Demonstration by Fluorescence Resonance Energy Transfer of Two Sites of Interaction between the Low-Density Lipoprotein Receptor-Related Protein and the Amyloid Precursor Protein: Role of the Intracellular Adapter Protein Fe65

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The Journal of Neuroscience, November 1, 2001, 21(21):8354-8361

Demonstration by Fluorescence Resonance Energy Transfer of Two Sites of Interaction between the Low-Density Lipoprotein Receptor-Related Protein and the Amyloid Precursor Protein: Role of the Intracellular Adapter Protein Fe65
Ayae Kinoshita¹, Christa M. Whelan¹, Carolyn J. Smith¹, Irena Mikhailenko², G. William Rebeck¹, Dudley K. Strickland², and Bradley T. Hyman¹
¹ Alzheimer's Disease Research Unit, Department of Neurology, Massachusetts General Hospital, Charlestown, Massachusetts 02129, and ² Department of Vascular Biology, Holland Laboratory, American Red Cross, Rockville, Maryland 20855

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Amyloid- $beta$ , the major constituent of senile plaques in Alzheimer's disease, is derived from the amyloid precursor protein (APP)by proteolysis. Kunitz protease inhibitor (KPI) containing formsof APP (APP751/770) interact with a multifunctional endocyticreceptor, the low-density lipoprotein receptor-related protein(LRP), which modulates its proteolytic processing affecting productionof amyloid- $beta$ . We used fluorescence resonance energy transfer (FRET)using labeled LRP and APP in H4 cell line to examine the subcellularlocalization and the molecular domains involved in the APP-LRPinteraction. KPI-containing forms of APP (APP770) demonstratedFRET with LRP that was sensitive to the LRP inhibitor receptor-associatedprotein (RAP), suggesting an interaction between the extracellulardomains of APP770 and LRP. APP695 also interacts with LRP to lesserdegree (as measured by extracellular domain probes), and thisectodomain interaction is not altered by RAP. By using C-terminallytagged LRP and APP, we demonstrate a second site of interactionbetween the C termini of both APP695 and APP770 and the C terminusof LRP, and that the interactions at these regions are not sensitiveto RAP. We next examined the possibility that the C-termini APP-LRPinteraction was mediated by Fe65, an adaptor protein that interactswith the cytoplasmic tails of LRP and APP. FRET studies confirmeda close proximity between the amino Fe65 phosphotyrosine binding(PTB) domain and LRP cytoplasmic domain and between the carboxylFe65 PTB domain and the APP cytoplasmic domain. These findingsdemonstrate that LRP interaction with APP occurs via both extracellularand intracellular protein interactiondomains.

Key words: amyloid precursor protein; APP; low-density lipoprotein receptor-related protein; LRP; adaptor protein Fe65; fluorescent resonance energy transfer; FRET; protein-protein interaction; secretory pathway; immunocytochemistry; confocal microscopy

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The pathological hallmarks of Alzheimer's disease are senile plaques and neurofibrillary tangles. The senile plaques containamyloid- $beta$ , which is generated by proteolysis of the amyloid precursorprotein (APP) (for review, see Selkoe, 1998; De Strooper and Annaert,2000). APP is a type I integral membrane protein in three majorisoforms generated by alternative splicing; APP695 is most abundantlyexpressed in the neurons, and two other splice variants, APP751and APP770, contain a Kunitz-type protease inhibitor domain (KPIdomain). APP is cleaved by $alpha$ - or $beta$ -secretases, releasing the 100-120kDa ectodomain of APP (soluble APP) and 10-12 kDa membrane-boundC-terminal fragments. An additional cleavage in the transmembranedomain by $gamma$ -secretase results in secretion of 4 kDa amyloid- $beta$ peptides.

Three pathways have been described that can lead to the processing of APP into amyloid- $beta$ : within the secretory pathway inthe endoplasmic reticulum-intermediate compartment pathway (Cooket al., 1997; Hartmann et al., 1997), a trans-Golgi network pathway(Xu et al., 1997), and the endosomal-lysosomal pathway (Haasset al., 1992; Koo and Squazzo, 1994). Recent data suggest thatendocytosis of APP holoprotein from the cell surface is an importantstep in amyloid- $beta$ synthesis in some systems (Perez et al., 1999).

The low-density lipoprotein (LDL) receptor-related protein (LRP) is a member of the LDL receptor family and is a ~600 kDasingle transmembrane endocytic receptor. The extracellular domaincontains four distinct ligand binding sites. It mediates internalizationand degradation of ligands involved in metabolic pathways of lipoproteinsand protease-protease-inhibitor complexes (Strickland et al.,1995), including $alpha$ -2-macroglobulin (Borth 1992), apolipoproteinE (Herz et al., 1988), and KPI domain in tissue factor plasminogenactivator (Bu et al., 1992). The binding of ligands to LRP canbe blocked by the receptor-associated protein (RAP) (Herz et al.,1991; Williams et al., 1992).

It has been demonstrated previously that LRP can serve as an internalization receptor for the KPI-containing (but not APP695)isoforms of soluble APP (Kounnas et al., 1995). These data ledto the hypothesis that the extracellular domains of LRP and APPinteract via a ligand-ligand binding domain interaction, and subsequentdata supported the idea that this interaction could also mediateAPP770-LRP interactions for cell surface APP, leading to APP endocytosis(Knauer et al., 1996; Ulery et al., 2000).

Our current studies examine the interaction of APP and LRP using confocal microscopy-based fluorescence resonance energy transfer(FRET) techniques that provide both exquisite subcellular localizationand information about protein-protein interactions in cells. Wedemonstrate that there are clear interactions at the cell surfaceand in the secretory pathway between LRP and APP770, and, surprisingly,between LRP and APP695. Studies of interactions of both the ectodomainsand the intracellular domains show that there are two distinctsites of interaction between APP and LRP: an RAP-sensitive extracellularinteraction between the APP KPI domain and a ligand binding domainof LRP, and an RAP-insensitive intracellular interaction betweenthe C terminus of APP and the C terminus of LRP. The latter maybe mediated partly by intracellular adaptor proteins such asFe65.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Generation of expression constructs and deletion mutants for human APP, LRP, Fe65, and RAP. Human APP770, APP695 cDNA lackingthe termination codon was generated by PCR with a set of primers:5'-ATAGCTAGCCACCATGCTGCCCGGTTTG-3' and 5'-TCGTCGACCTGTTCTGCATCTGCTCAAA-3'.The PCR product was digested with the restriction enzymes NheIand SalI and ligated in-frame to the NheI and SalI site of anexpression vector: pEGFP-N1 (Clontech, Palo Alto, CA) and pDsRed-N1(Clontech) (for reagent information, see Fig. 1).

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Figure 1. Reagents used in this study. This scheme shows the constructs used in this study. The membrane-spanning regions are shown in black. Both APP695 and APP770 are tagged at the C terminus with either myc or DsRed. The N-terminus truncated APPC99 is tagged with myc at the C terminus. Full-length LRP is tagged at the C terminus with either myc or EGFP (shown as GFP). The Fe65 construct is tagged either with EGFP at the N terminus or myc at C terminus. For the study of ectodomain interactions, anti-APP antibody (8E5) and anti-LRP antibody (R829), both of which are raised against the extracellular domain of APP or LRP, respectively, are used. For intracytoplasmic interaction, the combination of myc (detected with Cy3) and EGFP or the combination of DsRed and EGFP is used.

To make myc-tagged constructs for APP770, APP770 cDNA lacking the termination codon was generated by PCR and inserted intothe HindIII site of pcDNA3.1B (Invitrogen, Carlsbad, CA) in-frame.To make the myc-tagged construct for APP695, human APP695 cDNAlacking the termination codon was generated by PCR with a setof primers: 5'-TTAAAATTTGCTAGCACCGCCATGCTGCCCGG-3' and 5'-TTTAGCGGCCGCGTTCTGCATCTGCTCAAA-3'.The PCR product was digested with NheI and NotI and ligated intothe NheI and NotI site of pcDNA3.1A(Invitrogen).

A deletion mutant containing only the C-terminal 99 amino acids of full-length APP (APPC99) was generated by PCR with a setof primers: 5'GCAAGCTTGCAGAATTCCGACATGACTCAGGA-3' and 5'-TTCAAGAAACTCGTCTACGTCTTGCGAGCTCCG-3'.The PCR products were digested with HindIII and XhoI and ligatedinto the HindIII and XhoI site of an expression vector pSecTag2B(Invitrogen).

Authenticity of all PCR-generated constructs was confirmed by DNAsequencing.

Constructs of LRP-EGFP (enhanced green fluorescent protein) was generated from ligating human LRP cDNA digested with restrictionenzymes of XhoI and Bsu36I and synthetic oligomers of 5'-TGAGGACGAGATAGGGGACCCCTTGGCAA-3'and 5'-AGCTTTGCCAAGGGGTCCCCTATCTCGTCC-3' containing the last partof LRP without a stop codon and HindIII site. These were theninserted into the XhoI and HindIII site of expression vector pEGFP-N1(Clontech). LRP in pcDNA3.1A (Invitrogen) was also constructedin a similar manner (LRP-myc).

The generation of Fe65-myc, which has myc at its C terminus, has been reported previously (Borg et al., 1996). This constructlacks N-terminal 52 amino acids but maintains the WW and PTB domains.The Fe65-myc construct was digested by SalI and inserted intothe SalI site of the pEGFP-C3 vector (Clontech) to generate aGFP-Fe65construct.

Human RAP cDNA that was originally cloned into pGEX-2T (Amersham Pharmacia Biotech, Piscataway, NJ) vector (Williams et al.,1992) was cut by BamHI and EcoRI, recloned into the BamHI andEcoRI site of the pcDNAINeo vector (Invitrogen), and then furtherrecloned into the BamHI and XhoI sites of the expression vectorpcDNA3(Invitrogen).

Antibodies and proteins. Human RAP was expressed in bacteria as a fusion protein with glutathione S-transferase (GST) as describedpreviously (Williams et al., 1992). Cleavage through thrombinand purification of recombinant RAP was performed as describedpreviously (Williams et al., 1992). The rabbit polyclonal R829against LRP was raised in the same way as R777 as described previously(Kounnas et al., 1992). Monoclonal antibody 8E5 was raised against520-668 residues of APP770 and was a gift from Dr. P. Seubert(Elan Pharmaceuticals, South San Francisco, CA). Monoclonal antibody22C11 raised against 60-100 residues of APP was purchased fromChemicon (Temecula, CA). Mouse monoclonal anti-myc antibody waspurchased from Invitrogen. Rabbit polyclonal anti-myc antibodywas purchased from Upstate Biotechnology (Lake Placid, NY). Mousemonoclonal antibody 7F1 recognizes RAP (Kounnas et al., 1992).

Cell culture conditions and transient transfection. H4 cells derived from human neuroglioma cells used in this study wereobtained from the American Type Culture Collection (Manassas,VA). H4 cells were cultured in OPTI-MEMI with 10% fetal bovineserum, and Chinese hamster ovary (CHO) cells were cultured inHam's-F-12 with 10% fetal bovine serum. Transient transfectionof H4 cells were performed using a liposome-mediated method (FuGene6; Roche Molecular Biochemicals, Indianapolis, IN). Cells wereplated onto four-well chambers 1 d before the transfection. First,a mixture of 1 µg of plasmid DNA and 3 µl of Fugene6 was madein 100 µl of DMEM and left for 15-30 min at room temperature,and then 25 µl of this mixture was added to the medium in eachwell. The incubation time was from 24 to 48 hr. Double transfectionof APP and LRP plasmids was done in the same way. To investigatethe possible inhibition by RAP, some cells were also triple-transfectedwith APP, LRP, andRAP.

Immunohistochemistry. Immunostaining of cells was performed 24-48 hr after transfection. Cells were fixed in 4% paraformaldehyde(PFA) for 10 min, washed in Tris-buffered saline (TBS), pH 7.3,permeabilized by 0.5% Triton X-100 for 20 min, and blocked with1.5% normal goat serum for 1hr.

To detect C-terminal interactions, cotransfected cells of APP770-myc (or APP695-myc or APPC99-myc) and LRP-EGFP were used.Cells were immunostained by mouse anti-myc monoclonal antibody(1:1000 dilution; Invitrogen) for 1 hr at room temperature. Cellswere then washed three times in TBS and labeled by Cy3-conjugatedanti-mouse antibody (10 µg/ml; Jackson ImmunoResearch, West Grove,PA) for 1 hr at room temperature. Immunostained cells were storedin TBS at 4°C until the confocal imaging was performed. To confirmthe results, the C-terminal interaction was also studied by APP770-DsRed(or APP695-DsRed) and LRP-EGFP double-transfectedcells.

For the N-terminal interactions, cotransfected cells of APP770-myc (or APP695-myc) and LRP-myc were used. These cells werelabeled with antibodies against ectodomains of APP and LRP, 8E5(1:1000) and R829 (1 µg/ml), respectively, and then labeled byCy3-conjugated anti-mouse antibody and FITC-conjugated anti-rabbitantibodies,respectively.

To confirm the APP-LRP interaction in the secretory pathway, double-transfected cells of APP-myc and LRP-GFP were counterstainedwith mouse monoclonal anti-GM130 antibody, which stains the Golgiapparatus (1 µg/ml; Becton Dickinson/Transduction Laboratory,San Diego, CA). GM130 was visualized by Cy5-conjugated anti-mouseantibody (10 µg/ml; Jackson ImmunoResearch). Golgi staining wasconfirmed by confocal microscopy using the 647 line of the krypton-argonlaser.

To detect interactions occurring on the cell membrane, cells were incubated with primary antibodies against the extracellulardomain (8E5 and R829) in the culture media for 1 hr on ice, thenwashed with PBS, and fixed in 2% PFA for 10 min without permeabilization.Secondary antibodies conjugated to Cy3 or FITC were applied tovisualize the primaryantibodies.

RAP treatment was performed in two ways. To study APP-LRP interactions within the secretory pathway, RAP was cotransfectedinto cells. To observe the transfection efficiency of RAP, RAPwas also stained with anti-RAP antibody 7H1 (1:1000) and conjugatedwith Alexa350 anti-mouse antibody (10 µg/ml; Molecular Probes,Eugene, OR) in the cells triple-transfected cells of APP-DsRedor APP-myc, LRP-EGFP, and RAP. For the cells with APP-myc, rabbitpolyclonal anti-myc antibody was used instead. The RAP stainingon the triple-transfected cells was confirmed by the 4',6'-diamidino-2-phenylindolefilter of the confocal microscope. To study cell surface APP-LRPinteractions, a solution of 500 nM recombinant RAP (Williams etal., 1992) was applied in the culture media 24 hr after transienttransfection, and the same assay was performed 24 hr after additionofRAP.

FRET. Immunostaining was observed using a Bio-Rad (Hercules, CA) 1024 confocal microscope mounted on a Nikon (Tokyo, Japan)Eclipse TE300 inverted microscope; the krypton-argon laser (emission,488 and 568 nm lines) was used to excite the fluorescein or EGFPand Cy3 or DsRed,respectively.

FRET was measured using a method developed for laser-scanning confocal microscopy (Knowles et al., 1999; McLean et al., 2000),which is analogous to the technique used by Rocheville et al.(2000) to study interactions of receptor subunits in cells. Theenergy transfer was detected as an increase in donor fluorescence(FITC or EGFP) after complete photobleaching of the acceptor molecules(DsRed or Cy3). This technique is also referred to as donor dequenching(Kenworthy and Edidin, 1998; Siegel et al., 2000). The amountof energy transfer was calculated as the percentage of increasein donor fluorescence after acceptor photobleaching; initial scanwas obtained at low-laser energy using the 488 line of the krypton-argonlaser to record the fluorescein (or EGFP) signal. A second scanwas performed with the 568 line, and the area of colocalizationwas noted. A small part of the cells (~5 × 5 µm) was then photobleachedwith intense 568 nm light (laser power 100%) to destroy the acceptormolecules. The cells were then rescanned using 488 nm light. Anincrease of the fluorescein (or EGFP) within the photobleachedarea was used as a measure of the amount of FRET present. Exposingsingle-labeled FITC or EGFP cells to 568 nm light for equivalenttimes did not alter the amount of fluorescein emission. The ratioFl_D2/Fl_D1 (where Fl_D2/Fl_D1 indicates the ratio of donor fluorescenceafter photobleaching to donor fluorescence before photobleaching)was compared with the null hypothesis value of 1.0 by one-groupt tests. Comparison of multiple groups was by ANOVA, with Fisher'sPLSD post hoc test for significance. FRET can be detected onlyif the two fluorophores are in close physical proximity: betweenfluorophores (e.g., EFGP-DsRed) to be less than ~10 nm. In experimentsin which the epitopes are labeled by indirect immunofluorescence,the fluorophores must be <10 nm apart, and the distance betweenepitopes can be (maximally) 30 nm (e.g., using the R829-8E5 pair)(Chin et al., 2000). This provides a >10-fold increase in resolutioncompared with double staining with conventional confocal microscopy,which has a resolution of ~500nm.

Negative controls for FRET experiments included the following: no FRET was observed between APP-GFP and APP-DsRed when cotransfected;no FRET was observed if the primary or the secondary antibodywas omitted; and no FRET was observed when APP-GFP was immunostainedwith 22C11 against the distal N-terminal end of APP, despite thecomplete colocalization. Thus, we conclude that the donor dequenchingobserved after photobleaching of the acceptor reflectsFRET.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The H4 human neuroglioma cell line was used in this study, because it has been used for the study of APP processing (Kuentzelet al., 1993) and for investigating the effect of LRP on thisprocess (Ulery et al., 2000; Rebeck et al., 2001). EndogenousAPP and LRP, visualized by anti-APP (8E5) and anti-LRP (R829)antibodies, were weakly visible in the cell body of H4 cells usingconfocal microscopy. Transfection of H4 cells with various LRPand APP constructs revealed similar patterns of immunostainingin the transfected cells when compared with the parental cells.No apparent differences in distribution of the overexpressed proteinscompared with endogenous proteins were detected, and, in the currentstudy, the FRET experiments were all performed in H4 cells transfectedwith plasmids encoding taggedproteins.

Interaction between ectodomains

Previous experiments showed that soluble forms of APP containing the KPI domain is a ligand for LRP (Kounnas et al., 1995;Knauer et al., 1996). We therefore initially investigated FRETbetween the ectodomains of APP and LRP in intact H4 cells. Cellscotransfected with APP770-myc and LRP were immunostained withmonoclonal anti-APP (8E5) and polyclonal anti-LRP (R829) antibodies(both raised against ectodomains) and then labeled by Cy3-conjugatedanti-mouse antibody and FITC-conjugated anti-rabbit antibody,respectively. The amount of FRET was calculated as the percentageof increase in donor fluorescence (FITC) after acceptor (Cy3)photobleaching (Fl_D2/Fl_D1). The presence of FRET suggests thatthere is a close apposition between the ectodomains (ratio ofFl_D2/Fl_D1 = 1.47 ± 0.06; mean ± SE; n = 14; p < 0.0001) (Fig.2). Surprisingly, FRET occurs not only on the cell surface butalso in intracellular compartments, including the Golgi (confirmedby counterstaining with GM130; data not shown) and endoplasmicreticulum. As a negative control, FRET was assessed using theAPP770-myc-transfected cells labeled with monoclonal 8E5 directedagainst an extracellular APP domain and a polyclonal anti-mycantibody directed against an intracellular domain of APP770-myc;although there was absolute colocalization of the two fluorophores,no FRET was observed because the distance across the membraneis too far to allow FRET. Similarly, exposure of single-labeledFITC stained cells to intense 568 light did result in a changein FITC intensity. Thus, the increase in FITC brightness afteracceptor photobleaching indicates a sufficiently close associationbetween the FITC and Cy3 fluorophores to support FRET.

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Figure 2. Extracellular domains of APP and LRP are closely associated with each other. H4 cells were cotransfected with APP770-myc and LRP-myc, immunostained with anti-APP (8E5) and anti-LRP (R829) antibodies, and visualized with Cy3 and FITC, respectively. Here is shown a typical example of FRET between ectodomains of APP770 and LRP. A, Cy3 (APP770) signal after 568 nm excitation. B, A discrete area of the cell was photobleached using intense 568 nm laser. C, FITC signal (LRP) using 488 nm excitation before photobleaching. D, FITC signal (LRP) using 488 nm excitation after photobleaching of the acceptor fluorophore (Cy3) with intense 568 nm laser light. An increase in donor fluorescence is observed within the discrete area that was photobleached, showing the presence of FRET. In this example, the FITC signal increased by 51%.

To determine whether the APP770-LRP interaction occurred on the cell surface, H4 cells were cotransfected with APP770-mycand LRP. The 8E5 and R829 antibodies against the ectodomains ofAPP and LRP were then incubated with the transfected cells at4°C to allow binding but to prevent cellular mediated internalization.Cells were then fixed but not permeabilized, and labeled secondaryantibodies were added. APP and LRP were observed on the plasmamembrane by confocal microscopy (Fig. 3). FRET was also presentbetween APP770 and LRP on the cell membranes, as revealed by increasedFITC fluorescence after photobleaching of Cy3. The FRET ratioincrease (Fl_D2/Fl_D1) of 1.40 ± 0.04 (n = 23; p < 0.0001) was essentiallythe same as that determined after routine fixation and stainingof cells (Fig. 2). This result suggests a close proximity betweenthe ectodomains of APP770 and LRP on the plasma membrane, consistentwith an interaction between these two molecules on the cell surface.

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Figure 3. Extracellular domains of APP and LRP displayed FRET at the cell surface. H4 cells were cotransfected with APP770-myc and LRP-myc, immunostained with anti-APP (8E5) and anti-LRP (R829) antibodies without permeabilization, and visualized with Cy3 and FITC, respectively. APP and LRP on the cell surface were observed. A, Cy3 (APP770) signal using 568 nm excitation. B, Discrete area of the cell was photobleached using intense 568 nm laser. C, FITC signal (LRP) using 488 nm excitation before photobleaching. D, FITC signal (LRP) using 488 nm light after photobleaching the acceptor (Cy3) with intense 568 nm laser light. An increase in donor fluorescence is observed within the discrete area that was photobleached, showing the presence of FRET on the cell membrane. In this example, the FITC signal increased by 38%.

We next asked whether the association of APP770 and LRP occurred via an interaction of APP with the ligand binding regionof LRP. This was determined by measuring whether the presenceof FRET was sensitive to RAP, because RAP is known to inhibitthe binding of all LRP ligands (including soluble APP) to LRP(Kounnas et al., 1995). H4 cells were cotransfected with RAP,APP770-myc, and LRP-GFP. No change in subcellular distributionwas observed for APP or LRP. The FRET ratio observed for the APP770-LRPectodomain interaction was significantly diminished when H4 cellswere cotransfected with RAP, APP770-myc, and LRP-GFP (Fl_D2/Fl_D1= 1.17 ± 0.03; n = 15; p < 0.005 compared with cells transfectedwith APP770-myc and LRP-GFP), but surprisingly FRET was not reducedto 1.0 (Fig. 4). Thus, the FRET observed between APP770 and LRPis partially, but not completely, inhibited by RAP. Similarly,the APP-LRP interaction at the cell membrane was partially inhibitedby exogenous addition of RAP, which was shown as a decrease ofFRET ratio (Fl_D2/Fl_D1 = 1.16 ± 0.01; n = 22; p < 0.001 comparedwith cells transfected with APP770 and LRP-GFP not treated withRAP). This suggests that, on the plasma membrane and within intracellularcompartments such as the Golgi and endoplasmic reticulum, theremay be two components of APP770-LRP interactions: one APP770-LRPinteraction that is RAP-sensitive, and another APP770-LRP interactionthat is RAP-insensitive. The existence of an RAP-insensitive interactionbetween APP and LRP is interesting, because previous work usingsoluble forms of APP revealed that RAP was able to block the interaction(Kounnas et al., 1995). The RAP-insensitive interaction couldbe attributable to the presence of another (RAP-insensitive) siteof interaction in the extracellular domains or, more likely, toan intracellular interaction between the C-terminal tails of APPand LRP.

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Figure 4. The FRET ratio increase of ectodomains is shown as a percentage of increase of donor fluorescence between APP (APP770 and APP695) and LRP. Both APP770 and APP695 demonstrated increases in donor fluorescence significantly above zero (p < 0.0001; one-group t test), but the magnitude of the FRET ratio increase of APP695 was significantly less than that of APP770 (p < 0.0001; ANOVA; Fisher's PLSD post hoc test). Cotransfection with RAP significantly decreased the FRET ratio between APP770 and LRP (p = 0.00012; ANOVA; Fisher's PLSD post hoc test) but not APP695 and LRP. The APP695-LRP ectodomain interaction was not affected by RAP. The FRET ratio increase on the cell membrane is almost the same as that of the routinely fixed and permeabilized cells. Cotransfection with RAP also significantly decreased the FRET ratio between APP770 and LRP at the cell surface (p < 0.0001; ANOVA; Fisher's PLSD post hoc test).

These two possibilities were examined next. To test the former possibility, cells were cotransfected with LRP and APP695-myc,which lacks the KPI domain. We detected FRET between APP695 andLRP (Fl_D2/Fl_D1 = 1.17 ± 0.03; n = 16; p < 0.0001), which was highlystatistically significant, but the magnitude of the FRET was significantlyless than that observed for APP770 and LRP (p < 0.0001). UnlikeAPP770, the APP695-LRP ectodomain interaction was not affectedby cotransfection with RAP (Fl_D2/Fl_D1 = 1.18 ± 0.04; n = 9). Togetherwith the previous experiments, the results are consistent withthe hypothesis that there is both an RAP-sensitive and an RAP-insensitivecomponent of the interaction between APP and LRP, and that theRAP-sensitive component is dependent on the presence of the KPIdomain.

Interaction between cytoplasmic domains

One possible mechanism that might account for an RAP-insensitive APP-LRP interaction would be an interaction between the intracellularC-terminal domains of LRP and APP. To examine this possibility,cells were transfected with APP and LRP plasmids tagged with eitherfluorescent markers (EGFP or DsRed) or myc at the C termini. Theamount of FRET was again calculated as the percentage of increasein donor fluorescence (EGFP) after acceptor (Cy3 or DsRed) photobleaching.As shown in Figure 5, strong FRET was observed between the C terminiof APP770-myc (labeled with Cy3) and LRP-EGFP (Fl_D2/Fl_D1 = 1.46± 0.0.05; mean ± SE; n = 14; p < 0.0001), suggesting the presenceof close association between the cytoplasmic domains of thesemolecules throughout the cell. The same result was obtained withAPP770-DsRed and LRP-EGFP (Fl_D2/Fl_D1 = 1.55 ± 0.05; n = 10; p< 0.0001), excluding the possibility of false positive with theuse of secondary antibodies. As a negative control, we also examinedFRET between APP770-EGFP and APP770-DsRed and found it to be absent(Fl_D2/Fl_D1 = 1.01 ± 0.005; n = 10; not significant). Cotransfectionwith RAP partially inhibited the interaction and significantlydecreased the FRET ratio of APP770-myc and LRP-EGFP (Fl_D2/Fl_D1= 1.18 ± 0.04; n = 16; p < 0.0001 compared with no RAP) but againdid not reduce the interaction to zero.

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Figure 5. Intracellular domains of APP and LRP are closely associated. H4 cells were transiently transfected with APP770-myc and LRP-EGFP expression constructs. Cells were immunostained by anti-myc antibody conjugated with Cy3. A, Cy3 (APP770) signal using 568 nm excitation. B, Discrete area of the cell was photobleached using intense 568 nm laser. C, EGFP signal (LRP) using 488 nm excitation before photobleaching. D, EGFP signal (LRP) using 488 nm excitation after photobleaching of the acceptor (Cy3) fluorophore with intense 568 nm light. An increase in donor fluorescence is observed within the discrete area that was photobleached, showing the presence of FRET. In this example, the EGFP signal increased by 40%.

We repeated the experiment using APP695 and LRP to test whether the lack of the KPI domain altered the cytoplasmic interactionbetween APP and LRP. The C terminus of APP695 had an easily detectableand strong FRET with the C terminus of LRP: APP695-myc (labeledwith Cy3) and LRP-EGFP (Fl_D2/Fl_D1 = 1.37 ± 0.06; n = 10; p < 0.0001)(Fig. 6). This ratio was not significantly different from thatof APP770. That APP695 interacts with LRP at the C termini wasalso confirmed using the APP695-DsRed and LRP-EGFP constructs(Fl_D2/Fl_D1 = 1.53 ± 0.06; n = 14; p < 0.0001). However, unlikethe APP770-LRP C-terminal interaction, the APP695-LRP C-terminalinteraction was not RAP-sensitive. Cotransfection of RAP did notaffect the FRET ratio between APP695 and LRP (for APP695-myc andLRP-EGFP, Fl_D2/Fl_D1 = 1.33 ± 0.03, n = 9 , p < 0.0001; for APP695-DsRedand LRP $---$ EGFP, Fl_D2/Fl_D1 = 1.56 ± 0.05 , n = 9, p < 0.0001).

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Figure 6. The FRET ratio increase of intracellular domain is shown as a percentage of increase of donor fluorescence between APP and LRP. The FRET ratio increase in donor fluorescence (EGFP) after photobleaching of the acceptor molecule (APP-myc) was measured. The percentage of increase in donor fluorescence was shown in the graph. FRET was present between all of the APP constructs (APP770, APP695, and APPC99) tagged at the C terminal and LRP-EGFP, the ratio being significantly above zero (p < 0.0001; one-group t test). Cotransfection of RAP significantly decreased the FRET ratio increase of APP770 (p = 0.0001; ANOVA; Fisher's PLSD post hoc test), but there was no significant effect of RAP on APP695 or APPC99-LRP interactions.

These data demonstrate that APP770 interacts with LRP at both an RAP-sensitive and an RAP-insensitive site, whereas APP695interacts with LRP only at an RAP-insensitive site. As an additionaltest of the idea that APP-LRP C-terminal interactions occur independentlyof an interaction in the extracellular domain, we constructedAPPC99-myc, which is membrane tethered but does not have an ectodomain.FRET was observed between APPC99-myc (labeled with Cy3) and LRP-EGFP(Fig. 6), although the ratio was smaller than that observed forfull-length APP (Fl_D2/Fl_D1 = 1.26 ± 0.05, for APPC99-myc and LRP-EGFP;n = 17; p < 0.0001). This value did not change after the cotransfectionof RAP (Fl_D2/Fl_D1 = 1.27 ± 0.05; n = 9; p < 0.0001). Thus, theC-terminal domain of APP, in the absence of ectodomain, mediatessignificant interactions between APP andLRP.

Interactions among APP, LRP, and Fe65

Trommsdorff et al. (1998) used pull-down assays with GST fusion proteins to show that Fe65 associates with the cytoplasmicdomain of LRP and suggested a model in which cytosolic adapterproteins such as Fe65 could interact with both APP and LRP, forminga trimeric complex. The model suggests an association of the N-terminalphosphotyrosine binding (PTB) domain of Fe65 with LRP and an associationof the C-terminal PTB of Fe65 domain with APP. We used a FRETstrategy to test this hypothesis in H4 cells. Two Fe65 fusionproteins were constructed, one containing a myc tag at the C terminus(Fe65-myc) and a second with EGFP coupled to the N terminus (EGFP-Fe65).A close interaction was observed between the C-terminally taggedFe65-myc and APP770-GFP(Fl_D2/Fl_D1 = 1.46 ± 0.08; n = 7; p < 0.0001),but a much smaller interaction was observed between the N-terminallytagged EGFP-Fe65 and APP770-DsRed or APP770-myc (Fl_D2/Fl_D1 = 1.09± 0.03; n = 10; p = 0.02) (Fig. 7). In contrast, a close interactionwas observed between the N-terminally tagged EGFP-Fe65 and LRP-myc(labeled with Cy3) (Fl_D2/Fl_D1 = 1.42 ± 0.06; n = 13; p < 0.0001),whereas a much smaller interaction was observed between the Cterminus of Fe65-myc and LRP-EGFP (Fl_D2/Fl_D1 = 1.09 ± 0.02; n= 9; p = 0.001) (Fig. 7). Because the size of the Fl_D2/Fl_D1 ratioreflects the distance between fluorophores, these data are consistentwith a close interaction of the N terminal of Fe65 with LRP andof the C terminal of Fe65 with APP and provide support for a modelin which Fe65 interacts with both LRP and APP via cytoplasmicdomain interactions.

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Figure 7. The interaction between Fe65-APP and Fe65-LRP was investigated by FRET. The interaction between Fe65-APP and Fe65-LRP was measured by FRET ratio increase after photobleaching of acceptor molecules. A close interaction was observed between C-terminally tagged Fe65 [shown as Fe65(C)] and APP770, whereas N-terminally tagged Fe65 [shown as Fe65(N)] and APP770 showed a much smaller interaction (p < 0.0001; ANOVA; Fisher's PLSD post hoc test). In contrast, C-terminally tagged Fe65 and LRP showed much less FRET than N-terminally tagged Fe65 and LRP (p < 0.0001; ANOVA; Fisher's PLSD post hoc test).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study examines cellular interactions between different isoforms of APP and LRP. We use in this study an application ofdigital confocal microscopy combined with FRET (Knowles et al.,1999; McLean et al., 2000; Rocheville et al., 2000). This providessubcellular anatomical resolution with information about protein-proteininteractions, allowing the analysis of protein domain structurewithin the context of cellular systems. Although there are limitationsto FRET (for example, the absence of FRET between two epitopescannot be taken as conclusive evidence against an interaction),FRET is a powerful tool, especially to investigate the morphologicalrelationships of the molecules, and is a complement to biochemicalanalyses, such as coimmunoprecipitation. FRET has advantages overcoimmunoprecipitation in circumstances in which indirect molecularinteractions are sought. Even using indirect immunofluorescence(i.e., taking into account the size of the antibody molecules),the greatest distance between two molecules that have detectableFRET is expected to be <30 nm. Direct interactions between fluorophoressuch as EGFP and DsRed might be expected to be detected only ifthe fluorophores are less than ~10 nm apart (Siegel et al., 2000).The FRET ratio is interpreted as a reflection of the distancebetween fluorophores, so that a larger ratio implies a closerinteraction. In this context, the presence of detectable FRETin our study indicates a close interaction between APP andLRP.

The results of the current investigation reveal several novel observations. (1) We demonstrate the presence of a strong interactionbetween the KPI-containing APP770 and LRP in cells and show thatthis interaction is partially RAP-sensitive, suggesting that itis mediated by an interaction between an extracellular LRP ligandbinding domain and APP770. (2) APP and LRP show a close appositionboth at the cell surface and in intracellular organelles, includingthe Golgi, and the interaction of APP770 and LRP is diminishedin these compartments by cotransfection with RAP, suggesting anunexpected interaction of APP and LRP in the secretory pathway.(3) We also surprisingly find an RAP-insensitive interaction betweenAPP695 (which does not contain a KPI domain) and LRP. (4) We showthat the C termini of both APP695 and APP770 and LRP can interact,even using the construct encoding truncated APP protein in whichthe extracellular domains has been deleted, suggesting a second(intracellular) site of protein-protein interaction between APPand LRP. (5) Fe65, a multidomain intracellular adapter protein,shows FRET with both APP and LRP. Together, our data support amodel of strong APP-LRP cellular contacts mediated by both directextracellular and indirect intracellular interactions (Fig. 8).

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Figure 8. This scheme shows a hypothetical model of interactions of APP, LRP, and the cytoplasmic adaptor protein Fe65. Extracellularly, there may be an interaction between the ligand binding domain of LRP and KPI domain of APP, which is RAP-sensitive. Intracellularly, Fe65 may bind both APP and LRP. We show both interactions occurring in this figure. APP binding to LRP may cause endocytosis of APP and thus modulate amyloid- $beta$ (A $beta$ ) synthesis.

Previous studies of APP-LRP interactions from our laboratory have emphasized the role of KPI containing forms of APP becausesoluble forms of APP containing the KPI domain, but not thoselacking the KPI domain, were bound and cleared by LRP (Kounnaset al., 1995). In the present study, we studied the interactionof LRP with full-length, membrane-spanning APP and examined thepossibility that LRP interacts with APP770 (a KPI-containing formof APP) or with both APP695 (which does not contain a KPI domain)and APP770. We demonstrate through a series of FRET experimentsthat there is a close apposition of the extracellular domainsof LRP and APP770. This interaction is sensitive to RAP, suggestingthat it is a classic ligand-ligand receptor interaction, albeitbetween two type I transmembrane proteins. FRET between APP andLRP can be detected both at the cell surface and also in intracellularcompartments. Interestingly, cotransfection with RAP diminishesthe APP770-LRP interaction in the endoplasmic reticulum-Golgicompartments, supporting the possibility that APP-LRP interactionsoccur in the endoplasmic reticulum-Golgi, suggesting a previouslyunsuspected interaction in the secretorypathway.

Based on the observation that secreted forms of APP695 do not bind to LRP, we expected there to be little or no interactionof APP695 with LRP (Kounnas et al., 1995). Surprisingly, however,the extracellular domains of APP695 and LRP also show a closeapproximation. This interaction is not sensitive to RAP, implyingthat the interaction is mediated by a nonligand binding domainof LRP. In fact, even constructs encoding only the C-terminalportions of APP interact with LRP, showing that APP-LRP protein-proteininteractions are mediated by two sites, one located in the ectodomain(between APP770 and LRP) and one between the cytoplasmic termini(APP695 or APP770 and LRP). We interpret these data to suggestthat interaction of the intracellular domains of APP and LRP aresufficient to bring the extracellular domains into relativelyclose proximity, even in instances in which the ligand-ligandbinding interaction either is blocked (APP770 in the presenceof RAP) or does not occur (APP695). Coimmunoprecipitation experimentsdemonstrated that both APP751 and APP695 could be pulled downwith LRP, although the former appeared to have a fourfold strongerassociation (Rebeck et al., 2001). In the light of our currentdata, we hypothesize that, in H4 cells, APP770 interacts withLRP via an ectodomain binding site, as well as via an interaction,possibly indirect, occurring within the cytoplasmic domains ofthese two molecules. In contrast, APP695 seems to interact withLRP only via the intracellularinteraction.

Yeast two-hybrid and isolated protein pull-down experiments (Trommsdorff et al., 1998) suggested a model in which the intracellularportion of APP might interact with LRP via a trimeric complexwith Fe65, an intracellular adapter protein. Fe65 contains threedistinct interaction domains: one WW and two PTB domains. TheWW domain of Fe65 interacts with several proteins, one of whichis Mena, the mammalian ortholog of the product of the enabledgene of Drosophila (Ermekova et al., 1997). The N-terminal PTBdomain interacts with LRP (Trommsdorff et al., 1998), and theC-terminal PTB domain interacts with APP (Fiore et al., 1995;Borg et al., 1996; Guenette et al., 1996; Trommsdorff et al.,1998) in isolated systems. Our data showing strong FRET betweenthe N terminus of Fe65 and LRP and the C terminus of Fe65 andAPP (but weaker FRET between the N terminus of Fe65 and APP orthe C terminus of Fe65 and LRP) support the idea that these interactionsare robust in cells. Our data do not rule out the possibilitythat other adapter proteins might also mediate an APP-LRP cytosolictail interaction and even that different cell types or tissuesmay differ in endogenous adapter protein complement. For example,preliminary studies using CHO cells suggest a lesser degree ofAPP-LRP C-terminal interaction than seen in H4cells.

Our previous studies of APP-LRP interactions in CHO cells suggested that either genetic deletion of LRP or exogenous RAP treatmentcould markedly diminish amyloid- $beta$ production from APP770-transfectedcells but not from APP695-transfected cells (Ulery et al., 2000).Our current studies showed that there is an RAP-sensitive, KPIdomain-dependent interaction between APP and ligand binding sitesin the LRP ectodomain. Together, we hypothesize that this ectodomaininteraction alters the endocytic process to influence amyloid- $beta$ generation in the endocytic pathway. Specific analysis of APP-LRPinteractions during endocytosis for APP695 and APP770 will bethe target of futurestudies.

  FOOTNOTES

Received May 14, 2001; revised July 27, 2001; accepted Aug. 17, 2001.

This work was supported by National Institutes of Health Grants AG12406 (B.T.H.), AG14473 (G.W.R.), and HL50784 (D.K.S.).A.K. was supported by the Uehara MemorialFoundation.
Correspondence should be addressed to Dr. Bradley T. Hyman, Alzheimer Research Laboratory, Massachusetts General Hospital,114 16th Street, Room 2009, Charlestown, MA 02129. E-mail: b_hyman{at}helix.mgh.harvard.edu.

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