Abstract
Defects in endosomal sorting have been implicated in Alzheimerâs disease. Endosomal traffic is largely controlled by phosphatidylinositol-3-phosphate, a phosphoinositide synthesized primarily by lipid kinase Vps34. Here we show that phosphatidylinositol-3-phosphate is selectively deficient in brain tissue from humans with Alzheimerâs disease and Alzheimerâs disease mouse models. Silencing Vps34 causes an enlargement of neuronal endosomes, enhances the amyloidogenic processing of amyloid precursor protein in these organelles and reduces amyloid precursor protein sorting to intraluminal vesicles. This trafficking phenotype is recapitulated by silencing components of the ESCRT (Endosomal Sorting Complex Required for Transport) pathway, including the phosphatidylinositol-3-phosphate effector Hrs and Tsg101. Amyloid precursor protein is ubiquitinated, and interfering with this process by targeted mutagenesis alters sorting of amyloid precursor protein to the intraluminal vesicles of endosomes and enhances amyloid-beta peptide generation. In addition to establishing phosphatidylinositol-3-phosphate deficiency as a contributing factor in Alzheimerâs disease, these results clarify the mechanisms of amyloid precursor protein trafficking through the endosomal system in normal and pathological states.
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Introduction
Alzheimerâs disease (AD) is the most common neurodegenerative disorder and is characterized by a progressive decline in cognitive function1,2,3. Brain regions affected by AD display neuronal loss as well as amyloid plaques and neurofibrillary tangles. Amyloid plaques largely consist of the amyloid-β (Aβ) peptide, which is released by cleavage of amyloid precursor protein (APP) by the β-secretase Beta-site APP cleavage enzyme 1 (BACE1) and γ-secretase. Autosomal dominant mutations in the genes encoding APP and presenilins 1 and 2, the proteases of the γ-secretase complex, lead to rare early-onset familial cases of AD (FAD). In contrast, the majority of AD cases occur later in life (that is, late-onset AD or LOAD) with no precise cause, although an allelic variant of the gene-encoding apolipoprotein E, ApoE4, has been identified as a major risk factor3. Overall, the molecular and cellular mechanisms underlying LOAD are poorly understood.
APP traffics through organelles of the biosynthetic, secretory and endolysosomal pathways, and undergoes differential and compartment-specific processing by α-, β- and γ-secretases1,4. Several converging lines of evidence indicate that the amyloidogenic cleavage of APP occurs predominantly in endosomes4,5. First, the proteolytic activity of BACE1 is optimal at a mildly acidic pH, making the endosomal environment ideal for β-secretase-mediated cleavage of APP6. Second, APP appears to interact with BACE1 primarily in the endocytic pathway4,7,8,9. Third, reducing the access of APP or BACE1 to endosomes by blocking their internalization via clathrin or the small GTPase Arf6, respectively, decreases the amyloidogenic processing of APP4,9,10,11,12,13,14. Fourth, β-cleaved COOH-terminal fragments (CTFs) of APP have been shown to be produced in endosomes15, where they can be further processed by γ-secretase16. Consistent with all these observations, various studies have documented abnormal endosomal morphology and increased endosomal Aβ burden in the brain of individuals with AD, suggesting that endosomal dysfunction may be the key to AD pathogenesis5,17,18,19. Importantly, expression studies have identified LOAD-associated deficiencies in a range of molecules related to the retromer pathway, which regulates the sorting of transmembrane proteins from endosomes to the trans-Golgi network (TGN) or the cell surface20,21,22. These include retromer components (Vps26, Vps29, Vps35) and retromer receptors (SorL1 and SorCS1), which have been implicated in APP sorting and processing1,21,22,23. Finally, neurons derived from the fibroblasts of patients with presenilin mutations24, APP duplications or LOAD25 show an enlargement of early endosomes. Thus, endosomal dysfunction is increasingly viewed as a key cellular phenotype of AD.
A master organizer of endosomal sorting is the signalling phosphoinositide phosphatidylinositol-3-phosphate (PI3P)26,27, which acts by recruiting to endosomal membranes a variety of effectors containing PI3P-binding modules, such as PX (Phox homology) and FYVE (Fab1, YOTB, Vac1, EEA1) domains27. These effectors control trafficking aspects as diverse as the budding of retromer-coated tubules (for example, SNX1,2,6,27), the fusion of endosomes (for example, EEA1) and the ESCRT-dependent intraluminal sorting of ubiquitinated cargos in multivesicular endosomes (for example, Hrs). A major pathway for the synthesis of PI3P involves class III PI 3-kinase Vps34, which phosphorylates PI on the 3â²-position of the inositol ring27. Disrupting the function of Vps34 through various approaches causes pleiotropic defects in endosomal function27. Finally, PI3P controls macroautophagy, and regulators of this degradative pathway such as beclin1 act in part through a modulation of Vps34 and show decreased levels in brain from LOAD patients28,29.
As AD pathogenesis is linked to endosomal anomalies, we hypothesized that a perturbation of PI3P metabolism may occur in brain regions most affected by the disease, and that this disruption could contribute to pathogenic processes. Our study shows a selective PI3P deficiency in the prefrontal cortex (PFC) and entorhinal cortex (ERC) of LOAD-affected individuals as well as in FAD mouse models. We further show that silencing Vps34, and thus reducing PI3P levels, recapitulates several features of AD, including endosomal anomalies and enhanced amyloidogenic processing of APP. In addition, we establish that APP is both ubiquitinated and sorted into endosomal intraluminal vesicles (ILVs) via the PI3P-dependent ESCRT pathway, with major implications for its metabolism. Together, our results identify the PI3PâESCRT pathway as a novel contributing factor in APP biology and potentially, AD pathogenesis.
Results
PI3P levels are decreased in AD-affected brains
To test whether PI3P levels are aberrant in brain regions affected with LOAD, we optimized the high-performance liquid chromatography-mediated separation of PI3P and PI4P and were able to detect and quantify these two lipids using suppressed conductivity30,31 (Supplementary Fig. S1). Brain regions affected in the AD (PFC and ERC) or relatively spared (cerebellum (CRB)) were analysed. Although PI4P levels were unchanged, a deficiency of PI(4,5)P2 was observed in the PFC of AD patients, consistent with our studies showing that the metabolism of this lipid is disrupted by Aβ, particularly at synapses31,32. Importantly, a significant decrease in PI3P was found in PFC (~40%) and, to a lower extent, ERC (~25%), but not in the CRB from AD patients (Fig. 1a). PI3P levels were also measured in the forebrain of three commonly used transgenic mouse models of familial AD (FAD), namely, (i) PSEN1M146V (PS), (ii) the Swedish mutant of APPK670N,M671L (APP) and (iii) PS-APP double transgenic lines33. We found a selective decrease in PI3P levels in each of the mouse model of FAD (that is, an ~25% decrease in the APP and PS1 models and an ~40% decrease in the PS1-APP model; Fig. 1b). Importantly, when the phosphoinositide data was combined with a recent mass spectrometry-based lipidomic analysis of the same samples33 and expressed as a heat map, the PI3P deficiency was the only lipid alteration common to both human and mouse brain affected with AD out of ~330 lipid species and 29 lipid classes (Fig. 1c). These data indicate that the deficiency of PI3P observed in both LOAD- and FAD-affected brains is highly selective.
APP is found on PI3P- and Vps34-positive endosomes
We next investigated the relationship between APP, Vps34 and its product PI3P using confocal microscopy. Attempts to localize endogenous Vps34 were unsuccessful because of the lack of specific antibodies, so HeLa cells were transfected with tagged constructs of Vps34 (Vps34RFP), APP (APPmyc) and a genetically encoded probe for PI3P, that is, the tandem FYVE domain of EEA1 (FYVE-FYVEGFP)34. We found that the majority of APP immunoreactivity localizes to Vps34RFP- and PI3P-positive structures (Supplementary Fig. S2a), consistent with their predominant localization in endosomes. Both Vps34RFP and APPmyc colocalized with endogenous markers of early (EEA1) and, to a lesser extent, late (LAMP1) endosomal compartments (Supplementary Figs S2b and S3a,b). Of note, although ~65% of APP colocalizes with EEA1, a smaller pool (~35%) is found in the late Golgi, as revealed by an anti-giantin staining (Supplementary Fig. S2b), consistent with previous literature (see for instance ref. 35). Not only full-length APP, but also its CTFs were found to be enriched in endosomes obtained by subcellular fractionation of HeLa cell extracts (Supplementary Fig. S3c), suggesting extensive processing of APP in these organelles. Finally, because Vps34 has been implicated in autophagosome formation and maturation29 and that APP processing can also occur in these structures36, we examined the localization of APPRFP and the autophagosomal marker LC3 upon starvation and found no colocalization (Supplementary Fig. S3d), suggesting that APPRFP does not traffic through autophagosomes, at least under these conditions. Together, these data show a tight association between APP and the Vps34- and PI3P-positive endosomes.
Silencing Vps34 enhances amyloidogenic processing of APP
We next investigated the impact of PI3P deficiency on the processing of endogenous APP. Lentiviruses expressing short hairpin RNAs against murine Vps34 (shVps34) or control short hairpin RNAs (shRNAs) (shCTRL) were used to infect mature primary cortical neurons for 7 days. Aβ40 and Aβ42 levels were subsequently analysed in media. In the shVps34 conditions (Fig. 2a), levels of Aβ42 and Aβ40 peptides were each increased by ~2-fold (Fig. 2b), with no change in the Aβ42/Aβ40 ratio (Fig. 2c). Full-length APP showed a trend for an increase (Fig. 2a), although the APP messenger RNA was not upregulated (1.007±0.002 for the shVps34 condition compared with 1.000±0.318 for the shMock condition, in normalized units, P>0.05). Levels of the secreted fragment of APP produced by α-secretase (sAPP-α) were not affected by shVps34, although a trend for an increase in the levels of the secreted fragment of APP produced by β-secretase (sAPP-β) was observed (Fig. 2d). Unfortunately, endogenous APP CTFs were not detectable. Importantly, silencing Vps34 produced an ~45% increase in the size of EEA1-positive endosomal puncta (Fig. 2e), consistent with previous studies37. Together, these data demonstrate that a deficiency of Vps34 causes endosomal abnormalities and enhances the amyloidogenic processing of APP in neurons, establishing a link between PI3P deficiency, endosomal dysfunction and AD pathogenesis.
Silencing Vps34 perturbs APP trafficking
To test whether silencing Vps34 perturbs the endosomal localization of APP, we conducted confocal analyses of primary neurons immunostained with antibodies to the cytodomain of endogenous APP as well as to EEA1 and GM130 to label the endosomal and Golgi compartments, respectively (Fig. 3a,b). Silencing Vps34 produced a major loss of APP fluorescence from EEA1-positive endosomes (Fig. 3c) and an apparent and relative increase in the Golgi compartment, which primarily reflects the loss of endosomal fluorescence (Fig. 3d). As γ-secretase releases the cytodomain of APP in the cytosol, loss of the APP cytodomain immunoreactivity from endosomes may reflect increased processing of APP CTFs by γ-secretase because of Vps34 silencing. To test this, neurons infected with the shCTRL or shVps34 lentiviruses were treated with vehicle or a γ-secretase inhibitor, compound XXI. Although the γ-secretase inhibitor did not affect the localization of APP in shCTRL-treated neurons, it fully restored the normal distribution of APP in shVps34-treated neurons (Fig. 3c,d). These data suggest that the increased processing of APP occurring upon silencing of Vps34 primarily takes place in endosomes (although minor contributions from the Golgi cannot be excluded) and prompted us to investigate the precise role of this enzyme and its product PI3P in the endosomal sorting of APP.
APP is sorted into the ILVs of multivesicular endosomes
A key function of Vps34 and PI3P is to control the sorting of cargos into ILVs of multivesicular endosomes via the ESCRT pathway, which typically ensures their degradation in lysosomes38,39. We thus tested whether aberrant processing of APP caused by Vps34 deficiency reflects a contribution of this pathway. To begin to address this issue, we attempted to visualize intraluminal APP in HeLa cells using confocal microscopy, following expression of APPRFP and the constitutively active form of Rab5, Rab5Q79LGFP, which is locked in its GTP-bound form15,40. This mutant is known to produce an enlargement of endosomes, allowing for the discrimination between the limiting membrane of these organelles and their lumen, which contains the ILVs. Under these conditions, APPRFP, and probably CTFs thereof, were mostly observed within the endosomal lumen, in contrast to endosomal markers known to be associated with the limiting membrane, including Rab5 itself, EEA1, or the retromer component Vps35 (Fig. 4a). Analysis of APPRFP- and Rab5Q79LGFP-positive endosomes showed that ~70% of these structures display luminal fluorescence, probably reflecting an association of APPRFP with ILVs (Fig. 4b). Comparable results were obtained with the CTF-β (data not shown; see also ref. 15). Immunoelectron microscopic (EM) analysis of APPGFP using anti-green fluorescent protein (GFP) antibodies showed gold particles inside multivesicular structures, confirming the light microscopic observations (Supplementary Fig. S4a). Importantly, endogenous APP was also predominantly found (~80%) in the lumen of enlarged endosomes in cultured neurons expressing Rab5Q79LGFP, as shown by the immunostaining of its cytodomain (Fig. 4câf). The luminal localization of the APP cytodomain was also found in naturally occurring enlarged endolysosomal structures, as shown by costainings with anti-EEA1, -Vps35 and -LAMP1 antibodies (Supplementary Fig. S4b). Importantly, immuno-EM labelling of neurons with antibodies to APP cytodomain showed gold particles associated with ILVs of multivesicular endosomes, which were also LAMP1-positive (Fig. 4g).
To determine whether the pool of APP found on ILVs originates from the plasma membrane, we performed an anti-APP ectodomain antibody (22C11) uptake experiment in HeLa cells co-expressing APPRFP and Rab5Q79LGFP (Supplementary Fig. S4c). After antibody binding at 4â°C and 3âh of treatment with protein synthesis inhibitor (cycloheximide), the 22C11 immunoreactivity was mostly found at the plasma membrane, as shown by the punctate staining at the basal plane of the cells (Supplementary Fig. S4c). After a 15-min chase period, the 22C11 immunoreactivity was detected primarily on the limiting membrane of endosomes (Supplementary Fig. S4d). After 30âmin, the APPRFP fluorescence (labelling the COOH-terminus) and the 22C11 fluorescence (labelling the NH2-terminus) converged in part in the lumen of endosomes (Supplementary Fig. S4d). Thus, the pool of APP that is sorted into the ILVs originates from the plasma membrane and is endocytic in nature (although a pool of cell surface-derived APP also traffics to the TGN via endosomes; see for instance, ref. 41).
Vps34 controls the intraluminal sorting of APP in endosomes
To test whether targeting of APP to ILVs is PI3P dependent, we analysed the acute effect of wortmannin, a chemical inhibitor of class I and class III PI 3-kinases. To monitor PI3P levels, HeLa cells were transfected with FYVE-FYVEGFP together with APPRFP and subjected to a 30-min treatment with 100ânM wortmannin. As expected, the drug dramatically decreased the association of FYVE-FYVEGFP with endosomes, labelled with EEA1 and Vps35 (Supplementary Fig. S5a). Although the localization of retromer was perturbed by this treatment, no marked phenotype was observed for APPRFP (Supplementary Fig. S5a). However, when this experiment was repeated after Rab5Q79LGFP expression to visualize the endosomal lumen (Supplementary Fig. S5b), APPRFP was relocalized from the lumen of giant endosomes to their limiting membrane. The ratio of internal/peripheral APPRFP fluorescence in giant endosomes was quantified following wortmannin treatment in a time course-dependent fashion. APPRFP relocalization occurred very rapidly, as early as 10âmin after the beginning of the treatment (Supplementary Fig. S5b). HeLa cells were also transfected with short interfering RNAs (siRNAs)-targeting Vps34 (siVps34) or control siRNAs (MOCK), grown for 72âh, and were then transfected with APPRFP and Rab5Q79LGFP. The potent inhibition of Vps34 protein expression was confirmed by immunoblotting (Fig. 4h) and the reduction in the levels of PI3P was confirmed with a microscopic analysis of the fluorescent pattern of the FYVE-FYVE probe, either used as a glutathione S-transferase (GST) fusion for the staining of fixed cells34 (Supplementary Fig. S6a,b) or as a genetically encoded GFP fusion (Supplementary Fig. S6c). In addition, the silencing of Vps34 produced a significant loss of membrane association of retromer component Vps35, consistent with reduced levels of PI3P (Supplementary Fig. S6d). As observed with wortmannin, APPRFP was mostly localized to the limiting membrane of endosomes upon siVps34 treatment (Fig. 4i; quantification shown in Supplementary Fig. S7c), thus confirming the essential role of Vps34-mediated PI3P synthesis in the ILV sorting of APP.
The targeting of APP to ILVs is ESCRT dependent
A key player initiating the ESCRT cascade is Hrs, also known as an ESCRT0 component, which binds PI3P via a FYVE domain and ubiquitinated cargoes via a ubiquitin-interacting motif38,39. To investigate whether Hrs, like Vps34, has a role in the intraluminal sorting of APP, HeLa cells were transfected with siRNAs-targeting Hrs. Silencing Hrs (Supplementary Fig. S7a) produced an accumulation of APPRFP fluorescence on the limiting membrane of endosomes similar to siVps34 (Supplementary Fig. S7b,c). Comparable results were obtained upon silencing of ESCRT-I subunit Tsg101 and, to a lesser extent, SNX3, which has been shown to mediate the formation of ILVs in multivesicular endosomes42 (Supplementary Fig. S7). In contrast, silencing of beclin1, a major regulator of Vps34 in autophagy, did not affect the intraendosomal localization of APP (Supplementary Fig. S7). Together, our data demonstrate that the Vps34/PI3P/ESCRT pathway controls the intraluminal sorting of APP.
The targeting of APP to ILVs depends on its ubiquitination
The signal triggering ESCRT-mediated internalization of cargoes from the limiting membrane of endosomes to ILV is ubiquitination of their cytodomain on lysine residues, either with monoubiquitins or with lysine-63-linked polyubiquitin chains39,43. We therefore tested whether endogenous APP is ubiquitinated in the brain. APP was immunoprecipitated from mouse brain extracts using anti-APP cytodomain antibodies and bound material was analysed by immunoblotting using anti-APP and -ubiquitin antibodies (Fig. 5a). Ubiquitin immunoreactivity was found to comigrate with APP, but not control eluate, indicating that endogenous APP is indeed ubiquitinated.
To determine the main ubiquitination sites relevant for ILV sorting, HeLa cells were transfected with APPGFP and lysates were subjected to immunoprecipitation (IP) using anti-GFP antibodies. Immunoblotting of the immunoprecipitated material with an anti-ubiquitin antibody revealed that APPGFP is also ubiquitinated (Fig. 5b), similar to endogenous APP. A stretch of three lysines located in the cytoplasmic juxtamembrane region on positions 724â726 of human APP were good candidate ubiquitination sites (green residues in Fig. 5c), based on evidence from others indicating that lysines in the juxtamembrane region of proteins can be ubiquitinated44 and the recent finding that lysine 726 ubiquitination is relevant for proteasomal degradation of APP under conditions of overexpression of F box factor FBL245. To determine the role of these lysines, an APP mutant in which lysines 724â726 were substituted with arginines (referred to as APP3RGFP) was expressed in HeLa cells and showed a dramatic reduction in the ubiquitin signal relative to the control (Fig. 5d,e).
To test whether ubiquitination of these lysine residues is critical for ILV sorting, we expressed APP3RGFP and Rab5Q79Lmyc and examined the targeting of mutant APP to ILVs in giant endosomes. We found that APP3RGFP displayed a predominant association with the limiting membrane of endosomes at the expense of luminal localization (Fig. 6a,b). When expressed in hippocampal neurons alongside Rab5Q79LGFP, APP3R also exhibited decreased targeting to the lumen of enlarged endosomes relative to APPWT (Fig. 6c,d), although the missorting was not as striking as that observed in HeLa cells. Importantly, treatment with γ-secretase inhibitor (compound XXI) was applied in these experiments to enhance and better visualize the endosomal pool of APP, which otherwise undergoes significant processing by the secretase (see below). Together, our results demonstrate that ubiquitination of the cytodomain of APP on one or more of lysines 724â726 is important for the intraluminal sorting of APP through the Vps34/PI3P/ESCRT pathway.
The APP3R mutant shows altered sorting in neurons
Silencing Vps34 produced a dramatic loss of endogenous APP fluorescence in neuronal endosomes, a phenotype rescued by γ-secretase inhibitor treatment. If a key function of PI3P is to promote ILV sorting of APP into multivesicular endosomes through ESCRT, the traffic pattern of APP3R may phenocopy that of wild-type APP obtained upon Vps34 silencing. As hypothesized, the association of APP3R with neuronal endosomes positive for EEA1 (Fig. 7) or Vps35/retromer (Supplementary Fig. S8) was dramatically reduced, whereas that with the GM130-positive Golgi compartment was slightly enhanced (Supplementary Fig. S9) relative to APPWT. As seen with the Vps34 knockdown, treatment of neurons with the γ-secretase inhibitor restored the normal distribution of APP3R (Fig. 7, Supplementary Figs S8 and S9), although within endosomes, the APP3R mutant was preferentially localized on the limiting membrane (Fig. 6c,d).
Inhibiting ILV sorting of APP enhances Aβ levels
Our data suggest that APP3R is more extensively processed through the amyloidogenic pathway in endosomes, similar to endogenous APP in the Vps34 knockdown. We thus examined the impact of the 3R mutation on the metabolism of APP expressed exogenously with lentivirus in primary neurons (in the absence of Rab5Q79L expression). Constructs were comparably expressed, based on the lack of differences found for FL-APPWT and APP3R (Fig. 8a). Similar to the Vps34 knockdown, sAPP-α levels were unchanged (Fig. 8b), whereas a trend for an increase in sAPP-β was found for the APP3R mutant (Fig. 8c). Consistent with this trend, expression of APP3R caused an ~50% increase in Aβ40, although surprisingly Aβ42 levels were unchanged (Fig. 8d). Together, these data indicate that mutations that decrease the intraluminal sorting of APP in endosomes promote the generation of Aβ.
Discussion
Cell biological observations combined with results from expression and genetic profiling have suggested that defects in endosomal sorting and trafficking have a pathogenic role in AD1,4,5. Together with studies suggesting that amyloidogenic processing of APP predominantly occurs in endosomes, these reports indicate that these organelles are critical players in AD pathogenesis. Our study strongly supports this hypothesis by identifying a molecular defect, namely, a selective deficiency in PI3P, in affected brain regions from patients with LOAD as well as in the forebrain of mouse models of FAD. Remarkably, the deficiency of PI3P is the only lipid change common to both human and mouse brains affected by AD out of ~330 lipid species examined. As the PI3P deficiency does not correlate with the extent of neuronal death or AD pathology in AD-affected regions, it is unlikely to merely stem from neurodegeneration, although it may also reflect changes occurring in glial cells.
PI3P controls fundamental aspects of endosomal membrane dynamics26,27,39. In addition, PI3P regulates macroautophagy, which mediates via an interplay with endolysosomal compartments the clearance of defective organelles and intracellular aggregates, and has also been implicated in AD29,36. Although a deficiency of PI3P in AD may theoretically cause any of the abovementioned PI3P-dependent processes to function suboptimally, our study provides strong evidence that it affects endosome dynamics as well as the sorting and processing of APP, all of which are believed to have a role in AD pathogenesis. Indeed, modelling the PI3P deficiency by silencing Vps34, the main source of PI3P, produces endosomal enlargement, a perturbation of APP trafficking as well as increased production of Aβ. Interestingly, these phenotypes are partially shared in common by instances in which Rab5 is overexpressed5,12. However, the link between PI3P deficiency and Rab5 hyperactivation identified in LOAD is unclear, as Rab5 is known to activate Vps3446. We speculate that Rab5 hyperactivation may be compensating for the PI3P deficiency, although these phenomena may not be directly related.
Our cell culture studies indicate that APP is sorted and trafficked via ESCRT, and together with previous studies implicating the retromer pathway suggest a general mechanism for how PI3P deficiency observed in the disease can lead to APP missorting. In common with recent studies45,47, we found that APP is ubiquitinated on cytoplasmic lysine residues. However, extending on these observations, we found that ubiquitination, which we document also for the endogenous protein in the brain, mediates targeting of an endocytic pool of APP to ILVs via ESCRT, rather than to proteasomal degradation. Indeed, silencing key ESCRT components, such as Hrs and Tsg101, leads to an accumulation of APP on the limiting membrane of endosomes in HeLa cells, which express low levels of BACE1. Furthermore, substituting the lysine residues with arginines dramatically impairs ubiquitination of APP and also causes a shift of its localization to the limiting membrane of endosomes. Remarkably, ILV missorting correlates with elevation of Aβ secretion in neurons, although the pattern of secreted Aβ species varies depending on the specific manipulation; while Vps34 silencing causes an increase in both Aβ40 and 42, the APP3R mutant causes a differential elevation in Aβ40. This is consistent with the idea that the PI3P deficiency may also cause defects in APP trafficking and processing independently of those produced by reduced ESCRT-dependent sorting into ILV. In this respect, a key effect of PI3P deficiency may be to cause a dysfunction of retromer, whose knockdown phenocopies the increase in Aβ40 and 42 levels in neurons23. Interestingly, the selective increase in Aβ40 observed with the APP3R mutant may paradoxically confer protection against amyloidogenesis in vivo, based on the ability of this shorter peptide to counteract the aggregate-inducing property of Aβ42 (ref. 48). Regardless, our data suggest that Aβ generation predominantly occurs on the limiting membrane of neuronal endosomes, perhaps reflecting the presence there of highly active pools of BACE1 and/or presenilin. This is supported by our experiments showing that γ-secretase inhibitors restore an endosomal pool of APP that is otherwise drastically diminished by the silencing of Vps34 or the 3R mutation of APP. We note that some studies in non-neuronal cell lines have reported experimental manipulations that enhance the Golgi association of APP (at the expense of endosomes) as well as its amyloidogenic processing (see for instance, ref. 35). The use of γ-secretase inhibitors in those instances should help to resolve whether the loss of endosomal pool reflects enhanced processing in those organelles rather than a bona fide accumulation of APP in the Golgi compartment. We also note that a recent APP overexpression study conducted in non-neuronal cells reported that silencing various âearlyâ ESCRT components (for example, Hrs, Tsg101) causes a retention of APP in endosomes and a decrease of Aβ40 release. Conversely, silencing âlateâ ESCRT components (for example, CHMP6, Vps4) causes enhanced targeting of APP to the TGN and an increase in Aβ40 release41. Future work should address whether these experimental manipulations produce similar results in neurons.
Overall, our study and work from others suggest that the pathogenesis of AD, and LOAD in particular, is linked to the dysfunction of a number of genes involved in trafficking pathways identified in yeast as âvacuolar protein sortingâ (for example, Vps34 and beclin1/Vps30 (PI3K), Hrs/Vps27 and Tsg101/Vps23 (ESCRT), Vps26/29/35 (retromer), SorLa/SorCs1 (Vps10-like proteins))22,28,49. The identification of PI3P deficiency in affected brain regions of individuals with LOAD not only provides a potential mechanism explaining AD-associated endosomal anomalies and aberrant APP metabolism but also defects in autophagy28,36, which may reduce clearance of tau aggregates50. The precise genetic and/or environmental factors responsible for PI3P deficiency in FAD and LOAD are unknown, although we speculate they may affect the function of Vps34 complexes, perhaps in combination with that of alternate pathways controlling PI3P levels.
Finally, besides clarifying basic mechanisms of APP biology, our results may have clinical implications. In particular, our data suggest that as an enzyme that regulates PI3P levels, Vps34, as well as other lipid enzymes controlling PI3P levels through dephosphorylation mechanisms (for example, myotubularins) may be novel targets for drug discovery in attempting to improve APP missorting characteristic of LOAD. In this respect, targeting the metabolism of phosphoinositides, and more generally phospholipids, is emerging as a promising new avenue for AD therapy31,32,51,52,53. As recent studies have implicated defects either in lipid metabolism or in endosomal sorting in AD, our work establishes an important link between these two intracellular processes, and this converging view also provides a focus for developing novel therapeutic targets and agents.
Methods
Human and mouse brain tissue
Frozen post-mortem brain tissue samples were obtained from the New York Brain Bank at Columbia University Medical Center, and are described previously33. Three different brain regions were sampled: PFC, ERC and CRB. The diagnostic criteria for AD were based on the presence of neurofibrillary tangles, senile plaques and dementia. Wild-type, PS1, APP and PS1-APP mice, which were aged between 9 and 11.5 months, were described previously33. All mice were killed by cervical dislocation, the forebrain was dissected immediately and frozen in liquid nitrogen before storage at â80°C.
Cell transfection and lentivirus production
HeLa and HEK-293T cells were grown at 37â°C in a 5% CO2 incubator in MEM and DMEM, respectively (Invitrogen). HeLa cells were transiently transfected using Fugene-6 (Roche Diagnostics) or Lipofectamine 2000 (Invitrogen) for complementary DNA (from 24 to 48âh) and siRNA (72âh), respectively. Hippocampal cultures were obtained from P0 mice. Neurons were plated on poly-L-lysine-coated coverslips or six-well plates, and were incubated with Neurobasal media (Invitrogen) with 10% fetal bovine serum. After 5âh, neurons were transferred into serum-free medium supplemented with B27 (Invitrogen) and cultured for 9â12 days in vitro (DIV). In some experiments, neurons cultured for 8â9 days were transfected for 60âmin with 2âμl of Lipofectamine 2000 combined with 1âμg of DNA, washed and incubated for 24âh (APPWTGFP, APP3RGFP) or 4 days (shRNA) before immunofluorescence analysis. In other experiments, neurons were infected with shRNA lentivirus after 7 days in culture, and were cultured up to 14 days. Lentiviruses were generated by transfecting lentiviral vectors (APPWTGFP, APP3RGFP) or a mix of equal amounts of shVPS34-1 and shVPS34-2 into HEK-293T cells using lipofectamine LTX (Invitrogen). A pPACK-H1 packaging mix (System Biosciences) was added to the transfection reagents according to the manufacturerâs instructions. The medium was collected 48 and 72âh after transfection, passed through a 45-nm filter and applied at 1:4 ratio to media.
Antibodies and reagents
Antibodies were obtained from the following sources: rabbit polyclonal antibodies to Vps34 (Cell Signaling), APP (Calbiochem), sAPP-α and giantin (Covance), APP C-terminal fragments (APP-Cter; Invitrogen), LAMP1 and SNX3 (Abcam), red fluorescent protein (Rockland) and Hrs (a kind gift from G. Cesareni, University of Tor Vergata, Rome, Italy), a goat polyclonal antibody to Vps35 (Abcam), mouse monoclonal antibodies (mAbs) to actin (Novus), Tsg101 (Abcam), beta amyloid 1-42 12F4 (Covance), sAPP-α clone m3.2 (a kind gift from P. Matthews, Nathan Kline Institute, NY, USA), APP N-terminus A4 22C11 (Millipore), Rab5, Rab7 and Synaptotagmin1 (Synaptic Systems), GAPDH (EnCor Biotech), GFP (Roche Diagnostics), Myc 9E10 (Invitrogen), EEA1 and GM130 (BD Transduction Laboratories), ubiquitin P4D1 (Santa Cruz) and LC3 4E12 (MBL), and a rat polyclonal antibody to LAMP1 (BD Pharmingen). Peroxidase-conjugated secondary antibodies were from Bio-Rad and fluorescent secondary antibodies (Alexa and Cyanin) were from Jackson Immunoresearch and Invitrogen. PI3-kinase activity was blocked with 100ânM wortmannin (Invitrogen). To prevent autophagosome clearance, cells were treated with 50ânM bafilomycin A1 (Waco) for 1âh. γ-secretase was blocked for 24âh with 10âμM γ-secretase Inhibitor XXI, Compound E (both from Calbiochem).
Plasmids and RNA interference
Plasmids were kindly provided by the following sources: human Rab5Q79LGFP (M. Zerial, Dresden, Germany), Rab5Q79Lmyc (J. Gruenberg, Geneva, Switzerland), FYVE-FYVEGST and FYVE-FYVEGFP (H. Stenmark, Oslo, Norway), human Vps34RFP (N. Ktistakis, Cambridge, UK) and monomeric RFP (Roger Tsien, UCSD, California, USA). The APPGFP and APPMYC plasmids were constructed by excising the APP cDNA from APPRFP (derived from NM_201414.2) with SalI/HindIII, and subcloning it into pEGFP-N3 (Clonetech) and pCMV5A (Stratagene). APP3RGFP was generated by quick mutagenesis on APPGFP with the following primer and its antisense: 5â²-CACCTTGGTGATGCTGAgGAgGAgACAGTACACATCCATTC-3â². Human APPGFP and APP3RGFP lentiviruses were constructed by excising APPGFP and APP3RGFP, respectively, from pEGFP-N3 with NheI/NotI and ligating the cDNAs into pCDH-CMV-MCSr (System Biosciences). Human APPmCherry and APP3RmCherry were constructed by SalI/NotI replacement of GFP in APPGFP, and APP3RGFP with a mCherry including SalI/NotI overhangs. For RNA interference in HeLa cells, we used an equal mix of the following predesigned human siRNA sequences (Qiagen): Vps34 (SI00040950/SI00040971), Hrs (SI00288239/SI02659650), Tsg101 (SI02655184/SI02664522), SNX3 (S104309704/S103150280) and Beclin1 (S100055573/S100055580). Mouse Vps34-shRNA lentivectors were generated with the pSIH-H1 shRNA vector from System Biosciences. The control was pSIH1-H1-copGFP Luciferase shRNA, and the Vps34-shRNA targets were as follow: mVps34-1 shRNA, 5â²-GTGGAGAGCAAACACCACAAGCTTGCTCG-3â²; mVps34-2 shRNA, 5â²-CCTGACCTGCCCAGGAATGCCCAAGTGGC-3â².
Lipid analysis
Phosphoinositide-enriched lipid fractions were extracted from frozen brain tissue samples (80â120âmg), deacylated and analysed by anion-exchange high-performance liquid chromatography with suppressed conductivity detection as described 30,31 but with slight modification to the KOH gradient profile to better resolve PI4P and PI3P elution (Supplementary Fig. S1). Specifically, the elution was carried out in five stages: (1) a gradient change of 1.5â4âmM KOH from the injection time to 7âmin after injection, (2) 4â16âmM from 7â12âmin after injection, (3) 16â25.75âmM from 12â35âmin after injection, (4) 25.75â86âmM from 35â60âmin after injection and (5) 5âmin isoelectric elution with 86âmM KOH. A portion of the same tissues used above was subjected to lipidomics analysis using LCâMS, as previously described 33.
Fluorescence microscopy
Cells were fixed with 4% paraformaldehyde for 30âmin and permeabilized with 0.05% saponin together with primary antibodies in PBS supplemented with 5% fetal calf serum. For the anti-APP-Cter staining, neurons were permeabilized with 0.2% Triton X-100 for 10âmin. For other stainings, neurons were permeabilized with 0.01% digitonin. For the labelling of PI3P with FYVE-FYVEGST, cells were fixed and incubated for 1âh with purified FYVE-FYVEGST recombinant protein (20âμgâmlâ1 final concentration), washed with PBS and labelled with a FITC-conjugated anti-GST antibody (Abcam). Coverslips were mounted in mowiol or DAPI-mowiol (Sigma) or ProLong Gold (Invitrogen). Images were acquired by confocal laser scanning microscopy (Zeiss LSM 700 and 510) and analysed with Zeiss Zen and imageJ softwares.
Ultracryomicrotomy and immunogold labelling
Hippocampal neurons at 15 DIV were fixed with a mixture of 2% (wt/vol) PFA and 0.125% (wt/vol) glutaraldehyde in 0.1âM PBS, pH 7.4. Cell pellets were washed with PBS, embedded in 10% (wt/vol) gelatin and infused in 2.3âM sucrose 54. Mounted gelatin blocks were frozen in liquid nitrogen and ultrathin sections were prepared with an EM UC6 ultracryomicrotome (Leica). Ultrathin cryosections were collected with 2% (vol/vol) methylcellulose, 2.3âM sucrose and single or double immunogold labelled with antibodies and protein A coupled to 5 or 10ânm gold (PAG5 and PAG10; obtained from the Cell Microscopy Center of Utrecht University Hospital, Netherlands), as reported previously 54. Sections were observed under Philips CM-12 electron microscope (FEI; Eindhoven, The Netherlands) and photographed with a Gatan (4âk à 2.7âk) digital camera (Gatan, Inc., Pleasanton, CA, USA).
Protein biochemistry and immunoblotting
Total endosome fractions, comprising both early and late endosomal membranes, were generated as previously described 55. To detect ubiquitinated APP, HeLa cells were transiently transfected with human APPWTGFP or APP3RGFP and then lysed for 30âmin at 4â°C in IP buffer (0.5% NP-40, 500âmM TrisâHCl, pH 7.4, 20âmM EDTA, 10âmM NaF, 30âmM sodium pyrophosphate decahydrate, 2âmM benzamidine, 1âmM phenylmethanesulfonylfluoride, 1âmM N-ethyl-maleimide and a cocktail of protease inhibitors), centrifuged for 3âmin at 2000âg, and supernatants were precleared with protein G-coupled beads (Invitrogen) before an incubation for 2âh at 4â°C with protein G-coupled beads and 2âμg anti-GFP mAb. For IP using mouse brain, tissue was collected and homogenized on ice with a Dounce homogenizer in IP buffer. After 30âmin at 4â°C, homogenates were centrifugated at 13000âg for 5âmin. After preclearing, 500âμl of lysate were incubated for 2âh at 4â°C with protein G-coupled beads and 10âμg anti-APP-Cter polyclonal antibody or 3âμg anti-GFP mAb (as a control). After washing the beads with IP buffer, proteins were eluated, separated on a BisâTris gel (Invitrogen) and transferred by a semi-dry method on a nitrocellulose membrane. The latter was then probed sequentially with an anti-ubiquitin and anti-GFP antibody (after stripping). Quantification was made with Image J or the LAS4000 softwares. For all other immunoblots, cells were lysed for 30âmin at 4â°C in RIPA buffer with protease and phosphatase inhibitor cocktails, centrifuged for 15âmin at 13000âg, and proteins in the supernatant were processed for SDSâPAGE and immunoblotting. Please see Supplementary Fig. S10 for full scans of imunoblots.
Enzyme-linked immunosorbent assays
Murine Aβ1-40 and Aβ1-42 were measured from the medium of hippocampal cultures infected with a mix of shVps34 lentiviruses to monitor endogenous APP processing, and human Aβ1-40, Aβ1-42 and sAPP-β were quantified from the media of neurons infected with human APP-WT-GFP or APP3R-GFP lentiviruses. The enzyme-linked immunosorbent assay kits were from Invitrogen (Aβ) and Covance (sAPP-β), and the experiments were performed according to the manufacturerâs instructions. Briefly, neurons were infected 7 days after plating, and the medium was collected 7 days after infection and supplemented with 0.25âmgâmlâ1 Pefabloc SC 4-(2-Aminoethyl) benzenesulfonyl fluoride hydrochloride (Fluka Analytical). Each sample was then measured in duplicates.
Statistics
Statistical analysis was performed using the Studentâs t-test (for the comparison of two averages), the one-sample t-test (for the comparison of one average to a normalized value where variability is lost), the one-way analysis of variance test with post hoc least significant difference or Tukey test (for the comparison of three or more averages). In Fig. 1a, a one-tailed Studentâs t-test was exceptionally used for the PI(4,5)P2 data, based on predictions from previously published work showing Aβ disrupts the metabolism of this lipid 31.
Additional information
How to cite this article: Morel, E. et al. Phosphatidylinositol-3-phosphate regulates sorting and processing of amyloid precursor protein through the endosomal system. Nat. Commun. 4:3250 doi: 10.1038/ncomms3250 (2013).
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Acknowledgements
We are grateful to Etty Cortes at the New York Brain Bank for human brain preparation, Huasong Tian for generating the APPRFP construct, Akhil Bhalla for the neuronal culture and lentivirus production protocols, Laurence Abrami and Gisou Van Der Goot for the ubiquitin identification on transmembrane proteins protocol and Harald Stenmark for the kind gift of FYVE-FYVEGST probe. We also acknowledge the EM facilities at Yale University (Christhof Rahner, Morven Graham and Kim Zichichi) and at the New York Structural Biology Center, and we thank Kelly McGrath for critical reading of the manuscript. This work was supported by grants from the National Institute of HealthâR01 NS056049 (G.D.P.), P50 AG008702 (Shelanski, projects from G.D.P., B.D.M and C.D.A.), R01 AG025161 (S.A.S.) and 2T32MH015174-35 (Z.L.), the Alzheimerâs Association (S.A.S. and G.D.P.), the Broitman Foundation (S.A.S.) and a fellowship from the Swiss National Science FoundationâPA00P3_124149 (Z.C.).
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E.M. and Z.C. designed, coordinated and carried out the bulk of the experiments. Z.M.L. carried out immunofluorescence experiments in neurons. R.B.C. designed and carried out the lipid biochemistry. R.L.W., K.S.P. and C.V. helped with the characterization of APP metabolites in neurons. C.D.A. helped with the preliminary protein analyses on human brains and with the LC3 immunofluorescence experiments. S.S. performed the immunoelectron microscopy experiments in neurons. E.M., Z.C., R.B.C., Z.M.L., R.L.W., C.V. and B.D.M. edited the manuscript. E.M., Z.C., R.B.C., B.D.M., S.A.S. and G.D.P. designed research. E.M., Z.C., S.A.S. and G.D.P. wrote the manuscript. G.D.P. and S.A.S. conceived the project, co-supervised the study and are co-senior authors.
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Morel, E., Chamoun, Z., Lasiecka, Z. et al. Phosphatidylinositol-3-phosphate regulates sorting and processing of amyloid precursor protein through the endosomal system. Nat Commun 4, 2250 (2013). https://doi.org/10.1038/ncomms3250
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DOI: https://doi.org/10.1038/ncomms3250
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