ApoJ/Clusterin concentrations are determinants of cerebrospinal fluid cholesterol efflux capacity and reduced levels are associated with Alzheimer’s disease

Background

Alzheimer’s disease (AD) shares risk factors with cardiovascular disease (CVD) and dysregulated cholesterol metabolism is a mechanism common to both diseases. Cholesterol efflux capacity (CEC) is an ex vivo metric of plasma high-density lipoprotein (HDL) function and inversely predicts incident CVD independently of other risk factors. Cholesterol pools in the central nervous system (CNS) are largely separate from those in blood, and CNS cholesterol excess may promote neurodegeneration. CEC of cerebrospinal fluid (CSF) may be a useful measure of CNS cholesterol trafficking. We hypothesized that subjects with AD and mild cognitive impairment (MCI) would have reduced CSF CEC compared with Cognitively Normal (CN) and that CSF apolipoproteins apoA-I, apoJ, and apoE might have associations with CSF CEC.

Methods

We retrieved CSF and same-day ethylenediaminetetraacetic acid (EDTA) plasma from 108 subjects (40 AD; 18 MCI; and 50 CN) from the Center for Neurodegenerative Disease Research biobank at the Perelman School of Medicine, University of Pennsylvania. For CSF CEC assays, we used N9 mouse microglial cells and SH-SY5Y human neuroblastoma cells, and the corresponding plasma assay used J774 cells. Cells were labeled with [³H]-cholesterol for 24 h, had ABCA1 expression upregulated for 6 h, were exposed to 33 μl of CSF, and then were incubated for 2.5 h. CEC was quantified as percent [³H]-cholesterol counts in medium of total counts medium+cells, normalized to a pool sample. ApoA-I, ApoJ, ApoE, and cholesterol were also measured in CSF.

Results

We found that CSF CEC was significantly lower in MCI compared with controls and was poorly correlated with plasma CEC. CSF levels of ApoJ/Clusterin were also significantly lower in MCI and were significantly associated with CSF CEC. While CSF ApoA-I was also associated with CSF CEC, CSF ApoE had no association with CSF CEC. CSF CEC is significantly and positively associated with CSF Aβ. Taken together, ApoJ/Clusterin may be an important determinant of CSF CEC, which in turn could mitigate risk of MCI and AD risk by promoting cellular efflux of cholesterol or other lipids. In contrast, CSF ApoE does not appear to play a role in determining CSF CEC.

Alzheimer’s disease (AD), the most common cause of dementia, is characterized by the abnormal accumulation of amyloid-beta (Aβ) and hyperphosphorylated tau proteins, synaptic and neuronal dysfunction, neuroinflammation, and brain degeneration. Importantly, the brain is the most lipid-rich organ in the body and depends on tight regulation of lipid metabolism and transport to maintain proper neural signaling and cognitive function. This is particularly pertinent to AD, because increased cellular cholesterol content can increase Aβ production [1] and changes in cellular ceramides have demonstrable effects on Aβ production and aggregation into plaques [2,3,4]. Extensive genetics studies of AD have identified a number of genes that encode proteins associated with lipid metabolism, including apolipoproteins E and J and cellular lipid transporters ABCA1 and ABCA7 [5]. However, there is a distinct lack of information on lipid metabolism in the human brain and its relationship to AD.

Cholesterol biosynthesis occurs in all cells within the central nervous system (CNS) and some cell types can actively take up cholesterol from the extracellular space [6, 7]. Experimental evidence suggests that excessive cholesterol in neurons, astrocytes, and microglia promotes amyloid-beta (Aβ) accumulation and Aβ-driven inflammation in (AD) [8, 9]. While brain cells can convert cholesterol to 24S-hydroxycholesterol, they otherwise must efflux excess cholesterol (and 24S-hydroxycholesterol and potentially other lipid species) to acceptors in the extracellular space.

Cerebrospinal fluid (CSF) contains at least three apolipoproteins that are known to be lipid transport proteins and could serve as extracellular acceptors of cellular cholesterol and other lipids in the brain. ApoA-I, the major protein in plasma high density lipoproteins (HDL), is not synthesized in the brain, and CSF ApoA-I is derived from the plasma and is in concentrations in CSF approximately 1% of those in plasma [10] (and Supplemental Table 1). ApoE and ApoJ (also known as Clusterin) are both synthesized in the brain.

The cholesterol efflux capacity (CEC) assay was first developed by the Rader lab, using plasma [11] in order to measure the capacity of circulating plasma HDL to remove cholesterol from cholesterol-loaded macrophages. The assay is dependent on both the source cells and the acceptor media. With respect to cardiovascular disease, the source cells are cholesterol-rich macrophages that are a high source of transporters (e.g., ABCA1, ABCG1, and SRB1), which aid in the transport of the hydrophobic cholesterol molecule out of the membrane. Ex vivo analysis of serum CEC has been shown to be inversely and independently correlated with CVD [12,13,14,15]. Recently, we have shown that reverse cholesterol transport (RCT) can be measured in vivo [16]. In serum, ApoA1-containing lipoproteins are the main acceptors and are much higher in concentration than ApoE or ApoJ. Because cellular cholesterol is thought to play a role in AD, we adapted the CEC assay to use neuronal cells as source and CSF as acceptor [17]. Unlike serum, the concentration of ApoA1 is similar to that of ApoE and ApoJ in CSF such that all three may play a major role in efflux. Initial studies have shown that among the cells and conditions used, neuronal cells are a less important source cell than microglia, showing less efflux to ApoA1 and HDL [17].

We hypothesized that CSF CEC may be inversely associated with AD: high CSF CEC may facilitate cellular efflux of cholesterol (or other lipids) in a manner that is protective against AD, while low CSF CEC may have an opposite effect, potentially contributing to Aβ accumulation and the development of amyloid plaques in AD. We adapted our plasma CEC assay for CSF and showed that it is reproducible using several cell lines relevant to the CNS [17]. In that study, we found strong correlations between cholesterol efflux to CSF from the mouse microglial N9 cell line in our laboratory for assessing CEC in blood-based fluids. Here, we used this assay to measure CSF (and plasma) CEC in patients with AD, with mild cognitive impairment (MCI), and in cognitively normal (CN) controls, and also measured lipids, apolipoproteins, and known AD biomarkers in the same CSF samples.

Study design

CSF and plasma samples were obtained from the Biosample Repository of the Center for Neurodegenerative Disease Research (CNDR) at the Perelman School of Medicine (PSOM), University of Pennsylvania (Philadelphia, PA, USA). This case-control study examined participants enrolled in a prospective longitudinal study under the auspices of the National Institute on Aging (NIA)-funded Alzheimer’s Disease Clinical Center (ADCC) at PSOM. The participants were recruited at the Penn Memory Center, PSOM, and the Maria de los Santos Health Center (Philadelphia, PA, USA), following written informed consent under approval of the University of Pennsylvania Institutional Review Board.

Cases were classified as AD or MCI based on standard diagnostic criteria according to procedures established for ADCCs and the National Alzheimer’s Coordinating Center (NACC) [18,19,20,21]. From this cohort, we identified a subset of 127 CSF and plasma samples obtained on the same day from 112 unique participants and other CSF biomarker data (AD = 42, MCI = 20, and CN = 50). Four subjects were further removed due to major disruption of the blood brain barrier as adjudged by albumin and ApoB serum to CSF ratio (2 AD and 2 MCI samples, AD = 40, MCI = 18, and CN = 50). The total number of subjects used in this study is 108.

Subjects were selected from the Integrated Neurodegenerative Diseases Database (INDD) of the CNDR, using the web-based query tool INQUERY developed at CNDR. Neuropsychological testing was conducted including the Mini-Mental State Examination (MMSE) and/or tests of frontal executive function, memory, language, praxis, visuospatial construction, motor performance, mood, and function, based on the NACC Uniform Data Set (UDS) [21,22,23]. Details for CSF samples collection and for standardized Luminex assay for amyloid-beta (Aβ_1-42), total tau (TTau), and phosphorylated tau (pTau) at the threonine 181 are available in previous publications [24,25,26].

Plasma and CSF aliquots (0.5 mL) were retrieved from the UPenn biorepository, coded to allow assays to be performed without knowledge of subject characteristics, and transported or shipped on dry ice to the respective laboratories for biochemical analysis.

The criteria for selecting CSF and plasma samples from the biobank were as follows: (1) subject evaluated at Penn Memory Center; (2) diagnosis of AD, MCI, or CN; and (3) availability of CSF and plasma from the same date.

Biochemistry

Plasma cholesterol (Roche), ApoA-I (Roche), ApoB (Roche), and ApoE (Kamiya) concentrations were assayed on a Cobas C311 (Roche) and plasma and CSF human serum albumin by ELISA (E88-129; Bethyl Laboratories, Inc.). CSF cholesterol and triglyceride phospholipid were determined by fluorescence assays (A12216 (Invitrogen) and MAK122 (Sigma-Aldrich), respectively). CSF ApoA-I (DAPA10 (R&D Systems, Inc.)), ApoB (ab108807 (Abcam)), ApoE (ab108813 (Abcam)), and ApoJ (DCLU00 (R&D Systems, Inc.)) were determined by ELISA.

Cholesterol efflux capacity (CEC) assays

The CSF CEC assay using N9 microglial cells and SH-SY5Y neuroblastoma cells has been described previously [17]. Briefly, SH-SY5Y cells were maintained in DMEM/4.5 g/L D-glucose/4mM L-glutamine/110 mg/L sodium pyruvate, and N9 were maintained in RPMI 1640/2mM L-glutamine (both media from Life Technologies), supplemented with 10% FBS. In the CSF CEC assay, cells were seeded in 96 well plates and labeled with 2 μCi/mL [1,2-³H(N)] cholesterol overnight. On day 2, SH-SY5Y were treated with 2 μM T0901317, and N9 and J774 cells were treated with 0.3 mM 8-CPT-cAMP to upregulate ABCA1. Cells were exposed to 33 μl of individual CSF and cholesterol efflux was allowed to proceed for 2.5 h. Cell medium was counted upon removal of floating cells and cell lipids were extracted with isopropanol read in a scintillation counter. Cell cholesterol efflux was quantified as the percent of [³H]-cholesterol counts in the medium relative to the total counts in medium and cells. A reference CSF sample was included on each plate to decrease inter-assay variability, and CEC activity was calculated as a unitless ratio of cholesterol efflux to sample CSF normalized to the reference CSF.

A similar assay with J774 mouse macrophages was used to determine plasma CEC using 1% ApoB depleted plasma in place of CSF and is described in Khera et al. [15] and Horiuchi et al. [27].

Statistical analysis

For demographics, categorical variables are in percentages, and continuous variables as means with standard deviations or medians with range. Demographic statistics were computed using ANOVA and chi-square test for the continuous variable and categorical variables, respectively. For the post hoc multiple comparisons, we used the Tukey honestly significant difference (HSD) test. The correlation of efflux capacity between different cell lines was assessed with Spearman’s correlation coefficients. Correlations with P < 0.05 were considered significant. CEC values were log-transformed, and the N9 and SH-SY5Y CEC were not significant for the Shapiro-Wilk normality test (P = 0.58 for N9 and P = 0.66 for SH-SY5Y). For the association analysis, linear regression models were used to predict CEC, including lipoproteins and CSF biomarkers. Age, sex, race, and CSF (or plasma) storage time were incorporated as covariates in all analyses. We assessed the contribution of predictors in multinomial logistic regression, and calculated β, the logistic regression coefficient that shows the direction and size of the relationship between predictor and diagnosis. Odds ratio (OR) is the ratio of the odds that are calculated as the exponent of β with 95% confidence interval. The association between plasma CEC and biomarkers were analyzed using the same model. All analysis was carried out in the R application (v 3.6.0).

Study demographics

The characteristics of the study cohort are shown in Table 1. Among the 108 participants, 40 (37.0%) were diagnosed as AD, 18 (16.7%) as MCI, and 50 (46.3%) were CN. Mean age at lumbar puncture was 69.9 years. Fifty-three percent were female, and 9% were African American. There were no significant differences among the three groups except for the MMSE as expected. The prevalence of the ApoE ε4 allele was highest in the AD group (65%) and lowest in the CN group (24%) as expected. AD biomarker CSF Aβ_1-42 levels were significantly reduced in AD, whereas total Tau (TTau) and phosphorylated Tau (pTau) were significantly increased in AD. MCI subjects were intermediate between CN and AD in all cases (Supplemental Figure 1; Table 2).

CSF CEC, but not plasma CEC, is lower in MCI compared with controls

CSF CEC was measured using both N9 microglial cells and SH-SY5Y neuroblastoma cells. The correlation of CSF CEC between the two cell types was moderate (correlation coefficient = 0.54, P-value = 1.3e−09) (Supplemental Figure 2A). Importantly, there was no association between CSF CEC and plasma CEC (Supplemental Figure 2B-C). CSF CEC was significantly lower in MCI subjects in SH-SY5Y neuroblastoma cells (F = 3.212, P = 0.0442). We further investigated the relationship between groups using multinomial logistic regression and observed a significant difference between MCI and CN for CECs from both cell types (Fig. 1 and Table 2). CSF cholesterol was significantly associated with CSF CEC from SH-SY5Y neuroblastoma cells (B = 26.0, t = 2.289, P = 0.0243) and from N9 microglial cells (B = 48.605, t = 2.883, P = 4.9e−03) (Supplemental Figure 3). CSF phospholipids were not significantly associated with CSF CEC in either cell type. There was no difference in CSF phospholipid, CSF cholesterol, plasma CEC, or cholesterol by diagnosis (Table 2 and Supplemental Table 1).

Multinomial logistic regression analyses for CSF cholesterol efflux capacity (CEC). The predictions were evaluated for MCI and AD groups against CN. CSF cholesterol efflux capacity was measured in CN (n = 50), MCI (n = 18), and AD (n = 40). The CEC values were normalized to a standard CSF sample that was run on each plate to account for inter-assay variability. We then log normalized the data prior to regression analysis. A Multinomial logistic regression analysis showed N9 CEC has a significant prediction of MCI. B Multinomial logistic regression analysis showed SHSY-5Y CEC has a significant prediction of MCI Detailed statistics are shown in the lower part of the figure. CN, cognitively normal; MCI, mild cognitive impairment; AD, Alzheimer’s disease; CSF, cerebrospinal fluid; CEC, cholesterol efflux capacity

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CSF ApoJ/Clusterin and ApoA-I were significantly associated with CEC and were lower in MCI compared to CN. ApoA-I, ApoE, and ApoJ were measured in CSF samples and ApoA-I and ApoE were measured in plasma samples (Table 2 and Supplemental Table 1). CSF ApoA-I and CSF ApoJ were each strongly correlated with both measures of CSF CEC, but ApoE was not (Fig. 2). Although we observed that CSF ApoJ and ApoA-I are closely correlated (Fig. 3), CSF ApoA-I and ApoJ were not significantly correlated with each other when we adjust for age, sex, and race (Supplemental Figure 4) CSF ApoA-I and ApoJ/Clusterin were both significantly lower in MCI than CN but not in AD, whereas CSF ApoE was significantly lower in AD subjects than in CN controls but not in MCI (Fig. 4 and Table 2). CSF ApoE levels were significantly lower in APOE ε4 allele carriers, and the AD group had significantly more ε4 allele carriers (Supplemental Figure 5). CSF ApoA-I had no correlation with plasma ApoA-I, and plasma ApoA-I was not different among CN, MCI, and AD subjects (Supplemental Table 1). Similarly, CSF and plasma ApoE levels were not correlated, and in contrast to CSF ApoE, plasma ApoE levels did not differ by diagnosis (Supplemental Table 1).

Multivariate linear regression of CSF CEC and apolipoproteins CSF. CSF cholesterol efflux capacity was measured in CN (n = 50), MCI (n = 18), and AD (n = 40). Association between ApoA1, ApoE, and ApoJ with both CEC in human microglial and neuronal cells (N9 and SH-SY5Y, respectively). Association between ApoA1 significantly associated with N9 microglial and SH-SY5Yneuronal cell CEC (**P < 8.96e−11 and ***P < 3.244e−06, respectively), ApoJ is significantly associated with N9 microglial and SH-SY5Yneuronal cell CEC (**P < 2.22e−05 and *P < 1.22e−02, respectively). ApoE is not associated with either CEC measurement

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Heat map and hierarchical clustering of CSF CEC with apolipoproteins and biomarkers of AD. CSF CEC is closely associated with ApoA-I and Clusterin. Aβ_1-42 is associated with ApoE, and pTau, TTau, and pTau/Aβ_1-42 ratio

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Multinomial logistic regression analyses for CSF apolipoproteins and AD diagnosis. Apolipoproteins were measured in CN (n = 50), MCI (n = 18), and AD (n = 40). A Apo A1 displayed significant prediction of MCI diagnosis. B ApoE is significantly lower in AD (**P < 0.01). C ApoJ (Clusterin) is significantly lower in MCI (**P < 0.01) AD denotes Alzheimer’s disease, CSF cerebrospinal fluid, ApoA1 apolipoprotein A-I, ApoE apolipoprotein E, ApoJ/Clusterin, PL phosphorylated lipid, and Aβ_1-42 42 amino acid form of beta amyloid

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CSF AD biomarkers

We measured Aβ_1-42, total Tau (TTau), and phosphorylated-Tau (pTau) in the same CSF samples. Aβ_1-42 had a modestly significant association with CSF CEC in SH-SY5Y cells but not in N9 cells (Supplemental Figure 6). None of the other AD CSF biomarkers had an association with CSF CEC (Supplemental Figure 6). There was a strong and highly significant positive association between CSF Aβ_1-42 and CSF ApoE and a strong negative association between pTau/Aβ_1-42 ratio and CSF ApoE (Table 3; Supplemental Figure 6). Neither ApoA-I nor ApoJ had significant correlations with the AD biomarkers. We performed a pair-wise correlation analysis for all measurements made in the CSF (Fig. 3). ApoA-I, ApoJ, and the two CEC measurements clearly clustered together and were negatively associated with Tau and pTau. Aβ_1-42 was positively correlated with ApoE and negatively with Tau and pTau.

Dysregulation of cholesterol metabolism in the brain has been associated with neurodegenerative disorders including AD. However, the exact mechanisms linking cholesterol metabolism and AD pathogenesis are not well understood and current understanding is sometimes conflicting. Prior work employing genome-wide association studies (GWAS) identified several genes involved in cholesterol movement as risk factors, including ApoE, ApoJ, ABCA1, and ABCA7. In this study, we used CSF from subjects with AD and MCI as well as cognitively normal controls to measure CSF cholesterol efflux capacity from two different cell types as well as lipids, apolipoproteins, and AD biomarkers. We studied whether these data were associated with AD/MCI diagnosis as well as with each other. We observed that both AD and MCI patients had significantly lower CSF Aβ_1-42, increased CSF total and phosphorylated tau, lower CSF ApoE, and higher frequency of the APOE ε4 genotype, all of which have been reported and were positive controls for the experiment.

Our major findings are that reduced CSF CEC is a feature of MCI and early-stage AD, and the CSF CEC is strongly correlated with CSF ApoA-I and ApoJ, but not with CSF ApoE. CSF ApoA-I and ApoJ were significantly lower in MCI subjects than in controls, while ApoE is significantly lower in AD subjects compared to controls. Importantly, neither CSF CEC nor CSF ApoA-I were correlated with plasma CEC and ApoA-I; thus, plasma levels of ApoA-I and CEC cannot be used as surrogates for CSF.

Importantly, we measured CSF CEC with a novel approach using two different biologically relevant cell lines—the human microglial N9 cell line and the human neuronal SH-SY5Y cell line—by labeling the cells with radiolabeled cholesterol and then testing the capacity of the CSF samples to promote efflux. While previous studies have suggested decreased levels of CSF CEC in MCI and AD subjects [28, 29], they used different assays with murine J774 macrophages, CHO cells, and BHK cells that are less biologically relevant. Yassine et al. specifically focused on ABCG1-transporter-related efflux, using CHO or BHK cells transfected with ABCA1 transporter or J774 macrophages which have high ABCA1 relative to N9 and SH-SY5Y cells [28].

In our studies, the two independent CEC assays correlated well with each other. The most significant association with CSF CEC was with CSF ApoA-I and ApoJ, both of which are highly plausible acceptors of cellular cholesterol efflux. Indeed, ApoA-I and ApoJ are known to occur on the same lipoprotein particles in plasma [30]. One might postulate that an ApoA1/ApoJ complex is responsible for cholesterol efflux. However, in the CSF where ApoJ and ApoA1 are at similar concentrations, much of ApoJ is not associated with Apo A1 [10, 30, 31]. It is possible that ApoA-I and ApoJ may be important for promoting removal of cholesterol (and possibly other toxic lipids) from brain cells in a way that is protective against AD, although in CSF, ApoJ is also present on other lipoproteins as well as in soluble form [10].

The association between CSF ApoA-I and AD is not consistent in the literature [32,33,34,35,36]. Our results aligned with Saito et al. [36] that CSF ApoA-I is not associated with AD. Merched et al. reported a decrease in serum ApoA-I in AD subjects (with 59 CN and 98 AD) [37], and Smach et al. showed that serum ApoA-I is highly correlated with severity of AD [38], but we did not observe an association of plasma ApoA-I with AD or MCI. A notable finding of our study is that levels of CSF ApoJ (Clusterin) were significantly lower in MCI and trending in AD; they were also significantly positively associated with CSF CEC. Variants at the ApoJ/Clusterin locus have been significantly associated with AD by GWAS [39], suggesting that ApoJ/Clusterin has a causal role in influencing AD risk. Clusterin binds to Aβ_1-42, and the complex is transported across the blood brain barrier (BBB) into the circulation through low-density lipoprotein receptor related protein 2 (LRP2) to promote clearance of Aβ peptides from the brain [40, 41]. More recently it has been shown that ApoJ/Clusterin can reverse neuroinflammation and memory loss in mice [42].

We previously reported that ApoJ/Clusterin predicts CSF CEC from microglia and astrocytes [17]. In our current analysis, we confirm that CSF ApoJ/Clusterin was significantly associated with CSF CEC but not with Aβ_1-42, similar to a previous study [43]. Our results suggest that CSF ApoJ/Clusterin may protect against AD in part by promotion of lipid efflux from brain cells. Further studies are needed to investigate this hypothesis.

ApoE has a well-established role in AD [39], though the mechanisms remain unclear. CSF ApoE levels were lower in AD subjects, likely a reflection of the effect of the APOE ε4 allele in reducing CSF ApoE levels. Despite the fact that ApoE can act as an acceptor of cellular lipid efflux, we found no correlation of CSF CEC with CSF ApoE; we did, however, note a significant positive correlation between CSF ApoE and CSF Aβ_1-42. In a previous study, the concentration of CSF ApoE was not associated with Aβ_1-42 or clinical dementia diagnosis [44]. Another smaller study found CSF ApoE to be significantly associated with TTau, tau phosphorylated at Thr181 (pTau), and Aβ_1-42 [45]. Our study suggests that ApoE does not influence AD risk through its effect on CSF CEC.

In summary, we found that CSF CEC measured using two different brain-relevant cell types was significantly lower in MCI patients than in cognitively normal controls. Both CSF ApoA-I and ApoJ (but not ApoE) were significantly associated with CEC. In addition, CSF ApoJ was significantly associated with MCI (lower) and trending in AD. Our major conclusions are that impaired CSF CEC, determined in part by CSF ApoJ concentrations, is a risk factor for MCI and AD. We speculate that factors regulating the synthesis and secretion of ApoJ in the brain influence the ability to promote efflux of cholesterol (and possibly other toxic lipids) from brain cells and therefore influence the risk of AD.

All data are available through the SAGE Synapse database as part of the M2OVE-AD program.

P30-AG010124-27, “Alzheimer's Disease Core Center”; RF1-AG051550, “Metabolic Signatures Underlying Vascular Risk Factors for Alzheimer-type Dementias” (M2OVE AD).

Funding for ADMC (Alzheimer’s Disease Metabolomics Consortium, led by R.F.K.-D. at Duke University) was provided by the National Institute on Aging grant 3U01AG061359, 1RF1AG059093, 1FR1AG057452, and R01AG046171, a component of the Accelerating Medicines Partnership for AD (AMP-AD) Target Discovery and Preclinical Validation Project (https://www.nia.nih.gov/research/dn/amp-ad-target-discovery-and-preclinical-validation-project) and the National Institute on Aging grant RF1 AG0151550, a component of the M²OVE-AD Consortium (Molecular Mechanisms of the Vascular Etiology of AD – Consortium https://www.nia.nih.gov/news/decoding-molecular-ties-between-vascular-disease-and-alzheimers).

NNL was supported by a Scientist Development Grant (grant number 14SDG20230024) from the American Heart Association.

1. Yi-An Ko and Jeffrey T. Billheimer contributed equally to this manuscript.

2. John Q. Trojanowski is deceased.

Authors and Affiliations

1. Division of Translational Medicine and Human Research, Perelman School of Medicine, University of Pennsylvania, 11-125 Smilow Center for Translational Research, 3400 Civic Center Blvd, Philadelphia, PA, 19104-5158, USA

   Yi-An Ko, Jeffrey T. Billheimer, John Q. Trojanowski & Daniel J. Rader

2. Alzheimer’s Center at Temple, Department of Neural Sciences, Lewis Katz School of Medicine at Temple University, Philadelphia, PA, 19140, USA

   Nicholas N. Lyssenko

3. Department of Psychiatry and Behavioral Sciences, Duke University, Durham, NC, 27708, USA

   Alexandra Kueider-Paisley & Rima F. Kaddurah-Daouk

4. Department of Neurology, University of Pennsylvania, Philadelphia, PA, 19104, USA

   David A. Wolk

5. Department of Neurology, Massachusetts General Hospital, Harvard Medical School, Boston, MA, 02115, USA

   Steven E. Arnold

6. Penn Neurodegeneration Genomics Center, Department of Pathology and Laboratory Medicine, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA, 19104, USA

   Yuk Yee Leung

7. Department of Pathology and Laboratory Medicine, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA, 19104, USA

   Leslie M. Shaw

8. Duke Institute for Brain Sciences, Duke University, Durham, NC, 27708, USA

   Rima F. Kaddurah-Daouk

9. Department of Medicine, Duke University, Durham, NC, 27708, USA

   Rima F. Kaddurah-Daouk

10. Department of Geriatrics and Gerontology, New Jersey Institute for Successful Aging, Rowan University School of Osteopathic Medicine, 42 E. Laurel Rd., Suite 1800, Stratford, NJ, 08084, USA

    Mitchel A. Kling

11. Department of Psychiatry, Perelman School of Medicine, University of Pennsylvania, Philadelphia, Pennsylvania, USA

    Mitchel A. Kling

Contributions

J.T.B., N.N.L., D.A.W., S.E.A., J.Q.T., M.A.K., and D.J.R. participated in the sample collection and sample quality control. Y.-A.K., J.T.B., N.N.L., A.K.-P., D.A.W., S.E.A., Y.-Y.L., L.M.S., R.F.K.-D., M.A.K., D.J.R., Y.-A.K., J.T.B., M.A.K., and D.J.R. developed the concepts, methodology, and analyses. J.T.B., M.A.K., D.J.R., and R.F.K.-D. supervised the study. Y.-A.K., J.T.B., M.A.K., and D.J.R. wrote the manuscript with input from N.N.L. A.K.-P., D.A.W., S.E.A., Y.-Y.L., L.M.S., J.Q.T., and R.F.K.-D. All authors discussed and approved the results and implications and commented on the manuscript at all stages.

Corresponding authors

Correspondence to Mitchel A. Kling or Daniel J. Rader.

Ethics approval and consent to participate

All subjects gave written informed consent under research protocols approved by the University of Pennsylvania Institutional Review Board and agreed to the use of their data for research purposes. Samples were retrieved from the biobank of the Center for Neurodegenerative Disease Research (CNDR) at the Perelman School of Medicine, University of Pennsylvania, with approval from its governing body. Clinical, demographic, and genotype data were obtained from the Integrated Neurodegenerative Diseases Database maintained by CNDR using structured queries.

Consent for publication

Not applicable.

Competing interests

R.F.K.-D. is inventor on key patents in the field of metabolomics including applications for Alzheimer’s disease. She holds equity in Metabolon Inc. R.F.K-D. formed Chymia LLC and PsyProtix, a Duke University biotechnology spinout aiming to transform the treatment of mental health disorders.

L.M.S. received research support from NIH/NIA, Alzheimer’s Disease Neuroimaging Initiative (ADNI) (AG024904), and University of Pennsylvania ADCC Biomarker Core (AG010124), Michael J. Fox Foundation for Parkinson’s Research, Roche, and Lilly; provides QC oversight for Roche Elecsys CSF AD biomarker immunoassays for ADNI; and is a consultant for Roche, Lilly, and Novartis.

D.A.W. reports grants from Merck, Biogen, and Eli Lilly/Avid and additional fees from GE Healthcare, Functional Neuromodulation, Eli Lilly, Qynapse, and Neuronix, all outside of this work.

S.E.A. has received fees for serving on advisory boards for Allyx Therapeutics, Inc., Bob’s Last Marathon, Cassava, Cortexyme, Inc., Sage Therapeutics, Inc., vTv Therapeutics, Inc., and for consulting to AbbVie, Inc., Boyle Shaughnessy Law, Cognito Therapeutics, Inc., EIP Pharma, Inc., M3 Biotech, Inc., Orthogonal Neuroscience, Inc., and Risen Pharmaceutical Technology Co, Ltd. He has received sponsored research grant support from the following commercial entities: AbbVie, Inc., Amylyx, Inc., Athira Pharma, Inc., Chromadex, Inc., EIP Pharma, Inc., Janssen Pharmaceuticals, Inc., Novartis AG, Seer Biosciences, Inc., and vTv Therapeutics, Inc. He has received sponsored research grant support from the following non-commercial entities: Alzheimer’s Association, Alzheimer’s Drug Discovery Foundation, Challenger Foundation, John Sperling Foundation, and the National Institutes of Health.

D.J.R. serves on the scientific advisory boards of Alnylam, Novartis, Pfizer, and Verve Therapeutics and is a Founder of Vascular Strategies and Staten Biotechnologies. He has received sponsored research support from Biogen Inc.

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