ApoE4-associated phospholipid dysregulation contributes to development of Tau hyper-phosphorylation after traumatic brain injury

The apolipoprotein E4 (ApoE4) genotype combines with traumatic brain injury (TBI) to increase the risk of developing Alzheimer’s Disease (AD). However, the underlying mechanism(s) is not well-understood. We found that after exposure to repetitive blast-induced TBI, phosphoinositol biphosphate (PIP2) levels in hippocampal regions of young ApoE3 mice were elevated and associated with reduction in expression of a PIP2 degrading enzyme, synaptojanin 1 (synj1). In contrast, hippocampal PIP2 levels in ApoE4 mice did not increase after blast TBI. Following blast TBI, phospho-Tau (pTau) levels were unchanged in ApoE3 mice, whereas in ApoE4 mice, levels of pTau were significantly increased. To determine the causal relationship between changes in pTau and PIP2/synj1 levels after TBI, we tested if down-regulation of synj1 prevented blast-induced Tau hyper-phosphorylation. Knockdown of synj1 decreased pTau levels in vitro, and abolished blast-induced elevation of pTau in vivo. Blast TBI increased glycogen synthase kinase (GSK)-3β activities in ApoE4 mice, and synj1 knockdown inhibited GSK3β phosphorylation of Tau. Together, these data suggest that ApoE proteins regulate brain phospholipid homeostasis in response to TBI and that the ApoE4 isoform is dysfunctional in this process. Down-regulation of synj1 rescues blast-induced phospholipid dysregulation and prevents development of Tau hyper-phosphorylation in ApoE4 carriers.

Taken together, research on this field suggests that the pathogenic relationships between ApoE4 genotype, TBI, and the risk they collectively confer for AD and CTE have yet to be fully elucidated. Neuropathological studies of human TBI cases have described the development of neurofibrillary tangles and amyloid plaques associated with neurodegenerative processes 22,23 . Recent studies in animal models also demonstrated TBI-linked Tau neuropathology and neurobehavioral deficits [24][25][26][27] . However, the mechanistic influence of ApoE4 genotype on developing neurodegeneration after TBI is unclear.
We have recently shown that ApoE proteins are critical determinants of brain phospholipid homeostasis and that the ApoE4 isoform is dysfunctional in this process 28 . We have demonstrated that the levels of PIP 2 are reduced in aged human and mouse brain tissues of ApoE4 carriers as compared to levels in ApoE3 carriers. These changes are secondary to increased expression of a PIP 2 degrading enzyme, synj1 in ApoE4 carriers. PIP 2 is a signaling lipid involved in ion channel regulation, exocytosis, endocytosis, actin cytoskeleton rearrangement, and cell signaling 29 . PIP 2 dephosphorylation at the synapse is mediated primarily by synj1, a phosphoinositol phosphatase that is expressed and enriched at the synapse and plays a role in endocytosis, presynaptic vesicle recycling, and postsynaptic receptor trafficking 29,30 . Interestingly, PIP 2 and synj1 have been recently linked to AD 31,32 . Recently, we have shown that reduction of synj1 accelerates lysosomal clearance of Aβ in APP/PS1 transgenic mice 33 , and rescues AD-related cognitive deficits by restoring brain PIP 2 homeostasis in ApoE4 mice 28 .
Based on these findings, we tested the hypotheses that ApoE proteins regulate changes in brain phospholipid homeostasis in response to TBI and that ApoE4-associated phospholipid dysregulation may promote development of TBI-associated amyloid and Tau pathologies. In the present study, we utilize well-established experimental models of human ApoE variants [34][35][36][37] and a battlefield-relevant mouse model of blast-induced TBI [24][25][26] to investigate the effects of ApoE isoforms on brain phospholipid composition, Aβ accumulation and Tau hyper-phosphorylation after blast-induced neurotrauma.

Results
Changes in hippocampal PIP 2 levels in response to blast-induced TBI exposure in ApoE3 and ApoE4 mice. We have recently shown that ApoE4 specifically induces reduction in brain PIP 2 levels in both aged ApoE4 human and mouse brains. However, these changes in PIP 2 levels were not seen in young ApoE4 mouse brains by 3 months of age 28 . In this study, we investigated if blast overpressure (BOP)-induced TBI could alter brain PIP 2 homeostasis in young ApoE4 mice when PIP 2 changes are yet to be manifested at this age.
At 3-4 months of age, ApoE3 or ApoE4 mice were exposed to three BOP injuries over the course of three days (once per day) while briefly anesthetized each time with isoflurane (see Methods) using an established pneumatic shock tube approach 26,38,39 . Non-blast sham control mice received the same exposure to anesthesia as blast-exposed mice. The BOPs used for this study (Fig. 1) simulated the blast forces that would be generated by approximately 14.3 kg of trinitrotoluene (TNT) detonated in the open field at a distance of approximately 6 meters (mean peak pressure 20.0 ± 0.3 psi; primary peak duration 6.0 ± 0.1 ms; impulse 40.0 ± 10.0 psi ms). Ninety-seven percent of blast-exposed mice (37/38, 97.4%) survived the 3X treatment regimen, which was not statistically different from the survival rate of sham controls (40/40, 100%, Fisher's Exact Test, p = 0.475). Immediately after recovering from anesthesia (approximately five minutes), 100% of the blast-exposed and control mice (38/38 blast-exposed and 40/40 sham controls) displayed intact visually-guided forepaw grasping responses while elevated from the tail as they were brought within reach of a foothold. In addition, all mice were monitored for two hours post-exposure (blast or sham treatments) in their home cages for adverse responses to treatment before being returned to the animal housing facility. By the end of this observation period, 97.4% of blast-exposed mice displayed normal appearing voluntary ambulation, breathing, movement responses to handling, and righting responses that by inspection were comparable to sham controls. One-hundred percent sham control and 97.4% blast-exposed mice (40/40 sham controls and 37/38 blast-exposed) survived to the conclusion of the study without veterinary intervention. Upon tissue collection, inspection of the brains revealed no indication of gross contusions or hemorrhages, including the one blast-exposed mouse that was euthanized within ten minutes after exposure to BOP due to breathing difficulty. These acute responses and experimental parameters are consistent with mild-to-moderate blast exposures in mice 39,40 .
Following 3X blast exposure, the levels of hippocampal PIP 2 in ApoE3 mice were increased 24 hours after BOP exposure ( Fig. 2A: ApoE3 blast 131.0 ± 9.8% of controls, N = 13, versus sham 100 ± 4.7%, N = 15; one-way ANOVA F(3,54) = 3.587, p = 0.0194; Tukey's multiple comparison test ApoE3 blast versus sham adjusted p = 0.022), whereas those levels in ApoE4 mouse hippocampal regions remained unchanged (ApoE4 blast 102.8 ± 4.5%, N = 15, versus sham 113.8 ± 9.0% of controls, N = 15; Tukey's multiple comparison test ApoE4 blast versus ApoE4 sham adjusted p = 0.69; ApoE3 blast versus ApoE4 blast adjusted p = 0.04). No statistically significant changes were seen in levels of other phospholipids such as phosphoinositol phosphate (PIP), phosphoinositol (PI), phosphatidic acid, cardiolipin and phosphoserine in ApoE4 or ApoE3 mice 24 hours after blast TBI exposure. On the other hand, the levels of PIP 2 were not significantly changed in neocortex, striatum or cerebellum in ApoE3 or ApoE4 mice in response to blast TBI (see Supplementary Fig. S1). No significant changes were seen in levels of other phospholipids in these brain regions. Together, these data suggest that blast exposure induces elevation of hippocampal PIP 2 levels in ApoE3 mouse brains, whereas ApoE4 genotype blunts these changes in response to blast TBI.
Hippocampal synj1 expression levels in ApoE3 and ApoE4 mice after blast TBI exposure. We have previously found that ApoE4 reduces brain PIP 2 levels due to the elevated expression of the rate-limiting enzyme of brain PIP 2 pathway, synj1 28 . Therefore, we next investigated whether blast-induced changes in brain PIP 2 levels in ApoE3 mouse hippocampal regions are secondary to decreased expression and/or enzymatic activities of synj1. We found that no statistically significant changes were seen in levels of synj1 mRNA in ApoE3 or ApoE4 mouse hippocampal brain regions 24 hours post blast TBI exposure (see Supplementary Fig. S2). On the other hand, there was a trend of reduction in synj1 protein levels in ApoE3 hippocampal regions 24 hours after BOP exposure (Fig. 2B: ApoE3 blast 50.3 ± 11.3% of control, N = 5, versus sham 100 ± 15.8%, N = 5; one-way ANOVA F(3,26) = 3.416, p = 0.0321; Tukey's multiple comparison test ApoE3 blast versus ApoE3 sham adjusted p = 0.0796, ApoE3 blast versus ApoE4 sham adjusted p = 0.028). These changes are consistent with the elevation in PIP 2 levels in ApoE3 mouse hippocampal regions after BOP exposure ( Fig. 2A). There was a similar but modest trend of reduction in synj1 protein levels in ApoE4 mouse brain post blast exposure ( Fig. 2B: ApoE4 blast 81.8 ± 12.0%, N = 10, versus sham 101.5 ± 7.3% of controls, N = 10; Tukey's multiple comparison test ApoE4 blast versus sham adjusted p = 0.500). No significant differences were seen in levels of synj1 protein or synj1 mRNA at baseline between ApoE3 and ApoE4 mouse brains without BOP (sham controls), which are consistent with our prior observations of ApoE mice at this age 28 . Together, these results suggest that changes in synj1 protein levels in response to blast TBI in ApoE3 mice are likely to be through translational or post-translational regulation.
Hippocampal pTau and Tau levels in ApoE3 and ApoE4 mice after blast exposure. Following blast exposure, the levels of pTau determined by AT8 antibodies using western blot analysis were significantly elevated 24 hours post-BOP in ApoE4 hippocampal brain regions (  Tukey's multiple comparison test adjusted p = 0.71). These results suggest that ApoE isoforms have differential effects on pTau/Tau processing, and that ApoE4 genotype may exacerbate Tau hyper-phosphorylation in the presence of blast exposure. These patterns of changes in pTau and total Tau levels in response to BOP-induced TBI were only seen in hippocampal brain regions, but not in cortical, striatal or cerebellar brain regions, suggesting regional vulnerability of hippocampi in response to blast TBI.
We also investigated the effects of ApoE4 and TBI on Aβ accumulation and ApoE secretion, and found that there were no significant changes in levels of mouse Aβ 40 or Aβ 42 , or in levels of secreted human ApoE in ApoE4 and ApoE3 hippocampal regions after BOP exposure (see Supplementary Fig. S3).

Reduction of synj1 decreases pTau levels in N2a cells.
We have demonstrated that there were differential changes in hippocampal PIP 2 /synj1 levels, as well as pTau/Tau levels in young ApoE3 versus ApoE4 mice after BOP exposure. Therefore, we determined whether there is a causal relationship between blast TBI-induced changes in PIP 2 /synj1 levels and changes in pTau/Tau levels. We first investigated the effects of down-regulation of synj1 on Tau phosphorylation in vitro. Using a N2a cell line stably transfected with human wild-type Tau, we found that levels of pTau were significant reduced ( Fig. 4A and B: 53.5% of reduction, T(4) = 14.79, p = 0.0001) with synj1 knockdown (KD) by synj1 siRNA, whereas levels of total Tau were slightly elevated although changes did not achieve statistical significance (113.8% of controls, T(4) = 1.365, p = 0.2441). The levels of holoAPP were not changed with synj1 siRNA treatment, which is consistent with our previous observations 33 . Down-regulation It was also noted that with reduction of pTau (mainly in cytosol) in synj1 KD conditions, the amount of cytosolic total Tau was increased as compared to controls. The reduction of synj1 expression in KD conditions was confirmed by fluorescent signals recognized by synj1 antibodies (see Supplementary  Fig. S4).
Together, our results suggest that synj1 down-regulation abolishes dysregulation of PIP 2 levels and hyper-phosphorylation of Tau in response to blast injury exposure in ApoE4 mice. Blast induces GSK3β activation in ApoE4 mice and synj1 knockdown reduces pTau partially through inactivation of GSK3β. We next determined whether blast injury induces any changes in the levels of two common Tau phosphorylation kinases: GSK3β and cyclin dependent kinase 5 (CDK5) in ApoE3 and ApoE4 mouse brains. As shown in Fig. 6A after blast exposure, levels of active GSK3β (pGSK3β recognized by an antibody against Y216) 41 were significantly increased in ApoE4 mice (ApoE4 sham 134.9 ± 38.6%, ApoE4 blast 241.0 ± 27.0%; N = 5/group, one-way ANOVA F(3,16) = 29.36, p < 0.0001), whereas levels of inactive GSK3β (pGSK3β recognized by antibody at Ser9) 42 were higher in ApoE3 mice but did not achieve statistical significance (Fig. 6B: ApoE3 sham 100 ± 25.8%, ApoE3 blast 156.5 ± 53.4%; N = 5/group, one-way ANOVA F(3,16) = 10.34, p = 0.0005, Turkey's comparison test: ApoE3 sham versus ApoE3 blast adjust p = 0.067). There were trends of higher basal levels of active GSK3β and lower basal levels of inactive GSK3β in ApoE4 sham mice compared to ApoE3 counterparts, but these differences did not achieve statistical significance (active GSK3β: ApoE4 sham 134.9 ± 38.6% versus ApoE3 sham 100.0 ± 11.8%, adjusted p = 0.22; inactive GSK3β: ApoE4 sham 60.11 ± 25.1% versus ApoE3 sham 100.0 ± 25.8%, adjusted p = 0.26). However, there were no significant changes in total GSK3β levels of ApoE4 or ApoE3 mouse brains in response to blast TBI exposure (ss Supplementary Fig. S6A and S6B: Tukey's multiple comparison test: ApoE4 blast versus ApoE4 sham adjusted p = 0.90, ApoE3 sham versus ApoE4 sham p = 0.21). On the other hand, the levels of CDK5 were not significantly changed in ApoE4 mice in response to blast exposure, whereas there was a trend of increased CDK5 levels in ApoE3 mice after BOP exposure (see Supplementary Fig. S6C). It was noted that basal levels of CDK5 in ApoE4 sham mouse brains were higher than those of ApoE3 counterparts.

Discussion
The ApoE-genotype dependent responses to TBI have been studied with many mechanisms proposed including alterations in neurogenesis, cholesterol trafficking, amyloid deposition and cholinergic dysfunction 43,44 . Our study investigates the association between a known genetic susceptibility factor (ApoE4) and an environmental risk factor (TBI) for the development of neurodegeneration and AD. We demonstrate that there are ApoE-genotype specific changes in brain PIP 2 homeostasis in response to blast injury, and that such changes contribute to the development of Tau pathology after blast. Therefore, our findings (as summarized in Table 1) are the first mechanistic studies that link ApoE4 genotype-specific changes in brain phospholipid homeostasis to the development of neurodegenerative processes after blast-induced TBI in ApoE4 carriers. These results implicate a novel mechanism by which ApoE4 genotype promotes the development of neurodegeneration after TBI.
Our study examines the effect of repetitive blast-TBI in the context of well-established genetic risk factors for Alzheimer's disease. In designing the current study we had concerns that a single blast exposure would more likely yield minimally interpretable negative results, as well as being less relevant to the exposure conditions of the Veterans we seek to model in mice. Single mild TBI exposures are typically reported to develop transient and relatively low levels of Alzheimer's-associated pathology. Conversely, repetitive TBI has gathered significant attention for its strong association with more persistent pathology, such as synapse loss, vasculopathy and Tau burden, which contributes to development of Alzheimer's disease. Studies by others 43 support the notion that significant and long-lasting ApoE-associated phospholipid changes are greater with more severe TBI injuries.
In addition, we have considerable experience at this point in the effects of single versus multiple blast exposures. Overall, we have found that one blast exposure causes modest and short-lived effects on neuropathology and behavior. For example, we found that at 30 days post-exposure a single blast has no residual effect on performance on the rotarod, whereas 3 blast exposure does 38 . More importantly, this is a positive translational implication using this experimental paradigm, in that persistent behavioral and neurological effects are most consistent with findings among Veterans who have experienced repetitive blast-related mTBIs. Therefore, we examined how repetitive mild TBI produces similar Alzheimer's disease-associated changes in manners dependent on ApoE genotypes and synj1 expression.
Our data support specific effects of both TBI and ApoE isoforms in hippocampus, which are consistent with previous studies 43,45 . We have shown that changes in PIP 2 homeostasis and pTau levels are most dramatic in hippocampal regions of ApoE3 and ApoE4 mice, suggesting specific vulnerability of hippocampal regions in response to TBI. Several hypotheses have been proposed in relation to hippocampal vulnerability following TBI such as direct biomechanical forces, excitotoxic neuropathological changes, vascular compromise, metabolic changes, and/or transneuronal degeneration 46,47 . Evidence also suggests that injuries resulting from blast are distinct from those arising from blunt force or other types of TBI 48 . Blast exposure produces intense shock waves that may injure brain tissue by various biophysical means that distort vascular and/or neural tissue, and produce inertial injury from rapid acceleration/deceleration of the brain 49,50 . It is possible that hippocampal brain regions are more susceptible to blast force induced injury due to heightened anatomical and vascular susceptibility 51 . On the other hand, it is possible that hippocampal PIP 2 is among the most sensitive lipid species in the brain, where levels are altered in response to a wide array of central nervous system insults including trauma, ApoE4 genotype 28 , and other factors known to promote neurodegenerative processes. Our results suggest that elevation of brain PIP 2 through reduction of synj1 expression could be a potential therapeutic strategy to prevent the development of neurodegeneration after TBI, and to possibly improve clinical outcomes of those affected by TBI-AD particularly in ApoE4 carriers.
Interestingly, our results suggest differential effects of ApoE genotype on development of Tau hyper-phosphorylation after blast TBI, which could be modulated by brain synj1 expression and PIP 2 levels. We are currently investigating whether down-regulation of synj1 with resultant elevation of brain PIP 2 levels in ApoE4 mice is sufficient to protect brains from development of long-term neurodegenerative processes. The regulation of Tau phosphorylation by PIP 2 /synj1 is at least partially mediated through inhibition of GSK3β (Fig. 6). The crosstalk between PIP 2 and GSK3β has been described previously in insulin signaling pathways by which insulin activates PI-3-kinase that converts PIP 2 to phosphoinositol triphosphate (PIP 3 ) which subsequently activates protein kinase B (PKB) leading to phosphorylation and inhibition of GSK3β 52 . It is possible that reducing synj1 prevents dephosphorylation of PIP 2 which could favor the generation of PIP 3 from PIP 2 and activate downstream signaling by PKB to inhibit GSK3β and reduce Tau phosphorylation.
It should be noted that we did not see any differences in the levels of Aβ 40 and Aβ 42 between blast versus sham conditions in our ApoE4 or ApoE3 mice (see Supplementary Fig. S3A and S3B). It is well established that ApoE plays a critical role in mediating Aβ clearance 53,54 . Overall, 10% of non-ApoE4, 35% of heterozygous ApoE4, and 100% of homozygous ApoE4 cases present with Aβ plaques after TBI 55 . We speculate that the differences in Aβ accumulation and clearance in different ApoE genotypes after TBI may take longer to develop. Alternatively, it is possible that we examined endogenous mouse Aβ levels, which are relatively low. To study amyloid plaque  Table 1. Summary of changes in different ApoE mice in response to blast TBI. Blast induces PIP 2 elevation and synj1 reduction in ApoE3 but not in ApoE4 mice. Blast induces Tau elevation with no changes in p-Tau in ApoE3 mice, whereas blast induces p-Tau elevation with no changes in Tau in ApoE4 mice. In ApoE3 synj1 +/− mice, pTau is reduced after blast, whereas blast-induced pTau elevation is abolished in ApoE4 synj1 +/− mice.
pathologies induced by TBI, we may need to utilize ApoE mice with an AD transgenic background. Moreover, we did not observe any changes in ApoE secretion in ApoE3 or ApoE4 mouse brains after blast (see Supplementary  Fig. S3C), which does not support the hypothesis that differential effects of ApoE genotypes on brain lipids may be mediated through differences in secreted ApoE levels after TBI. It should also be noted that we used all male ApoE mice in our study to avoid any potential gender confounding effects on our results. However, previously published epidemiologic and neuroimaging data suggest that ApoE4 has a stronger effect in promoting AD risk in females than in males 56 . It would be interesting in the future studies to perform comparative evaluations in both male and female mice after TBI exposure and determine any sex-specific impact on blast-induced phospholipid dysregulation development of Tau hyper-phosphorylation in different ApoE groups. One interesting aspect based on our results is that the influence of ApoE4 on responses to TBI may be a loss of reparative function rather than a gain of negative function. We speculate that elevated PIP 2 levels in ApoE3 mice after blast exposure may function as a protective mechanism to activate repair machinery, and ameliorate injury-related neurodegenerative processes like Tau hyper-phosphorylation. In contrast, the ApoE4 genotype blunts any changes in brain PIP 2 and synj1 in response to blast TBI which may contribute to the development of ApoE4-induced Tau hyper-phosphorylation.
It should be noted that reduction in synj1 protein levels in ApoE3 mouse hippocampal regions in response to blast TBI exposure is not likely due to transcriptional regulation because changes in synj1 mRNA levels were not seen (see Supplementary Fig. S2). Since synj1 protein is highly enriched at the synapse 29, 30 , we speculate that these changes in synj1 protein levels post-BOP occur at local synaptic terminals, possibly through post-translational regulation such as accelerated degradation of synj1 proteins in response to blast TBI. We have previously shown that the ApoE4 genotype perturbs neuronal, especially synaptic PIP 2 homeostasis, by altering synj1 expression at synapses, which could contribute to development of ApoE4-induced cognitive deficits and synaptic dysfunction 28 . Interestingly, key neuropathological features of AD development as late complications of TBI include hippocampal neuron loss and synaptic dysfunction [57][58][59] . Therefore, it is possible that TBI may exacerbate ApoE4-associated synaptic PIP 2 dyshomeostasis, which could contribute to TBI-induced neurodegenerative processes.
In recent years, phospholipid profiles in plasma and cerebrospinal fluid samples of TBI patients 60,61 , and in ApoE mouse brains 62,63 have been studied. To our knowledge, no report to date has examined phospholipid profiles of ApoE mouse models after blast TBI. Our studies had a specific focus on low abundance phosphoinositol species such as PIP and PIP 2 28, 32, 33 , and indicated that hippocampal PIP 2 levels were lower ( Fig. 2A) after blast TBI in ApoE4 mouse brain regions, associated with a trend to higher PI levels, as compared to sham controls or to their ApoE3 counterparts after blast exposure. It is possible that more drastic changes in PI/PIP/PIP 2 homeostasis of ApoE4 mouse brains may occur during chronic phases of blast injury. Studies are currently ongoing to investigate the effects of ApoE4 and TBI on brain phospholipid profiles at subacute and chronic stages of TBI.
In summary, our results in this study suggest that ApoE4 genotype specific PIP 2 dyshomeostasis contributes to the development of Tau hyper-phosphorylation after blast TBI exposure, and that elevation of brain PIP 2 levels by reducing synj1 expression may ameliorate TBI-associated Tauopathy in ApoE4 carriers.
Blast overpressure (BOP) exposure. Experimental blast exposure was performed using a pneumatic shock tube designed to recapitulate open-field blast forces caused by explosive detonation as described previously 26,38 . Briefly, all mice (blast-exposed and sham controls) were anesthetized using an isoflurane gas anesthesia system and placed onto a restraint grid in the shock tube in a supine orientation for approximately 3-5 minutes. Blast-exposed mice received BOP exposures (mean peak pressure: 20.0 ± 0.30 pounds per square inch (psi), primary peak duration: 6.0 ± 0.1 milliseconds (ms), impulse: 40.0 ± 10.0 psi · ms); once per day for three consecutive days followed by brain tissue harvest 24 hours after the last blast. Of the 38 blast-exposed mice used in this study only 1 was euthanized for humane reasons prior to study endpoint. All animal procedures were approved by The Institutional Animal Care and Use Committee (IACUC) of JJP VAMC and VAPSHCS and performed in accordance with the guidelines of Association for Assessment and Accreditation of Laboratory Animal Care (AAALAC).

Phospholipid analysis.
Blast or sham exposed mouse brain samples were used for lipid extraction, followed by anion-exchange high pressure liquid chromatography quantification as described previously 33 Message RNA (mRNA) extraction. mRNA was extracted using an RNeasy spin column kit (Qiagen).
Levels of synj1 mRNA were determined by quantitative Real time polymerase chain reaction. Controls included mouse 18S ribosomal subunit and glyceraldehyde-3-phosphate dehydrogenase (GADPH).

Cell lines and immunocytochemical studies. Mouse N2a neuroblastoma cells stably transfected
with cDNA encoding human wildtype Tau441 were maintained in medium containing 50% DMEM and 50% OPTI-MEM, supplemented with 5% fetal bovine serum, antibiotics, and 200 µg/ml G418 (Invitrogen). N2a cells were transfected with synj1 small interfering RNA (siRNA) and maintained for 4-5 days to achieve ~50-80% knockdown of synj1 protein levels as previously described 33 at which time SDS-PAGE and western blotting were performed to determine levels of pTau, total Tau, synj1, holo amyloid precursor protein (APP), β-actin and tubulin. In some experiments, cells transfected with synj1 siRNA were treated with a GSK3 inhibitor (indirubin at 5 µM or kenpaullone at 10 µM; Sigma), or vehicle control (DMSO) for 24 hours before subjected for analysis of pTau, Tau, pGSK3β and GSK3β levels. Alternatively, cells transfected with siRNA were fixed and stained for imaging analysis using a Zeiss LSM510 confocal microscope. Levels of pTau and total Tau were determined by immunostained with AT8 antibodies followed by Texas red anti-mouse immmunoglobulin (IgG), and then sequentially immunostained with Tau5 antibodies followed by Alexa 488 conjugated anti-mouse IgG. In parallel, levels of synj1 were determined by immunostained with synj1 antibody followed by Texas red anti-rabbit immunoglobulin (IgG). The immunofluorescence intensity was quantified after normalized by DAPI signals.
Statistical analysis. Levels of synj1, pTau and total Tau, pGSK3β (inactive and active forms) and total GSK3β were normalized to tubulin levels and expressed as a percentage of control (±SEM). Absolute Aβ 40 , Aβ 42 and ApoE concentrations were quantitatively determined by ELISA (Wako and ABCAM, Inc.) and expressed as a percentage of control (±SEM). Levels of pTau, total Tau and synj1 immunofluorescence signals were normalized to DAPI levels and expressed as a percentage of control (±SEM). Independent-sample t tests were used to determine significant mean differences (the threshold for significance sets at p < 0.05, two-tailed). To determine the overall statistical significance of differences between multiple groups, analysis of variance (ANOVA) was performed followed by post-hoc Tukey tests to determine the significance of differences between pairs of means. All statistical analyses were performed using GraphPad Prism 6.0 (GraphPad Software, Inc.).