c-Jun N-Terminal Kinase (JNK)-Interacting Protein-1b/Islet-Brain-1 Scaffolds Alzheimer's Amyloid Precursor Protein with JNK

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (116)

Citing Articles via Google Scholar

Google Scholar

Articles by Matsuda, S.

Articles by Nishimoto, I.

Search for Related Content

PubMed

PubMed Citation

Articles by Matsuda, S.

Articles by Nishimoto, I.

Pubmed/NCBI databases
Gene GEO Profiles
HomoloGene Protein
UniGene
Compound via MeSH
Substance via MeSH
Medline Plus Health Information
Alzheimer's Disease

Previous Article  |  Next Article

The Journal of Neuroscience, September 1, 2001, 21(17):6597-6607

c-Jun N-Terminal Kinase (JNK)-Interacting Protein-1b/Islet-Brain-1 Scaffolds Alzheimer's Amyloid Precursor Protein with JNK
Shuji Matsuda¹, Takashi Yasukawa¹, Yasuko Homma¹, Yuko Ito¹, Takako Niikura¹, Takako Hiraki¹, Shuichi Hirai², Shigeo Ohno², Yoshiko Kita¹, Masaoki Kawasumi¹, Keisuke Kouyama¹, Tokuo Yamamoto³, John M. Kyriakis⁴, and Ikuo Nishimoto¹
¹ Department of Pharmacology and Neurosciences, KEIO University School of Medicine, Shinjuku-ku, Tokyo 160-8582, Japan, ² Department of Molecular Biology, Yokohama City University School of Medicine, Kanazawa-ku, Yokohama 236-0004, Japan, ³ Tohoku University Gene Research Center, Aoba-ku, Sendai 981-8555, Japan, and ⁴ Diabetes Research Laboratory, Massachusetts General Hospital-East, Charlestown, Massachusetts 02129

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Using a yeast two-hybrid method, we searched for amyloid precursor protein (APP)-interacting molecules by screening mouseand human brain libraries. In addition to known interacting proteinscontaining a phosphotyrosine-interaction-domain (PID) $---$ Fe65, Fe65L,Fe65L2, X11, and mDab1, we identified, as a novel APP-interactingmolecule, a PID-containing isoform of mouse JNK-interacting protein-1(JIP-1b) and its human homolog IB1, the established scaffold proteinsfor JNK. The APP amino acids Tyr⁶⁸², Asn⁶⁸⁴, and Tyr⁶⁸⁷ in the G⁶⁸¹YENPTY⁶⁸⁷ region were all essential for APP/JIP-1b interaction, but neitherTyr⁶⁵³ nor Thr⁶⁶⁸ was necessary. APP-interacting ability was specific for thisadditional isoform containing PID and was shared by both humanand mouse homologs. JIP-1b expressed by mammalian cells was efficientlyprecipitated by the cytoplasmic domain of APP in the extreme Gly⁶⁸¹-Asn⁶⁹⁵ domain-dependent manner. Reciprocally, both full-length wild-typeand familial Alzheimer's disease mutant APPs were precipitatedby PID-containing JIP constructs. Antibodies raised against theN and C termini of JIP-1b coprecipitated JIP-1b and wild-typeor mutant APP in non-neuronal and neuronal cells. Moreover, humanJNK1 $beta$ 1 formed a complex with APP in a JIP-1b-dependent manner.Confocal microscopic examination demonstrated that APP and JIP-1bshare similar subcellular localization in transfected cells. Thesedata indicate that JIP-1b/IB1 scaffolds APP with JNK, providinga novel insight into the role of the JNK scaffold protein as aninterface of APP with intracellular functionalmolecules.

Key words: JIP-1b/IB1; amyloid precursor protein; phosphotyrosine-interaction-domain; scaffolding protein; c-Jun N-terminal kinase

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alzheimer's disease (AD) is the most prevalent neurodegenerative disease pathologically characterized by senile plaques inthe brain. The major constituent of the plaques is A $beta$ , cleavedoff from the transmembrane precursor, termed amyloid precursorprotein (APP). Genetic studies of familial AD (FAD) (Hardy, 1992)demonstrated that structural alterations in APP cause AD, basedon the finding that certain FAD patients carry V642I/F/G mutationsor an NL mutation (K595N/M596L) in APP₆₉₅, a 695 residue version(Kang et al., 1987). However, how these mutations cause pathophysiologyin AD and how wild-type APP (wt APP) contributes to normal functionshave been little understood. Yet multiple studies (Qiu et al.,1995; Coulson et al., 1997; Gillian et al., 1997; Perez et al.,1997) have shown that wt APP performs physiological functionson the surface of neurons relevant to neurite outgrowth, neuronaladhesion, and axonogenesis, aside from its pathological role asan A $beta$ precursor. Rohn et al. (2000) and Sudo et al. (2000) independentlyfound that anti-APP antibody treatment causes death in neuronalcells. Consistently, considerable amounts of APP are found onthe surface of neurons (Jung et al., 1996; Brouillet et al., 1999;Sudo et al., 2000).

Parallel to these studies on wt APP, FAD-associated V642 mutants of APP have been shown to induce neuronal apoptosis (Wolozinet al., 1996; Yamatsuji et al., 1996a; Zhao et al., 1997; Luoet al., 1999). Toxicity by FAD mutants of APP and presenilin (PS)-2is most likely a controllable process, mediated by pertussis toxin(PTX)-sensitive G-proteins (PG) (Wolozin et al., 1996; Yamatsujiet al., 1996a,b; Giambarella et al., 1997; Hashimoto et al., 2000).Furthermore, V642I-specific toxicity does not occur when APP lacksthe His⁶⁵⁷-Lys⁶⁷⁶ region, termed Domain 20 (Yamatsuji et al., 1996a,b; Hashimotoet al., 2000). Okamoto et al. (1995, 1996) showed in vitro thatwt APP and V642I-APP exert antibody-dependent and constitutivePG-activating functions, respectively, both through Domain 20.Sudo et al. (2000) confirmed that cell-surface wt APP triggersneuronal death antibody dependently in a PTX-sensitive manner.These findings suggest that APP, through PG, performs signalingfunctions mediated by Domain20.

On the other hand, the study of Murayama et al. (1996) suggested that wt APP could also trigger PTX-resistant signaling pathways.Consistently, Hashimoto et al. (2000) found that FAD-associatedNL mutant of APP not only exerted PTX-sensitive toxicity throughDomain 20 but also exerted PTX-resistant neurotoxicity throughthe Met⁶⁷⁷-Asn⁶⁹⁵ region, termed Domain 19. These findings suggest that APP hasa PG-independent signaling function mediated by Domain 19. Inaccord with this idea, Lu et al. (2000) found that the Ala⁶⁶⁵-Asn⁶⁹⁵ peptide, the C-terminal fragment generated through APP cleavageby caspases, is cytotoxic. This study was thus conducted to investigatehow the C terminus of APP can contribute to the regulation ofintracellular signals. Here we report a novel function of APPto interact with JIP-1b/IB1, which provides the scaffold withc-Jun N-terminal kinase(JNK).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Oligonucleotides. The nucleotide sequences of oligonucleotides used were as follows: SM60, 5'-aattttacccatatgatgtgccagattatgcctctcccgaattcggatccc-3';SM61, 5'-tcgagggatccgaattcgggagaggcataatctggcacatcatatgggtaa-3';SM71, 5'-gatccgaattcgcggccgcgtcgactctagactcgagaagctt-3'; SM72,5'-aattaagcttctcgagtctagagtcgacgcggccgcgaattcg-3'; SM74, 5'-ggccgaattccgcaagaagaaaccctatgg-3';SM78, 5'-agctccgccatgggatacccttatgatgtgccagattatgccggatccccggaattc-3';SM79, 5'-ctaggaattccggggatccggcataatctggcacatcataagggtatcccatggcgg-3';SM108, 5'-ggccgaattcaagatggatgcagagttcggacatgattcaggatttgaag-3';SM109, 5'-ggccgaattcaagaagaaacagtacacatccatcc-3'; SM110, 5'-ggccctcgagttagttctgcatttgctcaaagaacttg-3';SM121, 5'-ggccgaattcaggaagaggcagtacgg-3'; SM122, 5'-ggccctcgagttaaatctgcatctgctccagg-3';SM123, 5'-ggccctcgagtcagttctgctgcatcttggag-3'; SM124, 5'-gaattcaagaagaaacaggccacatccatccatcatg-3';SM125, 5'-cgccgccgtggaaccagaggagc-3'; SM126, 5'-gatgcagcagaacggaggtgagaatccaacttac-3';SM127, 5'-gcagaacggatatgaggctccaacttacaagttc-3'; SM132, 5'-cggatatgagaatccaactgccaagttctttgagc-3';SM138, 5'-ggccgaattcagcgactggattgaccag-3'; SM139, 5'-ggccctcgagctactccaagtagatatcttctg-3';SM143, 5'-gcagcccttgccaaaaacagctgtgtccttgagatcag-3'; SM241, 5'-gcctcgagtcaagcatccagacacttctggt-3';and SM242, 5'-gcggatccttcgctgtgcgctcc-3'.

Plasmid construction. The sequences of all constructs were verified by dideoxy-termination using ABI310 sequencer (PE AppliedBiosystems, Foster City, CA). PCR inserts were amplified by deepvent DNA polymerase (New England Biolabs, Beverly, MA) or KODDNA polymerase (Toyobo, Osaka, Japan). Mouse brain cDNA used forRT-PCR was prepared from total RNA of ICR adult mouse, isolatedusing an RNeasy kit (Qiagen GmbH, Hilden, Germany) and reversetranscribed using Superscript II and an Oligo-dT primer (LifeTechnologies Oriental, Tokyo, Japan). pEG202-NLS polylinker portionwas exchanged with the corresponding EcoRI-XbaI fragment of pEG202;then hemagglutinin (HA) epitope, encoding YPYDVPDYA, was insertedbetween EcoRI and XhoI using linkers SM60/SM61 (pEG202-NLS-HA).The coding sequences of APP, APLP1, and APLP2 and their variantswere PCR amplified and cloned into pEG202 and pEG202-NLS-HA usingEcoRI/XhoI. APP fragments were amplified from mouse APP₆₉₅ withthe following primers: APP_649-695, SM109/SM110; APP_595-695,SM108/SM110; and APP_649-680, SM109/SM123. The cytoplasmicdomain of APLP1 (APLP1_607-653) was amplified with PCR fromAPLP1 plasmid obtained in another two-hybrid screening using SM74.The cytoplasmic domain of APLP2₇₅₁ (APLP2_705-751) was clonedby RT-PCR using primers SM121/SM122. The point mutants of cytoplasmicdomain fragments of APP were constructed by PCR-directed mutagenesisof APP_649-695 and APP_649-680 and cloned into pEG202and pEG202-NLS-HA using the following primers: Y653A, SM124; T668E,SM125; Y682G, SM126; N684A, SM127; and Y687A, SM132, respectively.Among the prey fusion plasmids used in the interaction mating,JIP-1_493-660 was PCR constructed from JIP-1b_493-707using SM143. JIP-1b_557-707 was PCR constructed using primesSM138/SM139. Other prey fusions were directly cloned in the screening.All prey fusions were cloned into EcoRI/XhoI of pJG4-5.

JIP-1b was cloned by RT-PCR and cloned into KpnI/XbaI of pcDNA3.1-HisA (Invitrogen, Carlsbad, CA) (T7-JIP-1b). JIP-1 constructswere created using the prey fusion of JIP-1_493-660 and T7-JIP-1b.T7-JIP-1b_1-272 was constructed by deleting XhoI fragmentfrom T7-JIP-1b. In constructing T7-JIP1_271-660, T7-JIP-1b_365-707,and T7-JIP-1_365-660, corresponding fragments were clonedinto pcDNA3.1-HisC (Invitrogen). pcDNA3 (Invitrogen) was modifiedusing linkers SM78/SM79 and SM71/SM72 to insert Kozak's consensussequence followed by HA epitope MGYPYDVPDYAGSP. IB1_360-711was cloned into the EcoRI/XhoI site of this vector (HA-IB1_360-711).pGEX-2T (Amersham Pharmacia Biotech, Uppsala, Sweden) polylinkerwas modified by the insertion of the linker SM71/SM72, using BamHI/EcoRI(pGEX-2Tm). Glutathione S-transferase (GST)-fusion proteins usedfor bacterial protein expression were constructed by cloning thesame PCR inserts used for yeast bait vectors in EcoRI/XhoI ofpGEX-2Tm. Full-length mouse wt APP and its FAD mutants were clonedinto pEF-BOS (Mizushima and Nagata, 1990).

Corresponding portions of IB1, JIP-1b, and JIP-1 were cloned into pEBG (Sanchez et al., 1994), a mammalian expression vectorof GST, in constructing GST-IB1_360-711, GST-JIP-1b_493-707,and GST-JIP-1b_540-707. pEBG without insert was used as GSTcontrol. GST-JNK1 $beta$ 1 was constructed by cloning the BglII fragmentof SRHis-JNK1 $beta$ 1 (Hirai et al., 1996) into the BamHI site ofpEBG.

Corresponding portions of JIP-1b, mDab1, and X11, obtained in the two-hybrid screening, were cloned into pET28(a) (JIP-1band mDab1) or pET28(c) (X11) (Novagen, Madison, WI). The regioncontaining two PIDs of Fe65 was PCR amplified from a Fe65 cloneobtained in the screening using SM241/SM242 and cloned into pET28(a).These pET constructs were used to produce His-tagged JIP-1b_493-707,His-tagged mDab1_2-217, His-tagged X11_37-680, and His-taggedFe65_370-662,respectively.

Antibodies. Anti-T7 antibody (Novagen), anti-HA antibody (12CA5: Roche Diagnostics, Basel, Switzerland), anti-APP antibody(22C11: Roche Diagnostics), and anti-GST antibody (MAB2510: UpstateBiotechnology, Lake Placid, NY) were used for immunoblotting.Rabbit antisera were raised for CGGAASPPAASPFLGLHIASPPNFR correspondingto residues 10-33 of JIP-1b ( $alpha$ JIPN) and RAFQQFYKQFVEYTCPTEDIYLEcorresponding to residues 685-707 of JIP-1b ( $alpha$ JIPC).

Yeast two-hybrid method. A LexA yeast two-hybrid system was purchased from OriGene Technologies (Rockville, MD). Yeast two-hybridscreening was performed according to standard procedures (Ausubelet al., 1999), using the yeast transformation method of Gietzand Schiestl (1995). All bait constructs of APP and its mutantsfailed to activate LEU2 or LacZ reporters. EGY48 (MAT $alpha$ , trp1,his3, ura3, leu2:: 6 ops-LEU2) was used for the screening withpEG202-NLS-HA- APP_595-695, and EGY188 (MAT $alpha$ , trp1, his3,ura3, leu2:: 2 ops-LEU2) was used for pEG202-NLS-HA-APP_649-695.pSH18-34 (Ausubel et al., 1999) was used for the LacZ reporter.The positive control bait was pSH17-4 (GAL4 activation domainfused to LexA), and the negative control baits were pRFHM1 (homeodomainof bicoid fused to LexA) and pEG202-Max (Max fused to LexA), providedin the kit. The human adult AD patient library was constructedusing the method of Gubler and Hoffman (1983), using cDNA obtainedfrom a brain of a patient diagnosed as having AD by necropsy,according to institutional guidelines. The mouse adult brain librarywas purchased from Clontech (Palo Alto, CA). Yeast strains werecultured on YPAD plates, or on minimal plates with these combinationsof the following conditions: containing glucose (SD plates), orcontaining galactose and raffinose (Gal plates), or containing5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside (X-gal), or lackingthe combinations of histidine (-his), uracil (-ura), tryptophan(-trp), or leucine (-leu), as described in Ausubel et al. (1999).To extract yeast proteins, cells with the same optical densitywere collected and suspended with 2× sample buffer, frozen, andthen boiled, according to the protocol of Ausubel et al. (1999).Yeast interaction mating was performed according to the methodsof Finley and Brent (1994) and Meroni et al. (1997). Briefly,the bait constructs were transformed into RFY206 (MATa, trp1 $Delta$ ::hisG, his3 $Delta$ 200, ura3-52, leu2-3, lys2 $Delta$ 201) simultaneously withthe LacZ reporter and grown as patches on SD-his-ura plates. Thevarious fragments of genes cloned into pJG4-5 prey vectors weretransformed into EGY48 and grown as lawns on SD-trp plates. Themating was performed as follows. On the first day, the patchesof RFY206 bait transformants and the lawns of EGY48 prey transformantswere replica plated on the same YPAD plates. The next day, themated yeast on the YPAD plates was replica plated on SD-his-ura-trp-leuand Gal-his-ura -trp-leu plates and incubated for an additional48 hr to monitor cell growth reflecting galactose-induced LEU2reporter activity, and on SD-his-ura-trp plates to select themated yeast. On the third day, the patches grown on the replicaplated SD-his-ura-trp plates were again replica plated on SD (X-gal)-his-ura-trpand Gal (X-gal)-his-ura-trp plates and incubated an additional24 hr to monitor galactose-induced LacZ reporteractivity.

Bacterial protein production and purification. GST fusion proteins were expressed using BL21-Gold (Stratagene, La Jolla, CA)and purified with glutathione Sepharose 4B (Amersham PharmaciaBiotech), according to the manufacturer's protocol. The purifiedproteins were dialyzed three times against 100 vol of buffer A(20 mM Tris/HCl, pH 8.0, 1 mM DTT, 1 mM EDTA), and frozen at $-$ 80°Cuntil use. His-tagged proteins were expressed using BL21(DE3)(Novagen) and purified with Chelating Sepharose Fast Flow (AmershamPharmacia Biotech) loaded with NiSO₄, according to the manufacturer'sprotocol. The purified proteins were dialyzed against buffer Aand frozen until use, asabove.

Transfection and cell lysate. COS7 cells (1 × 10⁶) were seeded in 10 cm dishes the day before the transfection in high-glucoseDMEM supplemented with 10% fetal bovine serum (FBS), 100 U/mlof penicillin, and 100 µg/ml of streptomycin sulfate. The cellswere transfected with 6 µg of DNA using DEAE-dextran. NT2 cells(Stratagene), human neuronal precursor cells, were seeded at 1× 10⁶ in 10 cm dishes the day before the transfection in 50% DMEM,50% Ham's F-12 supplemented with 10% FBS, 100 U/ml of penicillin,100 µg/ml of streptomycin, and 2 mM L-glutamine. They were thentransfected with 12 µg of DNA using LipofectAMINE (Life TechnologiesOriental).

Forty-eight hours after the initiation of transfection, the cells were washed once with PBS, lysed for 30 min at 4°C in bufferB [20 mM HEPES/NaOH, pH 7.4, 1 mM DTT, 1 mM EDTA, 150 mM NaCl,0.5% (w/v) Triton X-100], supplemented with 10% (v/v) glycerol,1 mM phenylmethylsulfonylfluoride, 10 µg/ml of aprotinin, and10 µg/ml of leupeptin with occasional gentle shaking. The lysedcells were collected and centrifuged at 20000 × g for 15 min,and cleared lysates were used for furtheranalysis.

Bacterial GST pull-down. In pull-down experiments using His-tagged proteins, 6 µg of GST-fusion protein was incubated with20 µl of glutathione beads in a total volume of 0.5 ml of bufferA for 1 hr at 4°C and washed once with buffer C [20 mM Tris/HCl,pH 7.4, 1 mM DTT, 1 mM EDTA, 150 mM NaCl, 0.1% (w/v) Triton X-100].His-tagged proteins of various concentrations were adjusted to150 mM NaCl and 0.1% Triton X-100, mixed with beads immobilizingGST-fusion protein for 2 hr at 4°C with rotation, and washed threetimes with buffer C. The washed beads were mixed with 90 µl of1× sampling buffer, boiled, and subjected to immunoblotting andCoomassie brilliant blue (CBB) staining. In the pull-down experimentsusing COS cell lysate, 30 µg of GST fusion proteins were immobilizedon 30 µl of glutathione beads as above, and washed once with bufferB. Lysates (0.5 mg protein) were incubated with the beads immobilizingGST-fusion protein for 2 hr at 4°C with rotation, and washed threetimes with buffer B. The washed beads were mixed with 90 µl of1× sample buffer, boiled, and subjected to further analysis asabove.

Immunoprecipitation. Cell lysates (0.5 mg protein) were incubated with $alpha$ JIPN or $alpha$ JIPC or corresponding preimmune sera for1 hr at 4°C, and mixed with 10 µl of Protein G-Sepharose 4 FastFlow (Amersham Pharmacia Biotech) for an additional 1 hr withrotation at 4°C. Immunocomplexes were washed three times withbuffer B, boiled in 1× sample buffer, and subjected toimmunoblotting.

Immunoblotting. Protein samples were submitted to SDS-PAGE, transferred to nitrocellulose membranes (BA85; Schleicher & Schuell,Dassel, Germany) using a semidry system, and blocked overnightwith TBS (50 mM Tris/HCl, pH 7.5, 200 mM NaCl) plus 5% skim milk.The membranes were incubated 1 hr at room temperature with theprimary antibodies or antisera diluted in the same buffer, andthen washed five times with TBS containing 0.05% Tween 20. Thesecondary antibodies, horseradish peroxidase-conjugated anti-rabbitgoat polyclonal antibody (Bio-Rad, Hercules, CA) and horseradishperoxidase-conjugated anti-mouse rabbit polyclonal antibody (Bio-Rad),were diluted in TBS containing 5% skim milk. After washing, themembranes were visualized using an ECL kit (Amersham PharmaciaBiotech) and developed using x-ray films (Fujifilm, Tokyo,Japan).

Cell staining. COS cells (3 × 10⁵) were seeded in 60 mm dishes on the previous day and transfected with 2 µg of plasmids usingLipofectAMINE (Life Technologies Oriental), and reseeded on coverslipsthe next day. Forty-eight hours after the initiation of the transfection,cells were fixed with 0.1 M phosphate buffer, pH 7.4, containing4% paraformaldehyde for 20 min at room temperature. After extensivewashing with PBS, the fixed cells were incubated with $alpha$ JIPN, $alpha$ JIPC,preimmune sera, anti-APP antibody (22C11), or mouse IgG (CortexBiochem, San Leandro, CA) in PBS containing 3% BSA and 0.1% TritonX-100 overnight at 4°C, and visualized by goat fluorescein isothiocyanate(FITC)-conjugated anti-rabbit IgG or horse Texas Red-conjugatedanti-mouse IgG (Vector Laboratories, Burlingame, CA) in PBS containing3% BSA. DNA was stained by incubating coverslips in PBS containing0.2 µM 2'-[4-ethoxyphenyl]-5-[4-methyl-1-piperazinyl]-2,5'-bi-1H-benzimidazole(Hoechst 33342; Sigma-Aldrich Japan, Tokyo, Japan), and washedfive times with PBS. Coverslips were mounted to slides with Vectashield(Vector Laboratories). Digital images were taken with an LSM310laser scanning microscope (Carl Zeiss, Jena,Germany).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Screening of molecules interactive with cytoplasmic domains of APP

Twenty million transformants of an adult mouse brain library were screened with the transmembrane plus cytoplasmic domainAPP_595-695 and the cytoplasmic domain APP_649-695 (Fig.1A). All retransformation-positive clones carried a PID (Kavanaughand Williams, 1994; Bork and Margolis, 1995; Kavanaugh et al.,1995) that was implicated in the binding to the NPXY motif. Inaddition to known APP-binding proteins $---$ such as Fe65 (Fiore etal., 1995), Fe65L (Guenette et al., 1996), Fe65L2 (Duilio et al.,1998), X11 (Borg et al., 1996), and mDab1 (Trommsdorff et al.,1998) $---$ a novel APP-interacting protein was found to be JIP-1b (Whitmarshet al., 1998; Kim et al., 1999), a PID-containing form of JIP-1(Dickens et al., 1997).

View larger version (26K):
[in this window]
[in a new window]
Figure 1. The bait used and clones recovered in the two-hybrid screening. A, An illustration of the regions of mouse APP₆₉₅ used as bait. APP_595-695 starts from the two amino acids Lys⁵⁹⁵-Met⁵⁹⁶, mutated to Asn-Leu in the Swedish type of FAD. APP_649-695 encodes the entire cytoplasmic domain of APP, the amino acid sequence of which is conserved between human and mouse APP. The $alpha$ -, $beta$ -, and $gamma$ -secretase cleavage sites are also indicated. B, The clones recovered from the screening and the domain organization of mouse JIP-1b and its human homolog IB1. The portions coded by the recovered plasmids are indicated as lines with their amino acid positions in parentheses. The boxes indicate JNK binding domain (JBD), src-homology region 3 (SH3), and PID, with their amino acid positions in numbers.

Because the recovered plasmids from the two different series of screening were almost identical, and APP_649-695 showedstronger interaction with PID-containing clones than APP_595-695in a two-hybrid assay (data not shown), the human adult brainlibrary of an AD patient was screened only with APP_649-695.After screening 14 million transformants, we found three interactingmolecules: Fe65, X11L (Tomita et al., 1999), and IB1 (Bonny etal., 1998). X11L is the homolog of mouse X11 (Tomita et al., 1999),and IB1 is the human homolog of mouse JIP-1b (Bonny et al., 1998).Because JIP-1b and IB1 were novel APP-interacting proteins, andcloned from both the adult mouse brain library and the human patientbrain library, we further analyzed JIP-1b/IB1 in this study. Theregions encoded by the recovered JIP-1b/IB1 plasmids are indicatedin Figure 1B.

Requirement of PID in JIP-1b/IB1 and Y⁶⁸², N⁶⁸⁴, and Y⁶⁸⁷ in G⁶⁸¹YENPTY⁶⁸⁷ of APP

To determine the critical amino acids necessary for interaction of JIP-1b/IB1 with the APP cytoplasmic domain, various APPmutants (Fig. 2A) were constructed in both pEG202 and pEG202-NLS-HAbait vectors and transformed into RFY206 with LacZ reporter pSH18-34.When the transformants of pEG202-NLS-HA fusions were submittedto immunoblot analysis using anti-HA antibody, a single immunoreactiveband corresponding to the expected size of the bait fusions wasdetected in each lane of transformants (Fig. 2B). Various JIP-1b/IB1fusions in the prey vector pJG4-5 (Fig. 2D) were transformed intoan EGY48 yeast strain. The array of two patches of each RFY206bait transformant harboring the bait constructs (Fig. 2C) wasmated with the lawns of EGY48 prey transformants, and the matedcells were grown on minimal medium containing glucose or galactoseand lacking histidine, uracil, tryptophan, and leucine, to assaygalactose-induced LEU2 reporter activity, as shown in Figure 2D.

View larger version (38K):
[in this window]
[in a new window]
Figure 2. Requirement of both PID of JIP-1b/IB1 and G⁶⁸¹YENPTY⁶⁸⁷ of APP for JIP-1b/IB1 interaction with APP. A, The indicated amino acid residues were changed by site-directed mutagenesis. APP_649-695 and APP_649-680 are designated as cyt and $Delta$ NPTY, respectively. The G⁶⁸¹YENPTY⁶⁸⁷ region is boxed. B, Proteins of RFY206 yeast cells transformed with fusions of various mutants of the APP cytoplasmic domain were probed with anti-HA antibody. The bait fusions used are identified under each lane. Their designations are as described in A. The numbers on the left are the relative molecular weights of the size markers in kilodaltons. C, Two patches of each bait fusion transformant of the RFY206 strain were arranged as indicated. The names of APP bait variants are described in A. Two negative controls (pRFHM1 and pEG202-Max) and a positive control (pSH17-4) are also included. D, Interaction-mating of APP variants and JIP-1b/IB1 or other prey fusions. The left column of pictures shows the growth of mated yeast cells on glucose plates (Glucose), and the right column shows the growth of mated yeast cells on galactose and raffinose (Galactose) plates, as described in Materials and Methods. Galactose-dependent LEU2 activity was displayed by the difference in the growth of the mated cells between that in the glucose plates, which suppress the expression of the prey fusions, and that in the galactose plates, which induce it. The two negative controls (pRFHM1, pEG202-Max) showed no growth in any combination. The prey fusions are indicated at the right of the columns. The illustration of the fusions indicates the regions coded by the cDNA and the constructs as thin and thick lines, respectively. The first and last amino acids of cDNA and regions encoded by the constructs are indicated, except for mDab1_2-217, which starts at the second codon. PID regions were indicated as black boxes, except for JIP-1_493-660, which has incomplete PID. APP residues critical for the interaction are noted at the right side, except for JIP-1_493-660, which displayed no interaction with any APP variants. The GenBank accession numbers and amino acids corresponding to the PIDs were IB1, NM005456, 557-711; JIP-1b, AF054611, 557-707; JIP-1, AF003115, no PID; Fe65, AF206270, 364-505 and 535-660; X11, L34676, 297-460; mDab1, Y08381, 37-175. L34676 is a partial clone that lacks N-terminal 69 amino acids in its human or rat counterpart.

The fusions of IB1_360-711, JIP-1b_493-707, JIP-1b_540-707, and JIP-1b_557-707, all of which contain intactPID, interacted with APP_649-695 (cyt) and its Y653A andT668E mutants [cyt (Y653A), cyt (T668E)]. In contrast, no interactionwas observed with the other mutants of APP_649-695 [cyt (Y682G),cyt (N684A), and cyt (Y687A)] or APP_649-680 ( $Delta$ NPTY), norwith any of its mutants [ $Delta$ NPTY (Y653A), $Delta$ NPTY(T668E)] (Fig. 2D).This indicates that (1) the extreme C-terminal 15 amino acidsof APP harboring G⁶⁸¹YENPTY⁶⁸⁷ are necessary for the interaction of JIP-1b/IB1 with APP; (2)Tyr⁶⁸², Asn⁶⁸⁴, and Tyr⁶⁸⁷, contained in this region, are all critical for this interaction;and (3) the 151 amino acid PID region contained in the shortestconstruct, JIP-1b_557-707, is sufficient for the interactionwith APP. In further support of this observation, the fusion ofJIP-1_493-660, which is equivalent to the JIP-1b_493-707lacking 47 amino acids in the PID region, exhibited no interactionwith the cytoplasmic domain of wt APP or APP mutants (Fig. 2D).This observation suggests that the PID region was sufficient andnecessary for the interaction of JIP-1b withAPP.

Other PID-containing fusions obtained in the same screening were also examined for their ability to interact with cytoplasmicdomain mutants of APP, as shown in Figure 2D. Fe65_254-708,X11_37-680, and mDab1_2-217 all displayed G⁶⁸¹YENPTY⁶⁸⁷-dependent interaction with the cytoplasmic domain of APP, asevidenced by their positive interaction with cyt, cyt (Y653A),and cyt (T668E), and their negative interaction with $Delta$ NPTY, $Delta$ NPTY(Y653A), and $Delta$ NPTY (T668E) (Fig. 2D). However, the critical APPresidues necessary for the interactions were different in thethree constructs. Fe65_254-708 required Tyr⁶⁸², but not Asn⁶⁸⁴ or Tyr⁶⁸⁷; X11_37-680 required Tyr⁶⁸² and Asn⁶⁸⁴, but not Tyr⁶⁸⁷; mDab1_2-217 required Tyr⁶⁸² and Asn⁶⁸⁴, as well as Tyr⁶⁸⁷, the same residues necessary for JIP-1b/IB1 constructs containingPID (Fig. 2D). Therefore, in this experiment, the mode of APPinteraction with JIP-1b/IB1 was distinct from that with Fe65 andX11, but indistinguishable from that withmDab1.

These observed interactions were confirmed by replica-plating the mated yeast cells to minimal plates, containing X-gal, andcontaining glucose or galactose, and lacking histidine, uracil,and tryptophan. The LacZ reporter activity visualized by the bluecolor development displayed the same patterns as in Figure 2D(data not shown). The same set of cytoplasmic domain mutants ofAPP fused to pEG202 bait vector displayed the same results asthose of pEG202-NLS-HA fusion constructs (data not shown). Thesedata indicate that JIP-1b/IB1 interacts with APP in a manner distinctfrom already known interactions of Fe65 or X11 with APP, and bothPID of JIP-1b/IB1 and the G⁶⁸¹YENPTY⁶⁸⁷ region of APP, especially Tyr⁶⁸², Asn⁶⁸⁴, and Tyr⁶⁸⁷, are essential for theinteraction.

Purified JIP-1b protein binds to the cytoplasmic domain of APP with affinity comparable to that of mDab1, X11, and Fe65

To compare the binding affinity of JIP-1b PID with that of other PID-containing proteins, His-tagged JIP-1b_493-707,which contains a part of SH3 domain and the entire PID (the sameregion illustrated in Fig. 2D), was expressed in bacteria, purified,and subjected to pull-down experiments using bacterially producedrecombinant APP cytoplasmic domain fused to GST (GST-cyt). His-taggedJIP-1b at various concentrations was mixed with glutathione beadsimmobilizing an equivalent amount of GST-cyt, and each precipitant(ppt) was probed for GST-cyt by CBB staining (Fig. 3A, top panel),and for the bound His-tagged protein by immunoblotting using anti-T7antibody (Fig. 3A, bottom panel). A similar amount of GST-cytwas detected in all precipitants (Fig. 3A). When the bound His-taggedJIP-1b was plotted against the concentration used for the bindingexperiment, the bound protein showed saturable binding to GST-cytwith half-maximal binding at ~0.4 µM (Fig. 3A). His-tagged JIP-1bdid not bind to GST at all concentrations tested, indicating thatthe binding of His-tagged JIP-1b to GST-cyt is specific (datanot shown).

View larger version (35K):
[in this window]
[in a new window]
Figure 3. Purified JIP-1b binds to the cytoplasmic domain of APP with affinity comparable to those of other PID-containing proteins. A, His-tagged JIP-1b_493-707, at the concentrations indicated under each lane, was precipitated with glutathione beads immobilizing the APP cytoplasmic domain fused to GST (GST-cyt). Precipitated GST-cyt was visualized with CBB staining (top panel), and bound His-tagged JIP-1b_493-707 in the precipitants was detected with anti-T7 antibody (bottom panel). The numbers on the left are the relative molecular weights of the size markers in kilodaltons. The bound JIP-1b, calculated from the pixels of scanned image and a standard curve, was plotted against the concentration of JIP-1b used for the binding. B, Similar experiments were performed using His-tagged mDab1_2-217. The bands corresponding to mDab1 are faintly visible in CBB staining (top panel). C, Similar experiments were performed using His-tagged X11_37-680. D, Similar experiments were performed using His-tagged Fe65_370-662. The bands corresponding to Fe65 are visible in CBB staining (top panel). E, CBB staining of the purified His-tagged proteins used.

Similar experiments were performed using His-tagged mDab_2-217 (the same region illustrated in Fig. 2D), His-tagged X11_37-680(the same region illustrated in Fig. 2D), and His-tagged Fe65_370-662(the region containing its two PIDs). Again, a similar amountof GST-cyt was detected in all precipitants (Fig. 3B-D, top panels).When the bound PID-containing proteins were plotted against theirconcentration used for the binding, the binding curves showedsaturable binding with the concentration of mDab1, X11, and Fe65required for their half-maximal binding at ~0.5, 0.5, and 0.15µM, respectively (Fig. 3B-D). None of these His-tagged proteinsbound to GST at any of the concentrations tested, which confirmedthe specificity of their binding (data not shown). The purityof the recombinant proteins used for these binding experimentsas revealed by SDS-PAGE and CBB staining is shown in Figure 3E.

Therefore, bacterially expressed and purified JIP-1b bound to the cytoplasmic domain of APP in a specific and saturable manner,and it showed half-maximal binding at a submicromolar concentration,which is comparable with the half-maximal binding concentrationsof other PID proteins $---$ mDab1, X11, and Fe65. In addition, the datathat purified recombinant JIP-1b bound to purified GST-cyt suggestthat JIP-1b directly binds to the cytoplasmic domain of APP, asmDab1, X11, and Fe65. As assessed by the common T7-antigenicity,the maximal binding of JIP-1b to the cytoplasmic domain of APPwas relatively lower than that of the other PID proteins, suggestingthat the APP/JIP-1b complex might be a minority among all APP/PID-proteincomplexes under the conditions in which other PID proteins arealso present. However, considering its comparably high affinityto those of other PID proteins, this feature of APP/JIP-1b interactioncould be useful for signal transduction of high timeresolution.

C terminus of APP precipitates JIP-1b/IB1 in a G⁶⁸¹YENPTY⁶⁸⁷-dependent manner

To confirm the protein interaction of JIP-1b/IB1 with APP, the lysate of COS cells transfected with HA-IB1_360-711 weremixed with various GST fusion proteins immobilized on glutathionebeads, and the lysate and precipitants were analyzed by immunoblottingusing anti-HA antibody (Fig. 4B). HA-IB1_360-711 was detectedin the precipitant of GST fused with the cytoplasmic domain ofAPP (GST-cyt), but not in those of GST alone, GST fused with thecytoplasmic domain of APP lacking C-terminal 15 amino acids (GST- $Delta$ NPTY),or GST fused with the cytoplasmic domain of APLP1 (GST-APLP1cyt).Minor immunoreactive bands of lower relative molecular weightswere attributed to partial degradation of the expressed protein.A faint band was detected occasionally in the precipitant of GSTfused with the cytoplasmic domain of APLP2 (GST-APLP2cyt) (Fig.4B). It is thus highly likely that IB1_360-711 binds to thecytoplasmic domain of APP, which contains G⁶⁸¹YENPTY⁶⁸⁷ shown to be necessary by the interaction-mating experiment (Fig.2D). It was also noted that IB1_360-711 more preferentiallybound to the cytoplasmic domain of APP than the cytoplasmic domainsof APLP1 and APLP2, under the conditions that were used.

View larger version (33K):
[in this window]
[in a new window]
Figure 4. JIP-1b/IB1, not JIP-1, is precipitated by the cytoplasmic domain of APP, but little by those of APLP1 and APLP2. A, An illustration of the JIP/IB1 constructs used in the bacterial GST-fused protein pull-down experiments. HA and T7 tags are boxed. Other designations are the same as the illustration of the fusions in Figure 2D. B, The lysates prepared from the COS cells transfected with HA-IB1_360-711, T7-JIP-1b_365-707, and T7-JIP-1_365-660 were precipitated with glutathione beads immobilizing GST, GST-APP_649-695 (GST-cyt), GST-APP_649-680 (GST- $Delta$ NPTY), GST-APLP1_607-653 (GST-APLP1cyt), and GST-APLP2_705-751 (GST-APLP2cyt), and the lysate and the precipitants were visualized with anti-HA and anti-T7 antibodies as indicated. The precipitants were also stained with CBB, which shows the presence of a similar amount of GST-fusion protein. The numbers on the left are the relative molecular weights of the size markers in kilodaltons. Each datum presented in Figure 4 is the representative of three independent experiments. C, The lysates prepared from mock-transfected COS cells were precipitated using GST-cyt. The lysates (lysate) and precipitants (ppt) were visualized with anti-HA and anti-T7 antibody, indicating the absence of nonspecific bands in GST-cyt precipitants.

This IB1-APP interaction was reproduced by using its mouse counterpart, T7-JIP-1b_365-707, the homologous region encodedby HA-IB1_360-711. When the lysate of COS cells transfectedwith T7-JIP-1b_365-707 was again precipitated with GST-fusedproteins immobilized on glutathione beads, a weak but significantband corresponding to JIP-1b_365-707 was detected in theGST-cyt precipitant, but not in any of the other precipitants(Fig. 4B). The weakness of the JIP-1b immunoreactivity in theGST-cyt precipitant was attributed to proportionally weak expressionof T7-JIP-1b_365-707. Therefore, JIP-1b bound to the cytoplasmicdomain of APP in a manner similar to that observed for its humanhomologIB1.

When T7-JIP-1_365-660, equivalent to JIP-1b_365-707 lacking 47 amino acids in the PID region, was examined by thesame GST-cyt pull-down experiment, no anti-T7-immunoreactive bandwas observed in the precipitants, although the construct was expressedsufficiently in the lysate (Fig. 4B). These results indicate thatthe PID region is essential for the JIP interaction with APP,the same observation obtained by the interaction-mating experimentshown in Figure 2D. The amounts of GST-fusion proteins containedin the precipitants were similar in all experiments above. Thetypical CBB staining is shown (Fig. 4B, CBB).

As negative controls, the lysate of mock-transfected cells was precipitated with immobilized GST-cyt, and their lysates andthe ppts were subjected to immunoblotting using anti-HA and anti-T7antibodies. Anti-HA antibody detected faint bands in the lysate,which are different in size from those found in the lysate ofcells transfected with HA-IB1_360-711, but none in the precipitant.No immunoreactive bands were detected in either lysate or theprecipitant with anti-T7 antibody (Fig. 4C). This confirms thatthe bands detected in the lysates or precipitants in Figure 4Bwere derived from the transfectedplasmids.

We were unable to perform interaction-mating assays using the bait fusions of the cytoplasmic domain of APLP1 and APLP2 becauseof their autoactivation of the LEU2 reporter gene (data notshown).

GST-fused JIP-1b/IB1 can precipitate full-length APP with or without FAD mutations

To further confirm the interaction of JIP-1b/IB1 with APP, reciprocal pull-down experiments were performed using GST-fusedJIP-1b/IB1 constructs and full-length wt APP. When the lysatesof COS cells transfected with wt APP and GST, GST-IB1_360-711,GST-JIP-1b_493-707, or GST-JIP-1b_540-707, APP immunoreactivitywas found in the glutathione-bead precipitants from lysates transfectedwith any GST-JIP-1b/IB1 construct but not in the precipitant fromthe lysate transfected with GST alone (Fig. 5A). Similar amountsof APP were detected in lysates of these transfected cells (Fig.5A). Thus, GST-fused JIP-1b/IB1 constructs interacted with full-lengthwt APP.

View larger version (32K):
[in this window]
[in a new window]
Figure 5. The C terminus of JIP-1b/IB1 precipitates wild-type and FAD mutant APPs. A, COS cells were cotransfected with wt APP with GST, GST-IB1_360-711, GST-JIP-1b_493-707, or GST-JIP-1b_540-707 (lanes 1-4, respectively) and precipitated with glutathione beads. The presence of APP and GST-fused proteins were probed with anti-APP antibody and anti-GST antibody, respectively. The numbers on the left are the relative molecular weights of the size markers in kilodaltons. Each datum presented in Figure 5 is the representative of three independent experiments. B, COS cells were cotransfected with GST-IB1_360-711 with pEF-BOS (vec), wt APP (wt), NL-APP (NL), V642G-APP (Gly), V642F-APP (Phe), or V642I-APP (Ile) as indicated and precipitated with glutathione beads. Immunoreactivities of APP and GST-IB1_360-711 contained in the lysates (lysate) or precipitants (ppt) were detected by anti-APP antibody and anti-GST antibody, respectively. C, Similar experiments were performed with COS cells transfected with GST-JIP-1b_540-707 instead of GST-IB1_360-711. Other conditions and designations are the same as in B.

We next examined whether this interaction was affected by FAD mutations in APP. For this purpose, COS cells were transfectedwith GST-IB1_360-711 and pEF-BOS, wt APP, or four FAD mutantsof APP₆₉₅ [K595N/M596L-APP (NL-APP), V642G-APP, V642F-APP, andV642I-APP] (Fig. 5B). The levels of expression of APP constructswere similar among wt APP and mutant APPs (Fig. 5B). When theselysates were precipitated with glutathione beads, APP immunoreactivitywas detected in the precipitants from lysates transfected witheither APP construct. This finding indicates that GST-IB1_360-711can interact, to similar degrees, with full-length APP with orwithout FAD-associated mutations. Similar results were obtainedby a pull-down experiment using GST-JIP-1b_540-707 insteadof GST-IB1_360-711 (Fig. 5C). JIP-1b/IB1 thus interactedsimilarly with wt APP and four FAD mutants (NL and V642I/F/G).

Anti-JIP-1b antisera precipitate full-length wt APP and APP mutants with JIP-1b expressed in COS cells and neuronal NT2 cells

When lysates of COS cells transfected with T7-JIP-1b_1-272 or T7-JIP-1b_1-707 were probed with rabbit antiserumraised against the N-terminal residues 10-33 of JIP-1b ( $alpha$ JIPN),the major immunoreactive bands at ~40 and ~120 kDa were thosecorresponding to the bands detected with anti-T7 antibody. Incontrast, preimmune serum from the same rabbit failed to detectthem (data not shown). Likewise, when lysates of cells transfectedwith T7-JIP-1_271-660 or T7-JIP-1b_1-707 were probedwith rabbit antiserum raised against the C-terminal residues 685-707of JIP-1b ( $alpha$ JIPC), the major immunoreactive bands at ~70 and ~120kDa were those corresponding to the bands detected with anti-T7antibody, but its preimmune serum could not detect them (datanot shown). This indicates that both $alpha$ JIPN and $alpha$ JIPC antiseracan specifically recognize transfected JIP-1b or itsvariants.

To further confirm the interaction of full-length JIP-1b with full-length APP, various combinations of plasmids were transfectedinto COS cells (Fig. 6A). When the lysates of transfected cellswere analyzed by immunoblotting with anti-APP antibody, significantand similar amounts of wt APP and NL-APP were detected in thelysates of cells transfected with cognate constructs of APP, butlittle immunoreactivity of APP was detected in those transfectedwith the empty vector alone. Anti-T7 immunoreactivity of JIP-1bwas detected in the lysates transfected with T7-JIP-1b cDNA, butlittle immunoreactivity was detected in those transfected withan empty vector control (Fig. 6A). These lysates were immunoprecipitatedwith the antisera, as indicated in Figure 6B, using $alpha$ JIPN or itspreimmune serum. The precipitants were subjected to immunoblotanalysis using anti-APP and anti-T7 antibodies to detect wt APPor NL-APP and T7-JIP-1b, respectively. Significant immunoreactivityof JIP-1b was detected in the $alpha$ JIPN precipitants from all of theT7-JIP-1b-transfected lysates, but no immunoreactivity was detectedin those from the empty vector-transfected cells, nor was it detectedin the precipitants by preimmune serum (Fig. 6B). This indicatesthat $alpha$ JIPN antiserum precipitated JIP-1b in the presence or absenceof exogenous APP expression. When the precipitants were probedusing anti-APP antibody, APP immunoreactivity was detected inthe $alpha$ JIPN precipitants of cells transfected with both T7-JIP-1band either wt APP or NL-APP, but not in the precipitant by preimmuneserum. No APP immunoreactivity was detected when empty vectorcontrols were used in place of either JIP-1b or APP (Fig. 6B).This indicates that the immunoprecipitation of JIP-1b was specificand that exogenous JIP-1b expression was required for APP to beprecipitated by $alpha$ JIPN antiserum.

View larger version (22K):
[in this window]
[in a new window]
Figure 6. JIP-1b precipitates wild-type and FAD mutant APP in COS and NT2 cells. A, COS cells were transfected with the various combinations of wt APP, NL-APP, or their empty vector (wt, NL, or $-$ in APP, respectively), and T7-JIP-1b or its empty vector (+ or $-$ in JIP-1b). The presence of APP and JIP-1b in the lysates was detected with anti-APP and anti-T7 antibody, respectively. The numbers on the left are the relative molecular weights of the size markers in kilodaltons. Each datum presented in Figure 6 is the representative of three independent experiments. B, The same lysates prepared from the transfectants of indicated plasmids were immunoprecipitated with the antisera $alpha$ JIPN (N) or its preimmune serum (P). APP and JIP-1b were detected as in A. Other designations are the same as in A. C, Similar experiments were performed with $alpha$ JIPC (C) or its preimmune serum (P). Other conditions and designations are the same as in B. D, Similar experiments were performed using neuronal NT2 cells transfected with the indicated combinations of wt APP and T7-JIP-1b and $alpha$ JIPC (C) or its preimmune serum (P). Their lysates (lysate) and precipitants (ppt) were probed for the presence of APP and JIP-1b. Other conditions and designations are the same as in C.

Essentially the same immunoprecipitation experiments were performed using $alpha$ JIPC, yielding results similar to those obtainedin the $alpha$ JIPN experiments (Fig. 6C). Furthermore, similar resultswere obtained when similar immunoprecipitation was performed usingV642I-APP instead of NL-APP (data not shown). Full-length JIP-1bthus interacted with full-length APP with or without FADmutations.

To further confirm the interaction of JIP-1b and APP in neuronal cells, wt APP and T7-JIP-1b or their corresponding emptyvectors were transfected to NT2 cells, human neuronal precursorcells (Pleasure and Lee, 1993), as indicated in Figure 6D. Whenthe lysates were subjected to immunoblotting and probed for thepresence of APP and JIP-1b using anti-APP and T7-antibodies, respectively,APP and JIP-1b were detected in the lysates of cells transfectedwith their cognate plasmids. Significant amounts of APP of highermolecular weights were also detected in all lysates, includingthat of empty vector-transfected NT2 cells. These lysates wereimmunoprecipitated using $alpha$ JIPC and its preimmune serum, and theprecipitants were again probed for the presence of APP and JIP-1b.As in the experiments using COS cells, both JIP-1b and APP couldbe detected in the precipitant from the lysate of NT2 cells transfectedwith both plasmids and precipitated with $alpha$ JIPC, but not in theother combinations tested (Fig. 6D). The expression of JIP-1bin untransfected NT2 cells could not be detected using $alpha$ JIPN or $alpha$ JIPC (data notshown).

GST-fused JNK1 $beta$ 1 precipitates wild-type and FAD mutant APP in the presence of exogenously expressed JIP-1b

To investigate whether JIP-1b can scaffold JNK and APP, various combinations of plasmids were transfected to COS cells, andtheir lysates were probed with anti-APP, anti-T7, or anti-GSTantibody to detect wt APP-, T7-JIP-1b-, and GST-fused proteins,respectively (Fig. 7, lysate). The protein expression of wt APPand JIP-1b was confirmed in the lysates of cells transfected withcorresponding plasmids, but not in empty vector controls. Likewise,GST and GST-JNK1 $beta$ 1 were detected in cells transfected with theencoding plasmids, as the bands of the corresponding sizes oftheir expressed proteins (Fig. 7, lysate).

View larger version (26K):
[in this window]
[in a new window]
Figure 7. GST-fused JNK1 $beta$ 1 can precipitate APPs in a JIP-1b-dependent manner. COS cells were transfected with the indicated combinations of wt APP or its empty vector (+ or $-$ in wt APP), T7-JIP-1b or its empty vector (+ or $-$ in JIP-1b), and GST or GST-JNK1 $beta$ 1, as indicated with + under each lane, and their lysates were precipitated with glutathione beads. The presence of APP, JIP-1b, and GST-fused proteins in lysate (lysate) and precipitants (ppt) was detected with anti-APP, anti-T7, and anti-GST antibodies, respectively. Other designations are the same as in Figure 6. The data in this figure are representative of three independent experiments.

These lysates were precipitated with glutathione beads and subjected to immunoblot analyses (Fig. 7, ppt). GST or GST-JNK1 $beta$ 1was detected in all precipitants from lysates transfected withthe corresponding GST constructs. JIP-1b was detected in the precipitantfrom the lysate of cells transfected with both JIP-1b and GST-JNK1 $beta$ 1,but not in that from the lysate of cells transfected with GSTalone nor the empty vector control of JIP-1b. This suggests thatJIP-1b was specifically precipitated by JNK1b1. When the sameprecipitants were probed with anti-APP antibody, APP immunoreactivitywas detected only when wt APP, JIP-1 $beta$ , and GST-JNK1 $beta$ 1 were cotransfected.In contrast, no APP immunoreactivity was detected in either precipitantfrom lysates transfected in the other combinations. This providesevidence that wt APP forms a complex with JNK1 $beta$ 1 through the scaffoldingby JIP-1b.

JIP-1b and APP share similar subcellular localization

To further confirm the interaction of JIP-1b with APP in vivo, subcellular localization of JIP-1b and APP was examined byimmunocytochemical analysis using confocal microscopy. When COScells transfected with wt APP cDNA were stained with anti-APPantibody and visualized with Texas Red-conjugated secondary antibody,cells showed cytoplasmic staining but not nuclear staining (Fig.8). No staining was observed when the same transfected cells werestained with control mouse IgG or when untransfected cells werestained with anti-APP antibody (data not shown).

View larger version (35K):
[in this window]
[in a new window]
Figure 8. APP and JIP-1b share similar subcellular localization. COS cells were transfected with APP, JIP-1b, or both. JIP-1b expression was detected with $alpha$ JIPN and visualized with FITC-conjugated secondary antibody (green). APP expression was detected with 22C11 (anti-APP antibody) and visualized with Texas Red-conjugated secondary antibody (red). DNA was visualized with Hoechst 33342 (blue), as described in Materials and Methods. The yellow area in the merged section shows where JIP-1b and APP share similar subcellular localization. Scale bars, 10 µm. The same set of experiments was repeated at least three times and yielded similar results.

When T7-JIP-1b-transfected cells were stained with $alpha$ JIPN antiserum and visualized with FITC-conjugated secondary antibody,JIP-1b staining was observed in the cytoplasm and absent in thenucleus. Staining using $alpha$ JIPC yielded similar results (data notshown). No staining was observed when untransfected cells werestained with $alpha$ JIPN or $alpha$ JIPC or when corresponding preimmune serawere used to stain T7-JIP-1b-transfected cells (data notshown).

To investigate whether JIP-1b and APP share subcellular localization, cells were cotransfected with T7-JIP-1b and APP anddoubly stained by $alpha$ JIPN and anti-APP antibody (Fig. 8). The immunostainingof JIP-1b (stained green) and that of APP (stained red) significantlyoverlapped in the shared subcellular localization, as revealedby the yellow area in the merged picture. These observations areconsistent with the notion that a certain fraction of JIP-1b interactswith APP in vivo.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have herein identified JIP-1b/IB1 as a novel APP-interacting molecule that indicated an affinity for the cytoplasmic domainof APP comparable to those of other known PID-containing APP-interactingproteins. JIP-1 was initially characterized as a cytoplasmic inhibitorof JNK family kinases (Dickens et al., 1997) and subsequentlyfound to interact with MKK7, MLK, DLK, and HPK-1 in addition toJNK (Whitmarsh et al., 1998). Coexpression of JIP-1 and JNK withMKK7 or MLK3 increased JNK activation (Whitmarsh et al., 1998).These findings have established that JIP-1 scaffolds the kinasecomponents of the JNK signaling pathway (Davis, 2000). An additionalisoform of JIP-1 has been reported in mouse (JIP-1b) (Whitmarshet al., 1998; Kim et al., 1999), rat [islet-brain-1 (IB1)] (Bonnyet al., 1998), and human (IB1) (Mooser et al., 1999). This isoformcontains a 47-residue insertion that completes the PID regionat the C terminus, which was originally identified in Shc interactionwith NPXY in the cytoplasmic domain of the epidermal growth factorreceptor (Kavanaugh and Williams, 1994; Kavanaugh et al., 1995).Neither the physiological nor the pathological role of the JIP-1proteins has become totally clear, whereas expression of JIP-1has been reported to transcriptionally activate the GLUT2 promoter(Bonny et al., 1998) and is implicated in the pathogenesis ofa form of type 2 familial diabetes mellitus (Waeber et al., 2000)and in the cytoprotection of insulin-secreting cells (Bonny etal., 2000). The present study thus provides the first line ofevidence that the JNK scaffold protein, abundant in the brainand in islet $beta$ -cells, could be relevant to Alzheimer's disease.Interestingly, it has been reported that in vivo, neurotoxicityby hippocampal administration of Ab1-42 occurs only in diabeticrats (Smyth et al., 1994).

Analysis of subcellular localization using transfected cells indicates that JIP-1b and APP colocalized in the cytoplasm butboth were not detected in the nuclei. Similar cytoplasmic localizationof JIP-1b was reported by Dickens et al. (1997) and Whitmarshet al. (1998), although Bonny et al. (1998) reported that IB1is a nuclear protein. Coffey et al. (2000) showed nuclear localizationof JIP-1 proteins in cerebellar granule cells, and Meyer et al.(1999) showed that JIP-1 proteins localize in the cytoplasm inunpolarized NIE115 and PC12 cells but are concentrated at neuriteswhen the cells are polarized. These differences in JIP-1 localizationthus may reflect different functions of JIP-1 proteins assignedin different cell environments. Although the present study providesevidence that JIP-1b interacts with APP inside the transfectedcells, it would be necessary to investigate whether endogenousAPP and JIP-1b interact in nontransfected cells. Yet the notionthat JIP-1b/IB1 colocalizes with APP is consistent with earlierstudies (Becker et al., 1999; Kim et al., 1999; Yasuda et al.,1999; Marcinkiewicz and Seidah, 2000; Pellet et al., 2000) indicatingthat the subcellular and brain regional localizations of JIP proteinsconsiderably overlap with those of APP. Because the putative $alpha$ -secretaseADAM10 and the putative $beta$ -secretase BACE are expressed in thesame neurons that express APP in the mouse brain (Marcinkiewiczand Seidah, 2000), APP cleavage by these putative secretases wouldlose the interaction of APP with JIP-1b/IB1, causing, in turn,a loss in the ability of JIP-1b/IB1 to specifically colocalizesignaling molecules with APP. Although so far we have been unableto coimmunoprecipitate APP with IB1 from rat brain homogenates(data not shown), it remains unclear whether this failure is causedby inappropriate experimental conditions for specific immunoprecipitationof the APP/IB1 complex from solubilized brain homogenates or whetherit implies that, with the APP/IB1 complex being a minor fraction,the majority of APP and IB1 in the brain does not complex witheach other or form complexes with different partners. The latternotion is consistent, at least in part, with the observed relativelylower maximal binding of JIP-1b to the cytoplasmic domain of APP,as compared with those of the other PID-containing proteinstested.

By constructing deletion and point mutants, we have shown that the domains necessary for the APP/JIP-1b interaction are thecytoplasmic G⁶⁸¹YENPTY⁶⁸⁷ region in APP and the PID region in JIP-1b, completed by theinsertion specific for this isoform. This accounts for the PID-nonbearingisoform JIP-1 not interacting with APP. As noted above, X11, Fe65,Fe65L, and mDab1 have been shown to interact with the C terminusof APP. The present study indicates that the APP/JIP-1b interactionrequires Tyr⁶⁸², Asn⁶⁸⁴, and Tyr⁶⁸⁷ contained in the G⁶⁸¹YENPTY⁶⁸⁷ region. This is different from the mode of APP interaction withFe65 and X11 and similar to that with mDab1. The observed aminoacids required for the interaction of Fe65 or X11 concur witha previous report (Borg et al., 1996). Interestingly, the JIP-1bisoform, which is interactive with APP, is the major transcriptin the brain, and the noninteractive JIP-1 transcript is hardlydetected (Coffey et al., 2000; Pellet et al., 2000), pointingto certain specific roles of the JIP-1b isoform in neuronalfunctions.

The mechanism underlying the observed JIP-1b/IB1 interaction with APP is thus consistent with the established NPXY motif interactionof PID in Shc (Kavanaugh and Williams, 1994; Kavanaugh et al.,1995; Songyang et al., 1995) and IRS-1(Pawson and Scott, 1997).Yet in the present GST pull-down experiments, the cytoplasmicdomains of APP, APLP1, and APLP2, all of which contain the sameNPXY structure GYENPTY, showed largely different binding intensitiesfor JIP-1b/IB1, with APP being the strongest among them. Thesedifferent binding characteristics might reflect the differencein the primary to ternary structures surrounding the NPXY motif,suggesting the presence of an additional structural requirementallowing NPXY to interact efficiently with PID. In support ofthis idea, the most recent literature, in which PID of JIP-1bis shown to interact with p190 rhoGEF (Meyer et al., 1999), indicatesthat the binding region of p190 does not contain the classicalNPXYmotif.

Because JIP-1b showed binding similar to full-length APP regardless of the presence of four different FAD mutations, JIP-1bis most likely involved in the basic function of APP. Althoughthe binding of Fe65 or X11 to APP has been shown to affect A $beta$ secretion from APP (Borg et al., 1998; Sastre et al., 1998; Saboet al., 1999; Tomita et al., 1999), so far we have not observedremarkable changes in A $beta$ 42 secretion from NL-APP by cotransfectionwith JIP-1b (Z. Shao, S. Matsuda, and I. Nishimoto, unpublishedobservation). The JIP-1 proteins have been shown to serve as scaffoldproteins for the organization of active JNK signaling complexes(Whitmarsh et al., 1998). In fact, we have shown in this studythat APP associates with JNK via JIP-1b. It has also been establishedthat APP interacts with the GTP-binding protein G_o through themiddle portion in the APP cytoplasmic domain adjacent to the NPXY-containingC terminus (Nishimoto et al., 1993; Okamoto et al., 1995; Brouilletet al., 1999). It is likely, therefore, that APP may serve asa membrane-anchoring protein that further scaffolds the JIP-scaffoldingcomplex with other signaling molecules. Taking into account therecently cloned members of the JIP family, JIP2 and JIP3 (Yasudaet al., 1999; Kelker et al., 2000) $---$ PID is contained in JIP2 butnot in JIP3 $---$ it would deserve investigation whether APP might regulatethe JNK signaling pathway through the binding of these variousJIP proteins to the cytoplasmic domain ofAPP.

  FOOTNOTES

Received May 7, 2001; revised June 11, 2001; accepted June 13, 2001.

This work was supported in part by grants from the Ono Medical Research Foundation, the Ministry of Education, Culture, Sports,Science, and Technology of Japan, and the Organization for PharmaceuticalSafety and Research (OPSR). We especially thank Yukiko Yoshimoto-Matsudaand Tomo Yoshida for excellent assistance and generous encouragementthroughout the course of this study; Yumi and Yoshiomi Tamai forindispensable support; Masao Kaneki for cooperation; and KazumiNishihara and Dovie Wylie for expert technicalassistance.
Correspondence should be addressed to Ikuo Nishimoto, Department of Pharmacology and Neurosciences, KEIO University Schoolof Medicine, Shinjuku-ku, Tokyo 160-8582, Japan. E-mail: nisimoto{at}mc.med.keio.ac.jp.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ausubel FM, Brent R, Kingston RE, Moore DD, Seidman JG, Smith JA, Struhl K (1999) In: Current protocols in molecular biology. New York: Wiley.
Becker AJ, Gillardon F, Blumcke I, Langendorfer D, Beck H, Wiestler OD (1999) Differential regulation of apoptosis-related genes in resistant and vulnerable subfields of rat epileptic hippocampus. Mol Brain Res 67:172-176[Medline].
Bonny C, Nicod P, Waever G (1998) IB1, a JIP-1-related nuclear protein present in insulin-secreting cells. J Biol Chem 273:1843-1846[Abstract/Free Full Text].
Bonny C, Oberson A, Steinmann M, Schorderet DF, Nicod P, Waeber G (2000) IB1 reduces cytokine-induced apoptosis of insulin-secreting cells J Biol Chem 275:16466-16472[Abstract/Free Full Text].
Borg J-P, Ooi J, Levy E, Margolis B (1996) The phosphotyrosine interaction domains of X11 and Fe65 bind to distinct sites on the YENPTY motif of amyloid precursor protein. Mol Cell Biol 16:6229-6241[Abstract].
Borg J-P, Yang Y, De Taddeo-Borg M, Margolis B, Turner RS (1998) The X11 $alpha$ protein slows cellular amyloid precursor protein processing and reduces A $beta$ 40 and A $beta$ 42 secretion. J Biol Chem 273:14761-14766[Abstract/Free Full Text].
Bork P, Margolis B (1995) A phosphotyrosine interaction domain. Cell 80:693-694[Web of Science][Medline].
Brouillet E, Trembleau A, Galanaud D, Volovitch M, Bouillot C, Valenza C, Prochiantz A, Allinquant B (1999) The amyloid precursor protein interacts with G_o heterotrimeric protein within a cell compartment specialized in signal transduction. J Neurosci 19:1717-1727[Abstract/Free Full Text].
Coffey ET, Hongisto V, Dickens M, Davis RJ, Courtney MJ (2000) Dual roles for c-Jun N-terminal kinase in developmental and stress responses in cerebellar granule neurons. J Neurosci 20:7602-7613[Abstract/Free Full Text].
Coulson EJ, Barrett GL, Storey E, Bartlett PF, Beyreuther K, Masters CL (1997) Down-regulation of the amyloid protein precursor of Alzheimer's disease by antisense oligonucleotides reduces neuronal adhesion to specific substrata. Brain Res 770:72-80[Medline].
Davis RJ (2000) Signal transduction by the JNK group of MAP kinases. Cell 103:239-252[Web of Science][Medline].
Dickens M, Rogers JS, Cavanagh J, Raitano A, Xia Z, Halpern JR, Greenberg ME, Sawyers CL, Davis RJ (1997) A cytoplasmic inhibitor of the JNK signal transduction pathway. Science 277:693-696[Abstract/Free Full Text].
Duilio A, Faraonio R, Minopoli G, Zambrano N, Russo T (1998) Fe65L2: a new member of the Fe65 protein family interacting with the intracellular domain of the Alzheimer's $beta$ -amyloid precursor protein. Biochem J 330:513-519.
Finley Jr R, Brent R (1994) Interaction mating reveals binary and ternary connections between Drosophila cell cycle regulators. Proc Natl Acad Sci USA 91:12980-12984[Abstract/Free Full Text].
Fiore F, Zambrano N, Minopoli G, Donini V, Duilio A, Russo T (1995) The regions of the Fe65 protein homologous to the phosphotyrosine interaction/phosphotyrosine binding domain of Shc bind the intracellular domain of the Alzheimer's amyloid precursor protein. J Biol Chem 270:30853-30856[Abstract/Free Full Text].
Giambarella U, Yamatsuji T, Okamoto T, Matsui T, Ikezu T, Murayama Y, Levine MA, Katz A, Gautam N, Nishimoto I (1997) G protein $beta$ $gamma$ complex mediated apoptosis by familial Alzheimer's disease mutant of APP. EMBO J 16:4897-4907[Web of Science][Medline].
Gietz RD, Schiestl RH (1995) Transforming yeast with DNA. Mol Cell Biol 5:255-269.
Gillian AM, McFarlane I, Lucy FM, Overly C, McConlogue L, Breen KC (1997) Individual isoforms of the amyloid $beta$ precursor protein demonstrate differential adhesive potentials to constituents of the extracellular matrix. J Neurosci Res 49:154-160[Medline].
Gubler U, Hoffman BJ (1983) A simple and very efficient method for generating cDNA libraries. Gene 25:263-269[Web of Science][Medline].
Guenette SY, Chen J, Jondro PD, Tanzi RE (1996) Association of a novel human FE65-like protein with the cytoplasmic domain of the $beta$ -amyloid precursor protein. Proc Natl Acad Sci USA 93:10832-10837[Abstract/Free Full Text].
Hardy J (1992) Framing $beta$ -amyloid. Nat Genet 1:233-234[Web of Science][Medline].
Hashimoto Y, Niikura T, Ito Y, Nishimoto I (2000) Multiple mechanisms underlie neurotoxicity by different types of Alzheimer's disease mutations of amyloid precursor protein. J Biol Chem 275:34541-34551[Abstract/Free Full Text].
Hirai S, Izawa M, Osada S, Spyrou G, Ohno S (1996) Activation of the JNK pathway by distantly related protein kinases, MEKK and MUK. Oncogene 12:641-650[Web of Science][Medline].
Jung SS, Nalbantoglu J, Cashman NR (1996) Alzheimer's $beta$ -amyloid precursor protein is expressed on the surface of immediately ex vivo brain cells: a flow cytometric study. J Neurosci Res 46:336-348[Medline].
Kang J, Lemaire H-G, Unterback A, Salbaum JM, Masters CL, Grezeschik KH, Multhaup G, Beyreuther K, Müller-Hill B (1987) The precursor of Alzheimer disease amyloid A4 protein resembles a cell-surface receptor. Nature 325:733-736[Medline].
Kavanaugh WM, Williams LT (1994) An alternative to SH2 domains for binding tyrosine-phosphorylated proteins. Science 266:1862-1865[Abstract/Free Full Text].
Kavanaugh WM, Turck CW, Williams LT (1995) PTB domain binding to signaling proteins through a sequence motif containing phosphotyrosine. Science 268:1177-1179[Abstract/Free Full Text].
Kelkar N, Gupta S, Dickens M, Davis RJ (2000) Interaction of a mitogen-activated protein kinase signaling module with the neuronal protein JIP3. Mol Cell Biol 20:1030-1043[Abstract/Free Full Text].
Kim IJ, Lee KW, Park BY, Lee JK, Park J, Choi IY, Eom SJ, Chang TS, Kim MJ, Yeom YI, Chang SK, Lee YD, Choi EJ, Han PL (1999) Molecular cloning of multiple splicing variants of JIP-1 preferentially expressed in brain. J Neurochem 72:1335-1343[Medline].
Lu DC, Rabizadeh S, Chandra S, Shayya RF, Ellerby LM, Ye X, Salvesen GS, Koo EH, Bredesen DE (2000) A second cytotoxic proteolytic peptide derived from amyloid $beta$ -protein precursor. Nat Med 6:397-404[Web of Science][Medline].
Luo JJ, Wallace W, Riccioni T, Ingram DK, Roth GS, Kusiak JW (1999) Death of PC12 cells and hippocampal neurons induced by adenoviral-mediated FAD human amyloid precursor protein gene expression. J Neurosci Res 55:629-642[Web of Science][Medline].
Marcinkiewicz M, Seidah NG (2000) Coordinated expression of $beta$ -amyloid precursor protein and the putative $beta$ -secretase BACE and $alpha$ -secretase ADAM10 in mouse and human brain. J Neurochem 75:2133-2143[Web of Science][Medline].
Meroni G, Reymond A, Alcalay M, Borsani G, Tanigami A, Tonlorenzi R, Nigro CL, Messali S, Zollo M, Ledbetter DH, Brent R, Ballabio A, Carrozzo R (1997) Rox, a novel bHLHZip protein expressed in quiescent cells that heterodimerizes with Max, binds a non-canonical E box and acts as a transcriptional repressor. EMBO J 16:2892-2906[Web of Science][Medline].
Meyer D, Liu A, Margolis B (1999) Interaction of c-Jun amino-terminal kinase interacting protein-1 with p190 rhoGEF and its localization in differentiated neurons. J Biol Chem 274:35113-35118[Abstract/Free Full Text].
Mizushima S, Nagata S (1990) pEF-BOS, a powerful mammalian expression vector. Nucleic Acids Res 18:5322[Free Full Text].
Mooser V, Maillard A, Bonny C, Steinmann M, Shaw P, Yarnall DP, Burns DK, Schorderet DF, Nicod P, Waeber G (1999) Genomic organization, fine-mapping, and expression of the human Islet-Brain 1 (IB1)/c-jun-amino-terminal kinase interacting protein-1 (JIP-1) gene. Genomics 55:202-208[Medline].
Murayama Y, Takeda S, Yonezawa K, Giambarella U, Nishimoto I, Ogata E (1996) Cell surface receptor function of amyloid precursor protein that activates Ser/Thr kinases. Gerontology 42[Suppl 1]:2-11.
Nishimoto I, Okamoto T, Matsuura Y, Takahashi S, Okamoto T, Murayama Y, Ogata E (1993) Alzheimer amyloid protein precursor complexes with brain GTP-binding protein G_o. Nature 362:75-79[Medline].
Okamoto T, Takeda S, Murayama Y, Ogata E, Nishimoto I (1995) Ligand dependent G protein coupling function of amyloid transmembrane precursor. J Biol Chem 270:4205-4208[Abstract/Free Full Text].
Okamoto T, Takeda S, Giambarella U, Matsuura Y, Katada T, Nishimoto I (1996) Intrinsic G-coupling function of amyloid precursor protein as a novel target of V642 mutations linked to familial Alzheimer disease. EMBO J 15:3769-3777[Web of Science][Medline].
Pawson T, Scott JD (1997) Signaling though scaffold, anchoring, and adaptor proteins. Science 278:2075-2080[Abstract/Free Full Text].
Pellet J-B, Haefliger J-A, Staple JK, Widmann C, Welker E, Hirling H, Bonny C, Nicod P, Catsicas S, Waeber G, Riederer BM (2000) Spatial, temporal and subcellular localization of islet-brain 1 (IB1), a homologue of JIP-1, in mouse brain. Eur J Neurosci 12:621-632[Medline].
Perez RG, Zheng H, Van der Ploeg LHT, Koo EH (1997) The $beta$ -amyloid precursor protein of Alzheimer's disease enhances neuron viability and modulates neuronal polarity. J Neurosci 17:9407-9414[Abstract/Free Full Text].
Pleasure SJ, Lee VM (1993) NTera 2 cells: a human cell line which displays characteristics expected of a human committed neuronal progenitor cell. J Neurosci Res 35:585-602[Web of Science][Medline].
Qiu WQ, Ferreira A, Miller C, Koo E, Selkoe DJ (1995) Cell-surface $beta$ -amyloid precursor protein stimulates neurite outgrowth of hippocampal neurons in an isoform-dependent manner. J Neurosci 15:2157-2167[Abstract].
Rohn TT, Ivins KJ, Bahr BA, Cotman CW, Cribbs DH (2000) A monoclonal antibody to amyloid precursor protein induces neuronal apoptosis. J Neurochem 74:2331-2342[Medline].
Sabo SL, Lanier LM, Ikin AF, Khorkova O, Sahasrabudhe S, Greengard P, Buxbaum JD (1999) Regulation of $beta$ -amyloid secretion by FE65, an amyloid protein precursor-binding protein. J Biol Chem 274:7952-7957[Abstract/Free Full Text].
Sanchez I, Hughes RT, Mayer B, Yee K, Woodgett JR, Avruch J, Kyriakis JM, Zon LI (1994) Role of SAPK/ERK kinase-1 in the stress-activated pathway regulating transcription factor c-Jun. Nature 372:794-798[Medline].
Sastre M, Turner RS, Levy E (1998) X11 interaction with $beta$ -amyloid precursor protein modulates its cellular stabilization and reduces amyloid $beta$ -protein secretion. J Biol Chem 273:22351-22357[Abstract/Free Full Text].
Smyth MD, Kesslak JP, Cummings BJ, Cotman CW (1994) Analysis of brain injury after intrahippocampal administration of $beta$ -amyloid in streptozotocin-treated rats. Neurobiol Aging 15:153-159[Medline].
Songyang Z, Margolis B, Chaudhuri M, Shoelson SE, Cantley LC (1995) The phosphotyrosine interaction domain of Shc recognizes tyrosine phosphorylated NPXY motif. J Biol Chem 270:14863-14866[Abstract/Free Full Text].
Sudo H, Jiang H, Yasukawa T, Hashimoto Y, Niikura T, Kawasumi M, Matsuda S, Takeuchi Y, Aiso S, Matsuoka M, Murayama Y, Nishimoto I (2000) Antibody-regulated neurotoxic function of cell surface $beta$ -amyloid precursor protein. Mol Cell Neurosci 16:708-723[Medline].
Tomita S, Ozaki T, Taru H, Oguchi S, Takeda S, Yagi Y, Sakiyama S, Kirino Y, Suzuki T (1999) Interaction of a neuron-specific protein containing PDZ domains with Alzheimer's amyloid precursor protein. J Biol Chem 274:2243-2254[Abstract/Free Full Text].
Trommsdorff M, Borg JP, Margolis B, Herz J (1998) Interaction of cytosolic adaptor proteins with neuronal apolipoprotein E receptors and the amyloid precursor protein. J Biol Chem 273:33556-33560[Abstract/Free Full Text].
Waeber G, Delplanque J, Bonny C, Mooser V, Steinmann M, Widmann C, Maillard A, Milklossy J, Dina C, Hani EH, Vionnet N, Nicod P, Boutin P, Froguel P (2000) The gene MAPK8IP1, encoding islet-brain-1, is a candidate for type 2 diabetes. Nat Genet 24:291-295[Web of Science][Medline].
Whitmarsh AJ, Cavanagh J, Tournier C, Yasuda J, Davis RJ (1998) A mammalian scaffold complex that selectively mediates MAP kinase activation. Science 281:1671-1674[Abstract/Free Full Text].
Wolozin B, Iwasaki K, Vito P, Ganjei JK, Lacana E, Sunderland T, Zhao B, Kusiak JW, Wasco W, D'Adamio L (1996) Participation of presenilin 2 in apoptosis: enhanced basal activity conferred by an Alzheimer mutation. Science 274:1710-1713[Abstract/Free Full Text].
Yamatsuji T, Okamoto T, Takeda S, Fukumoto H, Iwatsubo T, Suzuki N, Asami-Odaka A, Ireland S, Kinane TB, Nishimoto I (1996a) Neuronal DNA fragmentation by familial Alzheimer's V642 mutants of APP via heteromeric G proteins. Science 272:1349-1352[Abstract].
Yamatsuji T, Okamoto T, Takeda S, Murayama Y, Tanaka N, Nishimoto I (1996b) Expression of V642 APP mutant causes cellular apoptosis as Alzheimer trait linked phenotype. EMBO J 15:498-509[Web of Science][Medline].
Yasuda J, Whitmarsh AJ, Cavanagh J, Sharma M, Davis RJ (1999) The JIP Group of mitogen-activated protein kinase scaffold proteins. Mol Cell Biol 19:7245-7254[Abstract/Free Full Text].
Zhao B, Chrest FJ, Horton Jr WE, Sisodia SS, Kusiak JW (1997) Expression of mutant amyloid precursor proteins induces apoptosis in PC12 cells. J Neurosci Res 47:253-263[Web of Science][Medline].

Copyright © 2001 Society for Neuroscience 0270-6474/01/21176597-11$05.00/0

This article has been cited by other articles:

K. Laky, W. Annaert, and B. J. Fowlkes
Amyloid precursor family proteins are expressed by thymic and lymph node stromal cells but are not required for lymphocyte development
Int. Immunol., October 1, 2009; 21(10): 1163 - 1174.
[Abstract] [Full Text] [PDF]

S. Matsuda, Y. Matsuda, and L. D'Adamio
BRI3 Inhibits Amyloid Precursor Protein Processing in a Mechanistically Distinct Manner from Its Homologue Dementia Gene BRI2
J. Biol. Chem., June 5, 2009; 284(23): 15815 - 15825.
[Abstract] [Full Text] [PDF]

K. Krause, S. Karger, S.-Y. Sheu, T. Aigner, R. Kursawe, O. Gimm, K.-W. Schmid, H. Dralle, and D. Fuhrer
Evidence for a role of the amyloid precursor protein in thyroid carcinogenesis
J. Endocrinol., August 1, 2008; 198(2): 291 - 299.
[Abstract] [Full Text] [PDF]

T. Suzuki, Y. Araki, T. Yamamoto, and T. Nakaya
Trafficking of Alzheimer's Disease-Related Membrane Proteins and Its Participation in Disease Pathogenesis
J. Biochem., June 1, 2006; 139(6): 949 - 955.
[Abstract] [Full Text] [PDF]

C. D'Ambrosio, S. Arena, G. Fulcoli, M. H. Scheinfeld, D. Zhou, L. D'Adamio, and A. Scaloni
Hyperphosphorylation of JNK-interacting Protein 1, a Protein Associated with Alzheimer Disease
Mol. Cell. Proteomics, January 1, 2006; 5(1): 97 - 113.
[Abstract] [Full Text] [PDF]

Z. Muresan and V. Muresan
Coordinated transport of phosphorylated amyloid-{beta} precursor protein and c-Jun NH2-terminal kinase-interacting protein-1
J. Cell Biol., November 21, 2005; 171(4): 615 - 625.
[Abstract] [Full Text] [PDF]

J. Zhou, B. K. Deo, K. Hosoya, T. Terasaki, I. G. Obrosova, F. C. Brosius III, and A. K. Kumagai
Increased JNK Phosphorylation and Oxidative Stress in Response to Increased Glucose Flux through Increased GLUT1 Expression in Rat Retinal Endothelial Cells
Invest. Ophthalmol. Vis. Sci., September 1, 2005; 46(9): 3403 - 3410.
[Abstract] [Full Text] [PDF]

Z. Muresan and V. Muresan
c-Jun NH2-Terminal Kinase-Interacting Protein-3 Facilitates Phosphorylation and Controls Localization of Amyloid-{beta} Precursor Protein
J. Neurosci., April 13, 2005; 25(15): 3741 - 3751.
[Abstract] [Full Text] [PDF]

O. Lazarov, G. A. Morfini, E. B. Lee, M. H. Farah, A. Szodorai, S. R. DeBoer, V. E. Koliatsos, S. Kins, V. M.-Y. Lee, P. C. Wong, et al.
Axonal Transport, Amyloid Precursor Protein, Kinesin-1, and the Processing Apparatus: Revisited
J. Neurosci., March 2, 2005; 25(9): 2386 - 2395.
[Abstract] [Full Text] [PDF]

E. Ghersi, C. Noviello, and L. D'Adamio
Amyloid-{beta} Protein Precursor (A{beta}PP) Intracellular Domain-associated Protein-1 Proteins Bind to A{beta}PP and Modulate Its Processing in an Isoform-specific Manner
J. Biol. Chem., November 19, 2004; 279(47): 49105 - 49112.
[Abstract] [Full Text] [PDF]

R. C. von Rotz, B. M. Kohli, J. Bosset, M. Meier, T. Suzuki, R. M. Nitsch, and U. Konietzko
The APP intracellular domain forms nuclear multiprotein complexes and regulates the transcription of its own precursor
J. Cell Sci., September 1, 2004; 117(19): 4435 - 4448.
[Abstract] [Full Text] [PDF]

M. S. Perkinton, C. L. Standen, K.-F. Lau, S. Kesavapany, H. L. Byers, M. Ward, D. M. McLoughlin, and C. C. J. Miller
The c-Abl Tyrosine Kinase Phosphorylates the Fe65 Adaptor Protein to Stimulate Fe65/Amyloid Precursor Protein Nuclear Signaling
J. Biol. Chem., May 21, 2004; 279(21): 22084 - 22091.
[Abstract] [Full Text] [PDF]

H. Taru and T. Suzuki
Facilitation of Stress-induced Phosphorylation of {beta}-Amyloid Precursor Protein Family Members by X11-like/Mint2 Protein
J. Biol. Chem., May 14, 2004; 279(20): 21628 - 21636.
[Abstract] [Full Text] [PDF]

U. Beffert, P. C. Stolt, and J. Herz
Functions of lipoprotein receptors in neurons
J. Lipid Res., March 1, 2004; 45(3): 403 - 409.
[Abstract] [Full Text] [PDF]

J.-H. Lee, K.-F. Lau, M. S. Perkinton, C. L. Standen, S. J. A. Shemilt, L. Mercken, J. D. Cooper, D. M. McLoughlin, and C. C. J. Miller
The Neuronal Adaptor Protein X11{alpha} Reduces A{beta} Levels in the Brains of Alzheimer's APPswe Tg2576 Transgenic Mice
J. Biol. Chem., November 21, 2003; 278(47): 47025 - 47029.
[Abstract] [Full Text] [PDF]

M. H. Scheinfeld, E. Ghersi, P. Davies, and L. D'Adamio
Amyloid {beta} Protein Precursor Is Phosphorylated by JNK-1 Independent of, yet Facilitated by, JNK-Interacting Protein (JIP)-1
J. Biol. Chem., October 24, 2003; 278(43): 42058 - 42063.
[Abstract] [Full Text] [PDF]

S. Matsuda, Y. Matsuda, and L. D'Adamio
Amyloid {beta} Protein Precursor (A{beta}PP), but Not A{beta}PP-like Protein 2, Is Bridged to the Kinesin Light Chain by the Scaffold Protein JNK-interacting Protein 1
J. Biol. Chem., October 3, 2003; 278(40): 38601 - 38606.
[Abstract] [Full Text] [PDF]

Y. Hashimoto, T. Niikura, T. Chiba, E. Tsukamoto, H. Kadowaki, H. Nishitoh, Y. Yamagishi, M. Ishizaka, M. Yamada, M. Nawa, et al.
The Cytoplasmic Domain of Alzheimer's Amyloid-{beta} Protein Precursor Causes Sustained Apoptosis Signal-Regulating Kinase 1/c-Jun NH2-Terminal Kinase-Mediated Neurotoxic Signal via Dimerization
J. Pharmacol. Exp. Ther., September 1, 2003; 306(3): 889 - 902.
[Abstract] [Full Text] [PDF]

C. Noviello, P. Vito, P. Lopez, M. Abdallah, and L. D'Adamio
Autosomal Recessive Hypercholesterolemia Protein Interacts with and Regulates the Cell Surface Level of Alzheimer's Amyloid {beta} Precursor Protein
J. Biol. Chem., August 22, 2003; 278(34): 31843 - 31847.
[Abstract] [Full Text] [PDF]

C. A. Marques, U. Keil, A. Bonert, B. Steiner, C. Haass, W. E. Muller, and A. Eckert
Neurotoxic Mechanisms Caused by the Alzheimer's Disease-linked Swedish Amyloid Precursor Protein Mutation: OXIDATIVE STRESS, CASPASES, AND THE JNK PATHWAY
J. Biol. Chem., July 18, 2003; 278(30): 28294 - 28302.
[Abstract] [Full Text] [PDF]

H. Inomata, Y. Nakamura, A. Hayakawa, H. Takata, T. Suzuki, K. Miyazawa, and N. Kitamura
A Scaffold Protein JIP-1b Enhances Amyloid Precursor Protein Phosphorylation by JNK and Its Association with Kinesin Light Chain 1
J. Biol. Chem., June 13, 2003; 278(25): 22946 - 22955.
[Abstract] [Full Text] [PDF]

E. A. Willoughby, G. R. Perkins, M. K. Collins, and A. J. Whitmarsh
The JNK-interacting Protein-1 Scaffold Protein Targets MAPK Phosphatase-7 to Dephosphorylate JNK
J. Biol. Chem., March 14, 2003; 278(12): 10731 - 10736.
[Abstract] [Full Text] [PDF]

D. Gianni, N. Zambrano, M. Bimonte, G. Minopoli, L. Mercken, F. Talamo, A. Scaloni, and T. Russo
Platelet-derived Growth Factor Induces the beta -gamma -Secretase-mediated Cleavage of Alzheimer's Amyloid Precursor Protein through a Src-Rac-dependent Pathway
J. Biol. Chem., March 7, 2003; 278(11): 9290 - 9297.
[Abstract] [Full Text] [PDF]

M. H. Scheinfeld, S. Matsuda, and L. D'Adamio
JNK-interacting protein-1 promotes transcription of Abeta protein precursor but not Abeta precursor-like proteins, mechanistically different than Fe65
PNAS, February 18, 2003; 100(4): 1729 - 1734.
[Abstract] [Full Text] [PDF]

J. Schoorlemmer and M. Goldfarb
Fibroblast Growth Factor Homologous Factors and the Islet Brain-2 Scaffold Protein Regulate Activation of a Stress-activated Protein Kinase
J. Biol. Chem., December 13, 2002; 277(51): 49111 - 49119.
[Abstract] [Full Text] [PDF]

P. H. Frederikse and X.-O. Ren
Lens Defects and Age-Related Fiber Cell Degeneration in a Mouse Model of Increased A{beta}PP Gene Dosage in Down Syndrome
Am. J. Pathol., December 1, 2002; 161(6): 1985 - 1990.
[Abstract] [Full Text] [PDF]

C. Lutz, J. Nimpf, M. Jenny, K. Boecklinger, C. Enzinger, G. Utermann, G. Baier-Bitterlich, and G. Baier
Evidence of Functional Modulation of the MEKK/JNK/cJun Signaling Cascade by the Low Density Lipoprotein Receptor-related Protein (LRP)
J. Biol. Chem., November 1, 2002; 277(45): 43143 - 43151.
[Abstract] [Full Text] [PDF]

C. Russo, V. Dolcini, S. Salis, V. Venezia, N. Zambrano, T. Russo, and G. Schettini
Signal Transduction through Tyrosine-phosphorylated C-terminal Fragments of Amyloid Precursor Protein via an Enhanced Interaction with Shc/Grb2 Adaptor Proteins in Reactive Astrocytes of Alzheimer's Disease Brain
J. Biol. Chem., September 13, 2002; 277(38): 35282 - 35288.
[Abstract] [Full Text] [PDF]

P. Bruni, G. Minopoli, T. Brancaccio, M. Napolitano, R. Faraonio, N. Zambrano, U. Hansen, and T. Russo
Fe65, a Ligand of the Alzheimer's beta -Amyloid Precursor Protein, Blocks Cell Cycle Progression by Down-regulating Thymidylate Synthase Expression
J. Biol. Chem., September 13, 2002; 277(38): 35481 - 35488.
[Abstract] [Full Text] [PDF]

H. Taru, K.-i. Iijima, M. Hase, Y. Kirino, Y. Yagi, and T. Suzuki
Interaction of Alzheimer's beta -Amyloid Precursor Family Proteins with Scaffold Proteins of the JNK Signaling Cascade
J. Biol. Chem., May 24, 2002; 277(22): 20070 - 20078.
[Abstract] [Full Text] [PDF]

P. E. Tarr, R. Roncarati, G. Pelicci, P. G. Pelicci, and L. D'Adamio
Tyrosine Phosphorylation of the beta -Amyloid Precursor Protein Cytoplasmic Tail Promotes Interaction with Shc
J. Biol. Chem., May 3, 2002; 277(19): 16798 - 16804.
[Abstract] [Full Text] [PDF]

M. J. Savage, Y.-G. Lin, J. R. Ciallella, D. G. Flood, and R. W. Scott
Activation of c-Jun N-Terminal Kinase and p38 in an Alzheimer's Disease Model Is Associated with Amyloid Deposition
J. Neurosci., May 1, 2002; 22(9): 3376 - 3385.
[Abstract] [Full Text] [PDF]

M. Hashimoto, L. J. Hsu, E. Rockenstein, T. Takenouchi, M. Mallory, and E. Masliah
alpha -Synuclein Protects against Oxidative Stress via Inactivation of the c-Jun N-terminal Kinase Stress-signaling Pathway in Neuronal Cells
J. Biol. Chem., March 22, 2002; 277(13): 11465 - 11472.
[Abstract] [Full Text] [PDF]

Q. Hu, B. H. Cool, B. Wang, M. G. Hearn, and G. M. Martin
A candidate molecular mechanism for the association of an intronic polymorphism of FE65 with resistance to very late onset dementia of the Alzheimer type
Hum. Mol. Genet., February 1, 2002; 11(4): 465 - 475.
[Abstract] [Full Text] [PDF]

M. Goldfarb
Signaling By Fibroblast Growth Factors: The Inside Story
Sci. Signal., October 30, 2001; 2001(106): pe37 - pe37.
[Abstract] [Full Text] [PDF]

M. H. Scheinfeld, R. Roncarati, P. Vito, P. A. Lopez, M. Abdallah, and L. D'Adamio
Jun NH2-terminal Kinase (JNK) Interacting Protein 1 (JIP1) Binds the Cytoplasmic Domain of the Alzheimer's beta -Amyloid Precursor Protein (APP)
J. Biol. Chem., January 25, 2002; 277(5): 3767 - 3775.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (116)

Citing Articles via Google Scholar

Google Scholar

Articles by Matsuda, S.

Articles by Nishimoto, I.

Search for Related Content

PubMed

PubMed Citation

Articles by Matsuda, S.

Articles by Nishimoto, I.

Pubmed/NCBI databases
Gene GEO Profiles
HomoloGene Protein
UniGene
Compound via MeSH
Substance via MeSH
Medline Plus Health Information
Alzheimer's Disease