Abstract
Recent evidence suggests that tau aggregation may spread via extracellular release and subsequent uptake by synaptically connected neurons, but little is known about the processes by which tau is released or the molecular forms of extracellular tau. To gain insight into the nature of extracellular tau, we used highly sensitive ELISAs, which, when used in tandem, are capable of differentiating between full-length (FL) tau, mid-region-bearing fragments, and C-terminal (CT) fragments. We applied these assays to the systematic study of the conditioned media of N2a cells, induced pluripotent stem cell-derived human cortical neurons, and primary rat cortical neurons, each of which was carefully assessed for viability. In all three neuronal models, the bulk of extracellular tau was free-floating and unaggregated and <0.2% was encapsulated in exosomes. Although most intracellular tau was FL, the majority of extracellular tau was CT truncated and appeared to be released both actively by living neurons and passively by dead cells. In contrast, only a small amount of extracellular tau was aggregation-competent tau (i.e., contained the microtubule-binding regions) and this material appears to be released solely due to a low level of cell death that occurs in all cell culture systems. Importantly, amyloid β-protein (Aβ)-induced neuronal compromise significantly increased the quantity of all forms of extracellular tau, but the presence of Aβ before detectable cell compromise did not increase extracellular tau. Collectively, these results suggest that factors that induce neuronal death are likely to be necessary to initiate the extracellular spread of tau aggregation.
SIGNIFICANCE STATEMENT Recent studies suggest that the transfer of tau between neurons underlies the characteristic spatiotemporal progression of neurofibrillary pathology. We searched for tau in the conditioned medium of N2a cells, induced pluripotent stem cell-derived human cortical neurons, and primary rat cortical neurons and analyzed the material present using four different tau ELISAs. We demonstrate that the majority of tau released from healthy neurons is C-terminally truncated and lacks the microtubule-binding region (MTBR) thought necessary for self-aggregation. A small amount of MTBR-containing tau is present outside of cells, but this appears to be solely due to cell death. Therefore, if propagation of tau aggregation is mediated by extracellular tau, our findings suggest that neuronal compromise is required to facilitate this process.
Introduction
The temporal and spatial accumulation of neurofibrillary tangles correlates well with the presentation and progression of symptoms typical of Alzheimer's disease (AD; Spillantini and Goedert, 2013). Animal (Clavaguera et al., 2009; Frost et al., 2009; de Calignon et al., 2012; Kfoury et al., 2012) and cell culture studies suggest that tau aggregation can propagate from neuron to neuron (Frost et al., 2009, Holmes et al., 2014) and there is growing interest in how tau is released and taken up by cells.
Tau does not contain a signal for secretion, yet it is readily detected in the CSF of normal humans (Blennow et al., 1995) and rodents (Barten et al., 2011; Mably et al., 2015) and burgeoning evidence suggests that tau can be detected in the medium of apparently healthy cells (Kim et al., 2010a; Chai et al., 2012; Karch et al., 2012; Plouffe et al., 2012; Simón et al., 2012; Pooler et al., 2013). In addition, the levels of CSF tau are elevated in AD and after acute neuronal injury resulting from stroke, traumatic brain injury, and Creutzfeldt–Jakob disease (Hesse et al., 2000). Therefore, it appears that tau may be released both as a result of neuronal compromise and by specific but poorly described secretion mechanisms (Barten et al., 2011; Chai et al., 2012). Although significant effort has been expended to understand the mechanisms of release, uptake, and propagation, little is known about the molecular forms of tau that are released from neurons.
Until very recently, most studies that measured tau in CSF used immunoassays based on mid-region-directed antibodies incapable of discriminating between full-length (FL) tau and fragments that retain mid-region epitopes. In the few studies to use reliable methodologies, only N-terminal and mid-region fragments of tau were detected in CSF (Johnson et al., 1997; Meredith et al., 2013; Wagshal et al., 2015). The microtubule binding repeat domains (MTBRs) of tau are important for formation of paired helical filaments and contain motifs known to drive aggregation (Barghorn et al., 2004; Goux et al., 2004; Mandelkow and Mandelkow, 2012) and most “seeding” studies have used MTBR-containing fragments (MTBR-CFs) of tau (Frost et al., 2009; Guo and Lee, 2011; Holmes et al., 2014). Given the established importance of MTBRs for aggregation but their apparent absence in biological fluids, we set out to determine whether FL tau or MTBR-CFs are present in the medium of healthy neurons and whether disease-relevant stresses affect their levels.
Using three different neuronal culture models, we found that tau is released by mechanisms both dependent on and independent of cell death and that the bulk of the released protein is free-floating (soluble) and unaggregated. ELISAs capable of detecting different regions of tau [FL, C-terminal (CT) fragments, and mid-region-containing fragments] revealed that the majority of extracellular tau is CT truncated. Importantly, the extracellular levels of both aggregation-prone MTBR-containing fragments and FL tau are increased when neuronal injury is induced by amyloid β-protein (Aβ). These results suggest that cellular compromise is the major mechanism by which MTBR-CFs and FL tau are released from neurons.
Materials and Methods
Reagents.
All chemicals and reagents were purchased from Sigma-Aldrich unless otherwise noted. The antibodies used and their source are described in Table 1. Synthetic Aβ(1–42) (human sequence) was synthesized and purified using reversed-phase HPLC by Dr. James I. Elliott at Yale University. Peptide mass and purity (>99%) were confirmed by reversed-phase HPLC and electrospray/ion trap mass spectrometry. All tissue culture reagents were obtained from Invitrogen and, where appropriate, the medium used to condition cells was centrifuged (100,000 × g for 18 h and 4°C) to remove exosomes (Théry et al., 2001).
N2a tissue culture.
N2a cells were grown on either 6-well plates or 75 cm2 flasks at 37°C in a 5% CO2 atmosphere in DMEM supplemented with 10% fetal bovine serum, 5% l-glutamine, and 5% penicillin/streptomycin. When cells reached 90% confluency, the medium was removed and washed once with growth medium. Fresh medium was added and incubated on cells for 6, 24, or 48 h. Cells were lysed in one of two ways: (1) by the addition of Triton X-100 to medium to a final concentration of 1% (v/v) and incubated at 37°C for 30 min or (2) by the removal of all the medium and addition of radioimmunoprecipitation assay (RIPA) buffer containing 1 mg/ml pepstatin A, 1 mm pefabloc, 1 mg/ml aprotinin, 5 mm EGTA, and 5 mm EDTA. Conditioned medium (CM) and cell lysates were centrifuged for 10 min at 200 × g or 16,000 × g, respectively, and 4°C, and used immediately (Fig. 1A).
Induced human cortical neuronal cultures.
Induced pluripotent stem cells (iPSCs) were obtained from the UCONN Stem Cell Core and used to produce neurons as described previously (Muratore et al., 2014a). Line YZ1 was produced by injecting iPSCs with retroviral vectors for the reprogramming factors OCT4, SOX2, NANOG, and LIN28 or c-Myc and KLF4 (Zeng, 2010). To ensure a stable chromosome number over time, the NanoString nCounter Human Karyotype Panel CNV CodeSet was used to assay genomic iPSC DNA every ∼10 passages. iPSCs were cultured in iPSC medium and fresh FGF2 (Millipore) was added daily at 10 ng/ml. Cultures were maintained at 37°C and 5% CO2 and were split as necessary based on colony growth (∼6 d). iPSCs were manually groomed by removing any colonies with irregular borders, spontaneous differentiation, or transparent centers, before splitting. iPSCs were maintained on a mouse embryonic fibroblast feeder layer at 1.7–2.0 × 105 cells/well of a 6-well plate (Globalstem). For the induction of forebrain cortical neurons, iPSCs were differentiated using an embryoid-body-based protocol (Muratore et al., 2014a). After 24 d of differentiation, iPSC-derived neuronal aggregates were dissociated to single cells with accutase (Invitrogen) and plated on Matrigel for final differentiation into induced human cortical neurons (iHCNs; 40,000–50,000 cells/well of 96-well plate) using N2/B27 medium supplemented with 10 μm ROCK inhibitor (StemRD; Muratore et al., 2014a). A full medium change was performed every 3 d and, on day 45, postdifferentiation medium was removed and fresh medium was added and incubated on cells for 48 h. For some assays, the medium was pooled across multiple wells of a 96-well plate. Neuronal cultures were characterized by qPCR, Nanostring, and immunostaining followed by confocal microscopy (Muratore et al., 2014a). Maximal expression of tau mRNA is attained between postdifferentiation days 40 and 60 with an approximate ratio of 3:1 3R:4R transcript.
Rat primary hippocampal neuronal cultures.
Neurons were prepared and grown essentially as described previously (Minogue et al., 2009, Walsh et al., 2009). Hippocampi were explanted from E18 Sprague Dawley rat pups in Hank's balanced salt solution and dissociated using 0.25% trypsin (Invitrogen) for 16 min at 37°C. Neurons were plated at a density of 3 × 104 cells on the inner 24 wells of poly-d-lysine-coated 48-well plates and cultivated in neurobasal medium supplemented with 0.5 mm Glutamax-I (Invitrogen) and B27 with antioxidants (Invitrogen). Seven days after plating, 10 μm 5-fluoro-2′-deoxyuridine was added to reduce glial proliferation. Cultures were kept in a humidified incubator at 37°C and 5% CO2 and, once per week, half of the medium was replaced with fresh neurobasal medium containing 0.5 mm Glutamax-I and B27 with antioxidants (Kaech and Banker, 2006). After 21 d in vitro (DIV), 50% of the medium was replaced with fresh medium and, after 24 h, the medium and cells were harvested. Medium was processed according to Figure 1A and cells were lysed using either 1% Triton X-100 or RIPA as described above for N2a cells.
Lactate dehydrogenase colorimetric assay.
Lactate dehydrogenase (LDH) activity was measured using the Promega cytotoxicity kit in accordance with the manufacturer's instructions. Samples were analyzed in duplicate, standards (bovine pancreatic LDH; 0.004–8 U/ml), and blanks in triplicate. Samples (50 μl) were diluted 1:2 with assay buffer and incubated for 30 min at room temperature. Stop solution (50 μl) was added and the absorbance at 490 nm was measured using a Spectramax plate reader (Molecular Devices). Standard curves were fitted to a five-parameter logistic function with 1/Y2 weighting, using MasterPlex ReaderFit (MiraiBio). The lower limit of quantification (LLOQ) is defined as the lowest standard point with a signal higher than the average signal for the blank plus 9 SDs and a percent recovery ≥100 ± 20% and was 0.03 U/ml. Where appropriate, samples were diluted so that the LDH activity exceeded the LLOQ but was lower than the 8 U/ml standard.
In certain experiments, the relative viability of primary rat neuron cultures was assessed by staining with propidium iodide and Hoechst 33258 (Aras et al., 2001). Propidium iodide (Life Technologies; 1 mm in sterile MQ water) was added to yield a concentration of 10 μm and incubated on cells for 1 h at 37°C. At the end of this time, Hoechst (Life Technologies; 1 mm in DMSO) was added to a concentration of 10 μm and cells were incubated for a further 30 min at 37°C. Live cultures were then immediately viewed using a Zeiss LSM710 confocal microscope and 10× objective lens and images were recorded using ZEN Black software. For each experiment, a total of three wells were examined, with one random field per well. The number of Hoechst- and propidium-iodide-positive cells were counted using ImageJ software. Hoechst is a cell-permeable dye and can stain the nuclei of both live and dead cells, whereas propidium iodide is cell impermeant and stains only the nuclei of compromised cells. The percentage cell death was determined using the following formula: % cell death = (no. of propidium-iodide-stained cells/no. total of Hoechst-stained cells) × 100.
β3-tubulin ELISA.
Black half-area high binding 96-well plates (Greiner Bio-One) were coated with the anti-β3-tubulin (β3T) antibody ab68193 (Abcam; diluted 1:250 in TBS, pH 7.4, at 25 μl/well) for 1 h at 37°C. All remaining steps were conducted at ambient temperature unless otherwise indicated. Wells were washed 5 times with TBS containing 0.05% Tween 20 (TBS-T) and then blocked with 3% (w/v) BSA in TBS for 2 h with shaking. Thereafter, wells were washed five times with TBS-T. Samples were analyzed in duplicate (25 μl/well), whereas blanks and standards (7.8–8000 ng/ml) were analyzed in triplicate. The β3T used as a calibrant was from Cytoskeleton. All samples were incubated overnight at 4°C. The next day, plates were shaken for 2 h to allow the assay to return to room temperature. Subsequently, 25 μl of TUJ1-alkaline phosphatase in TBS-T containing 1% (w/v) BSA was added to each well and incubated for 1 h with shaking. TUJ1 was conjugated to alkaline phosphatase using a Lightning-Link alkaline phosphatase conjugation kit (Innova Biosciences). Wells were washed five times and 50 μl of chemiluminescent substrate (Tropix CDP-Star Sapphire II; Applied Biosystems) was added and incubated with shaking for 30 min. Chemiluminescence was measured using a Synery H1 plate reader (Biotek). Standard curves were fitted to a five-parameter logistic function with 1/Y2 weighting, using MasterPlex ReaderFit (MiraiBio). The LLOQ of the assay was 125 ng/ml (Fig. 2A). Most CM samples contained little or no β3T and were analyzed without dilution but, where appropriate, CM and lysates were diluted so that the concentration of β3T exceeded the LLOQ but was lower than the 8000 ng/ml standard.
Recombinant production of tau proteins.
Escherichia coli strain BL21 (DE3) was transformed with expression vectors pNG2/hTau40, pNG2/K19, and pET17b-mTau2310 encoding human tau 441, K19, and rodent tau 430, respectively. The K19 construct contains a total of 98 residues and encompass repeat domains R1, R3, and R4. Proteins were expressed and purified as described previously (Barghorn et al., 2005, O'Dowd et al., 2013). Purity of the proteins was assessed by SDS-PAGE/sliver staining and reversed phase-HPLC. Concentrations were determined using absorbance at 280 nm and Beer–Lambert's law (ε280 = 7575, 1490, and 6085 M−1 cm−1 for human tau 441, K19, and rodent tau 430, respectively).
Mid-region tau ELISA.
This assay was performed essentially as described previously (Barten et al., 2011) and the procedure used for mid-region tau ELISA was similar to that used for the β3T ELISA. The anti-tau monoclonal antibody BT2 (Thermo Scientific) at 2.5 μg/ml in TBS was used for capture and Tau5 conjugated to alkaline phosphatase was used for detection (Fig. 3). Samples were analyzed in duplicate, whereas blanks and standards (mouse tau 430 or human tau 441; 7.8–8000 pg/ml) were analyzed in triplicate. Standard curves were fitted to a five-parameter logistic function with 1/Y2 weighting using MasterPlex ReaderFit (MiraiBio). The LLOQ of the assay was 30 pg/ml (Fig. 2B) and, where appropriate, samples were diluted so that the concentration of tau exceeded the LLOQ but was lower than the 8000 pg/ml standard.
CT tau ELISA 1.
CT tau ELISA 1 was performed in the same manner as the mid-region tau assay except that the polyclonal antibody K9JA was used both for capture and detection (Fig. 3). The LLOQ of the assay was 30 pg/ml (Fig. 2C).
CT tau ELISA 2.
This assay was performed in the same manner as the other tau assays except that the polyclonal antibody K9JA was used for capture and the monoclonal antibody Tau46 was used for detection (Fig. 3). The LLOQ of the assay was 125 pg/ml (Fig. 2D).
FL tau ELISA.
This assay was performed in the same manner as the other tau assays. Either monoclonal antibody H9.4 (for rodent tau) or Tau12 (for human tau) was used for capture and the monoclonal antibody Tau46 was used for detection (Fig. 3). The LLOQ of the assay was 125 pg/ml (Fig. 2E).
All tau assays produced concordant results when samples were serially diluted and displayed excellent recoveries (≥80% and ≤110%) when spiked with recombinant tau.
Immunoprecipitation ELISA.
To gain further insight about the aggregation state of extracellular tau, we used the MC1 antibody (which binds misfolded tau) to deplete samples of aberrantly folded tau and measured the concentration of BT2-Tau5 ELISA-detectable tau in samples with and without immunoprecipitation (IP). To control for the efficiency of the IP, we immunoprecipitated replicates of the same samples with BT2. For each IP, 5 μg/ml mAb and 7.5 μl of protein G beads (Thermo Scientific) were used. Two rounds of IP were sufficient to achieve maximal depletion with BT2 (data not shown), so each round of IP was performed twice. To remove antibody that could interfere with the ELISA, samples were subsequently incubated with protein G beads alone. Samples before and after each round of IP were analyzed by BT2-Tau5 ELISA and concentrations were normalized to control samples treated with PBS and beads instead of antibody and beads. Conditioned media and lysate were analyzed in duplicate. Lysates were diluted in 1% BSA/PBS to produce tau concentrations comparable to those of the corresponding CM samples.
Isolation of crude exosomes.
N2a cells were cultured in 75 cm2 flasks until 90% confluent. Cells were washed with 5 ml of growth medium and then incubated in 20 ml of exosome-depleted medium. Primary neurons were conditioned (in 48-well plates) for 24 h in 0.3 ml of medium per well and iHCNs were conditioned (in 96-well plates) for 48 h in 0.1 ml of medium per well. CM was centrifuged at 200 × g and 4°C for 10 min (Fig. 1A). The upper 95% of the supernatant (Sup 1) was removed and centrifuged at 2000 × g and 4°C for 10 min. Again, the upper 95% of the supernatant (Sup 2) was removed. This time Sup 2 was centrifuged at 10,000 × g and 4°C for 30 min. Supernatant 3 was centrifuged at 100,000 × g and 4°C for 2 h. The entire supernatant was poured off and the pellet (Pellet 1) resuspended in 30 ml of PBS and exosomes repelleted by centrifugation for 2 h at 100,000 × g and 4°C. The PBS wash was poured off. To remove proteins adventitiously associated with the surface of exosomes (Pellet 2), this material was resuspended in 30 ml of 0.1 m sodium bicarbonate, pH 11.4, and the washed exosomes collected by centrifugation at 100,000 × g and 4°C for 2 h (Pellet 3). Depending on the volume of CM, we used either an SW28 or SW41Ti rotor (Beckman Coulter) and an Optima L-90K ultracentrifuge (Beckman Coulter).
Sucrose gradient isolation of exosomes.
Crude exosomes (Fig. 1A) from each cell model were further fractionated on gradients of 0.25–2.3 m sucrose according to the method of Théry et al. (2001) (Fig. 1B). To investigate whether tau was present inside or on the surface of exosomes, Pellet 3 from 400 ml of N2a CM was resuspended in 400 μl of PBS and split in two. Each suspension was repelleted by centrifugation at 100,000 × g for 2 h. One pellet was held at 4°C; the other pellet was resuspended in 20 μl of 10% (v/v) Triton X-100 in PBS and subjected to two rounds of freeze-thawing using dry ice and a 37°C water bath. To ensure completed disruption of exosomes, the suspension was sonicated for 10 min. Thereafter, samples treated with or without Triton X-100 were applied to a 0.25–2.3 m linear sucrose gradient and centrifuged at 100,000 × g and 4°C for 18 h using an Optima L-90K ultracentrifuge and an SW41Ti rotor (Beckman Coulter). Sucrose gradients were prepared in 12 ml tubes using a peristaltic pump and a mixing chamber with 0.25 m sucrose in 20 mm HEPES, pH 7.4, in chamber A and 2.3 m sucrose in 20 mm HEPES, pH 7.4, in chamber B. After centrifugation, 1 ml fractions were collected by sequentially removing samples from the top of the tube (Fig. 1B). Aliquots (50 μl) of each fraction were used to measure refractive index. The remainder of the fractions were diluted 1:10 with PBS and then centrifuged at 100,000 × g and 4°C for 2 h using an Optima L-90K ultracentrifuge and an SW41Ti rotor (Beckman Coulter) to pellet exosomes. Supernatants were poured off and pellets resuspended in 60 μl of PBS containing 1% (v/v) Triton X-100 and 1% (w/v) BSA. These were then subjected to two freeze–thaw cycles and 10 min of sonication. For Western blot analysis, a starting volume of 200 ml of CM was used to isolate exosomes and the final pellet resuspended in 20 μl of Laemmli buffer. For electron microscopy (EM), a starting volume of 200 ml of CM was used to isolate exosomes and the final pellet was resuspended in 20 μl of PBS. For primary neurons and iHCNs, a starting volume of 35 ml of CM was used for sucrose-density isolation of exosomes.
Preparation of brain homogenates.
Cortical tissue (200 mg) from a male adult C57BL/6J mouse, a 93-year-old cognitively normal woman, and a female Sprague Dawley adult rat were each homogenized in 1 ml of ice-cold RIPA buffer containing 1 mg/ml aprotinin, 1 mg/ml pepstatin A, 1 mm pefabloc, 2 mm 1,10-phenanthroline, 5 mm EDTA, and 5 mm EGTA with 20 strokes of a Dounce homogenizer. Homogenates (1 ml) were clarified by centrifugation at 90,000 × g and 4°C for 60 min. The supernatant was removed and protein concentration determined using a BCA kit (Thermo Fisher Scientific). Thereafter, samples were either stored at −80°C or used directly. For dephosphorylation, lysates (0.2 mg of total protein) were incubated with 40 units of calf intestine alkaline phosphatase (New England Biolabs) at 37°C for 1 h.
Western blot.
Samples were electrophoresed on 4–12% polyacrylamide bis-tris gels in MOPS (for tau) or MES (for ALIX-1, Flotillin-1, PrP, and GM1) buffer (Invitrogen) and proteins transferred to nitrocellulose membranes at 400 mA for 2 h (Borlikova et al., 2013). Thereafter, membranes were boiled in PBS for 2 × 90 s (Ida et al., 1996) and blocked in 1% (w/v) BSA in PBS. For exosome experiments, membranes were cut to allow analysis of the same sample for ALIX-1, Flotillin-1, PrP, and GM1 ganglioside. The membranes were incubated overnight at 4°C in primary antibody solution, followed by a 6 × 10 min wash with PBS-T. The membranes were then incubated in secondary antibody solution for 1 h at room temperature, followed by a 6 × 10 min wash with PBS-T. See Table 1 for details of antibodies and concentrations used. Tau bands were visualized using Licor, whereas ECL Western blotting substrate (Thermo Fisher Scientific) and x-ray films were used for revelation of exosome markers.
A standard containing recombinant versions of all six human tau isoforms was obtained from Sigma-Aldrich and used as a positive control for Western blot experiments involving iHCN lysates.
Electron microscopy.
Sucrose-gradient-isolated exosomes from a starting volume of 200 ml of N2a CM were resuspended in 10 μl of PBS and adsorbed onto 2 formvar-coated copper grids. After 1 min, the grids were washed with water and then counterstained with 1% uranyl-formate for 1 min. Grids were blotted dry using Whatman filter paper and exosomes were visualized using a 1200EX microscope (JEOL).
Preparation of ½-tmax Aβ(1–42).
Half-tmax Aβ(1–42) was prepared essentially as described previously (Minogue et al., 2009). Aβ(1–42) monomer was isolated by SEC in 10.9 mm HEPES, pH 7.8, and filtered through a 0.22 μm filter (Millipore) in a sterile hood. An aliquot of the filtered sample was used for concentration determination by measuring the absorbance at 275 nm and using the extinction coefficient 1361 M−1 cm−1 (O'Malley et al., 2014). The remainder of the sample was diluted with sterile buffer to 80 μm and all further manipulations were performed on ice. Thioflavin T (ThT) was added to a portion of the stock Aβ solution and aliqouts added into a black 96-well plate (Nunc; Plate 1) and to a second sterile black 96-well plate (Plate 2). The remainder of the Aβ stock solution that did not contain ThT was added to Plate 2 and held on ice for 60 min. Plate 1 was incubated at room temperature (RT) with shaking (700 rpm) and fluorescence was monitored at 20 min intervals. After 60 min, Plate 2 was also incubated at RT and fluorescence was monitored in the wells containing Aβ plus ThT. Results from Plate 1 were used to estimate the incubation time required for the samples in Plate 2 to attain half maximal aggregation and the replicates containing ThT in Plate 2 to confirm that the initial phase of aggregation was similar to that observed for samples in Plate 1. ½tmax samples were then flash frozen on dry ice and stored at −80°C until used for toxicity experiments or for characterization using EM and analytical size exclusion chromatography (aSEC; O'Malley et al., 2014).
Preparation of amyloid β-derived diffusible ligands.
Amyloid β-derived diffusible ligands (ADDLs) were prepared essentially as described previously (Freir et al., 2011). Hexafluoro-2-propanol (HFIP; 222 μl) was added to 1 mg of Aβ(1–42) in a 2 ml of low-binding microcentrifuge tube (Eppendorf) to produce a peptide concentration of 1 mm. The solution was incubated at 37°C for 1 h and mixed briefly by vortexing every 10 min. The HFIP was evaporated under a nitrogen stream with rotation of the centrifuge tube to ensure formation of an even film of peptide on the lower walls of the tube. Dried peptide films were stored over desiccant at −20°C for a minimum of 14 h. The peptide film was then dissolved in 40 μl of anhydrous DMSO (Life Technologies) and 5 μl of the DMSO mixture was added stepwise to 960 μl of F-12 medium (Life Technologies), with vortexing between each addition. The solution was incubated at 4°C for 14–16 h and then centrifuged at 16,000 × g for 10 min. The upper 95% of the supernatant was transferred to a new microcentrifuge tube and ADDLs were buffer exchanged into 10.9 mm HEPES, pH 7.8, using a preequilibrated Zeba spin desalting column (7 kDa MWCO; Thermo Fisher Scientific). The concentration of Aβ oligomers was determined using the extinction coefficient, ε275 = 1361 M−1 cm−1 (O'Malley et al., 2014). After concentration determination, ADDLs were aliquoted, immediately frozen on dry ice, and then stored at −80°C. Once thawed, aliquots were characterize by aSEC and EM (O'Malley et al., 2014) or applied to cells.
Results
Tau is present in the medium of healthy N2a cells at levels slightly but significantly higher than marker cytosolic proteins
Most prior studies that have investigated the extracellular release of tau used transfected cells that overexpress tau (Kim et al., 2010a; Kim et al., 2010b; Chai et al., 2012; Karch et al., 2012; Plouffe et al., 2012; Saman et al., 2012; Simón et al., 2012), whereas we chose to focus on endogenous tau in CM of untransfected cells. Because even strongly expressing cells release only femtomolar levels of tau (Chai et al., 2012) and Western blotting is insufficiently sensitive for the detection of such low levels (Kuiperij and Verbeek, 2012; Petry et al., 2014), we used a well characterized ELISA capable of capturing all isoforms of tau that contain the mid-region residues 194–241 (Figs. 2B, 3; Barten et al., 2011). In preliminary experiments, we examined three neuroblastoma cell lines and found that N2a cells (Fig. 4A) have high levels of viability when grown under standard conditions, as evidenced by release of only low levels of LDH (Fig. 4D), and express appreciable levels of intracellular tau (Fig. 4B). Tau detected in CM could arise from at least three distinct sources: (1) nonspecific leakage due to cellular compromise (Jack et al., 2010), (2) release due to specific but undefined secretory mechanisms (Chai et al., 2012), or (3) release due to membrane turnover and/or vesicle release (Chai et al., 2012; Simón et al., 2012). Therefore, we were careful to compare the levels of tau in CM alongside those of LDH and β3T, two marker cytosolic proteins that are not known to be actively secreted by cells. In addition, to account for the very different intracellular concentrations of tau, LDH, and β3T, we measured protein levels or enzymatic activity (in the case of LDH) in CM and in lysates and used the values obtained to calculate the percentage of protein in CM relative to the total amount found in both CM and lysates. Using this approach, we examined the relative levels of tau, LDH, and β3T in medium conditioned by N2a cells for 6, 24, and 48 h. LDH levels were relatively low and remained constant between 6 and 24 h after medium change and β3T was not detected (Fig. 4C). However, after 48 h, LDH levels were significantly increased and β3T was readily detected. To minimize artifacts arising from cumulative levels of cell death, we conditioned cells for just 24 h. In multiple experiments, the amount of LDH activity found in medium after 24 h of conditioning was typically ≤1% of total LDH activity in the respective cell lysate (Fig. 4C,D). Careful inspection of cells using bright-field microscopy (Fig. 4A) and trypan blue exclusion (data not shown) indicated that <1.5% of cells were dead or damaged and no β3T release was detected. In contrast, even after only 6 h of incubation, N2a CM was found to contain significantly higher relative amounts of tau than LDH (Fig. 4C). Importantly, we confirmed that the differences in the detection of the tau, LDH, and β3T proteins in CM did not result from differences in sensitivity because, when total cell lysate was diluted into the medium, all three assays readily detected ≤0.1% of the respective protein present in lysate (data not shown). Moreover, when CM was removed from cells and incubated at 37°C for 24 h, the levels of tau, LDH, and β3T remained stable (data not shown). There are a number of probable explanations as to why the increase in tau relative to LDH is more readily detected at early time versus later time point. First, even if tau is released at a constant rate, some may interact with or be taken into cells or be degraded by membrane-bound proteases. Second, with increasing time in culture, there is more cell death and consequently disproportionately more LDH. Third, there may be a homeostatic mechanism that controls the levels of extracellular tau. Whatever the reason that the relative amount of tau to LDH does not increase over time, it is clear that at least a portion of tau detected in the CM of N2a cells is released from healthy cells.
Extracellular tau from N2a cells is largely free-floating and unaggregated
Next, we investigated whether the tau present in N2a CM was aggregated. We addressed this issue by using a conformation-directed mAb to capture and immunodeplete N2a CM of reactive tau species and then measure the amount of residual tau that could be detected using our Tau5-BT2 ELISA. In these experiments, each sample was subjected to two rounds of immunodepletion by either MC1 (conformation-directed) or BT2 (mid-region tau unaffected by posttranslational modifications). Excess mAb was removed by addition of protein G beads. In two separate experiments, BT2 immunodepletion decreased the Tau5-BT2 ELISA signal in CM by ∼100% and in lysates by ∼100%. In contrast, MC1 did not significantly change the amount of tau detected by the Tau5-BT2 ELISA in CM (783 ± 93 and 729 ± 73 pg/ml before vs after IP with MC1) or in lysates (310 ± 35 vs 305 ± 53 pg of tau/μg total protein before vs after IP with MC1), whereas MC1 did effectively immunodeplete recombinant aggregated FL tau. To search for aggregates of tau that might not be recognized by MC1, we centrifuged N2a CM under conditions known to pellet tau aggregates (100,000 × g for 2 h; Kumar et al., 2014), but again observed no change in the amount of tau in the supernatant (Fig. 5A). The results of the MC1 and centrifugation experiments indicate that the vast majority of tau present in the CM of healthy N2a cells is not aggregated. In the course of our centrifugation experiments, we probed the pellets to determine whether there were small quantities of pelletable tau the removal of which might not produce a detectable difference between the centrifuged sample and uncentrifuged N2a CM. Indeed, a very small amount of tau (equivalent to 0.1% of the mid-region ELISA signal in the CM) was recovered in the pellet and this amount was increased when the pellet was thoroughly disrupted (equivalent to 0.2% of the mid-region ELISA signal in the CM) with detergent and sonication (Fig. 5A: 0.60 vs 1.18 pg).
Less than 1% of extracellular tau in healthy N2a cultures is present in exosomes
Because a prior study reported that tau can be contained in small, extracellular microvesicles known as exosomes (Saman et al., 2012), we used the pellet produced by the 2 h 100,000 × g centrifugation as the starting point to isolate exosomes and determine whether tau could be detected therein. The 100,000 × g pellet from 400 ml of N2a CM was divided in half; one portion was treated with Triton X-100 to lyse any vesicles that might have been present and the other half was gently resuspended in PBS. The two samples were then fractionated on a sucrose gradient (Fig. 1B). Tau was detected in pellets from fractions with a buoyant density (1.10–1.15 g/ml sucrose; Fig. 5B, ▴) consistent with that reported for exosomes (Théry et al., 2001), whereas tau was not detected in the pellets from the corresponding fraction of the sample that had been pretreated with Triton X-100 (Fig. 5B, +). In the gradient bearing the pellet that had been treated with Triton X-100, tau was found in only the least dense fraction (#1), that is, the fraction expected to contain free-floating molecules or molecules from lysed vesicles (Fig. 5B, ○). Pelleted fractions from both gradients (i.e., from samples pretreated with and without Triton X-100) were analyzed for the presence of exosome markers by Western blotting and also examined by EM. As anticipated, exosome markers were not detected in pellets from any sucrose gradient fractions from the Triton X-100-pretreated sample (data not shown). In contrast, the pellets from gradient fractions #3–5 of the Triton X-100-free sample contained readily detectable levels of the exosome marker proteins Alix-1, Flotillin, and PrP, as well as the lipid GM1, which is abundant in exosomes (Fig. 5C). Moreover, the exosome-positive fractions did not contain detectable amounts of β3T, Prohibitin, or GRP78 (data not shown). EM examination of the pellets from gradient fractions #3–5 revealed the presence of ∼60-μm-diameter vesicles typical of exosomes (Théry et al., 2001; Fig. 5D). Therefore, it is apparent that a small amount of the tau released from healthy N2a cells is associated with exosomes.
Free-floating tau is found in conditioned media from iPSC-derived iHCNs
After the above identification of free-floating, unaggregated tau in N2a CM, we searched for tau in CM from an iHCN line. Cortical neurons were generated from iPSCs from a healthy control (YZ1) using protocols described previously (Muratore et al., 2014a, Muratore et al., 2014b). iHCNs were cultured for 45 d after differentiation (Fig. 6A)—a stage at which they display appropriate markers of forebrain neurons (Muratore et al., 2014a) and express appreciable levels of tau (Fig. 6B). The neurons were conditioned for 48 h and CM and lysates collected. In 6 separate experiments, <5.7% of total LDH enzymatic activity was present in CM and no β3T was detected in CM (Fig. 6C). The latter finding indicates that, even under conditions when cell compromise is detectable by LDH release and trypan blue uptake, β3T is not readily released from damaged cells and therefore its measurement is not a useful indicator of low levels (less than ∼5%) of cell compromise. Consistent with our N2a studies, tau was found in iHCN CM at levels disproportionately higher than LDH (Fig. 6C). Again, we used a combination of MC1 IP and Tau5-BT2 ELISA to search for potential tau aggregates. As before, the conformation-specific mAb, MC1, did not decrease the amount of tau detected by mid-region-ELISA in iHCN CM (11.9 ± 1.4 and 10.2 ± 1.5 ng/ml before vs after IP with MC1) or lysates (4130 ± 371 and 3830 ± 651 pg of tau/μg total protein before vs after IP with MC1), whereas BT2 IP completely depleted both CM and lysate of measurable tau. Again, similar to our N2a study, the amount of tau in iHCN CM was not detectably affected by high-speed centrifugation (Fig. 6D). These results indicate that the overwhelming majority of tau in iHCN CM is free-floating and unaggregated, but, as in N2a CM, small quantities of tau (equivalent to 0.01% of the mid-region ELISA-detected signal in iHCN CM) were recovered in the pellet of a sucrose gradient fraction having a buoyant density typical of exosomes (Fig. 6E).
Free-floating, truncated tau is found in conditioned media of PRNs
To determine whether expression of a more mature array of tau isoforms influence the amounts and forms of extracellular tau, we examined DIV 21 primary rat hippocampal neurons (PRNs; Fig. 7A,B). Neurons were conditioned for 24 h and the media and lysates collected. No β3T was detected in CM and staining with propidium iodide and Hoechst indicated that <1.5% of cells were dead (data not shown). In 8 separate experiments, the LDH activity in medium never accounted for >3.7% of total LDH activity (Fig. 7C). Consistent with our N2a and iHCN studies, tau was detected in the PRN CM at a level disproportionately higher than LDH (Fig. 7C). Again, IP with the conformation-specific mAb MC1 did not decrease the amount of tau detected by mid-region ELISA in PRN CM (1797 ± 232 and 1846 ± 147 pg/ml before vs after IP with MC1) or lysates (2645 ± 409 and 2715 ± 357 pg of tau/μg total protein before vs after IP with MC1), whereas BT2 effectively depleted all detectable tau. As with the CM from N2a and iHCN cells, high-speed centrifugation did not detectably lessen the amount of tau in PRN CM (Fig. 7D). These results indicate that the bulk of tau in PRN CM is unaggregated and free-floating, but, as with N2a cells and iHCNs, small quantities of tau (equivalent to 0.01% of the mid-region ELISA-detected signal in iHCN CM) were detected in buoyant vesicles with a density expected for exosomes (Fig. 7E).
Majority of tau in PRN CM is CT truncated
Although most prior studies on extracellular tau assumed that the material released was FL, the ELISAs that were used were incapable of differentiating between FL tau and fragments of tau that retain the mid-region epitopes relied upon for detection (Meredith et al., 2013, Pooler et al., 2013). Moreover, previous studies did not specifically identify extracellular CT fragments of tau. We addressed these important issues by developing and validating three new ELISAs (Figs. 2, 3): (1) one that readily detects FL tau but not fragments of tau (Fig. 2E) and assays that detect (2) any form of tau that contains all or part of the C terminus of tau (Fig. 2C) or (3) any form of tau with a fully intact C terminus (Fig. 2D). Using these new assays and the aforementioned mid-region ELISA (Fig. 2B), we measured the levels of tau in the CM and lysates of PRNs using the same recombinant FL tau standard for each assay. All four assays measured closely similar levels of tau in lysates (Fig. 8A), but yielded very different values for tau in CM (Fig. 8B).
The fact that all four assays reported similar levels of tau in lysates strongly suggests that the bulk of tau inside neurons is FL (Fig. 8B). In contrast, in PRN CM, the mid-region assay detected ∼10 times more tau than the FL assay, thus indicating that most extracellular tau is truncated and that FL tau only contributes a small percentage of the total tau found in CM (Fig. 8B). The two CT assays should be capable of detecting both FL tau and any N-terminally truncated fragments that need not extend beyond Gln244 (Fig. 3). Because the CT assays detected approximately twice as much tau in CM as was measured by the FL assay (Fig. 8B), we conclude that ∼50% of the CT assay signal is attributable to FL tau and 50% to forms of tau that contain an intact C terminus but are N-terminally truncated. The amount of tau detected in PRN CM with the mid-region assay was ∼4–5 times greater than the amount of tau detected by the CT assays. This suggests that ∼75% of the tau detected by the mid-region assay must contain all or most of the Tau5 epitope (210–241), but lacks sequence extending beyond Gln244. The N terminus of the BT2 epitope extends to Arg194 and, although we can only speculate as to how far N-terminally the fragments detected by the mid-region assay may extend (Fig. 3), recent studies on human CSF (Meredith et al., 2013; Wagshal et al., 2015) and iPS neurons (Bright et al., 2015) indicate that this material is likely to be highly heterogeneous with regard to N termini.
Because we had shown for each of the three neuronal systems that at least a portion of the tau in CM detected by the mid-region assay was present at levels higher than the percentage of released LDH (and therefore apparently independent of neuronal compromise), we investigated whether the relative amount of tau species detected by our other tau assays also exceeded that attributable to cell leakage. Importantly, the relative amount of extracellular tau measured by the FL and CT ELISAs in CM was lower than that of LDH in the same CM, suggesting that FL and CT fragments of tau were unlikely to be released by mechanisms independent of neuronal compromise. The difference in the ratio of extracellular to intracellular tau measured using the mid-region assay versus the other tau assays (Fig. 8C) further suggests that mid-region-containing fragments are specifically released from neurons by a process independent of cell compromise/death.
To investigate whether mid-region-containing fragments were generated by extracellular cleavage of FL tau, we conducted time course experiments in which PRN CM or PRN CM spiked with PRN lysate was incubated at 37°C with and without protease inhibitors and samples were analyzed using the FL tau (HJ9.4-Tau46) ELISA. The amount of FL tau detected in PRN CM was low and did not change upon incubation regardless of the presence of protease inhibitors. Neuronal lysates contain abundant FL tau (Fig. 8A) so that the addition of a small amount of lysate was sufficient to yield a FL tau concentration of ∼20 ng/ml; that is, a level ∼40-fold greater than the concentration of endogenous FL tau in PRN CM (cf. Fig. 8A,B,D). As with endogenous tau, the levels of the exogenous (lysate spike) FL tau remained constant throughout the 24 h incubation (Fig. 8D). As an additional control, we also measured tau using the mid-region (BT2-Tau5) ELISA. The amount of tau detected by the mid-region assay was ∼8–9% lower in samples without protease inhibitors, but did not change over time (Fig. 8E). Together, these results indicate that PRN CM contains little or no proteolytic activities capable of cleaving FL tau and that CT truncated tau fragments are likely to be produced inside neurons and then released.
Aβ-induced cell death leads to the release of multiple forms of tau from PRN
Given that certain assembly forms of the Aβ can influence aspects of tau biology and that Aβ-induced changes in tau are believed to be critically involved in AD pathogenesis (Spires-Jones and Hyman, 2014), we investigated whether Aβ can influence the levels and forms of tau released from neurons. We treated primary rat neurons with a partially aggregated preparation of Aβ(1–42) that contained both amyloid fibrils and Aβ monomer (Fig. 9A). This preparation is referred to as ½tmax because it is produced by incubating Aβ monomer for a period that yields half the maximal level of thioflavin T fluorescence (Fig. 9A; Minogue et al., 2009; O'Malley et al., 2014). In 5 separate experiments, 20 μm ½tmax caused a time-dependent decrease in neuronal viability such that, from day 5, the level of LDH in media was significantly elevated compared with the vehicle control (Fig. 9B, p > 0.005). When the same CM was analyzed using the BT2-Tau5 mid-region ELISA, the relative increase in extracellular tau signal (Fig. 9C) was similar to the increase seen in LDH (Fig. 9B), suggesting that the increase in tau was attributable to Aβ-induced neuronal compromise. Sister cultures treated with excitotoxic levels of glutamate (as a positive control) also evidenced a direct correspondence between the relative levels of tau and LDH detected in medium (cf. Fig. 9B,C). Given that these time course experiments (Fig. 9C) allowed us to analyze medium from cells treated with Aβ both before and after induction of cell leakage/death, it is clear that the addition of Aβ to the cultures per se did not alter the levels of tau detected by the mid-region ELISA. Therefore, treatment of neurons with a preparation of Aβ that over time induced toxicity did not cause any discernible change in extracellular tau before loss of membrane integrity.
It is possible that only certain forms of tau may be specifically altered by Aβ and that these changes are not detected using the mid-region BT2-Tau5 ELISA. In this context, we also measured tau in CM using our FL and CT ELISAs. In two separate experiments, both CT ELISAs revealed a time-dependent increase in extracellular tau from neurons treated with Aβ, whereas the level of tau in CM from vehicle-treated PRNs actually fell modestly (Fig. 9D,E). The levels of CT-tau in CM from PRNs treated with glutamate were elevated from day 1 compared with vehicle- or Aβ-treated cells and remained high throughout the 7 d experiment. Therefore, the changes seen with the mid-region and CT ELISAs were broadly similar (Fig. 9C–E). Remarkably, the levels of FL tau fell in PRNs treated with vehicle or glutamate (Fig. 9F), whereas the levels of FL tau were increased on days 5 and 7 after Aβ treatment (p < 0.02). In summary, time-dependent increases in extracellular tau were only evident in cultures with injured neurons and both glutamate and Aβ caused an increase in tau as measured using the mid-region and CT assays. Notably Aβ, but not glutamate, caused an increase in extracellular FL tau. Therefore, Aβ treatment that resulted in cell leakage/death caused a similar time-dependent increase in tau measured using four different ELISAs. The reason that the overt damage induced by glutamate did not increase extracellular FL tau but Aβ did hints that the mechanisms by which neurons die may influence the release of certain forms of tau (e.g., FL tau) and merits further investigation.
Because several different forms of Aβ have been shown to compromise normal neuronal activity and this can be accomplished at much lower concentrations than is required to induce cell death (Wang et al., 2002; Freir et al., 2011), we also investigated whether low concentrations of synaptotoxic Aβ could alter the amount or forms of extracellular tau. For this, we used an Aβ preparation known as ADDLs (Lambert et al., 1998; Wang et al., 2002; Hepler et al., 2006; Freir et al., 2011). Aliquots of preprepared ADDLs, which when applied to hippocampal slices at a concentration of 500 nm blocked LTP (data not shown), were thawed on ice and added directly to neurons or characterized by SEC and EM (Fig. 9G). At intervals, CM was removed and analyzed for LDH and tau. Consistent with prior experiments (Fig. 9B), LDH was increased in CM of cells treated with 20 μm glutamate versus the vehicle control at all time points studied (data not shown). Also in keeping with our other experiments (Fig. 9C), treatment with glutamate caused a time-dependent increase in tau detected by the mid-region assay (Fig. 9H) and an increase in CT1-detected tau was evident throughout the 7 d study. In contrast, 500 nm ADDLs did not increase extracellular levels of tau measured using either mid-region or CT1 ELISAs (Fig. 9H,I). Therefore, as with the results from the ½tmax studies, application of bioactive Aβ (in this case, ADDLs) did not alter extracellular tau in the absence of overt neuronal compromise.
Discussion
The possibility that aggregation of certain proteins linked to neurodegeneration may propagate in a manner analogous to that proposed for the prion protein has drawn much attention in recent years (Spires-Jones and Hyman, 2014). However, although there is clear evidence that extracellular application of exogenous tau aggregates to cultured cells or injection of aggregates into rodent brain can induce aggregation of endogenous tau, little is known about the fundamental processes involved and how they might be initiated in the human brain. A spread mechanism for a supposedly cytosolic protein such as tau must involve at least four phases: (1) release of tau from donor neurons, (2) aggregation of tau (this could occur before or after point 1), (3) uptake of tau into certain recipient neurons, and (4) induction of aggregation of tau in the recipient cells. Understanding the molecular forms of tau released and the mechanisms by which this is achieved are of obvious interest.
Several prior studies investigated the release of tau in various cell culture systems. Most used tau overexpression models (Kim et al., 2010a; Kim et al., 2010b; Chai et al., 2012; Plouffe et al., 2012; Simón et al., 2012), a few used untransfected cells (Chai et al., 2012; Karch et al., 2012; Bright et al., 2015), and two analyzed tau in medium from immature primary cortical rodent neurons (Karch et al., 2012, Pooler et al., 2013). All of these studies suggest that the tau detected in cell medium is released by an unconventional secretion mechanism (Kim et al., 2010a, b; Chai et al., 2012; Karch et al., 2012; Plouffe et al., 2012; Saman et al., 2012; Simón et al., 2012). Some groups reported that tau is released from cells in exosomes (Saman et al., 2012, Simón et al., 2012), whereas others found no evidence for tau in exosomes (Karch et al., 2012). Importantly, only one prior study rigorously controlled for the level of cell death (Chai et al., 2012), but these investigators used transfected HEK cells and measured tau using a mid-region ELISA incapable of distinguishing between FL tau and mid-region-containing fragments of tau (Chai et al., 2012).
Here, we report a series of systematic experiments that involved three distinct neuronal model systems; the use of highly sensitive ELISAs that differentiate between FL tau, mid-region-bearing fragments, and CT fragments; and careful assessment of cell viability. To determine whether the amount of tau in CM was higher than that attributable to cell rupture, we measured the levels of two marker cytosolic proteins (LDH and β3T) that are not actively secreted from cells and counted dead cells using trypan blue and/or propidium iodide/Hoechst. To control for differences in the expression of tau, LDH, and β3T, we measured protein levels or enzymatic activity in CM and in lysates and used the values obtained to calculate the percentage of protein in CM according to the following equation: ([analyte in CM])/([analyte in CM] + [analyte in lysate]) × 100. To ensure reproducibility, at least five replicate experiments were conducted for each neuronal cell model studied. In agreement with other reports, we found that the level of extracellular tau (measured using our mid-region ELISA) was higher than that which could be attributed to the low level of cell death evident in our cultures. Only a tiny portion of this released material was found in exosomes. Similar results were obtained in N2a cells, iHCNs, and mature PRNs. In contrast to the mid-region-detected material, the low signals for tau in PRN CM measured using assays specific for FL-tau- or CT-containing fragments are fully explainable by the low level of cell death evident in our (and all) cell cultures. In preliminary experiments, similar results were obtained when comparing mid-region, FL-detected tau, and CT-detected tau in CM and lysates of N2a cells, iHCNs, and mature human fetal neurons (data not shown). Therefore, in four distinct neuronal culture systems (N2a cells, iHCNs, PRNs, and human fetal neurons), different forms of tau are released from neurons by different processes. CT-truncated forms of tau are released by mechanisms that are both dependent and independent of cell death and FL and CT fragments of tau appear to be released only upon cell death.
The specific and sensitive detection of tau in biofluids is not trivial (Portelius et al., 2008; Kuiperij and Verbeek, 2012); up to six spliced isoforms can be present and tau is known to undergo multiple after translational modifications, including heterogeneous proteolysis (Lee and Leugers, 2012). In this study, we chose to investigate the molecular identity of extracellular tau using highly specific and sensitive ELISAs, which, when used in tandem, yielded significant information about the nature of tau in the medium of cultured neurons. The assays that we developed allow for the detection of very low levels of the protein regardless of aggregation and/or phosphorylation state; the ELISA signals are appropriately responsive to dilution and are abolished when samples are immunodepleted with relevant anti-tau mAbs. In future studies, it will be important to develop orthogonal methods to define more precisely the species detected by both our mid-region and CT ELISAs. Nonetheless, from our analysis, it is already clear that N-terminal fragments that are detected in the CM of healthy neurons by our mid-region assay share similar antigenic profiles as the heterogeneous mid-domain and N-terminal tau fragments recently described in human CSF (Meredith et al., 2013, Wagshal et al., 2015), whereas the FL and CT species released as a result of cell death are distinct.
Low levels of cell death among CNS neurons is inevitable (Spalding et al., 2013) and tau is a highly abundant protein (Lee and Leugers, 2012). Therefore, one would anticipate that, even in healthy brains, a small amount of MTBR-containing tau will be released as a consequence of cell death. The initial reports of the detection of extracellular tau in cultures of apparently healthy cells raised the hope that therapeutically inhibiting the active release of tau might attenuate the spread of tau aggregates in the brain (Mohamed et al., 2013). However, this strategy would be of use only if the forms of tau released were capable of aggregation. Therefore, our finding that only non-MTBR-containing forms of tau are actively released from healthy neurons suggests that there would be no benefit in inhibiting this process. Indeed, given the apparent specificity for the release from healthy neurons of mid-region-containing tau lacking the MTBRs, it is possible that these species may serve some normal extracellular function and that inhibition of their release could be detrimental (Mably et al., 2015). Similarly, it is conceivable that mid-region-containing fragments of tau could influence signal transduction pathways to affect neurodegeneration in ways yet to be discovered.
Because it is impossible to prevent the low level of neuronal death that occurs naturally, and many events can heighten such neuronal compromise, our demonstration that small amounts of MTBR-containing forms of tau are released during neuronal death have implications for understanding human tauopathies and developing therapies. If the “pathogenic spread” hypothesis, which has been so elegantly demonstrated in rodent models (Clavaguera et al., 2009; de Calignon et al., 2012) and cell culture (Frost et al., 2009; Kfoury et al., 2012; Holmes et al., 2014), has any relevance to human tauopathies, then the central question arises as to what is the first site of aggregation (intracellular or extracellular) and how is tau released. Our data suggest that aggregation-competent tau is released only upon cell compromise. However, none of the culture systems that we studied produced intraneuronal aggregates, so our work is presumably relevant only to the release of unaggregated forms of tau, some of which could later aggregate after release. Our study deliberately focuses on physiological forms of tau; however, further studies will be required to determine whether aggregates of tau are only released passively or if there are specific active release processes that can be targeted therapeutically. Furthermore, a rigorous analysis of the phosphorylation status of extracellular tau and the forms of tau found in exosomes is also merited.
With regard to the other self-aggregating protein in AD, addition of aggregated Aβ to PRNs induced cell compromise starting between days 3 and 5 after treatment and all 4 ELISAs recorded an elevation in tau coincident with the onset of neuronal death. Similar to what has been described in the CSF of APP transgenic mice (Maia et al., 2013; Mably et al., 2015), extracellular tau did not change in the early phase of Aβ toxicity, but increased only when cell loss became evident. Moreover, treatment of PRNs with ADDLs at a concentration that impairs synaptic plasticity but does not induce cell death did not alter the amount or form of extracellular tau. Therefore, if Aβ is the trigger that stimulates the initial release from neurons of aggregation-competent (i.e., MTBR-containing) tau in AD and models thereof, it would appear to require specific injury of certain neurons. Regardless of whether tau is released passively as a result of cell death or via active processes, the therapeutic use of antibodies that target aggregated tau or MTBR-containing aggregation-competent forms of tau appear to offer great promise (Gu and Sigurdsson, 2011; Castillo-Carranza et al., 2014; Holmes and Diamond, 2014). An extension of the work described here to elucidate further the molecular identities of extracellular tau should facilitate the better design of efficacious immunotherapy approaches.
Footnotes
This work was supported by the Cure Alzheimer Fund (D.M.W. and D.J.S.), the Foundation for Neurologic Diseases (D.M.W., T.L.Y.-P., and D.J.S.) and he Harvard NeuroDiscovery Center through a major gift from Rick and Nancy Moskovitz (D.M.W.). We thank Irene Griswold-Prenner and Alexandra Mably for useful discussions; Eva-Maria and Eckhard Mandelkow for expression vectors for hTau40 and K19; Peter Davies and David Holtzman for antibodies MC1 and HJ9.4, respectively; Donna Barten and Sethu Sankaranarayanan for invaluable advice on the ELISAs for β3T and mid-region tau; Maria Ericsson for assistance with electron microscopy; Matthew P. Frosch for human tissue; and Anna Krichevsky for human fetal neurons.
The authors declare no competing financial interests.
- Correspondence should be addressed to Dominic M. Walsh, Laboratory for Neurodegenerative Research, Center for Neurologic Diseases, Brigham and Women's Hospital, Harvard Institutes of Medicine, 77 Avenue Louis Pasteur, Boston, MA 02115. dwalsh3{at}partners.org