Systemic Amyloid Deposits in Familial British Dementia

doi:10.1074/jbc.M105956200

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Systemic Amyloid Deposits in Familial British Dementia^*

Jorge A. Ghiso^§^¶, Janice Holton^§§, Leticia Miravalle, Miguel Calero, Tammaryn Lashley^§§, Ruben Vidal, Henry Houlden^§§, Nicholas Wood^§§, Thomas A. Neubert^**, Agueda Rostagno, Gordon Plant, Tamas Révész^§§, and Blas Frangione^§

From the Departments of Pathology, ^§ Psychiatry, and ^** Pharmacology and Skirball Institute for Biomolecular Medicine, New York University School of Medicine, New York, New York 10016 and the Division of Neuropathology and ^§§ Department of Molecular Pathogenesis, Institute of Neurology and National Hospital for Neurology and Neurosurgery, London, WC1N 3BG, United Kingdom

Received for publication, June 26, 2001, and in revised form, September 12, 2001

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS AND DISCUSSION
REFERENCES

Familial British dementia (FBD) is an early onset inherited disorder that, like familial Alzheimer's disease (FAD), is characterizedby progressive dementia, amyloid deposition in the brain, andneurofibrillary degeneration of limbic neurons. The primary structureof the amyloid subunit (ABri) extracted from FBD brain tissues(Vidal, R., Frangione, B., Rostagno, A., Mead, S., Revesz, T.,Plant, G., and Ghiso, J. (1999) Nature 399, 776-781) is entirelydifferent and unrelated to any previously known amyloid protein.Patients with FBD have a single nucleotide substitution at codon267 in the BRI2 gene, resulting in an arginine replacing the stopcodon and a longer open reading frame of 277 amino acids insteadof 266. The ABri peptide comprises the 34 C-terminal residuesof the mutated precursor ABriPP-277 and is generated via furin-likeproteolytic processing. Here we report that carriers of the Stop-to-Argmutation have a soluble form of the amyloid peptide (sABri) inthe circulation with an estimated concentration in the range of20 ng/ml, several fold higher than that of soluble A $beta$ . In addition,ABri species identical to those identified in the brain were alsofound as fibrillar components of amyloid deposits predominantlyin the blood vessels of several peripheral tissues, includingpancreas and myocardium. We hypothesize that the high concentrationof the soluble de novo created amyloidogenic peptide and/or theinsufficient tissue clearance are the main causative factors forthe formation of amyloid deposits outside the brain. Thus, FBDconstitutes the first documented cerebral amyloidosis associatedwith neurodegeneration and dementia in which the amyloid depositionis alsosystemic.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS AND DISCUSSION
REFERENCES

Familial British dementia (FBD)¹ was originally described in 1933 by Worster-Drought et al. (1) as familial presenile dementiawith spastic paralysis. The pedigree has been followed and expandedsince then (2), and common ancestors have been identified incase reports by Griffiths et al. (3), and Love and Duchen (4).At present, the Worster-Drought pedigree comprises 343 individualsextending over nine generations dating back to ~1780 (5). Thedisease is clinically characterized by progressive dementia, spastictetraparesis, and cerebellar ataxia with an age of onset in thefifth decade. Brain MRI scans of FBD patients show the existenceof periventricular white matter hyperintensities resembling Binswanger'sleukoencephalopathy (2, 5). Neuropathological examinationof several FBD cases revealed a widespread severe amyloid angiopathywith perivascular deposits, amyloid plaques, and pre-amyloid lesionsaffecting the hippocampus and occasionally the cerebral cortex,and neurofibrillary tangles (NFTs) in hippocampal neurons (2,6, 7). Because of its clinical and neuropathological features,FBD has been previously interpreted as an atypical form of familialAlzheimer's disease (AD) (8), as an example of spongiform encephalopathy(9-11) and also regarded as a specific form of primary congophilicangiopathy (12).

We have recently reported that amyloid ABri, the main component of the parenchymal and vascular lesions in FBD, is a 4-kDapeptide derived from a type II transmembrane precursor moleculecodified by a single multiexonic gene BRI2 (also known as ITM2B(13)) located on the long arm of chromosome 13. A single substitutionin the BRI2 gene (TGA to AGA at codon 267) results in an argininereplacing the normally occurring stop codon in the wild type precursormolecule and a longer open reading frame of 277 amino acids (ABriPP-277)(14). Furin-like proteolytic processing releases the 34-aminoacid ABri peptide from the C terminus of the mutated precursorprotein (15). Amyloid isolated from leptomeningeal fibrillardeposits shows a high degree of polymerization and a post-translationallymodified N terminus (pyroglutamate) (14). Synthetic ABri peptidesare able to mimic in vitro the in vivo properties, namely thehigh tendency to polymerize and to form amyloid-like fibrils inphysiologic conditions (16).

The existence of circulating soluble precursors for both systemic and localized amyloid fibrils has been previously proposed(17) as a putative source of most amyloidogenic proteins. InAD, amyloid deposits are composed of A $beta$ , a 39-43-residue internalproteolytic fragment derived from a larger precursor protein A $beta$ PPwith a predicted structure of a multidomain, type I transmembranecell-surface receptor codified by a single gene on chromosome21 (reviewed in Ref. 18). A $beta$ species extracted from the tissuedeposits are heterogeneous at the N and C terminus and exhibita high tendency to form aggregates. A soluble form of A $beta$ (sA $beta$ )has been identified in body fluids, cell conditioned media, andbrain supernatants, consisting mainly of the first 40 residuesof the amyloid peptide. It has been demonstrated in guinea pigs,mice, and rats that the blood-brain barrier has the capabilityto modulate sA $beta$ transport in and out of the brain (19-21). Althoughthe contribution of circulating sA $beta$ to the deposited A $beta$ in ADbrains is still debatable, the circulating peptide has been postulatedto potentially contribute to the amyloid deposition (21). Inthe present report, we describe that in FBD-affected individuals,the de novo created ABri molecule is found not only in the circulationbut as the main constituent of amyloid deposits in peripheraltissues. The ABri species identified in systemic deposits areindistinguishable from those isolated form the brain. However,the circulating soluble ABri differs from the deposited peptidein that it lacks the post-translationally modified N-terminalpyroglutamate.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS AND DISCUSSION
REFERENCES

Immunohistochemistry-- Tissue blocks from different organs and skeletal muscle were taken at post mortem, fixed in 10% buffered formalin, and embeddedin paraffin. Seven-µm-thick sections pretreated with 99% formicacid were incubated at room temperature with anti-ABri polyclonalrabbit Ab 338 (specific for the ten C-terminal residues TVKKNIIEEN;1:2000) followed by biotinylated anti-rabbit IgG (1:200; Dako,Carpinteria, CA) and ABC complex (Dako). Color was developed withdiaminobenzinedine/H₂O₂. Double staining with Ab 338 and thioflavinS was carried out as described previously (6). Briefly, tissuesections were pretreated using 70% formic acid, blocked in drymilk solution, incubated with Ab 338 (1:2000) overnight at 4 °Cfollowed by biotinylated anti-rabbit antibody and ABC complex,and visualized using the tetramethylrhodamine signal amplificationkit (PerkinElmer Life Sciences). Sections were subsequently counterstainedin aqueous 1.0% thioflavin S (Sigma), differentiated with 70%ethanol, washed in phosphate-buffered saline, and viewed witha Zeiss Axioskop fluorescence microscope. Congo red staining wascarried out using a standard protocol and viewed under polarizedlight.

Amyloid Extraction-- Samples of pancreas, myocardium, and cerebral gray matter were homogenized at 4 °C in 10 mM phosphate buffer, pH 7.4, containing137 mM NaCl, 2.7 mM KCl, and protease inhibitors (Complete, Roche/RocheMolecular Biochemicals, Basel, Switzerland) and filtered through45-µm nylon mesh. The retained material, enriched in microvessels,was separately washed three times with the same buffer and centrifugedat 40,000 × g for 30 min at 4 °C, while the filtrated homogenatewas centrifuged at 100,000 × g for 45 min at 4 °C. The resultingpellets were subjected to collagenase (EC 3.4.24.3, Sigma typeI) digestion (1% w/w wet pellet) for 16 h at 37 °C followed bycentrifugation at 100,000 × g for 45 min at 4 °C, and the remaininginsoluble fractions, enriched in amyloid fibrils, were dissolvedin 99% formic acid and used for Western blot, N-terminal sequence,and mass spectrometryanalysis.

Plasma Samples-- Blood samples (7 ml) were collected from 15 normal controls and 20 affected and nonaffected FBD family members. After separationof plasma for immunoprecipitation experiments (see below), peripheralblood leukocytes were used for DNA isolation. After genomic DNAamplification by PCR, carriers of the Stop-to-Arg mutation wereconfirmed via restriction analysis with XbaI, as described previously(14).

Peptide Preparation-- Synthetic ABri peptide (EASNCFAIRHFENKFAVETLICSRTVKKNIIEEN) was synthesized at the W. M. Keck Foundation (Yale University)using solid-phase techniques. The peptide was purified by reverse-phasehigh performance liquid chromatography (C4; Vydac, Hesperia, CA)and its purity evaluated via amino acid sequence analysis andmass spectrometry. Oxidation of the cysteine residues with theconsequent formation of an intrachain disulfide bond was carriedout at pH 8.0 in the presence of air. The resulting mixture ofoxidized and nonoxidized ABri peptides was resolved by reverse-phasehigh performance liquid chromatography using a 40-min linear gradientof 20-80% acetonitrile in 0.05% trifluoroacetic acid and furtheranalyzed by mass spectrometry. Oxidized ABri exhibited a retentiontime of 27 min and an average mass of 3953.4 Da (expected 3953.3Da), while the reduced ABri peptide displayed a retention timeof 30 min and an average mass of 3955.2 Da (expected 3955.3Da).

Immunoprecipitation-- Fifty microliters of paramagnetic beads (Dynabeads M-450; Dynal Biotech, Lake Success, NY) coated with goat anti-rabbit IgGwere allowed to interact with polyclonal anti-ABri Ab 338 (3 h,room temperature), washed three times with phosphate-bufferedsaline and further incubated overnight at 4 °C with 200 µl ofplasma. After washing the beads three times with phosphate-bufferedsaline, bound components were eluted with 0.5 M acetic acid, pH2.5, and used for Western blots and mass spectrometryanalysis.

Western Blot Analysis-- Aliquots of both the isolated amyloid fractions and the immunoprecipitated components from biological fluids were separatedin Tris/Tricine gels under nonreducing and reducing conditions,transferred to a polyvinylidene difluoride membrane (Immobilon-P,Millipore Corp., Bedford, MA) using CAPS buffer, pH 11.0, containing10% (v/v) methanol and immunoreacted with Ab 338 (1:3000) followedby horseradish peroxidase-labeled anti-rabbit IgG (Amersham PharmaciaBiotech). Fluorograms were developed with ECL, exposed to HyperfilmECL (Amersham Pharmacia Biotech), and quantified by densitometryusing a standard curve (0.5 to 50 ng) of syntheticABri.

Sequence Analysis-- N-terminal sequence analysis of isolated ABri species was carried out by automatic Edman degradation on a 494 Procise ProteinSequencer (Applied Biosystems). Samples were separated on Tris/TricineSDS-polyacrylamide gel electrophoresis, transferred to Immobilonmembranes as described above, stained with Coomassie Blue, andthe pertinent bands excised andsequenced.

Mass Spectrometry-- Molecular masses of both the isolated amyloid fractions and the immunoprecipitated ABri components were determined at theNew York University Protein Analysis Facility. Amyloid-containingsamples (0.5 µl) were mixed with 0.5 µl of 10 mg/ml $alpha$ -cyano-4-hydroxycinnamicacid (Sigma-Aldrich) in 50% acetonitrile and 0.1% trifluoroaceticacid, air-dried, and analyzed on a Micromass TofSpec-2E (MALDI-TOF)mass spectrometer in linear mode using standard instrument settings.Internal and/or external calibration was carried out using syntheticA $beta$ 1-42 (average mass = 4513.1 Da), angiotensin I (average mass= 1296.5 Da), and insulin (average mass = 5733.5Da).

RESULTS AND DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS AND DISCUSSION
REFERENCES

A soluble form of ABri (sABri) in serum of patients with FBD was identified using a combination of immunoprecipitation, massspectrometry, and Western blot analysis. Immunoprecipitation experimentswith antibodies specific to the ten C-terminal residues of theABri peptide (TVKKNIIEEN; Ab 338 (14)) followed by Western blotand chemiluminescence identified a 4-kDa soluble component inall tested carriers of the Stop-to-Arg mutation (n = 8), and itwas consistently absent in noncarrier family members (n = 12)and normal controls (n = 15) (Fig. 1). In contrast to the brain-depositedABri (14), sABri was consistently monomeric and devoid of N-terminalpyroglutamate with an observed average mass of 3953.5 ± 0.5 Da(expected: 3953.3 Da for the ABri peptide with oxidized cysteineresidues). No obvious N- and/or C-terminal heterogeneity was observed.The experimental average mass was close to the theoretical massvalue of the oxidized ABri peptide, suggesting that some of thesoluble ABri molecules may contain a single intrachain disulfidebond. Consistent with these data is the mass spectrometry analysisof synthetic full-length ABri peptides either containing or lackinga single disulfide bond between cysteine residues 5 and 22. Theobserved average mass for the oxidized synthetic ABri was 3953.4Da versus 3955.2 Da for the reduced peptide (see "Materials andMethods"). A molecular mass of 3935.5 Da was previously reportedfor a secreted ABri species detected in conditioned medium ofN2a cells transfected with full-length ABriPP-277 cDNA containingthe Stop-to-Arg mutation, a mass value also consistent with thepresence of N-terminal glutamate and suggestive of oxidized cysteines(15).

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Fig. 1. Soluble ABri species in plasma. Mass spectrometry analysis of sABri immunoprecipitated with anti-ABri antibody (Ab 338) shows an average mass of 3954.5 Da (values expressed as M + H⁺). Inset, Western blot analysis of five plasma samples obtained from FBD family members. Soluble ABri is detected in three carriers of the Stop-to-Arg mutation (lanes 4-6), while it is absent in noncarrier family members (lanes 2 and 3). Immunoprecipitation of synthetic ABri used as a positive control is shown in lane 1.

The origin of the circulating soluble ABri is not clearly established yet; however, based on Northern blot analysis (14)it can be speculated that the brain, kidney, and pancreas mightbe the most likely sources. The plasma levels in the small numberof FBD carriers available (n = 8) was estimated in the range of20 ng/ml by means of scanning densitometry of the immunoprecipitatedbands. The existence of such elevated plasma levels of sABri mayimply that, in FBD patients, amyloid deposits could also occuroutside the central nervous system. Using conventional immunohistochemicalmethods, we searched for ABri deposits in systemic organs obtainedat autopsy from two FBD cases. As previously demonstrated forcerebral amyloid and pre-amyloid lesions (6, 14), Ab 338labeled Congo red (CR)-positive/thioflavin S (TS)-positive bloodvessels in organs such as pancreas (Fig. 2), adrenal gland, lung,myocardium, liver, spleen, and skeletal muscle (not shown). Parenchymaldeposits either CR-negative/TS-negative or CR-positive/TS-positivewere also seen in organs such as pancreas (Fig. 2), adrenal gland,myocardium, and skeletal muscle (not shown). Western blot analysisand mass spectrometry data of the amyloid material extracted fromeither vascular or parenchymal lesions of two peripheral organs(pancreas and heart) revealed ABri species identical to thosefound in the brain lesions. As illustrated in Fig. 3 for the parenchymaldeposits in pancreas, the pattern of ABri immunoreactivity (ABrimonomers, dimers, trimers, and larger oligomeric species) wascomparable with that of the amyloid isolated from the brain. N-terminalsequence analysis of the 4- and 8-kDa components rendered similarresults, two minor sequences SNXFAIRHF (corresponding to positions3-11 of ABri) and EASNXFAIX (corresponding to residues 1-8 ofABri) that represented less than 20% of the protein loaded, suggestinga blocked N terminus for the main deposited component, as previouslyreported for the leptomeningeal ABri amyloid (14).

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Fig. 2. Amyloid deposits in the brain and pancreas in a case of FBD. A-D, ABri deposits in the cerebellum and pancreas, visualized by fluorescence microscopy. Deposition of ABri (A), which is also thioflavin S-positive (B), is illustrated in a leptomeningeal blood vessel and cerebellar parenchyma. ABri deposition (C) in a similarly affected blood vessel and around parenchymal epithelial cells in the pancreas is also thioflavin S-positive (D). A and C, antibody 338 immunohistochemistry; B and D, thioflavin S staining; A-D, original magnification × 50.

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Fig. 3. Western blot analysis of amyloid fractions. Amyloid extracted from the pancreas (left lane) and the brain (right lane) was tested for immunoreactivity with Ab 338. Note the similar pattern of ABri polymerization.

Mass spectrometry analysis of the same fractions (depicted in Fig. 4) confirmed that the full-length ABri peptide featuringpyroglutamate at the N terminus with an observed average mass3935.7 ± 0.3 Da (expected 3935.5 Da) was the main constituentof both brain and peripheral deposits. The experimental mass obtained,3935.7 Da, was also close to the theoretical mass of the oxidizedpeptide and differed in 18 units from the ABri species found incirculation (average mass 3953.5 Da), a value accountable forthe loss of one molecule of water and the formation of pyroglutamate.Two minor components were also identified: (a) a full-length ABripeptide containing glutamic acid at the N terminus, identicalto sABri (observed average mass 3953.5 ± 0.4 Da; expected 3953.3Da) and (b) an N-terminal truncated ABri fragment starting atserine 3 (observed average mass 3753.4 ± 0.3 Da; expected 3,753.3Da), a product previously identified in cerebrovascular deposits.Collectively, the last two components accounted for less than20% of the systemic amyloid deposits and less than 10% of thebrain lesions, results consistent with the amino acid sequencedata. As also indicated in Fig. 4, formylated species of all theabove mentioned peptides, probably by-products of the extractionprocedure, were present in the samples. Almost identical resultswere obtained with the microvessels extracts (data not shown).When compared in terms of electrophoretic mobility, pattern ofpolymerization, immunoreactivity, and molecular mass, the ABriamyloid subunits deposited in the brain were chemically indistinguishablefrom that in the systemic organs studied, indicating that in bothcases, amyloid formation most likely occurs by a similar (if notidentical) biochemical mechanism.

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Fig. 4. Mass spectrometry analysis of amyloid fractions. Amyloid extracted from the pancreas (top) and the cerebral gray matter (bottom) was subjected to MALDI-TOF mass spectrometry analysis, as described under "Materials and Methods." Notation: 1, peaks with an average mass of 3936.8 Da (brain) and 3936.7 Da (pancreas) correspond to the ABri molecule bearing pyroglutamate at the N terminus; 2, peaks with an average mass of 3954.6 Da (brain) and 3954.5 Da (pancreas) represent ABri species containing glutamate at the N terminus; 3, peaks with an average mass of 3754.2 Da (brain) and 3754.4 Da (pancreas) correspond to ABri species starting at serine 3; *, indicates Abri-formylated species (average mass change of +28).

The neuropathology of FBD is strikingly similar to that of AD, i.e. both exhibit vascular amyloid and parenchymal amyloidand pre-amyloid deposition and NFTs (22). In AD, parenchymalA $beta$ deposits are mainly present in the hippocampus and the cerebralcortex, while A $beta$ vascular lesions are predominantly seen in leptomeningealand cortical vessels. Degenerating neurons containing NFTs arefrequent in limbic areas and in the neocortex. Paired helicalfilament-containing abnormal neurites, frequently co-localizewith amyloid deposits (neuritic plaques). In FBD, however, severeamyloid angiopathy with perivascular plaque formation occurs throughoutthe central nervous system. Parenchymal amyloid plaques and pre-amyloiddeposits together with neurofibrillary pathology predominantlyaffect limbic structures but rarely the cerebral cortex, clearlyindicating that amyloid deposition is of primary importance inthe initiation of neurodegeneration. The distribution of NFTsin FBD corresponds to stage IV in the system recommended by Braakand Braak for AD (23). Similar to AD, the NFTs in FBD are ultrastructurallycomposed of paired helical filaments; moreover, the electrophoreticpattern of abnormal hyperphosphorylated tau isolated from FBDbrain tissue is indistinguishable from that seen in AD (6,7). The presence of the soluble amyloid peptide sABri in plasmaadds another element to the striking pattern of similarities betweenFBD and AD, although the plasma levels of sABri surpasses by atleast 10-fold those of sA $beta$ . Despite this similitude, the ABriamyloid subunit forming the lesions in FBD is completely unrelatedin sequence to the A $beta$ molecule composing the fibrillar depositsin AD.

The N-terminal amino acid of many proteins, hormones, and neurotrasmitters is pyroglutamic acid. The pyroglutamyl moiety resultsfrom the post-translational modification of either glutamine orglutamic acid. Cyclization of glutamine to pyroglutamic acid involvesthe nucleophilic attack of the $alpha$ -amino group on the amidated carboxylgroup, and the reaction is catalyzed at neutral pH by an enzymeknown as glutamine cyclotransferase (24-26). Less is known aboutthe cyclization of glutamic acid in which the chemical reactioninvolves the loss of one molecule of water, although an apparentlyspecific enzymatic activity has been recently detected in Aplysianeurons (27). Analysis of the genes codifying the many moleculescontaining this post-translational modification indicate thatglutamine and not glutamate is the common precursor of the N-terminalpyroglutamic acid. However, few exceptions have been reported,among them processing products of pro-opiomelanocortin (28)and fragments of Alzheimer's A $beta$ peptide (29-31). In the later case,the use of mass spectrometry and specific antibodies have allowedthe identification in the brains of AD patients of deposited modifiedA $beta$ species A $beta$ pE3 and A $beta$ pE11 starting at residues 3 and 11 andcontaining N-terminal pyroglutamate. In both instances the originalamino acid is glutamic acid, as it is the case of the ABri amyloidas well as in the recently described ADan peptide, the main componentof cerebral amyloid deposits in familial Danish dementia (32).The mechanism that produce these N-terminal blocked peptides isnot entirely clear. In the case of ABri, it is released from itsprecursor ABriPP-277 by a furin-like proteolytic processing thatoccurs in the Golgi apparatus. Using N2a cells transfected withABriPP-277, the release of full-length ABri to the conditionedmedia was demonstrated (15). The peptide contained glutamatebut not pyroglutamate at the N terminus, and it was identicalin mass to the circulating sABri described above. Therefore, onelikely possibility is that the chemically irreversible conversionfrom glutamate to pyroglutamate in FBD takes place at the siteof deposition; alternatively, the rate of amyloid formation anddeposition may preferentially favor the pyroglutamate-containingpeptide. The finding that the same ABri species are found in thebrain and systemic organ amyloid deposits suggests that the pyroglutamate-formingmechanism is not neuron-specific. It is interesting to note thatA $beta$ and ABri may also share a similar mechanism for the releaseof the two N-terminal residues that generate A $beta$ 3-40/42 and ABri3-34. Both molecules contain an acidic N-terminal amino acid followedby alanine (Asp-Ala- $down-arrow$ in A $beta$ and Glu-Ala- $down-arrow$ in ABri), a likely substratefor dipeptidyl aminopeptidases II and IV (33, 34).

The presence of Congo red/thioflavin S-positive ABri amyloid deposits in systemic organs in individuals with FBD contrastswith the findings of Congo red-negative A $beta$ immunoreactivity innon-central nervous system tissues deposits in AD patients (35-37).Several elements may converge to produce systemic ABri amyloiddeposits in patients with FBD: (i) high levels of the putativecirculating precursor, increasing the probability of monomer-monomerinteractions resulting in polymerization; (ii) the presence ofN-terminal pyroglutamate, which facilitates aggregation and increasesthe resistance to proteolytic degradation by amino peptidases;(iii) the unlikelihood that specific cellular receptors participatein the physiologic clearance of the deposits, since sABri/ABriare de novo createdmolecules.

Amyloid deposits simultaneously present in the brain and in systemic organs have been previously found in another autosomaldominant disorder, hereditary cerebral hemorrhage with amyloidosis,Icelandic type (HCHWA-I). This disease, characterized by massiveamyloid deposition of mutant cystatin C Q68 (38) within smallarteries and arterioles of leptomeninges, cerebral cortex, basalganglia, brainstem, and cerebellum (39), also presents withsilent amyloid deposits in peripheral tissues such as skin, lymphnodes, spleen, salivary glands, and seminal vesicles (40). Despitethese similarities the main clinical hallmark of the disease iscerebral hemorrhage, not dementia, with fatal outcome in the thirdto fourth decade of life. The results reported here (summarizedin Fig. 5) indicate that FBD is the first documented cerebralamyloidosis associated with extensive neurofibrillar degenerationin which significant amyloid deposits are also found in peripheralorgans. The extent to which the systemic amyloid precursor peptidecontributes to the mechanism of cerebral amyloid formation remainsan open question. The corroboration of an active role of circulatingsABri in amyloid deposition in the brain and elsewhere will undoubtedlychange the therapeutic approaches proposed for inhibiting amyloidogenesisin the human brain.

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Fig. 5. Schematic summary of the deposited ABri species identified in the brain and pancreas in comparison with soluble ABri identified in plasma. The table at the righthand side of the figure shows the theoretical and experimental average masses (in daltons) of each of the identified ABri components.

	ACKNOWLEDGEMENT

We thank Yun Lu for expert technical assistance with MALDI-TOF massspectrometry.

	FOOTNOTES

^* This work was supported by National Institutes of Health (NIH) Grants AG05891 (MERIT) and AG08721, the Alzheimer's Association,The Brain Research Trust, and NIH Shared Instrumentation GrantsRR14662 and RR13077.The costs of publication of this article weredefrayed in part by the payment of page charges. The article musttherefore be hereby marked "advertisement" in accordance with18 U.S.C. Section 1734 solely to indicate thisfact.

^¶ To whom correspondence should be addressed: Dept. of Pathology, NYU School of Medicine, 550 First Ave., TH-432, New York,NY 10016. Tel.: 212-263-7997; Fax: 212-263-6751; E-mail: ghisoj01@popmail.med.nyu.edu.

Published, JBC Papers in Press, September 13, 2001, DOI 10.1074/jbc.M105956200

ABBREVIATIONS

The abbreviations used are: FBD, familial British dementia; NFT, neurofibrillary tangle; AD, Alzheimer's disease; Ab, antibody; CAPS, 3-(cyclohexylamino)propanesulfonic acid; Tricine, N-[2-hydroxy-1,1-bis(hydroxymethyl)ethyl]glycine; MALDI-TOF, matrix-assisted laser desorption ionization time-of-flight; CR, Congo red; TS, thioflavin S.

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