Increased Neuronal Endocytosis and Protease Delivery to Early Endosomes in Sporadic Alzheimer's Disease: Neuropathologic Evidence for a Mechanism of Increased beta -Amyloidogenesis

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Volume 17, Number 16, Issue of August 15, 1997 pp. 6142-6151
Copyright ©1997 Society for Neuroscience

Increased Neuronal Endocytosis and Protease Delivery to Early Endosomes in Sporadic Alzheimer's Disease: Neuropathologic Evidence for a Mechanism of Increased $beta$ -Amyloidogenesis

Anne M. Cataldo¹^,², Jody L. Barnett¹, Cristiana Pieroni¹, and Ralph A. Nixon¹^,²^,³
¹ Laboratories for Molecular Neuroscience, McLean Hospital, Belmont, Massachusetts 02178, ² Departments of Psychiatry and Neuropathology, and ³ Program in Neuroscience, Harvard Medical School, Belmont, Massachusetts 02178

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

The early endosome is the first vacuolar compartment along the endocytic pathway. It is the site of internalization and initialprocessing of amyloid precursor protein (APP) and apolipoproteinE (ApoE), two proteins of etiological importance in Alzheimer'sdisease, and a putative site of $beta$ -amyloid peptide (A $beta$ ) formation.Here, we identify early endosomes in human pyramidal neurons,using specific compartmental markers and morphometry, and showthat in Alzheimer's disease individual endosomes display up to32-fold larger volumes than the normal average. Endosomal enlargementcontributed to an average 2.5-fold larger total endosomal volumeper neuron, implying a marked increase in endocytic activity.Endosomal alterations were evident in most pyramidal neurons inAlzheimer brain, detectable at early stages of the disease butabsent in several other neurodegenerative disorders examined.In addition, mature and proenzyme forms of the proteases cathepsinB and cathepsin D, a candidate APP secretase, were identifiedin most early endosomes in Alzheimer brains but were detectablein only a minor proportion of endosomes in normal brain. Expressionof the cation-dependent 46 kDa mannose 6-phosphate receptor waselevated in pyramidal neurons of Alzheimer brains, which couldbe a possible basis for the altered cathepsin trafficking pattern.Enhanced endocytic activity, coupled with increased traffickingto endosomes of proteases, which may have the ability under pathologicalconditions to generate A $beta$ , constitutes a potential mechanism bywhich $beta$ -amyloidogenesis may become accelerated in sporadic ADand also be subject to influences by ApoE.
Key words: endocytosis; early endosome; protease; neurodegenerative disease; $beta$ -amyloidogenesis; lysosomal trafficking

INTRODUCTION

The neuronal endocytic pathway is a finely controlled and efficient intracellular trafficking system for internalizing andprocessing extracellular nutrients and trophic factors, for recyclingor catabolizing receptors and other integral membrane proteinsafter neurotransmitter release, and for directing informationto intracellular biosynthetic pathways. Endocytosis enables cellsto modify or degrade molecules within a continuum of morphologicallyand biochemically distinct vacuolar compartments. These compartmentsinclude early and late endosomes and lysosomes, which have differentcapabilities for processing substrates by proteolysis (Dimentet al., 1989; Casciola-Rosen and Hubbard, 1991; Berg et al., 1995).A variety of acid hydrolases is packaged within the Golgi apparatusand then trafficked by shuttle vesicles to these compartmentsunder the regulation of cation-dependent and cation-independentmannose 6-phosphate receptors (MP-R). The turnover of endocytosedmaterials originally was thought to be limited to lysosomes, butit is known now that in certain non-neuronal cells some acid proteasesmay be present in endosomes and can modify endocytosed proteins(Diment et al., 1989; Casciola-Rosen and Hubbard, 1991; Berg etal., 1995).

Interest in the neuronal endosomal-lysosomal (E-L) system and in the processing enzymes residing in its acidic compartmentshas grown recently because of the pathophysiological importanceof this system in Alzheimer's disease (AD). Proteins closely linkedto AD pathogenesis, such as altered amyloid precursor protein(APP), the $beta$ -amyloid protein (A $beta$ ), and apolipoprotein E (ApoE),are internalized and processed within the E-L system. The E-Lsystem, therefore, represents a shared cellular pathway in whichthese etiological influences may converge. Our previous studies(Nixon and Cataldo, 1993; Cataldo et al., 1995, 1996) of AD brainrevealed a marked upregulation of lysosomal activity at an earlystage in the metabolic compromise of neurons within affected regions,including marked upregulation of acid hydrolase synthesis andtwo- to sevenfold increases in the numbers of lysosomes. The accumulationof various acid hydrolases within late endosomes and lysosomes,including proteases with potential APP secretase activities suchas cathepsins B and D (Tagawa et al., 1991; Nixon and Cataldo,1993; Dreyer et al., 1994; Cataldo et al., 1995, 1996; Evin etal., 1995), the release of these enzymes after neuronal lysis(Nixon and Cataldo, 1993; Cataldo et al., 1994, 1995, 1996), andtheir persistence extracellularly in association with A $beta$ deposits(Nixon and Cataldo, 1993; Cataldo et al., 1994, 1995, 1996), hasbeen observed only in disorders in which A $beta$ is accumulated, suggestinga link between E-L system abnormalities and $beta$ -amyloidogenesis.

In this study we used immunocytochemical and morphometric approaches to identify neuronal early endosomes for the first timein situ. We used an antibody to rab5, the monomeric GTP-bindingprotein that modulates transport kinetics between the plasma membraneand early endosomes (Gorvel et al., 1991; Bucci et al., 1992;de Hoop et al., 1994), to label specifically the early endosomes.In cultured non-neuronal and neuronal cells, rab5 is localizedselectively to early endosomes and, to a lesser extent, clathrin-coatedvesicles and the plasmalemma. Immunocytochemical markers of lateendosomes (cation-independent 215 kDa MP-R) and lysosomes [acidhydrolases and lysosome-associated membrane proteins (LAMPs)]used in our previous studies (Cataldo et al., 1996), as well ascellular size and location criteria, enabled us to distinguishamong the major acidic compartments that make up the E-L system.In doing this, we identified striking alterations in the sizeand volume of early endosomal compartments in neurons of affectedregions of AD brains, as well as in the localization pattern ofacid hydrolases, in both their pro- and mature forms within thesesame compartments. These results, which support upregulation ofendocytosis and increased hydrolase delivery to early endosomesin neurons of vulnerable regions of AD brains, suggest how $beta$ -amyloidogenesismay be initiated in the early endocytic pathway and how ApoE mayexert its influence on AD pathogenesis.

MATERIALS AND METHODS
Tissue. Postmortem brain tissue from nine individuals with the probable clinical diagnosis of AD and eight age-matched 62-to 78-year-old neurologically normal controls were used in thisstudy. Tissue was procured from the Harvard Brain Tissue ResourceCenter at McLean Hospital (Belmont, MA) and the NeuropathologyCore Facility of the Massachusetts Alzheimer's Disease ResearchCenter (Massachusetts General Hospital, Boston, MA). Control brainsexhibited minimal histopathological changes (0-3 neuritic plaques/lowpower field; 0-6 neurofibrillary tangles/low power field). Thepresence and magnitude of neurodegeneration and neurofibrillaryhistopathology were confirmed with the use of Nissl and Bielschowskystains, and the diagnosis of AD was established by criteria fromthe Consortium to Establish a Registry for Alzheimer's Disease(Mirra et al., 1991). Brain tissue used for immunocytochemicalanalyses was immersion-fixed in cold 10% phosphate-buffered (0.15M) formalin, pH 7.4. The postmortem interval for all brain tissuewas $<=$ 6 hr, with a total fixation time of 2 weeks or less.

Antibodies. Immunocytochemical studies were performed with antibodies to the two lysosomal hydrolases, cathepsin D (Cat D)and cathepsin B (Cat B), and the rab-related GTP-binding proteinrab5. Anti-Cat D antiserum was prepared in our laboratory andraised in sheep against human brain Cat D (Nixon and Marotta,1984; Cataldo et al., 1990). Human liver anti-Cat B antiserumwas purchased commercially from ICN Biochemicals (Costa Mesa,CA). The anti-pro-Cat D antiserum was purchased commercially fromOncogene Science (Cambridge, MA). Antibody directed against rab5is a commercially prepared affinity-purified rabbit polyclonalantibody (Santa Cruz Biotechnology, Santa Cruz, CA) raised againsta synthetic peptide corresponding to amino acids 193-211 of theC-terminal domain of human rab5. An affinity-purified rabbit polyclonalantibody directed against the cytoplasmic tail of human 46 kDaMP-R was generously provided by Drs. Kurt von Figura and AnnetteReyfeld, Georg-August-Universitat, Göttingen, Germany (Steinet al., 1987a; Nadimpalli et al., 1991).

Immunocytochemistry. Immunoreactivity was demonstrated on 30- to 40-µm-thick vibratome sections, as previously described (Cataldoet al., 1990). Negative controls consisted of tissue sectionsincubated in preimmune antisera or in the absence of primary antisera.For immunofluorescence studies sections were double-immunostainedwith different hydrolase antisera and rab5, and immunoreactivitywas demonstrated with secondary antibodies conjugated to FITC,TRITC, or Texas Red (Cataldo et al., 1990, 1996).

Digital confocal analysis. High-resolution images of double-labeled neurons were viewed at high magnification with digitalconfocal microscopy. Images were created from representative neuronsthat displayed both Cat D or Cat B and rab5 immunofluorescence.Digital images were obtained as previously reported (Cataldo etal., 1996). A Z-series stack of high-magnification digitized imagesof representative neocortical layer III pyramidal neurons wasacquired through consecutive focal planes (Cataldo et al., 1996).For each single- and double-labeled neuron, two Z-series stackswere generated with FITC and TRITC filters, respectively. Parallelpairs of stacks were processed with a deconvolution subroutineof the BDS-IMAGE software, and images displaying the colocalizationof each fluoroprobe were generated by the Multicolor Registrationsubroutine (BDS-IMAGE software).

Morphometric analysis. Vibratome sections from the prefrontal cortices of eight age-matched controls and nine AD brains wereimmunostained in tandem under identical experimental conditionswith rab5 antiserum. Background staining intensities between ADand control sections were comparable in all cases, and all neuronswere intact. Small, medium, and large pyramidal neurons from corticallaminae III were selected at random (Cataldo et al., 1996). Thecross-sectional area, number of endosomes, average endosomal volume,and total early endosomal volume per cell were analyzed for eachneuron by the Bioquant System IV morphometry software package(R & M Biometrics, Nashville, TN) at 1000× magnification. Countsof rab5-positive endosomes were made by direct inspection in asingle plane of focus. To measure cross-sectional areas, we useda Leitz microscope with a low-light video camera attachment tocapture and display high-resolution images by a Targa frame grabber.Neurons were isolated and outlined with a Summagraphics digitizingtablet. For each brain 25 neurons were assessed at random withinseveral fields from neocortical layer III. In total, 200 neuronsfrom the control and 225 neurons from the AD cases were analyzed.For statistical comparisons based on endosomal size, each endosomewas assigned to one of four groups on the basis of volume: (inµm³) 0-0.35, 0.35-1.0, 1.0-2.1, 2.1-7+ µm. All data sets examinedshowed nonparametric distributions. ANOVA with the Kruskal-Wallistest (p < 0.05) showed significant differences between the Alzheimerand control groups analyzed. The Tukey-Kramer test (p > 0) wasused to demonstrate statistically significant differences in totalendosomal volume and individual endosomal size per cell betweenAlzheimer and control groups.

Vibratome sections from the prefrontal cortices of six control brains and seven age-matched AD brains were immunostained intandem under identical experimental conditions with anti-MP-R46antiserum. It should be noted that the background staining intensitiesbetween AD and control sections were comparable in all cases andthat all neurons counted were intact. Small, medium, and largepyramidal neurons from lamina III were selected at random, usinga 100 × oil immersion objective (N.A. 1.518). The cross-sectionalarea and MP-R density were analyzed for each of 25 neurons, aspreviously described (Cataldo et al., 1996). The image systemwas calibrated by placing an image box over the laminae of interestand recording the optical density [expressed as 0-255 levels ofgray scale: 0, lowest density; 255, highest density (Cataldo etal., 1995)].

For statistical comparisons based on cell size, each neuron was assigned to one of three groups on the basis of a real diameter:0-150, 151-225, and >225 µm². All data sets examined showed parametric distribution. Statisticalcomputations were performed with a Student's t test.

RESULTS

Rab5-positive early endosomes are a distinct group of hydrolase-containing organelles in human neurons
In tissue sections of human neocortex from normal individuals, anti-rab5 antiserum immunolabeled a population of small neuronalvacuolar compartments distributed close to the plasmalemma. Thislocalization is distinct from either the predominantly perinucleardistribution of late endosomes, the uniform cytoplasmic distributionof lysosomes (Fig. 1), or the basal location of lipopigment granules.Rab5-positive early endosomes were spherical in shape and relativelyuniform in size (100-250 nm), similar to those described in non-neuronalcell types (Gorvel et al., 1991; Bucci et al., 1992, 1994; deHoop et al., 1994). They were most numerous in the soma and proximaldendrites. As shown in our previous studies, antibodies to 215kDa MP-R selectively immunolabeled late endosomes and distinguishedthese compartments from MP-R-negative lysosomes (Fig. 1), whichcomprise the major subpopulation of acid hydrolase-containingorganelles. In neurons from aged control brains, late endosomesand lysosomes typically displayed diameters ranging from 100 to400 nm and from 50 to 400 nm (Nixon and Cataldo, 1995), respectively.Rab5 was absent from lipofuscin granules, which were identifiedon the basis of size (0.5-1.5 µm), the presence of autofluorescentlipopigment, and a concentration within the basal pole of thecell soma.
Fig. 1. Identification of early endosomes as distinct hydrolase-containing compartments in human pyramidal neurons. A, Consistentwith established morphological criteria, rab5-positive early endosomes(arrowhead) in cortical pyramids of aged control human brain weredistributed close to the plasmalemma and were relatively uniformin size. Immunoreactive endosomes were located principally inthe soma and proximal dendrites. We have shown that these structuresrepresent a subpopulation of neuronal acid-hydrolase-containingcompartments (see Fig. 3). B, We distinguished early endosomalcompartments from a smaller subgroup of hydrolase-containing,rab5-negative, MP-R215-positive late endosomes (arrowhead) thatdisplayed the typical perinuclear distribution. C, Lysosomes,which contain Cat D (arrow) and a number of other hydrolases,are MP-R-negative, rab5-negative, and distinct from early andlate endosomes. Lysosomes, which comprise the major populationof acidic vacuolar compartments, are typically 50-400 nm in diameterand are distributed uniformly throughout the cytosol. Magnificationin A-C, 4500×).
[View Larger Version of this Image (66K GIF file)]

Early endosomes in neurons of AD brain are abnormally large
We found a striking difference in the morphology of rab5-positive early endosomes in pyramids of at-risk neocortical regionsof AD brains, as compared with that of early endosomes in controlregions (Fig. 2). Pyramidal neurons in lamina III of the prefrontalcortex exhibited atypically large early endosomes resembling theones seen in baby hamster kidney (BHK) cells when the wild-typerab5 protein (Bucci et al., 1992) was overexpressed to stimulateendocytosis. In addition to being rab5-immunoreactive, the largeearly endosomes were distinguished from MP-R-positive, rab5-negativelate endosomes and rab-negative, MP-R-negative lysosomes on thebasis of size. Early endosomes in AD brains measured an averageof 487 nm in diameter (average diameter per brain ranged from400 to 620 nm), whereas late endosomes and lysosomes were consistentlyno larger than 400 nm in diameter. Large early endosomal profileswere found principally in at-risk pyramids of laminae III andV. In the less vulnerable neurons of laminae II and IV, the sizesof rab5-positive endosomes in small- to medium-sized pyramidalneurons, nonpyramidal neurons, and glia were equivalent to thosein controls.
Fig. 2. Morphometric analysis of rab5-positive early endosomes in control and Alzheimer's disease (AD) brains. High-magnificationimages of early endosomal compartments (arrows) in neocorticalneurons in lamina III of aged control (A) and AD (B) brains immunostainedwith rab5 and enhanced by Nomarski optics show the striking increasein the size of these compartments in AD brain, as compared withcontrol. In some, invaginations suggest a location at the plasmalemma.C, Percentage of cell area occupied by rab5-positive early endosomesplotted as a function of total cell area. Alterations in earlyendosomes were widespread in AD brains, and many pyramidal neuronsin AD brains (filled triangles) exhibited a significant increase(>2 SD higher than the control mean) in total endosomal volumeper cross-sectional cell area as compared with age-matched controls(open circles) (AD mean = 5.37% ± 0.19; control mean = 2.18% ±0.09). D, The size distributions of individual early endosomespresent in 25 lamina III pyramids from each of eight aged controland nine AD brains show that a substantial proportion of individualneuronal endosomes in the AD brains had volumes larger than thosein control brains. Endosomal volume is expressed as a functionof cell area for easier visualization of data. E, The percentageof abnormally large endosomal profiles that are >1 µm³. Values are mean percentage based on 25 pyramidal neurons perindividual brain (n = 9 AD and 8 controls). Approximately 10-foldhigher numbers are seen in AD brains as compared with controls(AD mean = 7.8% ± 1.65; control mean = 0.80% ± 0.13). Changesin endosomal volume as a function of cell area were not significantin AD and control brains. Magnification in A, B, 4700×.
[View Larger Version of this Image (43K GIF file)]

The size and/or number of early endosomes in neuronal and non-neuronal animal cells have been shown in vivo and in vitro tobe proportional to the rate of endocytic uptake (Parton et al.,1989, 1992; Stenmark et al., 1994). Therefore, to index this neuronalendocytic function, we used computerized morphometry to determinethe number and volumes of rab5-immunoreactive compartments in25 pyramidal neurons from lamina III of the prefrontal cortexin each of nine AD and eight age-matched control brains (Fig.2). Total numbers of early endosomes in neurons from AD brainswere markedly similar to those in neurons from control brains(AD average, 49 endosomes/cell; control average, 58 endosomes/cells).Of the neocortical pyramids in lamina III of AD brain, 48% hadabnormally large endosomal volumes (i.e., total endosome volume>1 SD higher than the control mean). The percentage of cell areaoccupied by rab5-positive early endosomes averaged 2.5-fold greater(p < 0.0001) in the pyramidal neurons of the AD brains than incontrols (AD mean = 5.37% ± 0.19; control mean = 2.18% ± 0.09)(Fig. 2C) $---$ a finding consistent with an upregulation of endocytosis(Parton et al., 1989, 1992; Gorvel et al., 1991; Bucci et al.,1992, 1994; Stenmark et al., 1994). Substantial numbers of individualendosomes were eightfold to 32-fold larger than the average sizeof endosomes in control neurons (Fig. 2D). The incidence of abnormallylarge early endosomes (>1 µm³) was ~ten-fold higher in AD brains than in controls (AD mean= 7.80 ± 1.65; control mean = 0.80 ± 0.13; p < 0.0001) (Fig. 2E).Similar abnormalities were detected in neuronal pyramids fromlamina V (data not shown). By contrast, cell size in neuronalpopulations within severely affected regions from cases of Pick'sdisease, Huntington's disease (grades 0-3), diffuse Lewy bodydisease, progressive supranuclear palsy, or encephalitis fellwithin the normal control range.

Immature and mature lysosomal proteases frequently are detected in the early endosomes of neurons in AD
Because early endosomes normally may contain low levels of acid hydrolases and because cathepsin expression is markedly upregulatedin AD brain (Nixon and Cataldo, 1993, 1995; Cataldo et al., 1994,1995, 1996), we evaluated whether the delivery of cathepsins toearly endosomes may be increased in AD. As we reported previously(Nixon and Cataldo, 1993, 1995; Cataldo et al., 1994, 1995, 1996),most pyramidal neurons of laminae III and V of AD brains exhibitedincreased numbers of hydrolase-positive compartments. Confocalimmunofluorescence image analyses of human brain sections double-labeledwith antibodies to rab5 and to the mature form of Cat D or torab5 and to mature Cat B demonstrated that, in most pyramidalneurons in vulnerable regions of AD brains, Cat D and Cat B colocalizedwithin the majority of rab5-positive vacuolar compartments (Fig.3). Colocalization was evident in 85% (±5%) of neuronal earlyendosomes of pyramidal neurons in AD brains but in only 25% (±5%)of the neuronal endosomes in control brains. In the AD brainshydrolase was localized more frequently within the larger rab5-positivecompartments than smaller ones (Fig. 3). As expected, both CatD and Cat B also were detected in rab5-negative compartments (e.g.,late endosomes, mature lysosomes, and lipofuscin).
Fig. 3. Colocalization of mature proteases in early endosomal compartments of human neurons. Immunofluorescence confocal images ofa neocortical pyramidal neuron from control (A-C) and AD (D-F)brains, using antisera to mature Cat B (red) and rab5 (green),demonstrate that mature lysosomal hydrolases often reside in earlyendosomes (yellow). The localization of mature protease in earlyendosomal compartments occurred to a greater extent in neuronsin the AD brains than in controls and more often in the largerendosomal profiles. Both Cat B and Cat D (not shown) were presentin rab5-positive early endosomes as well as rab5-negative lateendosomes, lysosomes, and lipofuscin. Magnification in A-F, 4000×.
[View Larger Version of this Image (114K GIF file)]

Human control and AD brain sections also were double-labeled with antisera to the proform of Cat D and rab5 by the ABC techniqueand two chromogens, DAB and SG, and visualized with bright-fieldmicroscopy. We found that in control brains pro-Cat D rarely colocalizedwith rab5-positive early endosomes, whereas >50% of the abnormallylarge rab5-positive early endosomal profiles in AD brains containedpro-Cat D immunoreactivity (Fig. 4).
Fig. 4. Immature proteases frequently are detected in early endosomes of AD neurons. Double-label immunocytochemical analysis withbright-field microscopy and antisera directed against pro-CatD (brown, left inset) and rab5 (blue, right inset) in this laminaIII pyramid from an AD brain is a representative example of thefrequent colocalization of immature proteases in the abnormallylarge early endosomes (arrows). Pro-Cat D is also present in apopulation of smaller immunoreactive vacuolar compartments, whichare consistent with late endosomes and are increased in numberin AD neurons, as compared with normal controls (see Fig. 1B).Magnification, 4350×; magnification in left and right insets,3600×; magnification in center inset, 6000×.
[View Larger Version of this Image (139K GIF file)]

MP-R46 content of neurons from affected regions of AD brains is increased
In pyramidal neurons from human brains, anti-MP-R46 antiserum was located principally in close apposition to the nucleus $---$ adistribution consistent with that of the Golgi apparatus (Fig.5). This perinuclear distribution was observed in lamina III pyramidsof both control and AD brains. We found that the qualitative levelsof MP-R46 immunoreactivity were increased in neocortical laminaIII neurons of the AD brains, as compared with the levels observedin age-matched control brains. In AD brains anti-MP-R46 antiserumalso immunolabeled a population of large vacuolar compartments(Fig. 5), which were not apparent in pyramids from age-matchedcontrols. MP-R46 immunoreactive vacuolar compartments were visualizedbest in pyramidal neurons exhibiting a lower density of staining.These profiles resembled the ones seen in lamina III pyramidsfrom at-risk AD brain regions labeled with rab5 antiserum (seeFigs. 2, 3, 4). Both the 215 and 46 kDa MP-Rs are distributedin the trans-Golgi apparatus, endosomes, and lysosomes (Brownet al., 1985; von Figura and Hasilik, 1986; Dahms et al., 1989;Jin et al., 1989). The MP-R215 is enriched in late endosomes andis accepted now as a marker of this compartment, although smallamounts have been detected in early endosomes and at the plasmamembrane (Fischer et al., 1980; Geuze et al., 1988; Griffithset al., 1988). Alternatively, MP-R46 is thought most likely toaccompany its ligand to early endosomes and the cell surface (Hasilikand von Figura, 1984; Chao et al., 1990). The large MP-R46-positivecompartments were similar in size and location to the abnormallylarge rab5-positive early endosomes. Double-label immunocytochemistrywith rab5 and MP-R46 antisera could not be performed because theseantibodies were both raised in rabbits.
Fig. 5. Levels of MP-R46 are elevated in neurons of AD brains. Immunocytochemical studies using antibody directed against MP-R46 showincreased levels of this receptor (arrows) in lamina III neuronsin the AD brains (B) than in controls (A). (The cells in A rangein optical density from 57 to 67, control mean = 54.14 ± 1.31;those in B range in optical density from 71 to 86, AD mean = 70.80± 1.38; p < 0.001. Percentage difference above the mean opticaldensity was equivalent for neurons in A vs B.) In AD brains displayinglower levels of immunostaining, MP-R46 immunolabeling could bevisualized clearly within large vacuolar profiles (B, inset, arrowhead)that resembled the abnormally large rab5-positive early endosomalprofiles. Semiquantitative morphometric analysis from sectionsof the prefrontal cortex revealed that cortical pyramids in laminaeIII of the AD brains ( filled triangles) exhibit increased MP-R46densities per cross-sectional area as compared with age-matchedcontrols (open circles). Magnification in A, B, B inset, 3600×.
[View Larger Version of this Image (53K GIF file)]

To assess the functional activity of MP-R46 as an alternate mechanism for the delivery of lysosomal proteases to the earlyendosomal pathway of neurons of at-risk regions of AD brains,we performed semiquantitative morphometric analyses to determinethe density of MP-R46-positive compartments in 25 lamina III pyramidsfrom seven AD brains and six age-matched controls (Fig. 5). TotalMP-R46 density per neuron in the AD brains was up to twofold higherthan the density of the MP-R46 in the age-matched control brains,and the average density was 30% higher (Student's t test, p <0.001; Fig. 5).

DISCUSSION

Early endosomes in neurons of human brain
This study is the first to our knowledge to identify and characterize early endosomal compartments in brain in vivo and hasrevealed a sizable population of early endosomes in normal neurons.The identity of early endosomes in human neurons is based on severallines of evidence. First, these vacuolar compartments were immunolabeledselectively by an antibody directed against rab5, a resident proteinof early endosomes and an established marker of this compartment(Parton et al., 1989, 1992; Gorvel et al., 1991; Bucci et al.,1992, 1994; de Hoop et al., 1994; Stenmark et al., 1994). Second,they were not labeled by immunocytochemical markers of other compartmentsof the E-L pathway, including MP-R215 (late endosomes) and LAMP-2(lysosomes; our unpublished results), and they contained no lipopigmentindicative of lipofuscin (Nixon and Cataldo, 1995; Cataldo etal., 1996). Furthermore, early endosomes predominantly were distributedclose to the cell surface and were prominent in both the cellsoma and processes, particularly proximal dendrites. This localizationpattern is consistent with that observed in a variety of culturedneurons and non-neuronal cells; however, the pattern differedfrom the perinuclear location of late endosomes and the diffusecytoplasmic localization of mature lysosomes that reside in boththe cell body and processes but predominate in the soma. A percentageof these vacuoles normally contain acid hydrolase, as predictedfrom other studies (Diment et al., 1989; Casciola-Rosen and Hubbard,1991; Berg et al., 1995), and this percentage was increased inAD brains. Finally, the sizes of rab5-positive vacuolar compartmentsin neurons from normal human brains ranged from 100 to 250 nmin diameter. Each of these characteristics of early endosomesis in agreement with what is known about these compartments fromstudies of non-neuronal (Parton et al., 1989; Gorvel et al., 1991;Bucci et al., 1992, 1994; Stenmark et al., 1994) and neuronal(Parton et al., 1992; de Hoop et al., 1994) cell lines and primarycultures of neurons (de Hoop et al., 1994).

Increased endocytic activity and cathepsin trafficking to early endosomes in AD
We found that total endosomal volumes of neurons within laminae III of AD brains were, on average, 2.5-fold larger than normaland that a high proportion of pyramidal cells exhibited theseabnormalities. Previous studies have shown that the size of earlyendosomal compartments reflects the degree of endocytic uptake.Rab5, which regulates the early endocytic pathway by modulatingplasma membrane uptake and trafficking and which regulates thefusion of endosomes derived from the plasma membrane (Parton etal., 1989; Gorvel et al., 1991; Bucci et al., 1992, 1994; de Hoopet al., 1994; Stenmark et al., 1994), seems to be a major determinantof this process. Increased rab5 expression stimulates endocyticuptake and expands the size of early endosomes (Gorvel et al.,1991; de Hoop et al., 1994), whereas the expression of mutantsdefective in rab5 decreases the rate of endocytic uptake (Gorvelet al., 1991; Stenmark et al., 1994). The appearance of abnormallylarge rab5-positive early endosomes in neurons of at-risk regionsof AD brains, therefore, strongly suggests an accelerated rateof endocytosis.

Previously, we showed that pyramidal neurons and other neuronal populations affected in AD contained abnormally high numbersof late endosomal and lysosomal compartments (Cataldo et al.,1994, 1996). The major acid hydrolase-containing compartmentsin the cell, late endosomes and lysosomes, are associated withterminal processing of substrates that arrive by the endocyticpathway, by autophagy (Gordon et al., 1992), or by direct scavengingof proteins from the endoplasmic reticulum to lysosomes (Nodaand Farquhar, 1992). Increased numbers of these organelles could,therefore, reflect the upregulation of one or both of these cellular-processingpathways. Our results demonstrate that increased activity in theearly endocytic pathway in sporadic AD is likely to account, inpart, for the massive activation of the lysosomal system. Consistentwith a more active rate of endocytosis, we observed that the geneexpression of Cat D and Cat B is upregulated (Cataldo et al.,1995) and that greater amounts of these proteases are being traffickedto neuronal early endosomes in AD brain. That acid hydrolasesof many types are present in greater amounts in lysosomes of affectedneurons in AD brain (Cataldo et al., 1991) raises the possibilitythat some of these enzymes also may be represented more highlyin early endosomes in AD. Early endosomes, unlike other compartmentsof the E-L pathway, normally contain low levels of cathepsins(Diment et al., 1989; Casciola-Rosen and Hubbard, 1991; Berg etal., 1995). In vitro studies (Ludwig et al., 1991) have shownthat the newly synthesized lysosomal hydrolases can be traffickedto the early endosome, but the trafficking mechanisms have yetto be elucidated. The presence of active proteases and perhapsother hydrolases in early endosomes provides a basis for partialproteolytic processing of endocytosed materials within these organelles,as shown for various substrates (Diment et al., 1989; Casciola-Rosenand Hubbard, 1991; Berg et al., 1995). The increased detectionof the proteases Cat D and Cat B in early endosomes observed inthis study, together with the findings of much larger early endosomesin pyramidal neurons of AD brains, indicates that traffickingof these proteases to this compartment is increased and supportsthe notion that proteolytic activity within early endosomes ismore active.

In response to increased endocytic uptake, an increased demand for hydrolases in early endosomes of neurons within affectedregions of AD brains may activate alternative mechanisms of enzymedelivery to this compartment. The trafficking of lysosomal hydrolasesto both early and late endosomes is compatible with the intracellulardistributions of the 215 and 46 kDa MP-Rs (Pfeffer, 1987; Geuzeet al., 1988; Griffiths et al., 1988; Bleekemolen et al., 1989).Delivery to late endosomes or lysosomes via the 215 kDa MP-R orto early endosomes/cell surface or lysosomes via the 46 kDa MP-Rmay be favored, depending on cellular alterations that promotedifferent transport routes (see Chao et al., 1990). We observedthat levels of MP-R46 immunoreactivity are increased markedlyin pyramidal neurons of lamina III of the neocortex of AD brains,as compared with aged controls. This receptor normally plays aless dominant role than the 215 kDa MP-R in the transport of newlysynthesized acid hydrolases to late endosomes and lysosomes (Steinet al., 1987b; Dahms et al., 1989) and mediates the transportof endogenous lysosomal enzymes to the plasma membrane and earlyendosomes but, unlike MP-R215, does not mediate the endocytosisof secreted hydrolase (Stein et al., 1987b; Dahms et al., 1989),which is believed to be the usual route of arrival of hydrolasesresiding in endosomes. The increase in content of MP-R46 in affectedneuronal populations suggests that trafficking pathways are activatedthat assist in the delivery of lysosomal hydrolases, includingthe proforms of these hydrolases, to early endosomes. This wouldbe expected to promote an earlier and more efficient processingof substrates arriving to early endocytic compartments at increasinglyrapid rates in affected neurons in AD.

Various antecedent events linked to the etiology and progression of AD could lead to the need for increased endocytic activityin neurons of at-risk regions of AD brains. These potentiallyimportant events include accelerated membrane turnover/repairresulting from cumulative membrane damage caused by aging, genetic,chemical and oxidative factors (Nixon and Cataldo, 1994), alterationsin membrane function or stability because of genetic or chemicalalterations of APP, and other membrane proteins accompanying AD(Chartier-Harlin et al., 1991; Terry et al., 1991; Levy-Lahadet al., 1995; Sherrington et al., 1995). ApoE, another criticallyimportant molecule in AD pathogenesis (Roses, 1995), is not synthesizedin neurons but is taken up by them, particularly during cell injury(Mahley, 1988). In Alzheimer brains increased levels of ApoE havebeen demonstrated in otherwise normal-appearing neurons of at-riskbrain regions and the same cell populations that display earlyE-L system alterations (Einstein et al., 1995), consistent withincreased uptake of ApoE and its subsequent trafficking throughthe E-L system. More importantly, the increased, and possiblyaltered, processing of ApoE through this pathway may be relateddirectly to greater levels of neuronal toxicity of the 22 kDaproteolytic fragment of the ApoE-e4 isoform versus the ApoE-e3isoform (Crutcher et al., 1996).

Implications for $beta$ -amyloidogenesis and pathogenesis in AD
Previous studies of cultured cell lines have implicated both the secretory (Busciglio et al., 1993; Morato and Mayor, 1993;Araki et al., 1994) and endocytic (Haass et al., 1992; Nordstedtet al., 1993; Koo and Squazzo, 1994; Refolo et al., 1995) pathwaysin APP processing and A $beta$ generation. The relative contributionof these two pathways to A $beta$ production is altered by the APP mutationthat causes early-onset AD (Citron et al., 1992; Suzuki et al.,1994). Involvement of the endocytic pathway in constitutive APPprocessing and A $beta$ production is supported by (1) the presenceof the consensus motif, NPTY, on the C terminus of APP, a signaltriggering receptor-mediated internalization from the cell surfaceto endosomes (Chen et al., 1990); (2) the detection of APP andAPP fragments in clathrin-coated vesicles (Nordstedt et al., 1993;Marks et al., 1994; Sapirstein et al., 1994); and (3) the abilityof treatments that reduce APP internalization to decrease A $beta$ releasein non-neuronal cell cultures (Koo and Squazzo, 1994).

The neuronal endocytic abnormalities we observed in the brains of Alzheimer patients now provide direct neuropathologicalsupport for a mechanism of accelerated $beta$ -amyloidogenesis in sporadicAD, which is also consistent with the foregoing data on the endocyticpathway in cultured cell systems (Haass et al., 1992; Nordstedtet al., 1993; Koo and Squazzo, 1994; Refolo et al., 1995). Thepersistent upregulation of endocytosis seen in pyramidal neuronsof Alzheimer brain, by itself, implies an abnormal stimulationof usual endocytic events that should include APP processing andnormal A $beta$ generation. A further acceleration of APP processingis expected if, as we observed, the trafficking to endosomes ofappropriate proteases is increased abnormally. In this regard,one of the cathepsins that we monitored in this study, Cat D,has $beta$ and $gamma$ secretase activity toward model peptides and/or recombinantAPP (Dreyer et al., 1994; Evin et al., 1995; Higaki et al., 1995;Chevallier et al., 1996). Other cathepsins also indirectly influenceA $beta$ formation (Sahasrabudhe et al., 1993; Bernstein and Wiedanders,1994; Munger et al., 1995). The identification of specific hydrolasesinvolved in constitutive A $beta$ production, however, is still notdefinitive. Whether or not the cathepsins are normally responsiblefor A $beta$ production, the possibility may be raised by our studiesthat, under pathological circumstances, proteases not normallyinvolved in constitutive A $beta$ formation become abnormally routedto a cellular compartment within which they now may contributedirectly or indirectly to A $beta$ production. The identification ofproteases that might become APP secretases under a specific pathologicalcondition would require the analysis of cell systems in whichthat condition is modeled appropriately. Although these effectson endocytosis could be a consequence of $beta$ -amyloid depositionrather than a cause, chromosome 14 mutations leading to AD areassociated with high levels of $beta$ -amyloid deposition, but no changesin the appearance of endosomes (A. Cataldo and R. Nixon, unpublishedresults), consistent with the existence of multiple pathways forA $beta$ production and evidence that increased $beta$ -amyloidogenesis insome forms of familial AD may occur by routes other than the endosomalpathway (Haass et al., 1995; Thinakaran et al., 1996).

Enhanced endocytosis is expected to influence ApoE internalization and function, a prediction consistent with the observationof elevated ApoE immunoreactivity in pyramidal neurons in AD.Because ApoE is not synthesized appreciably in neurons, intracellularuptake is critical, and early endosomes are among the few intracellularsites in which ApoE has the opportunity to interact extensivelywith APP and its cleaved derivatives (Crutcher et al., 1996).Evidence that ApoE isoforms have differential binding affinitiesfor A $beta$ and may serve, with varying degrees of effectiveness, aspathological chaperones in A $beta$ fibrillogenesis (Wisniewski et al.,1994) is another example of how the endocytic pathway representsa crossroad in which etiological factors in AD pathogenesis converge.

FOOTNOTES

Received Dec. 11, 1996; revised May 20, 1997; accepted May 23, 1997.

This project was supported by Public Health Service Grant 5R35 AG10916-05 to R.A.N. and Grant MH/NS31862 (Harvard Brain TissueResource Center). We thank Maureen Medeiros for secretarial assistanceand Lisa Kanaley-Andrews for technical expertise. Affinity-purifiedantiserum directed against the 215 kDa mannose 6-phosphate receptor(MP-R) was a generous gift from Dr. Stuart Kornfeld. Antibodiesdirected against the cation-dependent 46 kDa MP-R were kindlyprovided by Drs. Kurt von Figura and Annette Reyfeld.

Correspondence should be addressed to Dr. Anne M. Cataldo, Nathan Kline Institute for Psychiatry, New York University Schoolof Medicine, 140 Old Orangeburg Road, Orangeburg, NY 10962.

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Volume 17, Number 16, Issue of August 15, 1997 pp. 6142-6151 Copyright ©1997 Society for Neuroscience

Increased Neuronal Endocytosis and Protease Delivery to Early Endosomes in Sporadic Alzheimer's Disease: Neuropathologic Evidence for a Mechanism of Increased -Amyloidogenesis

Copyright ©1997 Society for Neuroscience 0270-6474/1997/176142-10$05.00/0

Volume 17, Number 16, Issue of August 15, 1997 pp. 6142-6151
Copyright ©1997 Society for Neuroscience

Increased Neuronal Endocytosis and Protease Delivery to Early Endosomes in Sporadic Alzheimer's Disease: Neuropathologic Evidence for a Mechanism of Increased $beta$ -Amyloidogenesis