Deadly Conformations: Protein Misfolding in Prion Disease
Models for the Conversion of PrPC to PrPSc
Conformational basis for prion strains
Cell, Vol. 89, 499-510, May 16, 1997 Arthur L. Horwich and Jonathan S. Weissman
Novel infectious particles, termed prions, composed largely and perhaps solely of a single protein, are the likely causative agents of a group of transmissible spongiform encephalopathies that produce lethal decline of cognitive and motor function. As if the notion of a transmissible pathogenic protein is not jarring enough, evidence indicates that the responsible protein arrives at a pathogenic state by misfolding from a normal form that has ubiquitous tissue distribution. The remarkable nature of these diseases and the nature of the prion protein conversion process as we currently understand it are reviewed below.
Transmissibility of kuru was first demonstrated following intracerebral inoculation of homogenate of kuru brain into chimpanzees (Gajdusek et al., 1966 ), but within the highlander population it was eventually surmised that transmission was occurring by ritual cannibalism (Gajdusek, 1977 ).
Figure 1. Neuopathological Findings in Transmissible Spongiform EncephalopathiesThree other clinically or pathologically similar neurodegenerative diseases have been recognized in humans, and for all of these, as with kuru, disease has been observed to be transmissible to experimental animals by intracerebral inoculation. In 1936, Gerstmann, Ströussler, and Scheinker described a condition with ataxia and progressive dementia, occurring after age 40, associated, as in kuru, with plaques in the brain of affected individuals (Gerstmann et al., 1936 ). Multiple affected family members were observed, in a pattern indicating autosomal-dominant inheritance. Similar genetic transmission has also been observed for a rare condition more recently described, familial fatal insomnia (FFI), exhibiting lethal insomnia and autonomic dysfunction associated with pathologic changes confined to nuclei in the thalamus (e.g., Manetto et al., 1992 ). By contrast, the more common condition, Creutzfeldt-Jakob disease (CJD), usually occurs sporadically and presents with dementia occurring after age 40, with pathology generally featuring spongiform degeneration.
(Top Row) Plaque lesions in Creutzfeldt-Jacob disease (CJD) (first panel); the variant form of CJD (vCJD), recently shown to be transmissible to primates from BSE-infected cattle (second panel); and Gerstmann-StraŞssler Scheinker disease (GSS) (third panel). In the first panel, the section is stained with PAS (periodic acid-Schiff reaction) and shows a centrally located plaque lesion exhibiting the "spiked ball" appearance typical of a kuru plaque). In the second panel, the section is stained with PAS and shows a number of so-called "florid plaques" typical of vCJD, in each case with a central plaque lesion surrounded by a daisy-like pattern of vacuoles. The third panel is a section immunostained after hydrolytic autoclaving with anti-PrP antiserum, revealing the presence of PrP in the plaque lesions of GSS.
(Middle Row) Spongiform changes typical of CJD. Section obtained from an affected transgenic mouse, carrying a chimeric mouse-human-mouse transgene, that had been inoculated with brain homogenate from a human sporadic CJD case .
(Bottom Row) Histoblot analysis of brain section from an individual with CJD and from an unaffected individual. Staining is with anti-PrP antibody, showing extensive staining of PrP in the cortical mantle of the affected individual ).
While most CJD cases are sporadic in occurrence, autosomal-dominant transmission accounts for 10% of cases. Horizontal transmission of CJD to chimpanzee was demonstrated early (Gibbs et al., 1968 ), but particularly notable have been cases of transmission between humans iatrogenically, through transplantation of infected corneas or injection of growth hormone derived from human pituitaries (see DeArmond and Prusiner, 1996 ).
Even more striking have been a number of early-onset CJD cases with atypical pathology recently reported from Great Britain (Will et al., 1996 and see Figure 1), suggested to have been transmitted by consumption of meat from cows suffering from mad cow disease, a spongiform encephalopathy recently epidemic in British herds (see Anderson et al., 1996 , concerning progression of the epidemic). The recent reports of production of a clinically and pathologically similar CJD in macaques by intracerebral injection of brain homogenate from afflicted cows (Lasm╚zas et al., 1996b ), and of biochemical properties shared between the human cases and bovine spongiform encephalopathy (BSE) (Collinge et al., 1996 ), suggest that BSE is transmissible to man.
This led to a number of hypotheses about the nature of the infectious agent, ranging from a replicating polysaccharide to a nucleoprotein complex (for review, see Prusiner, 1982 ). Among these models was a prescient speculation, in which Griffith suggested that "conversion" of a protein from a normal energetically favored conformation to another conformation, either spontaneously or by exogenous introduction of the altered conformation, could explain these diseases (Griffith, 1967 ).
The molecular nature of the infectious agent lay largely untested for 15 years until Stanley Prusiner and coworkers achieved the biochemical enrichment of infectious activity and showed its association with a specific protein. In early 1982, Prusiner and coworkers reported a 1000-fold enrichment of scrapie infectivity from homogenate of infected brain, achieved through a series of steps including polyethylene glycol precipitation, micrococcal nuclease digestion, limited proteinase K digestion, and sucrose density gradient centrifugation (Prusiner et al., 1982 ; Prusiner, 1982 ). The highest activity came from a fraction at the interface between 25% and 60% sucrose, where aggregates composed of amorphous material and flattened rods measuring 25 nm x 100-200 nm were observed. The enriched activity was inactivated by proteinase K, diethylpyrocarbonate, urea, chaotropes, phenol, and SDS, but was not abolished by nuclease treatments or UV irradiation. This behavior, typical of a protein, gave rise to the name attached by Prusiner and coworkers, "prion," for proteinaceous infectious particle (Prusiner, 1982 ; see also Prusiner et al., 1980 ).
The same workers identified a protein, designated PrP, resistant to limited proteinase K digestion, that was specifically present in infected hamster brain but not in normal brain and exhibited a relative migration in SDS-PAGE of 27-30 kDa (Bolton et al., 1982 ; Prusiner et al., 1982 ). Whether this species was a byproduct of infection, or was directly responsible, could not be immediately distinguished, although the copurification of proteinase K-resistant PrP 27-30 with infectivity offered circumstantial evidence that it was involved with causation. Similarly, rod structures, first observed by Merz et al., 1981 , were observed in the proteinase K-treated extracts of infected brain and were found also to contain the PrP 27-30 core product. Preparations enriched for these rods were shown to be highly infectious (Prusiner et al., 1983 ; Diringer et al., 1983 ), although subsequent studies have shown that preparations devoid of visible structures can also be infectious. Coenrichment of PrP 27-30 and infectivity was observed in another setting, when immunoaffinity purification of detergent-lipid-solubilized infected brain extract was carried out, showing several 1000-fold enrichment of both PrP 27-30 and infectivity (Gabizon et al., 1988 ).
This was consistent with the notion that there is tight linkage between infectivity and the presence of some form of the PrP protein. Nonetheless, despite years of effort, even in the purest samples, the ratio of PrP molecules to infectious units is 105. At such low infectivity, it is impossible to exclude the possibility that other components, or covalent modifications, are required for infectivity. However, highly-purified infectious material has been shown to contain less than one molecule of nucleic acid larger than 100 nt for a particle-to-infectivity ratio near unity (Kellings et al., 1992 ). Thus, it seems likely that demonstration of the protein only hypothesis will require the production of infectious particles in vitro from purified PrP protein (that has a level of impurity of less than 1 part per infectious unit).
Antibodies generated against PrP 27-30 identified the PrP protein not only in the brain of uninfected animals but also in many visceral tissues as a 33-35 kDa glycosylated species, termed PrPC. A protein of identical size was also observed in scrapie-infected brain extracts. Strikingly, when limited proteinase K digestion was carried out, PrPC was completely degraded, whereas a fraction of the protein in infected brain, termed PrPSc, was only partially cleaved, removing 66 NH2-terminal amino acids to produce the species PrP 27-30. Thus, the PrP protein appears to have at least two distinct conformational states: a protease-sensitive one found ubiquitously, and a protease-resistant one in the setting of infection. Perhaps linked to such protease-resistant behavior is the additional observation that, while PrPC is a soluble protein, the PrPSc form is stubbornly insoluble, localizing in the amorphous aggregates in enriched fractions from infected brain (e.g., Meyer et al., 1986 ). In any case, the protease resistance of the PrPSc form has been relied on to allow the detection of PrPSc in situ in both experimental and clinical diagnosis. This is accomplished by pretreatment with proteinase K to remove PrPC, followed by guanidine treatment to expose epitopes of PrPSc for immunolocalization (Taraboulos et al., 1992 see Figure 1 histoblot).
Given the same primary structure of PrPC and PrPSc, the process whereby the normal state of PrP protein is "converted" to the infection-associated form seemed likely to involve either posttranslational modification or a change in conformation (e.g., Hope et al., 1986 ). Extensive biochemical characterization has failed to find any covalent difference between the PrPC and PrPSc proteins (e.g., Stahl et al., 1993 ). By contrast, physical measurements have demonstrated a dramatic conformational difference in the PrP forms. For example, Fourier transform infrared spectosocopy and circular dichroism indicate that the -helical content of the PrPC form is 40%, with little or no ■ sheet (Pan et al., 1993 ).
By contrast, the PrP 27-30 form contains 50% ■ sheet and only 20% helix (Caughey et al., 1991 ; Pan et al., 1993 ; Safar et al., 1993 ). The recently presented solution structure of a fragment of the mouse PrPC has allowed a direct determination of secondary structure content of this portion of PrPC (Riek et al., 1996 ). The agreement with the FTIR study is excellent: out of 109 resolvable residues in the PrP 121-232 species, 43 lie in helix (40%), while only 8 residues lie in two short antiparallel ■ strands (7%) (see Figure 3B).
Figure 2. Schematic Model for the Conversion of PrPC to PrPSc
In the nucleation-polymerization model, conversion between the PrPC form (circles) and PrPSc form (squares) is inherently fast. However, in the absence of an aggregate large enough to act as a stable nucleus, designated by the collective of PrPSc squares, the PrPC form is thermodynamically favored. In the template assistance model, the conversion of PrPC or an altered conformation, PrPInt, to PrPSc is extremely slow in the absence of PrPSc, but the conversion process is effectively irreversible. The PrPSc is able to propagate itself by catalyzing the conversion of other PrPInt molecules to the PrPSc conformation. Additional unidentified factors, e.g., a molecular chaperone, might also be involved in the conversion process (see text).
Figure 3. Structure of Prion Protein
(A) Primary structure of mature human PrP. The sequence of the mature protein, residues 23-231, after proteolytic processing of the NH2-terminal secretory signal and the COOH-terminal region beyond the GPI anchor site, is shown. Mutations involved with inherited human disease are indicated in red, above the line, and naturally occurring polymorphisms are shown as numerator/denominator on the line, in purple. The asterisk indicates a mutation producing a stop codon at amino acid 145. Residues implicated in species barriers are also shown, between human and mouse (backlit in blue), and between mouse and hamster (backlit in yellow). Secondary structure of corresponding region 123-231 of mouse PrP, determined from the NMR structure (Riek et al., 1996 ), is shown above the primary sequence, with ■ strands represented by arrows and helices by cylinders.
(B) Structure of mouse prion protein domain PrP121-231. Two opposite faces are shown of the mouse PrP121-231 structure recently determined by NMR (taken from Riek et al., 1996 , with permission). Ribbon diagrams are shown in the two left panels, displaying the three helices and the short antiparallel two-stranded ■ sheet. In the top left panel, green indicates well resolved loop structure, whereas purple indicates poorly resolved loop structure. A disulfide bond is shown in white. In the bottom left panel, side chains associated with inherited prion disease are shown in red, and residues that may be involved in the species barrier between mouse and human are shown in blue (Q168 side chain is not shown). (Note that side chain numbering corresponds to the human sequence shown in [A]). Two solvent-accessible glycosylation sites are also shown in green and the disulfide bond in yellow. Electrostatic potential plots are shown in the two right panels, displaying positive charge as blue and negative charge as red. The aspect of the molecule shown in the top panel has been suggested to possibly face a membrane, whereas the opposite, negatively-charged aspect (lower panels) may present a binding surface for an as yet unidentified ligand (see text).
Two different genetic studies with mice have provided perhaps the strongest evidence arguing that infectious particles are generated from the endogenous PrPC protein. In one, spontaneous prion disease was observed in uninoculated transgenic mice expressing a mouse PrP with a substitution homologous to that in GSS patients (Hsiao et al., 1990 ; Hsiao et al., 1994 ; Telling et al., 1996a ). Importantly, brain homogenates from these mice can transfer prion disease when inoculated into transgenic mice expressing low levels of the same mutant PrP protein, that would not otherwise develop disease (Hsiao et al., 1994 ; Telling et al., 1996a ). Thus, all the components required to form infectious particles appear to be present endogenously in the mice. Moreover, it appears that removal of the endogenous PrP gene in the latter study led to earlier onset of disease and more severe pathology in the uninoculated transgenic strain, reflecting that the presence of wild-type PrP somehow interfered with disease production from the mutant transgene.
In a second avenue of study, a requirement for PrPC protein in generating infectivity was demonstrated directlymice with a disruption in the endogenous PrP gene (Prnp0/0) were both resistant to prion disease and unable to generate new infectious particles (BŞeler et al., 1993 ; Prusiner et al., 1993 ). A straightforward hypothesis suggested by these observations is that endogenous PrPC is converted to PrPSc conformation by the action of an infectious form of the PrP molecule. However, given the low specific activity of even the purest PrPSc samples and the observation that under some circumstances it appears that there can be both disease and infectivity in the absence of protease-resistant material (e.g., the GSS mice), it remains possible that the infectious form of PrP is distinct from the protease-resistant PrPSc form.
As would be predicted for a homologous conversion reaction in which new PrPSc is generated from the endogenous PrPC, when the species of PrPSc in the brains of transgenic mice expressing the hamster PrPC was determined following challenge with hamster prions, the hamster PrPSc protein was observed (Prusiner et al., 1990 ). Correspondingly, if the transgenic animals were inoculated with mouse prions, mouse PrPSc was observed in the infected brain.
The location in the PrPC structure of the homologous interaction with PrPSc was probed by producing transgenic mice bearing chimeric genes. When the midportion of the hamster sequence (codons 94-188), differing at 5 residues from mouse, was substituted for the corresponding region of mouse PrP, the transgenic mice were observed to become susceptible to hamster prions, producing, as expected, chimeric PrPSc (Scott et al., 1993 and see Figure 3A).
Supporting the proposal that the in vitro reaction faithfully reproduced that in vivo, species specificity in the conversion reaction between hamster, mouse, and the hamster-mouse chimeras was reproduced by the in vitro reaction (Kocisko et al., 1995 ). Moreover, there was preservation of "strain" specificity in vitro (discussed below), insofar as the distinct proteinase K resistance patterns of PrPSc from two mink prion strains, presumably reflecting different PrPSc conformations, were reproducible in the in vitro system (Bessen et al., 1995 ).
In one model, formation of PrPSc is a nucleation-dependent polymerization process. In the absence of a preexistent aggregate, the conversion between PrPC and PrPSc is reversible, but PrPSc monomer is less stable than PrPC. PrPSc aggregates, however, promote the conversion of PrPC by binding to and stabilizing the otherwise unfavored PrPSc conformation. The barrier to a stable conversion process thus lies at the level of the initial nucleation process, in which formation of low order aggregates is not favored, since the free energy gained from intermolecular interactions does not outweigh the entropic cost of binding until a minimum size nucleus is attained.
The requirement that a nucleus be formed before conversion is stable predicts certain characteristics of the aggregation process, including dependence on exceeding a critical protein concentration for the initial formation of aggregates, and kinetics displaying a lag phase. The in vitro conversion process appears to show such features (Caughey et al., 1995 ), but whether a PrPSc nucleus is already present is unclear from the design of the study. The relatively large size of the minimum stable nucleus would tend to make such a particle insoluble and could therefore account for the observation in the in vitro reaction that fractions containing higher-order PrPSc aggregates greater than 300 kDa in size could mediate the conversion to protease resistance while smaller-sized fractions could not. Infection would thus circumvent the slow step of nucleation by introducing a "seed" that initiates aggregation.
In a second proposed mechanism, the PrPSc form is inherently more stable than PrPC, but kinetically inaccessible (Prusiner, 1991; Figure 2). In this case, PrPSc could promote conversion by catalyzing the rearrangement of a molecule of PrPC, or of a partially destabilized intermediate, to the more stable PrPSc conformation (Figure 2). Infectivity would then rely on the ability of the PrPSc molecule to bind to and catalyze the conversion of existing intermediate molecules. By this template assistance model, the genetically inherited diseases result from mutations that increase the population of the unstable intermediate and/or enhance the rate at which this form spontaneously converts to PrPSc.
For both of the proposed mechanisms, there are physical precedents. In the case of nucleation-polymerization, there is a resemblance to tubulin polymerization, crystal growth, sickle hemoglobin formation, viral capsid assembly, and bacterial flagellar polymerization. Flagellar polymerization may be particularly instructive. The soluble monomer unit, flagellin, becomes incorporated into the growing end of a flagellum (Asakura et al., 1964 Asakura et al., 1966 ). Monomers in solution, even at nearly millimolar concentration, occupy a conformation unable to spontaneously nucleate, but if a seed of fragmented flagellum is placed into the mixture, then polymerization rapidly ensues. Interestingly, the polymerizing monomers can assume the conformation of even heterologous seed material, reflecting a "templating" behavior. It should be pointed out that while the foregoing "aggregates" adopt a regular repeating structure, there is nothing in the physics underlying a nucleation process that requires that the aggregates formed must have long-range order.
There is also precedent for the template-assisted, catalyzed conversion mechanism, in which PrPC is a metastable conformation that does not spontaneously form the more stable PrPSc at any appreciable rate. During the past few years, a number of proteins have been observed to occupy such conformations under kinetic control, i.e., they are separated from their true free energy minima by a large barrier. These include influenza hemagglutinin (Baker and Agard, 1994a ), the serpin family of protease inhibitors (Sifers, 1995 ), and a number of proteases including subtilisin and -lytic protease (Baker and Agard, 1994b ). This last case of alpha-lytic protease is particularly revealing.
Here, the interconversion between a molten globule-like intermediate, I, and the native state, N, is extremely slow, allowing little or no conversion over the course of a month (reflecting a barrier of 25 kcal/mole). Conversion, however, is dramatically accelerated by binding of the naturally-occurring propeptide region, in either cis or trans, allowing folding to N to occur within minutes (the propeptide lowers the barrier by 14 kcal/mole). This behavior raises the possibility that folding of PrP is also under kinetic control, with the PrPSc state thermodynamically favored but kinetically inaccessible. Infectious prion disease could then result if PrPSc were able to accelerate the conversion of PrPC to PrPSc in a manner analogous to the catalyzed conversion between the I and N states of -lytic protease.
It is important to note that the nucleation and catalyzed conversion mechanisms are not mutually exclusive. For example, there could be a hybrid mechanism by which the surface of an aggregate, which is initially formed by a nucleation process, catalyzes the conformational change of unconverted monomers. Indeed, in the case of flagella formation in vitro, kinetic studies show a lag between the initial, reversible, binding, and stable incorporation into the flagellum (Asakura, 1968 ). Moreover, NMR studies indicate that the NH2 and COOH termini of flagellin, disordered in the monomers in solution, become ordered during the process of polymerization (Aizawa et al., 1990 ). By analogy, it seems attractive to consider that PrPC could become converted in this manner, after an initial interaction with a PrPSc aggregate.
Other amyloid-forming diseases offer further opportunity for examining the mechanism of conformational rearrangement. There are at least 15 human diseases in which an accumulation of a specific protein can occur in characteristic insoluble fibers known as amyloid, which are typically 60-100 ë in diameter and exhibit characteristic birefringence when stained with the dye Congo Red (for review, see Kelly, 1996 ). These amyloid diseases result in a variety of different clinical presentations, dependent on the sites of amyloid deposition, and include Alzheimer's disease, where neurodegeneration occurs in association with deposition of the amyloid ■ protein.
Despite distinct folds in the native state, all of the proteins involved in these diseases undergo conformational alteration to a common structure in the amyloid fibril, a "cross ■" repeat structure in which ■ strands are aligned perpendicular to the axis of the amyloid fiber. A recent fiber diffraction study with synchrotron radiation suggests that, in fact, it is ■ sheets that are positioned perpendicular to the fiber axis and that they are arrayed as a continuous helix (Blake and Serpell, 1996 ). As with prion disease, the other amyloidoses can be initiated by inherited mutations in the respective coding sequences, which apparently destabilize the native state of these proteins, enabling them to rearrange to the common conformation in amyloid. Such destabilization has been elegantly demonstrated recently for two purified amyloidogenic lysozyme variants while they were enzymatically active and crystallized in conformations nearly identical to wild-type, they exhibited little or no protection from deuterium exchange when incubated in solution at 37âC, unlike wild type (Booth et al., 1997 ). Lysozyme fibrils isolated from patient material, however, contained only the mutant lysozymes the wild-type protein present in the heterozygous individuals was not recruited. This underscores the major difference that sets prion disease apart from other amyloidoses, namely that the aggregated form of PrP is also able to promote the rearrangement of unmutated protein, thereby allowing transmission of disease.
Recent studies with another amyloidosis, familial amyloidotic polyneuropathy, provide further insight into an amyloidogenic conversion process (Kelly, 1996 ; Lai et al., 1996 ). The involved protein, transthyretin (TTR), is, in native form, a homotetramer whose subunits are eight-stranded ■ sheet sandwiches. In vitro, upon exposure to pH 4-5, TTR dissociates to monomers that undergo tertiary structural rearrangement, and amyloid formation ensues (Lai et al., 1996 ). As with prion conversion, control of TTR amyloid formation could lie either at the step of production of the amyloid aggregate or at the step of monomer rearrangement, invoking kinetic control. Both mechanisms have been observed with TTR in vitro. In support of a nucleation step, fibril formation was observed to exhibit a lag phase and to be accelerated after initiation by addition of amyloidogenic monomer. In support of kinetic control, a greater amount of TTR amyloid was formed at pH 4.4 during refolding from denaturant than was observed starting with native protein, reflecting a kinetic barrier between the amyloidogenic intermediate and the native tetramer.
Thus, for TTR, while both types of control have been observed in vitro, it remains unclear what step is rate limiting in vivo. How high is the kinetic barrier to formation of the amyloidogenic form at physiological temperature, pH, and ionic strength? In particular, without catalyzed formation of the amyloidogenic intermediate, how could there be enough accumulation of this intermediate to form a stable nucleus that would promote efficient polymerization?
Alternatively, if the barrier to production of the intermediate is so high in vivo that a catalytic event is required, what mediates such an event in the absence of preexisting converted protein? Finally, given the observation of seeding phenomena in vitro, why is it that, unlike prions, TTR aggregates are apparently noninfectious? Is this a property of the greater stability of PrPSc? Or are the respective aggregates processed differently by the various organ systems involved?
Concerning such potentially different physiology, two observations seem worth noting. In the case of TTR, a mechanism that clears TTR fibrils has recently been shown (Tan et al., 1995 ); and, in the case of prion disease, it has been observed that, even following intracerebral inoculation of mice with prions, there is early acquisition of infectivity in the spleen, long preceding any appearance of infectivity in the brain (Eklund et al., 1967 ; Kimberlin and Walker, 1979 ; Weissmann et al., 1997 ). Consistent with a primary replication step in the lymphoreticular system that favors neuroinvasion, SCID mice were relatively resistant to CNS disease following intraperitoneal inoculation (only 6 affected out of 18 animals), compared with immunocompetent littermates (13 of 14 animals) (Lasm╚zas et al., 1996a ; see also Kitamoto et al., 1991 ). Presumably, those SCID animals that developed disease acquired CNS infection by direct neural spread, suggested in early studies to extend from peripheral nervous system to spinal cord to brain (e.g., Kimberlin and Walker, 1979 ).
These different conformations could represent either different tertiary structures or, alternatively, different quaternary assemblies of the same fold. The latter case seems reminiscent of the ability of many proteins to pack their native forms into different crystal lattices, or of assembly of flagellar filaments, in which addition of different seeds results in the formation of distinct structures. Such diversity can be considerable, as in the case of the popular object of crystallization, hen egg lysozyme, shown to pack into at least five different crystallographic space groups.
Alternatively, it remains possible that there are modifications such as N-linked glycosylation that confer strain-specific properties, although this modification does not appear to be necessary for acquisition of a proteinase K-resistant PrPSc in a cultured cell system (Taraboulos et al., 1990 ). Regardless of whether conformation or covalent differences are responsible, it seems possible that strain-specific properties of incubation time and brain localization may reflect targeting of different forms of PrPSc to specific CNS cells. These cells would then impart the same form to the newly-converted molecules (Hecker et al., 1992 ; Weissmann et al., 1997 ).
While primary structural differences are not necessary to produce different strains, an example of primary sequence origin of strain properties in human prion disease has recently been reported (Telling et al., 1996b ). Human D178N FFI is associated with a proteinase K-resistant PrPSc of 19 kDa after deglycosylation, while both familial and sporadic CJD are associated with a 21 kDa species. Inoculation of the respective human brain homogenates into Prp-deleted mice containing a chimeric mouse-human mouse (MHuM) PrP transgene produced disease associated with the respectively sized PrPSc, indicating that the two distinct PrPSc species can template a single primary MHuM PrP structure into different conformations.
The importance of studying the origin and nature of strain differences has been emphasized recently by the reports of a number of cases of vCJD that appear to be linked to BSE epidemic in British cattle (Will et al., 1996 ). Despite the small number of cases, a number of observations suggests that nvCJD represents a novel disease distinct from sporadic CJD. First, nvCJD has a distinct pathology characterized by abundant "florid plaques," decorated by a daisy-like pattern of vacuolation (Figure 1). Second, there is a far younger age of onset than in sporadic CJD. The notion that nvCJD could be transmitted from cattle to primates was supported by the observation that intracerebral inoculation of BSE-infected brain extract into Macaque monkeys produced disease and pathology resembling that in the nvCJD patients (Lasm╚zas et al., 1996b ).
This raised the possibility that nvCJD was a newly-identified strain of prion that was less restricted by the species barrier. This was supported recently by studies examining the pattern of proteinase K-resistant PrPSc species from the nvCJD patients, in particular comparing di-, mono-, and non-glycosylated species with those from brain homogenates of patients with sporadic or iatrogenic CJD, and homogenates from BSE-infected animals including cats and macaque (Collinge et al., 1996 ). nvCJD was observed to share a common pattern with BSE-infected animals, distinct from that of sporadic or acquired CJD. The proteinase K-resistant diglycosylated species was particularly prominent, raising questions of whether this form of PrPC is more susceptible to BSE-mediated conformational change or whether a population of cells preferentially producing diglycosylated PrP may be more readily targeted by BSE (Aguzzi and Weissmann, 1996 ).
Additional studies in the cultured cell system showed that conversion to PrPSc could be blocked by addition of exogenous PI-specific phospholipase C or by proteases, suggesting that PrPC undergoes conversion either at the cell surface or after internalization from the cell surface into the endocytic pathway (Caughey and Raymond, 1991 ; Borchelt et al., 1992 ). In support of a requirement for internalization, low temperature incubation (18âC), which retards endocytosis, also blocked production of PrPSc (Borchelt et al., 1992 ). Additional efforts to refine the localization have noted that GPI-anchored proteins localize at the cell surface in cholesterol-rich plasma membrane invaginations that are Triton X-100 insoluble, known as DIGS (detergent-insoluble glycosphingolipid-enriched membranes) (Brown and Rose, 1992 ; Smart et al., 1995 ). Supporting a role of such a compartment, treatment of the cultured cell system with the inhibitor of cholesterol biosynthesis, lovastatin, blocked the conversion process, but it was unclear whether this effect was mediated by failure of PrPC to reach the cell surface or by disruption of the DIGS where conversion might take place (Taraboulos et al., 1995 ). Additional uncertainty is cast by the observation that absence of the GPI anchor from a truncated PrP inhibited but did not prevent production of the proteinase K-resistant PrPSc species in the cultured cells (Rogers et al., 1993 ).
Whatever the specific compartments involved, it seems clear that PrPC reaches the cell surface and that this localization may make it an easily accessible target for exogenous PrPSc, although it seems equally clear that PrPSc presented from outside the cell could internalize down the same pathway as PrPC and mediate conversion internally. Whichever the site, the notion that conversion could take place in a specific membranous compartment containing a specific subset of proteins has potential for reconstitution studies. If such a PrPC-containing compartment is isolable as a low density Triton-insoluble membrane fraction, it should be possible to test for conversion with the isolated fraction, potentially allowing the delimiting of components that are critical to conversion.
Recent transgenic studies on the susceptibility of mice expressing chimeric human-mouse PrPC suggest that at least one host factor other than PrPC, tentatively termed factor X, might be involved in susceptibility to infection (Telling et al., 1995 ). Conceivably, factor X could be a molecular chaperone that binds to PrPC and assists in altering its conformation. A precedent for chaperone involvement in a conversion process comes from recent studies in yeast, where the cytosolically localized product of the SUP35 gene, involved with translational termination, can be converted to a biologically inactive aggregated molecule, conferring a phenotype of nonsense suppression (PSI+) (Chernoff et al., 1995 ; Patino et al., 1996 ; Paushkin et al., 1996 ; see also Masison and Wickner, 1995 ).
The SUP35 aggregates appear to act as a nucleus, promoting the aggregation of newly synthesized SUP35 protein, allowing propagation of the PSI+ state in a manner analogous to the PrPC-to-PrPSc conversion process. Strikingly, maintenance of the PSI+ state was found to depend on the molecular chaperone, Hsp104, a large homohexameric single ring structure with two ATP-binding sites in each of its subunits, which has previously been shown to have a propensity to dissociate protein aggregates produced by heat shock (Parsell et al., 1994 ). Remarkably, either deletion of Hsp104 or its overexpression resulted in concordant disappearance of the SUP35 aggregates and loss of the PSI+ state. In the case of PrP conversion, a general chaperone component like Hsp104 has not so far been identified in the cellular locations where conversion appears to occur.
The secondary structure of PrP121-231 features three helices and two short antiparallel ■ strands (Figure 3B). Glockshuber, Wuthrich, and coworkers speculate that this latter feature could be a "nucleation site" for a conformational transition to the ■ sheet-rich PrPSc form, that could presumably incorporate neighboring loops. Interestingly, the methionine/valine polymorphism affecting disposition to CJD maps into one of these strands. The observation that heterozygosity for Met/Val at this position is protective (Palmer et al., 1991 ) leaves one to wonder whether these strands might also be involved in intermolecular contacts involved in either the conversion process or in aggregation of PrPSc.
Analysis of the surface properties of the PrP121-231 molecule reveal two disparate faces (Figure 3B). One is overall electrostatically positive but contains intermingled hydrophobic patches, suggesting that it could face the cell membrane. The opposite face, by contrast, is electrostatically negative, containing the two sites of glycosylation. Riek et al. suggest that it could be a site of binding of an as yet unidentified ligand. (Could this be PrPC itself, on another cell, for example?) In addition, this surface bears at one edge containing the first helix, a region suggested to act as an accessible binding site for PrPSc. This region contains 5 of 14 residues implicated by chimeric transgenic studies to be important for either the human-mouse or hamster-mouse species barrier (Figure 3A and Figure 3B). Three of the remaining residues involved in the species barrier lie at the opposite edge of the molecule, located in a loop region between the second ■ strand and the second helix (only 166 is shown in Figure 3B). The remaining five residues form a third putative PrPSc binding site located between residues 90 and 122, a region not present in the structure.
Interestingly, the sites of the species barrier and of disposing human mutations appear to be, so far, mutually exclusive. Whereas the region including helix 1 appears to be a determinant of the species barrier, human mutations disposing to disease map to the region of the two other helices, with three mapping into the hydrophobic core and three to the electrostatically negative surface. Such mutations could, correspondingly, either destabilize the structure or affect ligand binding.
With structural information of this sort now in hand, it will be possible to carry out a host of structure-function studies relating the regions of the species barrier and human mutations to the conversion process. For example, it should be possible to assess the relative importance of the three structural regions implicated in the species barrier. In addition, designed mutants with either decreased or increased PrPC stability, measured in vitro with purified recombinant protein, will make it possible to test directly whether destabilization of the native PrPC structure facilitates conversion in vivo. Finally, antibodies generated against peptides that are buried in the native PrPC structure may potentially provide reagents for specifically detecting the PrPSc form. While PrPC is at last yielding to structural analysis, by contrast, in the absence of protocols for solubilizing PrPSc, structural information on the converted form may require nonsolution techniques such as solid state NMR (e.g., Heller et al., 1996 ).
On the other hand, these clinical and pathologic features of PrPC deficiency fail to recapitulate those of classic prion disease. Conversely, can production of PrPSc alone produce disease? An elegant study of Aguzzi, Weissmann, and coworkers has recently addressed this question (Brandner et al., 1996a ). They engrafted brain tissue from a PrPC-expressing normal mouse into a knockout animal and then inoculated with mouse prions. They observed the characteristic pathology of prion disease precisely within the engrafted tissue, but not within the knockout tissue. Nevertheless, PrPSc produced within the diseased tissue migrated into the neighboring null tissue.
Thus, PrPSc by itself was insufficient to produce disease, i.e., simple exposure to exogenous PrPSc is insufficient for cytotoxicity. Rather, PrPSc may be toxic only when formed within the cell, or when presented from outside to a cell already expressing PrPC, so that conversion ensues either at the cell surface or in an internalized compartment. Furthermore, Brandner and colleagues have also shown that propagation of infection across neural pathways in the CNS requires the presence of PrPC along the pathway (Brandner et al., 1996b ), insofar as grafts in null animals did not become infected following intraocular inoculation. Thus, in all cases, it appears that the presence of PrPC is required for pathogenesis.
Aguzzi, A., and Weissmann, C. (1996). A suspicious signature. Nature 383, 666-667.[Medline] Aizawa, S.-I., Vonderviszt, F., Ishima, R., and Akasaka, K. (1990). Termini of Salmonella flagellin are disordered and become organized upon polymerization into flagellar filament. J. Mol. Biol. 211, 673-677.[Medline] Alper, T., Haig, D.A., and Clarke, M.C. (1966). The exceptionally small size of the scrapie agent. Biochem. Biophys. Res. Commun. 22, 278-284.[Medline] Alper, T., Cramp, W.A., Haig, D.A., and Clarke, M.C. (1967). Does the agent of scrapie replicate without nucleic acid? Nature 214, 764-766.[Medline] Anderson, R.M., Donnelly, C.A., Ferguson, N.M., Woolhouse, M.E.J., Watt, C.J., Udy, H.J., MaWhinney, S., Dunstan, S.P., Southwood, T.R.E., and Wilesmith, J.W. et al. (1996). Transmission dynamics and epidemiology of BSE in British cattle. Nature 382, 779-788.[Medline] Asakura, S., Eguchi, G., and Iino, T. (1964). Reconstitution of bacterial flagella in vitro. J. Mol. Biol. 10, 42-56. Asakura, S., Eguchi, G., and Iino, T. (1966). Salmonella flagella: in vitro reconstruction and over-all shapes of flagellar filaments. J. Mol. Biol. 16, 302-316.[Medline] Asakura, S. (1968). A kinetic study of in vitro polymerization of flagellin. J. Mol. Biol. 35, 237-239.[Medline] Baker, D., and Agard, D.A. (1994). Influenza hemagglutinin: kinetic control of protein function. Structure 2, 907-910.[Medline] Baker, D., and Agard, D.A. (1994). Kinetics versus thermodynamics in protein folding. Biochemistry 33, 7505-7509.[Medline] Basler, K., Oesch, B., Scott, M., Westaway, D., Walchli, M., Groth, D.F., McKinley, M.P., Prusiner, S.B., and Weissmann, C. (1986). Scrapie and cellular PrP isoforms are encoded by the same chromosomal gene. Cell 46, 417-428.[Summary] Bessen, R.A., and Marsh, R.F. (1992). Biochemical and physical properties of the prion protein from two strains of the transmissible mink encephalopathy agent. J. Virol. 66, 2096-2101.[Medline] Bessen, R.A., and Marsh, R.F. (1994). Distinct PrP properties suggest the molecular basis of strain variation in transmissible mink encephalopathy. J. Virol. 68, 7859-7868.[Medline] Bessen, R.A., Kocisko, D.A., Raymond, G.J., Nandan, S., Lansbury, P.T., and Caughey, B. (1995). Non-genetic propagation of strain-specific properties of scrapie prion protein. Nature 375, 698-700.[Medline] Blake, C., and Serpell, L. (1996). Synchrotron X-ray studies suggest that the core of the transthyretin amyloid fibril is a continuous ■-sheet helix. Structure 4, 989-998.[Medline] Bolton, D.C., McKinley, M.P., and Prusiner, S.B. (1982). Identification of a protein that purifies with the scrapie prion. Science 218, 1309-1311.[Medline] Booth, D.R., Sunde, M., Bellotti, B., Robinson, C.V., Hutchinson, W.L., Fraser, P.E., Hawkins, P.N., Dobson, C.M., Radford, S.E., Blake, C.C.F., and Pepys, M.B. (1997). Instability, unfolding and aggregation of human lysozyme variants underlying amyloid fibrillogenesis. Nature 385, 787-793.[Medline] Borchelt, D.R., Scott, M., Taraboulos, A., Stahl, N., and Prusiner, S.B. (1990). Scrapie and cellular prion proteins differ in their kinetics of synthesis and topology in cultured cells. J. Cell Biol. 110, 743-752.[Medline] Borchelt, D.R., Taraboulos, A., and Prusiner, S.B. (1992). Evidence for synthesis of scrapie prion proteins in the endocytic pathway. J. Biol. Chem. 267, 16188-16199.[Medline] Brandner, S., Isenmann, S., Raeber, A., Fischer, M., Sailer, A., Kobayashi, Y., Marino, S., Weissmann, C., and Aguzzi, A. (1996). Normal host prion protein necessary for scrapie-induced neurotoxicity. Nature 379, 339-343.[Medline] Brandner, S., Raeber, A., Sailer, A., Blöttler, T., Fischer, M., Weissmann, C., and Aguzzi, A. (1996). Normal host prion protein (PrPC) is required for scrapie spread within the central nervous system. Proc. Natl. Acad. Sci. USA 93, 13148-13151.[Medline] Brown, D.A., and Rose, J.K. (1992). Sorting of GPI-anchored proteins to glycolipid-enriched membrane subdomains during transport to the apical cell surface. Cell 68, 533-544.[Summary] Bruce, M.E., Dickinson, A.G., and Fraser, H. (1976). Cerebral amyloidosis in scrapie in the mouse: effect of agent strain and mouse genotype. Neuropathol. Appl. Neurobiol. 2, 471-478. BŞeler, H., Fischer, M., Lang, Y., Bluethmann, H., Lipp, H.-P., DeArmond, S.J., Prusiner, S.B., Aguet, M., and Weissmann, C. (1992). Normal development and behaviour of mice lacking the neuronal cell-surface PrP protein. Nature 356, 577-582.[Medline] BŞeler, H., Aguzzi, A., Sailer, A., Greiner, R.-A., Autenried, P, Aguet, M., and Weissmann, C. (1993). Mice devoid of PrP are resistant to scrapie. Cell 73, 1339-1347.[Summary] Butler, D.A., Scott, M.R.D., Bockman, J.M., Borchelt, D.R., Taraboulos, A., Hsiao, K.K., Kingsbury, D.T., and Prusiner, S.B. (1988). Scrapie-infected murine neuroblastoma cells produce protease-resistant prion proteins. J. Virol. 62, 1558-1564.[Medline] Carp, R.I., and Callahan, S.M. (1991). Variation in the characteristics of 10 mouse-passaged scrapie lines derived from five scrapie-positive sheep. J. Gen. Virol. 72, 293-298.[Medline] Caughey, B., Race, R.E., Ernst, D., Buchmeier, M.J., and Chesebro, B. (1989). Prion protein-biosynthesis in scrapie-infected and uninfected neuro-blastoma cells. J. Virol. 63, 175-181.[Medline] Caughey, B.W., Dong, A., Bhat, K.S., Ernst, D., Hayes, S.F., and Caughey, W.S. (1991). Secondary structure analysis of the scrapie-associated protein PrP27-30 in water by infrared spectroscopy. Biochemistry 30, 7672-7680.[Medline] Caughey, B., and Raymond, G.J. (1991). The scrapie-associated form of PrP is made from a cell surface precursor that is both protease- and phospholipase-sensitive. J. Biol. Chem. 266, 18217-18223.[Medline] Caughey, B., Kocisko, D.A., Raymond, G.J., and Lansbury, P.T. (1995). Aggregates of scrapie-associated prion protein induce the cell-free conversion of protease-sensitive prion protein to the protease-resistant state. Chem. Biol. 2, 807-817.[Medline] Chernoff, Y.O., Lindquist, S.L., Ono, B., Inge-Vechtomov, S.G., and Liebman, S.W. (1995). Role of the chaperone protein Hsp104 in propagation of the yeast prion-like factor (psi+). Science 268, 880-884.[Medline] Chesebro, B., Race, R., Wehrly, K., Nishio, J., Bloom, M., Lechner, D., Bergstrom, S., Robbins, K., Mayer, L., and Keith, J.M. et al. (1985). Identification of scrapie prion protein-specific mRNA in scrapie-infected and uninfected brain. Nature 315, 331-333.[Medline] Cohen, F.E., Pan, K.-M., Huang, Z., Baldwin, M., Fletterick, R.J., and Prusiner, S.B. (1994). Structural clues to prion replication. Science 264, 530-531.[Medline] Collinge, J., Whittington, M.A., Sidle, K.C.L., Smith, C.J., Palmer, M.S., Clarke, A.R., and Jefferys, J.G.R. (1994). Prion protein is necessary for normal synaptic function. Nature 370, 295-297.[Medline] Collinge, J., Sidle, K.C. L., Meads, J., Ironside, J., and Hill, A.F. (1996). Molecular analysis of prion strain variation and the aetiology of 'new variant' CJD. Nature 383, 685-690.[Medline] DeArmond, S.J., Yang, S.-L., Lee, A., Bowler, R., Taraboulos, A., Groth, D., and Prusiner, S.B. (1993). Three scrapie prion isolates exhibit different accumulation patterns of the prion protein scrapie isoform. Proc. Natl. Acad. Sci. USA 90, 6449-6453.[Medline] DeArmond, S.J., and Prusiner, S.B. (1995). Etiology and pathogenesis of prion diseases. Am. J. Pathol. 146, 785-811.[Medline] DeArmond, S.J., and Prusiner, S.B. (1996). Molecular neuropathology of prion diseases. In The Molecular and Genetic Basis of Neurological Disease, Second Edition, R.N. Rosenberg, S.B. Prusiner, S. DiMauro, and R.L. Bacchi, eds. (Stoneham, MA: Butterworth-Heinemann), pp. 145-163. Diringer, H., Gelderblom, H., Hilmert, H., Ozel, M., Edelbluth, C., and Kimberlin, R.H. (1983). Scrapie infectivity, fibrils and low molecular weight protein. Nature 306, 476-478.[Medline] Eklund, C.M., Kennedy, R.C., and Hadlow, W.J. (1967). Pathogenesis of scrapie virus infection in the mouse. J. Infect. Dis. 117, 15-22.[Medline] Fischer, M., Rulicke, T., Raeber, A., Sailer, A., Moser, M., Oesch, B., Brandner, S., Aguzzi, A., and Weissmann, C. (1996). Prion protein (PrP) with amino-proximal deletions restoring susceptibility of PrP knockout mice to scrapie. EMBO J. 15, 1255-1264.[Medline] Fraser, H., and Dickinson, A.G. (1973). Scrapie in mice. Agent-strain differences in the distribution and intensity of grey matter vacuolation. J. Comp. Pathol. 83, 29-40.[Medline] Gabizon, R., McKinley, M.P., Groth, D., and Prusiner, S.B. (1988). Immunoaffinity purification and neutralization of scrapie prion infectivity. Proc. Natl. Acad. Sci. USA 85, 6617-6621.[Medline] Gajdusek, D.C., and Zigas, V. (1959). Kuru. Clinical, pathologic, and epidemiologic study of an acute progressive degenerative disease of the central nervous system among natives of the eastern highlands of New Guinea. Am. J. Med. 26, 442-469. Gajdusek, D.C., Gibbs, C.J., and Alpers, M. (1966). Experimental transmission of a kuru-like syndrome to chimpanzees. Nature 209, 794-796.[Medline] Gajdusek D.C. (1977). Unconventional viruses and the origin and disappearance of kuru. Science 197, 943-960.[Medline] Gajdusek, D.C. (1988). Transmissible and non-transmissible amyloidoses: Autocatalytic post-tranlsational conversion of host precursor proteins to ■-pleated configurations. J. Neuroimmunol. 20, 95-110.[Medline] Gerstmann, J., Ströussler, E., and Scheinker, I. (1936). Uber eine egenartige hereditar-familiare Erkrankung des Zentralnervensystems zugleich ein Beitrag zur frage des vorzeitigen lokalen Alterns. Z. Neurol. 154, 736-762. Gibbs, C.J., Gajdusek, D.C., Asher, D.M., Alpers, M.P., Beck, E., Daniel, P.M., and Matthews, W.B. (1968). Creutzfeldt-Jakob Disease (spongiform encephalopathy): transmission to the chimpanzee. Science 161, 388-389.[Medline] Gordon, W.S. (1946). Advances in veterinary research. Vet. Rec. 58, 518-525. Griffith, J.S. (1967). Self-replication and scrapie. Nature 215, 1043-1044.[Medline] Hadlow, W.J. (1959). Scrapie and kuru. Lancet 2, 289-290. Hecker, R., Taraboulos, A., Scott, M., Pan, K.-M., Yang, S.-L., Torchia, M., Jendroska, K., DeArmond, S.J., and Prusiner, S.B. (1992). Replication of distinct scrapie prion isolates is region specific in brains of transgenic mice and hamsters. Genes Dev. 6, 1213-1228.[Medline] Heller, J., Kolbert, A.C., Larsen, R., Ernst, M., Bekkar, T., Baldwin, M., Prusiner, S.B., Pines, A., and Wemmer, D.E. (1996). Solid-state NMR studies of the prion protein H1 fragment. Prot. Sci. 5, 1655-1661. Hope, J., Morton, L.J.D., Farquhar, C.F., Multhaup, G., Beyreuther, K., and Kimberlin, R.H. (1986). The major polypeptide of scrapie-associated fibrils (SAF) has the same size, charge distribution and N-terminal protein sequence as predicted for the normal brain protein (PrP). EMBO J. 5, 2591-2597.[Medline] Hsiao, K., Baker, H.F., Crow, T.J., Poulter, M., Owen, F., Terwilliger, J.D., Westaway, D., Ott, J., and Prusiner, S.B. (1989). Linkage of a prion protein missense variant to Gerstmann-Straussler syndrome. Nature 338, 342-345.[Medline] Hsiao, K.K., Scott, M., Foster, D., Groth, D.F., DeArmond, S.J., and Prusiner, S.B. (1990). Spontaneous neurodegeneration in transgenic mice with mutant prion protein. Science 250, 1587-1590.[Medline] Hsiao, K.K., Groth, D., Scott, M., Yang, S.-L., Serban, H., Rapp, D., Foster, D., Torchia, M., DeArmond, S.J., and Prusiner, S.B. (1994). Serial transmission in rodents of neurodegeneration from transgenic mice expressing mutant prion protein. Proc. Natl. Acad. Sci. USA 91, 9126-9130.[Medline] Jarrett, J.T., and Lansbury, P.T. (1993). Seeding "one-dimensional-crystallization" of amyloid: a pathogenic mechanism in Alzheimer's disease and scrapie? Cell 73, 1055-1058.[Summary] Kellings, K., Meyer, N., Mirenda, C., Prusiner, S.B., and Riesner (1992). Further analysis of nucleic acids in purified scrapie prion preparations by improved return refocusing gel electrophoresis. J. Gen. Virol. 73, 1025-1029.[Medline] Kelly, J.W. (1996). Alternative conformations of amyloidogenic proteins govern their behavior. Curr. Opin. Struct. Biol. 6, 11-17.[Medline] Kimberlin, R.H., and Walker, C.A. (1979). Pathogenesis of mouse scrapie: dynamics of agent replication in spleen, spinal cord and brain after infection by different routes. J. Comp. Pathol. 89, 551-562.[Medline] Kimberlin, R.H., Walker, C.A., and Fraser, H. (1989). The genomic identity of different strains of mouse scrapie is expressed in hamsters and preserved on reisolation in mice. J. Gen. Virol. 70, 2017-2025.[Medline] Kitamoto, T., Muramoto, T., Mohri, S., Doh-Ura, K., and Tateishi, J. (1991). Abnormal isoform of prion protein accumulates in follicular dendritic cells in mice with Creutzfeldt-Jakob disease. J. Virol. 65, 6292-6295.[Medline] Kocisko, D.A., Come, J.H., Priola, S.A., Chesebro, B., Raymond, G.J., Lansbury, P.T., and Caughey, B. (1994). Cell-free formation of protease-resistant prion protein. Nature 370, 471-474.[Medline] Kocisko, D.A., Priola, S.A., Raymond, G.J., Chesebro, B., Lansbury, P.T., and Caughey, B. (1995). Species specificity in the cell-free conversion of prion protein to protease-resistant forms: a model for the scrapie species barrier. Proc. Natl. Acad. Sci. USA 92, 3923-3927.[Medline] Lai, Z., Colon, W., and Kelly, J.W. (1996). The acid-mediated denaturation pathway of transthyretin yields a conformational intermediate that can self-assemble into amyloid. Biochemistry 35, 6470-6482.[Medline] Lasm╚zas, C.I., Cesbron, J.-Y., Deslys, J.-P., Demaimay, R., Adjou, K.T., Rioux, R., LeMaire, C., Locht, C., and Dormont, D. (1996). Immune system-dependent and -independent replication of the scrapie agent. J. Virol. 70, 1292-1295.[Medline] Lasm╚zas, C.I., DesIys, J.-P., Demaimay, R., Adjou, K.T., Lamoury, F., Dormont, D., Robain, O., Ornside, J., and Hauw, J.-J. (1996). BSE transmission to macaques. Nature 381, 743-744.[Medline] Latarjet, R., Muel, B., Haig, D.A., Clarke, M.C., and Alper, T. (1970). Inactivation of the scrapie agent by near monochromatic ultraviolet light. Nature 227, 1341-1343.[Medline] Lledo, P.M., Tremblay, P., DeArmond, S.J., Prusiner, S.B., and Nicholl, R.A. (1996). Mice deficient for prion protein exhibit normal neuronal excitability and synaptic transmission in the hippocampus. Proc. Natl. Acad. Sci. USA 93, 2403-2407.[Medline] Manetto, V., Medori, R., Cortelli, P., Montagna, P., Tinuper, P., Baruzzi, A., Rancurel, G., Hauw, J.-J., Vanderhaeghen, J.-J., and Mailleux, P. et al. (1992). Fatal familial insomnia: clinical and pathological study of five new cases. Neurology 42, 312-319.[Medline] Masison, D.C., and Wickner, R.B. (1995). Prion-inducing domain of yeast Ure2p and protease resistance of Ure2p in prion-containing cells. Science 270, 93-95.[Medline] Merz, P.A., Somerville, R.A., Wisniewski, H.M., and Iqbal, K. (1981). Abnormal fibrils from scrapie-infected brain. Acta Neuropathol. 54, 63-74.[Medline] Meyer, R.K., McKinley, M.P., Bowman, K.A., Braunfeld, M.B., Barry, R.A., and Prusiner, S.B. (1986). Separation and properties of cellular and scrapie prion proteins. Proc. Natl. Acad. Sci. USA 83, 2310-2314.[Medline] Muramoto, T., Kitamoto, T., Tateishi, J., and Goto, I. (1992). The sequential development of abnormal prion protein accumulation in mice with Creutzfeldt-Jakob disease. Am. J. Pathol. 140, 1411-1420.[Medline] Muramoto, T., Scott, M., Cohen, F.E., and Prusiner, S.B. (1996). Recombinant scrapie-like prion protein of 106 amino acids is soluble. Proc. Natl. Acad. Sci. USA 93, 15457-15462.[Medline] Oesch, B., Westaway, D., Walchli, M., McKinley, M.P., Kent, S.B.H., Aebersold, R., Barry, R.A., Tempst, P., Teplow, D.B., Hood, L.E., Prusiner, S.B., and Weissmann, C. (1985). A cellular gene encodes scrapie PrP 27-30. Cell 40, 735-746.[Summary] Palmer, M.S., Dryden, A.J., Hughes, J.T., and Collinge, J. (1991). Homozygous prion protein genotype predisposes to sporadic Creutzfeldt-Jakob disease. Nature 352, 340-342.[Medline] Pan, K.-M., Baldwin, M., Nguyen, J., Gasset, M., Servban, A., Groth, D., Mehlhorn, I., Huang, Z., Fletterick, R.J., Cohen, F.E., and Prusiner, S.B. (1993). Conversion of -helices into ■-sheets features in the formation of the scrapie prion proteins. Proc. Natl. Acad. Sci. USA 90, 10962-10966.[Medline] Parsell, D.A., Kowal, A.S., Singer, M.A., and Lindquist, S. (1994). Protein disaggregation mediated by heat-shock protein Hsp104. Nature 372, 475-478.[Medline] Patino, M.M., Liu, J.-J., Glover, J.R., and Lindquist, S. (1996). Support for the prion hypothesis for inheritance of a phenotypic trait in yeast. Science 273, 622-626.[Medline] Paushkin, S.V., Kushnirov, V.V., Smirnov, V.N., and Ter-Avanesyan, M.D. (1996). Propagation of the yeast prion-like [psi+] determinant is mediated by oligomerization of the SUP35-encoded polypeptide chain release factor. EMBO J. 15, 3127-3134.[Medline] Prusiner, S.B., Groth, D.F., Cochran, S.P., Masiarz, F.R., McKinley, M.P., and Martinez, H.M. (1980). Molecular properties, partial purification, and assay by incubation period measurmeents of the hamster scrapie agent. Biochemistry 19, 4883-4891.[Medline] Prusiner, S.B. (1982). Novel proteinaceous infectious particles cause scrapie. Science 216, 136-144.[Medline] Prusiner, S.B., Bolton, D.C., Groth, D.G., Bowman, K.A., Cochran, S.P., and McKinley, M.P. (1982). Further purification and characterization of scrapie prions. Biochemistry 21, 6942-6950.[Medline] Prusiner, S.B., McKinley, M.P., Bowman, K.A., Bolton, D.C., Bendheim, P.E., Groth, D.F., and Glenner, G.G. (1983). Scrapie prions aggregate to form amyloid-like birefringent rods. Cell 35, 349-358.[Summary] Prusiner, S.B., Groth, D.F., Bolton, D.C., Kent, S.B., and Hood, L.E. (1984). Purification and structural studies of a major scrapie prion protein. Cell 38, 127-134.[Summary] Prusiner, S.B., Scott, M., Foster, D., Pan, K.-M., Groth, D., Mirenda, C., Torchia, M., Yang, S.-L., Serban, D., Carlson, G.A., Hoppe, P.C., Westaway, D., and DeArmond, S.J. (1990). Transgenetic studies implicate interactions between homologous PrP isoforms in scrapie prion replication. Cell 63, 673-686.[Summary] Prusiner, S.B. (1991). Molecular biology of prion diseases. Science 252, 1515-1522.[Medline] Prusiner, S.B., Groth, D., Serban, A., Koehler, R., Foster, D., Torchia, M., Burton, D., Yang, S.-L., and DeArmond, S.J. (1993). Ablation of the prion protein (PrP) gene in mice prevents scrapie and facilitates production of anti-PrP antibodies. Proc. Natl. Acad. Sci. USA 90, 10608-10612.[Medline] Prusiner, S.B. (1996). Prion diseases of human and animals. In The Molecular and Genetic Basis of Neurological Disease, Second Edition, R.N. Rosenberg, S.B. Prusiner, S. DiMauro, and R.L. Bachi, eds. (Stoneham, MA: Butterworth-Heinemann), pp. 165-186. Riek, R., Hornemann, S., Wider, G., Billeter, M., Glockshuber, R., and Wuthrich, K. (1996). NMR structure of the mouse prion protein domain PrP(121-231). Nature 382, 180-182.[Medline] Rogers, M., Yehiely, F., Scott, M., and Prusiner, S.B. (1993). Conversion of truncated and elongated prion proteins into the scrapie isoform in cultured cells. Proc. Natl. Acad. Sci. USA 90, 3182-3186.[Medline] Safar, J., Roller, P.P., Gajdusek, D.C., and Gibbs, C.J. (1993). Thermal stability and conformational transitions of scrapie amyloid (prion) protein correlate with infectivity. Prot. Sci. 2, 2206-2216. Sakaguchi, S., Katamine, S., Nishida, N., Moriuchi, R., Shigematsu, K., Sugimoto, T., Nakatani, A., Kataoka, Y., Houtani, T., and Shirabe, S. et al. (1996). Loss of cerebellar Purkinje cells in aged mice homozygous for a disrupted PrP gene. Nature 380, 528-531.[Medline] Scott, M., Foster, D., Mirenda, C., Serban, D., Coufal, F., Walchli, M., Torchia, M., Groth, D., Carlson, G., and DeArmond, S.J. et al. (1989). Transgenic mice expressing hamster prion protein produce species-specific scrapie infectivity and amyloid plaques. Cell 59, 847-857.[Summary] Scott, M., Groth, D., Foster, D., Torchia, M., Yang, S.-L., DeArmond, S.J., and Prusiner, S.B. (1993). Propagation of prions with artificial properties in transgenic mice expressing chimeric PrP genes. Cell 73, 979-988.[Summary] Sifers, R.N. (1995). Defective protein folding as a cause of disease. Nat. Struct. Biol. 2, 355-357.[Medline] Smart, E.J., Ying, Y.-S., Mineo, C., and Anderson, R.G.W. (1995). A detergent-free method for purifying caveolae membrane from tissue culture cells. Proc. Natl. Acad. Sci. USA 92, 10104-10108.[Medline] Stahl, N., Borchelt, D.R., Hsiao, K., and Prusiner, S.B. (1987). Scrapie prion protein contains a phosphatidylinositol glycolipid. Cell 51, 229-240.[Summary] Stahl, N., Baldwin, M.A., Teplow, D.B., Hood, L., Gibson, B.W., Burlingame, A.L., and Prusiner, S.B. (1993). Structural studies of the scrapie prion protein using mass spectrometry and amino acid sequencing. Biochemistry 32, 1991-2002.[Medline] Tan, S.Y., Pepys, M.B., and Hawkins, P.N. (1995). Treatment of amyloidosis. Am. J. Kidney Dis. 26, 267-285.[Medline] Taraboulos, A., Rogers, M., Borchelt, D.R., McKinley, M.P., Scott, M., Serban, D., and Prusiner, S.B. (1990). Acquisition of protease resistance by prion proteins in scrapie-infected cells does not require asparagine-linked glycosylation. Proc. Natl. Acad. Sci. USA 87, 8262-8266.[Medline] Taraboulos, A., Jendroska, K., Serban, D., Yang, S.-L., DeArmond, S.J., and Prusiner, S.B. (1992). Regional mapping of prion proteins in brain. Proc. Natl. Acad. Sci. USA 89, 7620-7624.[Medline] Taraboulos, A., Scott, M., Semenov, A., Avraham, D., Laszlo, L., and Prusiner, S.B. (1995). Cholesterol depletion and modification of COOH-terminal targeting sequence of the prion protein inhibit formaiton of the scrapie isoform. J. Cell Biol. 129, 121-132.[Medline] Telling, G.C., Scott, M., Mastrianni, J., Gabizon, R., Torchia, M., Cohen, F.E., DeArmond, S.J., and Prusiner, S.B. (1995). Prion propagation in mice expressing human and chimeric PrP transgenes implicates athe interaciton of cellular PrP with another protein. Cell 83, 79-90.[Summary] Telling, G.C., Haga, T., Torchia, M., Tremblay, P., DeArmond, S.J., and Prusiner, S.B. (1996). Interactions between wild-type and mutant prion proteins modulate neurodegeneration in transgenic mice. Genes Dev. 10, 1736-1750.[Medline] Telling, G.C., Parchi, P., DeArmond, S.J., Cortelli, P., Montagna, P., Gabizon, R., Lugaresi, E., Gambetti, P., and Prusiner, S.B. (1996). Evidence for the conformation of the pathologic isoform of the prion protein enciphering and propagating prion diversity. Science 274, 2079-2082.[Medline] Weissmann, C., Fischer, M., Raeber, A., Bueler, H., Sailer, A., Shmerling, D., Rulicke, T., Brandner, S., and Aguzzi, A. (1997). The role of PrP in pathogenesis of experimental scrapie. Cold Spring Harbor Symp. Quant. Biol. 61, 511-522. Westaway, D., Goodman, P.A., Mirenda, C.A., McKinley, M.P., Carlson, G.A., and Prusiner, S.B. (1987). Distinct prion proteins in short and long scrapie incubation period mice. Cell 51, 651-662.[Summary] Whittington, M.A., Sidle, K.C. L., Gowland, I., Meads, J., Hill, A.F., Palmer, M.S., Jefferys, J.G.R., and Collinge, J. (1995). Rescue of neurophysiological phenotype seen in PrP null mice by transgene encoding human prion protein. Nat. Genet. 9, 197-201.[Medline] Will, R.G., Ironside, J.W., Zeidler, M., Cousens, S.N., Estibeiro, K., Alperovitch, A., Poser, S., Pocchiari, M., Hofman, A., and Smith, P.G. (1996). A new variant of Creutzfeldt-Jakob disease in the United Kingdom. Lancet 347, 921-925.[Medline]