3).

    Overall, a correlation was found between NPTX2 and age (rs=−0.141; p=0.033) (online supplementary figure 1); this correlation was also found in mutation carriers alone (rs=−0.205; p=0.009) but not in non-carriers alone (rs=0.070; p=0.566). NPTX2 levels did not differ by sex (p=0.976).

    Supplemental material

    Diagnostic accuracy of NPTX2

    The AUC for NPTX2 to distinguish symptomatic from presymptomatic mutation carriers was 0.71 (95% CI 0.63 to 0.80), with an optimal cut-off of 895 pg/mL (sensitivity 82%, specificity 56%) (online supplementary figure 2). The AUC to distinguish symptomatic mutation carriers from non-carriers was 0.71 (95% CI 0.61 to 0.80), with an optimal cut-off of 945 pg/mL (sensitivity 83%, specificity 53%). NPTX2 did not distinguish presymptomatic mutation carriers from non-carriers (AUC 0.50 (95% CI 0.41 to 0.58)).

    Supplemental material

    NPTX2 and clinical and neuroimaging data

    NPTX2 levels in mutation carriers correlated significantly with grey matter volume of the whole brain, frontal, temporal and parietal lobes and insula, and in symptomatic mutation carriers alone, with whole brain volume, frontal lobe and insular volume (figure 2A,B, table 2, online supplementary figure 3). In presymptomatic mutation carriers, NPTX2 levels were associated with frontal lobe volume but this was no longer significant after multiple testing correction (table 2). Among non-carriers (n=64), no significant associations were found with any of the regional grey matter volumes (online supplementary table 1). Results were unchanged after repeating the analyses with raw grey matter volumes (ie, not corrected for TIV).

    Supplemental material

    Figure 2

    Relationship between NPTX2 and (A) frontal lobe volume (n=126), (B) insular volume (n=126), (C) Mini Mental State Examination (MMSE) (n=145) and (D) Clinical Dementia Rating scale (CDR) plus FTD modules (n=120) among mutation carriers. b and p were obtained through multiple linear regression with square-root transformed NPTX2 as the dependent variable, adjusting for age, gender and study site; for MMSE, we also included years of education as a covariate. CSF, cerebrospinal fluid; FTD, frontotemporal dementia; NPTX, neuronal pentraxin; TIV, total intracranial volume.

    Table 2

    Relationship between NPTX2 and grey matter volume. Results were obtained through multiple linear regression with square-root transformed NPTX2 as dependent variable, adjusting for age, gender and study site. All grey matter volumes were corrected for total intracranial volume

    Among mutation carriers, NPTX2 levels correlated with MMSE, TMT-B, phonemic verbal fluency, CDR plus FTD modules and CBI-R (table 3, figure 2C,D). In symptomatic mutation carriers alone, these correlations were similarly present for MMSE, TMT-B, CDR plus FTD modules and CBI-R. In presymptomatic mutation carriers alone, an association was found for TMT-B, which was no longer statistically significant after correction for multiple testing (table 3).

    Table 3

    Relationship between NPTX2 and disease severity scores, obtained through multiple linear regression with square-root transformed NPTX2 as dependent variable, adjusting for age, gender, study site and, in analyses of MMSE, TMT-B and letter fluency, years of education

    NPTX2 and NFL concentration

    Symptomatic mutation carriers had significantly higher NfL levels than presymptomatic carriers (2575 pg/mL (1218–4592) vs 471 pg/mL (305–729); p<0.001) and non-carriers (421 pg/mL (298–555); p<0.001). These differences were also found for each genetic group separately (online supplementary figure 4). No differences were seen between presymptomatic mutation carriers and non-carriers (p=0.517). Similar results were obtained after exclusion of nine outliers (values>3*IQR from the median) and after exclusion of subjects with ALS without FTD (n=3).

    Supplemental material

    NPTX2 concentration across all mutation carriers was inversely associated with NfL concentration (b=−5.69E-4; p=0.010; n=156) (figure 3). This correlation was not observed for symptomatic (b=−3.61E-4; p=0.141; n=50) or presymptomatic mutation carriers (b=−3.64E-5; p=0.971; n=106) alone. Repeating the analyses for symptomatic mutation carriers after exclusion of patients with concomitant or isolated ALS revealed a trend towards association between NfL and NPTX2 (b=−7.55E-4; p=0.061; n=43).

    Figure 3

    Correlation between NPTX2 and NfL levels in presymptomatic (n=106) and symptomatic (n=50) mutation carriers. NfL is plotted on a log-scale for visualisation purposes. b and p were obtained through multiple linear regression with square-root transformed NPTX2 as the dependent variable, adjusting for age, gender and study site. CSF, cerebrospinal fluid; NfL, neurofilament light chain; NPTX, neuronal pentraxin.

    Longitudinal NPTX2 measurements

    Longitudinal CSF samples were available in 10 presymptomatic mutation carriers (of whom two had converted to the symptomatic stage at follow-up CSF collection), two symptomatic mutation carriers and one non-carrier. The median time between samples was 2.0 years (IQR 1.8–2.1).

    In the MAPT converter, visually, a decrease in NPTX2 was observed in two presymptomatic samples, with a further decrease in the symptomatic sample (figure 4). In the GRN converter, NPTX2 was already below the proposed cut-off level 1.2 years before symptom onset, with a further decrease in the symptomatic sample. Both symptomatic mutation carriers demonstrated NPTX2 decreases over time. Lower NPTX2 levels at follow-up were observed in all presymptomatic mutation carriers over the age of 50 years, while in younger presymptomatic carriers, NPTX2 trajectories seemed to be more varied. NPTX2 in one non-carrier subject was visually stable (figure 4).

    Figure 4

    Longitudinal NPTX2 levels plotted against age in 13 subjects with multiple CSF samples. A line is drawn between NPTX2 levels of follow-up samples. Presymptomatic samples are shown as green squares, symptomatic samples as red triangles and the non-carrier as blue circles. GRN mutation carriers are shown as open symbols, C9orf72 mutation carriers as filled symbols and the MAPT mutation carrier as half-filled symbols. Dotted horizontal line indicates median NPTX2 level in presymptomatic mutation carriers (1003 pg/mL); dashed horizontal line indicates median in symptomatic mutation carriers (644 pg/mL). For blinding purposes, a jitter of ±2 years was applied to all subjects. CSF, cerebrospinal fluid; NPTX, neuronal pentraxin.

    There was no correlation between change in NPTX2 levels and time interval between CSF collections (rs=−0.116; p=0.705) (online supplementary figure 5).

    Supplemental material

    NPTX2 and subsequent cognitive decline

    NPTX2 was significantly associated with annualised change in phonemic verbal fluency (b=0.004; p=0.001; n=118), and CDR plus FTD modules (b=−0.001; p=0.025; n=105). The former remained significant after adjusting for clinical status, frontal lobe volume and CSF NfL. A trend was found for annualised change in MMSE (b=0.001; p=0.077; n=136). NPTX2 level was not associated with annualised change in CBI-R (p=0.200; n=93) or TMT-B (p=0.693; n=107) (online supplementary table 2, figure 6).

    Supplemental material

    NPTX1 and NPTXR concentration

    NPTX1 levels were significantly lower in symptomatic mutation carriers compared with presymptomatic carriers (median 54% (36–88) vs 86% (55–118); p<0.001) and non-carriers (92% (61–123); p<0.001). Similar results were found for NPTXR (symptomatic vs presymptomatic: 51% (27–85) vs 81% (51–147); p=0.002; symptomatic vs non-carriers: 51% vs 76% (51–133); p<0.001) (figure 5). Separated by genetic group, symptomatic C9orf72 and MAPT mutation carriers had significantly lower NPTX1 and NPTXR levels than non-carriers. In GRN mutation carriers, a similar pattern was observed, although not statistically significant. NPTX1 and NPTXR levels were strongly correlated with NPTX2 (rs=0.828 and rs=0.850, respectively, both p<0.001) (online supplementary figure 7).

    Supplemental material

    Figure 5

    NPTX1 and NPTXR levels as measured by Western blot. (A) Representative (cropped) Western blots of NPTX1 and NPTXR (n=230); (B, C) NPTX1 and NPTXR levels across groups, expressed as a percentage of band intensity compared with non-carriers. Whiskers indicate minimum and maximum values. Displayed significance levels are from analysis of covariance (ANCOVA) on square-root transformed relative band intensities of NPTX1 and NPTXR with age as a covariate. *p<0.05; **p<0.01. CSF, cerebrospinal fluid; NPTX, neuronal pentraxin; PRE, presymptomatic mutation carrier; SYM, symptomatic mutation carrier.

    Discussion

    The present study of a large international cohort of genetic FTD reports low levels of NPTX2, NPTX1 and NPTXR in the symptomatic stage, with correlations between NPTX2 and both disease severity and grey matter volume. We propose NPTX2 as a novel synapse-derived biomarker of disease progression in genetic FTD.

    The decreased levels of CSF NPTXs in patients with GRN-associated, C9orf72-associated and MAPT-associated FTD probably reflect a loss or dysfunction of their synaptic sources.32 Complexes of NPTXs accumulate at excitatory synapses between glutamatergic pyramidal neurons and parvalbumin-expressing (PV) interneurons in the cerebral cortex, hippocampus and cerebellum.32 NPTXs modulate the strength of these synapses through recruitment of AMPA-type glutamate receptors (AMPARs) to the postsynaptic membrane, thereby regulating excitatory drive of pyramidal neurons onto PV-interneurons.4 12 32 PV-interneurons in turn contact surrounding pyramidal neurons and prevent neural circuits from becoming too active (diagram provided in Hanson33).34 The expression of NPTX2—but not NPTX1 or NPTXR—is induced by synapse activity,3 35 and the relative ratio of the NPTXs in the complex is dynamically dependent on the neuron’s activity. Of the three proteins, NPTX2 is most effective at AMPAR recruitment, but their combined expression is synergistic.3 NPTX2 knockout mice have reduced AMPARs, resulting in less inhibitory PV-interneuron activity; the subsequent disruption of pyramidal neuron—PV-interneuron circuits is thought to underlie cognitive impairment, and NPTX2 loss has been hypothesised to drive neurodegeneration.12 Restoring these circuits is emerging as a potential treatment strategy in neurodegenerative disease36; in this regard, measuring NPTX2 in CSF could be especially relevant to select and monitor patients with aberrant pyramidal neuron-PV interneuron circuits.12 36 The lack of correlation in the current study between NPTX2 and brain volume in healthy non-carriers reflects that NPTX2 is not merely a measure of synapse density.

    The present study reports low NPTX2 levels in all included forms of genetic FTD. The lack of significant differences between presymptomatic and symptomatic MAPT mutation carriers likely reflects insufficient statistical power given the small sample size, or could reflect differences in underlying pathology (eg, tau pathology in MAPT-associated FTD vs TDP-43 pathology in GRN-associated and C9orf72-associated FTD).1 While these findings are novel in FTD, a few studies have identified reduced NPTXs in AD, both in brain and in CSF,12–19 although mostly through mass spectrometry approaches (box 1). The observed reductions in both FTD and AD suggest that reduced NPTXs reflect general rather than gene-specific or disease-specific pathological alterations. To date, CSF NPTX2 levels in other neurodegenerative diseases have not been reported; future research should focus on the measurement of CSF NPTXs across a broader range of neurodegenerative diseases, including sporadic FTD and Parkinson’s disease.37

    Box 1

    CSF NPTXs in other neurodegenerative diseases

    • Cerebrospinal fluid (CSF) neuronal pentraxin (NPTX)2 levels are reduced in patients with Alzheimer’s disease (AD) compared with controls.12 14 17 In AD, low CSF NPTX2 levels are associated with cognitive impairment and subsequent memory decline, as well as hippocampal atrophy and subsequent medial temporal lobe atrophy.12 17

    • To date, CSF NPTX2 levels have not been reported in other neurodegenerative diseases, such as sporadic FTD and Parkinson’s disease.

    • Differentially regulated levels of CSF NPTX1 and NPTXR have been reported in patients with AD, mostly identified through mass spectrometry approaches.13 15 16 18–20 In presymptomatic stages of autosomal dominant AD, mild cognitive impairment and early-stage AD, a transient increase in NPTXs has been observed.15 16 19 20

    • In brain tissue, NPTX2 levels are decreased in patients with AD.12 Conversely, one study has reported accumulation of NPTX2 in Lewy bodies in patients with Parkinson’s disease.37

    The correlations between NPTX2 concentration and several disease severity measures suggest that NPTX2 might further decrease with disease progression. This is supported by longitudinal NPTX2 decreases over time in two symptomatic mutation carriers and could reflect a link between progressive synapse pathology and cognitive decline; more longitudinal data is needed to confirm this. The association between NPTX2 levels and subsequent decline in phonemic verbal fluency and CDR plus FTD modules indicates that NPTX2 may have prognostic significance and is in line with previous findings in AD. The correlations between NPTX2 and grey matter volume in regions typically affected in FTD, including the frontal lobe and insula,23 are comparable to the previously reported correlations with hippocampal volume in AD and provide further evidence for NPTX2 as a disease progression marker.12 17

    Longitudinally, we observed strong NPTX2 decreases in two converters; in the MAPT converter, this decrease was already observed in two presymptomatic samples; similarly, in the GRN converter, NPTX2 levels were already low in the presymptomatic sample. Although these results must be interpreted with caution due to the small sample size, they provide tentative evidence that NPTX2 might be an early disease marker. The overall lack of differences in NPTXs between presymptomatic mutation carriers and non-carriers might reflect the inclusion of mutation carriers of all ages; therefore, time to symptom onset was highly variable. Remarkably, in presymptomatic autosomal dominant AD, mild cognitive impairment and early stage AD, a transient increase in NPTXs has been observed, with a subsequent decline as the disease progresses.15 16 19 20 This discrepancy in NPTXs dynamics may result from differences in underlying pathophysiology.

    The diagnostic accuracy of NPTX2 of 71% to distinguish symptomatic from presymptomatic mutation carriers is comparable to that of neurogranin, the most evaluated synapse-derived CSF biomarker for AD.38 Its longitudinal evaluation, especially in the late-presymptomatic stage, might be more valuable than cross-sectional measurements. It is promising that Ma et al 39 observed a correlation between NPTX1 in plasma and brain tissue; further studies are warranted to investigate whether NPTX2 can also be reliably measured in the blood, which would offer opportunities for longitudinal studies with larger numbers of samples.

    We found an inverse correlation between NPTX2 and NfL in mutation carriers. NfL is a sensitive marker of neuroaxonal degeneration which is elevated in CSF and blood in the symptomatic stage of genetic FTD40 and in various other neurological disorders.21 Although a trend was found for symptomatic carriers alone after exclusion of ALS patients (who are known to have very high NfL levels),21 the lack of a stronger correlation probably reflects that NPTX2 and NfL are markers of different pathological processes which do not occur simultaneously.

    Strengths of this study include the large sample size, despite the relative rarity of the disease, and the availability of corresponding clinical and brain imaging datasets. The inclusion of subjects with specific genetic defects allowed us to define pathologically homogeneous groups. Our NPTX2 findings are supported by similar results in NPTX1 and NPTXR, which correlated strongly with NPTX2, and indicate an overall reduction in NPTXs in genetic FTD.

    The findings of this study must be viewed in light of some limitations. First, our longitudinal NPTX2 measurements were too limited in number to draw strong conclusions and require replication and more extensive statistical analyses in larger datasets. Second, using diagnostic criteria to label mutation carriers as presymptomatic or symptomatic may have failed to recognise subjects in a very early symptomatic stage. We calculated disease duration based on estimated time of symptom onset, rather than diagnosis, to ensure that any diagnostic delay did not affect correlative analyses. Third, three C9orf72 mutation carriers had ALS without FTD, which, although increasingly recognised as part of the FTD spectrum,1 represents a clinically distinct phenotype. We ensured that these subjects did not affect our main results by repeating group comparisons after exclusion of these subjects. Finally, although brief medical and neurological history and examination did not reveal any significant neurological comorbidities, asymptomatic diseases, including cerebrovascular disease, could have confounded NPTX measurements. Future research focusing on potential confounding factors will be an important next step.

    In conclusion, we provide evidence for NPTX2 as a novel CSF biomarker in genetic FTD. Its synaptic localisation and correlation with disease progression indicates that NPTX2 decreases probably reflect synaptic dysfunction or loss, providing novel opportunities for in vivo monitoring of synaptic integrity in genetic FTD. Treatment strategies aimed at improving synaptic connectivity may benefit from the use of NPTX2 as a tool to select and monitor patients with neural circuit dysfunction. More longitudinal data on NPTXs in presymptomatic and symptomatic mutation carriers might verify their value as (pre-)clinical biomarkers.

    Acknowledgments

    We thank all the participants and their family members for taking part in this study. Several authors of this publication are members of the European Reference Network for Rare Neurological Diseases—Project ID no. 739510.

    References

    Footnotes

    • Collaborators GENFI Consortium members: Martin N Rossor, Jason D Warren, Nick C Fox (Dementia Research Centre, Department of Neurodegenerative Disease, UCL Queen Square Institute of Neurology, London, UK); Rita Guerreiro, Jose Bras (Center for Neurodegenerative Science, Van Andel Research Institute, Grand Rapids, Michigan, USA); Jennifer Nicholas (Department of Medical Statistics, London School of Hygiene and Tropical Medicine, London, UK); Simon Mead (MRC Prion Unit, Department of Neurodegenerative Disease, UCL Institute of Neurology, Queen Square, London, UK); Lize Jiskoot, Lieke Meeter, Jessica Panman (Department of Neurology, Erasmus Medical Centre, Rotterdam, Netherlands); Rick van Minkelen (Department of Clinical Genetics, Erasmus Medical Centre, Rotterdam, Netherlands); Myriam Barandiaran, Begoña Indakoetxea (Cognitive Disorders Unit, Department of Neurology, Donostia University Hospital, San Sebastian, Gipuzkoa, Spain; Biodonostia Health Research Institute, San Sebastian, Gipuzkoa, Spain); Alazne Gabilondo, Mikel Tainta, Maria de Arriba, Ana Gorostidi, Miren Zulaica (Neuroscience Area, Biodonostia Health Research Institute, San Sebastian, Gipuzkoa, Spain); Jorge Villanua (OSATEK, University of Donostia, San Sebastian, Gipuzkoa, Spain); Zigor Diaz (1CITA Alzheimer, San Sebastian, Gipuzkoa, Spain); Sergi Borrego-Ecija, Jaume Olives, Albert Lladó, Mircea Balasa, Anna Antonell (Alzheimer’s disease and Other Cognitive Disorders Unit, Neurology Service, Hospital Clínic, Barcelona, Spain); Nuria Bargallo (Imaging Diagnostic Center, Hospital Clínic, Barcelona, Spain), Enrico Premi, Maura Cosseddu, Stefano Gazzina, Alessandro Padovani (Centre for Neurodegenerative Disorders, Neurology Unit, Department of Clinical and Experimental Sciences, University of Brescia, Brescia, Italy); Roberto Gasparotti (Neuroradiology Unit, University of Brescia, Brescia, Italy); Silvana Archetti (Biotechnology Laboratory, Department of Diagnostics, Spedali Civili Hospital, Brescia, Italy), Sandra Black, Sara Mitchell (Sunnybrook Health Sciences Centre, Sunnybrook Research Institute, University of Toronto, Toronto, Canada); Ekaterina Rogaeva (Tanz Centre for Research in Neurodegenerative Diseases, University of Toronto, Toronto, Canada); Morris Freedman (Baycrest Health Sciences, Rotman Research Institute, University of Toronto, Toronto, Canada), Ron Keren (The University Health Network, Toronto Rehabilitation Institute, Toronto, Canada); David Tang-Wai (The University Health Network, Krembil Research Institute, Toronto, Canada); Linn Öijerstedt (Department of Geriatric Medicine, Karolinska University Hospital-Huddinge, Stockholm, Sweden); Christin Andersson (Department of Clinical Neuroscience, Karolinska Institutet, Stockholm, Sweden); Vesna Jelic (Division of Clinical Geriatrics, Karolinska Institutet, Stockholm, Sweden); Hakan Thonberg (Center for Alzheimer Research, Divison of Neurogeriatrics, Karolinska Institutet, Stockholm, Sweden); Andrea Arighi, Chiara Fenoglio, Elio Scarpini (Fondazione IRCCS Ca’ Granda Ospedale Maggiore Policlinico, Neurodegenerative Diseases Unit, Milan, Italy; University of Milan, Centro Dino Ferrari, Milan, Italy); Giorgio Fumagalli (Fondazione IRCCS Ca’ Granda Ospedale Maggiore Policlinico, Neurodegenerative Diseases Unit, Milan, Italy; University of Milan, Centro Dino Ferrari, Milan, Italy; Department of Neurosciences, Psychology, Drug Research and Child Health (NEUROFARBA), University of Florence, Florence, Italy); Thomas Cope, Carolyn Timberlake, Timothy Rittman (Department of Clinical Neurosciences, University of Cambridge, Cambridge, UK); Christen Shoesmith (Department of Clinical Neurological Sciences, University of Western Ontario, London, Ontario Canada); Robart Bartha (Department of Medical Biophysics, The University of Western Ontario, London, Ontario, Canada; Centre for Functional and Metabolic Mapping, Robarts Research Institute, The University of Western Ontario, London, Ontario, Canada); Rosa Rademakers (Department of Neuroscience, Mayo Clinic, Jacksonville, Florida, USA); Carlo Wilke (Department of Neurodegenerative Diseases, Hertie-Institute for Clinical Brain Research and Center of Neurology, University of Tübingen, Tübingen, Germany; Center for Neurodegenerative Diseases (DZNE), Tübingen, Germany), Hans-Otto Karnarth (Division of Neuropsychology, Hertie-Institute for Clinical Brain Research and Center of Neurology, University of Tübingen, Tübingen, Germany); Benjamin Bender (Department of Diagnostic and Interventional Neuroradiology, University of Tübingen, Tübingen, Germany), Rose Bruffaerts (Laboratory for Cognitive Neurology, Department of Neurosciences, KU Leuven, Leuven, Belgium); Philip Vandamme (Neurology Service, University Hospitals Leuven, Belgium, Laboratory for Neurobiology, VIB-KU Leuven Centre for Brain Research, Leuven, Belgium); Mathieu Vandenbulcke (Geriatric Psychiatry Service, University Hospitals Leuven, Belgium; Neuropsychiatry, Department of Neurosciences, KU Leuven, Leuven, Belgium); Catarina B Ferreira (Laboratory of Neurosciences, Institute of Molecular Medicine, Faculty of Medicine, University of Lisbon, Lisbon, Portugal); Gabriel Miltenberger (45Faculty of Medicine, University of Lisbon, Lisbon, Portugal); Carolina Maruta (Laboratory of Language Research, Centro de Estudos Egas Moniz, Faculty of Medicine, University of Lisbon, Lisbon, Portugal); Ana Verdelho (Department of Neurosciences and Mental Health, Centro Hospitalar Lisboa Norte - Hospital de Santa Maria & Faculty of Medicine, University of Lisbon, Lisbon, Portugal); Sónia Afonso (Instituto Ciencias Nucleares Aplicadas a Saude, Universidade de Coimbra, Coimbra, Portugal); Ricardo Taipa (Neuropathology Unit and Department of Neurology, Centro Hospitalar do Porto - Hospital de Santo António, Oporto, Portugal); Paola Caroppo, Giuseppe Di Fede, Giorgio Giaccone, Sara Prioni, Veronica Redaelli, Giacomina Rossi, Pietro Tiraboschi (Fondazione IRCCS Istituto Neurologico Carlo Besta, Milano, Italy); Diana Duro, Maria Rosario Almeida, Miguel Castelo-Branco (Faculty of Medicine, University of Coimbra, Coimbra, Portugal), Maria João Leitão (Centre of Neurosciences and Cell biology, Universidade de Coimbra, Coimbra, Portugal), Miguel Tabuas-Pereira, Beatriz Santiago (Neurology Department, Centro Hospitalar e Universitario de Coimbra, Coimbra, Portugal); Serge Gauthier (Alzheimer Disease Research Unit, McGill Centre for Studies in Aging, Department of Neurology & Neurosurgery, McGill University, Montreal, Québec, Canada), Pedro Rosa-Neto (Translational Neuroimaging Laboratory, McGill Centre for Studies in Aging, McGill University, Montreal, Québec, Canada), Michele Veldsman (Nuffield Department of Clinical Neurosciences, Medical Sciences Division, University of Oxford, Oxford, UK); Toby Flanagan (Faculty of Biology, Medicine and Health, Division of Neuroscience and Experimental Psychology, University of Manchester, Manchester, UK); Catharina Prix, Tobias Hoegen, Elisabeth Wlasich, Sandra Loosli, Sonja Schonecker (Neurologische Klinik, Ludwig-Maximilians-Universität München, Munich, Germany); Elisa Semler, Sarah Anderl-Straub (Department of Neurology, University of Ulm, Ulm); Luisa Benussi, Giuliano Binetti, Roberta Ghidoni, Michela Pievani (Instituto di Recovero e Cura a Carattere Scientifico Istituto Centro San Giovanni di Dio Fatebenefratelli, Brescia, Italy); Gemma Lombardi, Benedetta Nacmias, Camilla Ferrari, Valentina Bessi (Department of Neuroscience, Psychology, Drug Research, and Child Health, University of Florence, Florence, Italy).

    • Funding This study was supported in the Netherlands by two Memorabel grants from Deltaplan Dementie (The Netherlands Organisation for Health Research and Development and Alzheimer Nederland; grant numbers 733050813 and 733050103), the Bluefield Project to Cure Frontotemporal Dementia, the Dioraphte foundation (grant number 1402 1300) and the European Joint Programme—Neurodegenerative Disease Research and the Netherlands Organisation for Health Research and Development (PreFrontALS: 733051042, RiMod-FTD: 733051024); in Belgium by the Mady Browaeys Fonds voor Onderzoek naar Frontotemporale Degeneratie; in the UK by the MRC UK GENFI grant (MR/M023664/1); JR is supported by an MRC Clinician Scientist Fellowship (MR/M008525/1) and has received funding from the NIHR Rare Disease Translational Research Collaboration (BRC149/NS/MH); KM is supported by an Alzheimer’s Society PhD Studentship (AS-PhD-2015-005); JBR is supported by the Wellcome Trust (103838); in Spain by the Fundació Marató de TV3 (20143810 to RSV); in Germany by the Deutsche Forschungsgemeinschaft (DFG, German Research Foundation) under Germany’s Excellence Strategy within the framework of the Munich Cluster for Systems Neurology (EXC 2145 SyNergy—ID 390857198) and by grant 779357 ‘Solve-RD’ from the Horizon 2020 Research and Innovation Programme (to MS); in Sweden by grants from the Swedish FTD Initiative funded by the Schörling Foundation, grants from JPND PreFrontALS Swedish Research Council (VR) 529-2014-7504, Swedish Research Council (VR) 2015-02926, Swedish Research Council (VR) 2018-02754, Swedish Brain Foundation, Swedish Alzheimer Foundation, Stockholm County Council ALF, Swedish Demensfonden, Stohnes foundation, Gamla Tjänarinnor, Karolinska Institutet Doctoral Funding, and StratNeuro.

    • Competing interests None declared.

    • Patient consent for publication Obtained.

    • Ethics approval Local ethics committees at each site approved the study.

    • Provenance and peer review Not commissioned; externally peer reviewed.

    • Data availability statement The raw data of this project is part of GENFI and de-identified patient data can be accessed upon reasonable request to j.c.vanswieten@erasmusmc.nl and j.rohrer@ucl.ac.uk.