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Structural evidence for the critical role of the prion protein hydrophobic region in forming an infectious prion


Authors: Romany Abskharon aff001;  Fei Wang aff003;  Alexandre Wohlkonig aff001;  Juxin Ruan aff003;  Sameh Soror aff001;  Gabriele Giachin aff006;  Els Pardon aff001;  Wenquan Zou aff007;  Giuseppe Legname aff008;  Jiyan Ma aff003;  Jan Steyaert aff001
Authors place of work: Structural Biology Brussels, Vrije Universiteit Brussel (VUB), Brussels, Belgium aff001;  VIB-VUB Center for Structural Biology, Vlaams Instituut Biotechnologie (VIB), Brussels, Belgium aff002;  Center for Neurodegenerative Science, Van Andel Institute, Grand Rapids, Michigan, United States of America aff003;  National Institute of Oceanography and Fisheries (NIOF), Cairo, Egypt aff004;  Center of Excellence, Helwan Structural Biology Research, Faculty of Pharmacy, Helwan University, Cairo, Egypt aff005;  Structural Biology Group, European Synchrotron Radiation Facility, Grenoble, France aff006;  Departments of Pathology and Neurology, Case Western Reserve University School of Medicine, Cleveland, Ohio, United States of America aff007;  Laboratory of Prion Biology, Department of Neuroscience, Scuola Internazionale Superiore di Studi Avanzati (SISSA), Trieste, Italy aff008
Published in the journal: Structural evidence for the critical role of the prion protein hydrophobic region in forming an infectious prion. PLoS Pathog 15(12): e32767. doi:10.1371/journal.ppat.1008139
Category: Research Article
doi: https://doi.org/10.1371/journal.ppat.1008139

Summary

Prion or PrPSc is the proteinaceous infectious agent causing prion diseases in various mammalian species. Despite decades of research, the structural basis for PrPSc formation and prion infectivity remains elusive. To understand the role of the hydrophobic region in forming infectious prion at the molecular level, we report X-ray crystal structures of mouse (Mo) prion protein (PrP) (residues 89–230) in complex with a nanobody (Nb484). Using the recombinant prion propagation system, we show that the binding of Nb484 to the hydrophobic region of MoPrP efficiently inhibits the propagation of proteinase K resistant PrPSc and prion infectivity. In addition, when added to cultured mouse brain slices in high concentrations, Nb484 exhibits no neurotoxicity, which is drastically different from other neurotoxic anti-PrP antibodies, suggesting that the Nb484 can be a potential therapeutic agent against prion disease. In summary, our data provides the first structure-function evidence supporting a crucial role of the hydrophobic region of PrP in forming an infectious prion.

Keywords:

Lipids – Crystal structure – Antibodies – Enzyme-linked immunoassays – Animal prion diseases – Prion diseases – Cell binding assay – Crystallization

Introduction

Prion diseases, also known as transmissible spongiform encephalopathies (TSEs), are a group of fatal neurodegenerative diseases affecting both humans and animals[1]. The prion protein (PrP) exists in two forms: the physiological cellular isoform, PrPC, and the disease-associated infectious isoform, denoted as prion or PrPSc[2]. The host-encoded PrPC is a cell surface glycosylphosphatidylinositol (GPI)-anchored glycoprotein containing a flexible N-terminal fragment and a well-folded α-helical C-terminus. PrPSc, however, is composed almost entirely of β-sheets[3]. The conversion from normal PrPC to prion is the underlying pathogenic event of prion diseases[4]. Detailed three-dimensional (3D) structures of different mammalian PrPC have been solved[57], but little atomic-level information is available on the PrPSc structure except for a recent study that proposes the 4-rung β-solenoid architecture of PrPSc[8]. Thus far, the molecular mechanisms of the conformational conversion of PrPC into infectious prions and other key neurodegenerative processes in prion diseases remain unclear, which is a road block for developing effective therapeutic strategies against these devastating neurodegenerative disorders[8].

Previous structural studies have established that PrPC features an intrinsically unstructured N-terminal region, a globular C-terminal domain containing three α-helices and two short β-strands—forming a unique β1-α1- β2- α2- α3 fold in which the β-strands come together to form an anti-parallel β-ribbon (SCOP classification) and a highly conserved middle region that links the flexible N-terminus and globular C-terminus. This conserved middle region consists of a cluster of four positively-charged lysine residues (101, 104, 106 and 110, human numbering) and a hydrophobic region (residues 112–135, human numbering), which has a high propensity for β-sheet secondary structure[9, 10]. Therefore, the hydrophobic region has been proposed to be involved in PrP conformational changes or prion propagation, which occurs when PrPSc acts as a template and induces the seeded conformational change of PrPC into PrPSc, and causes prion disease.

A large number of anti-PrP antibodies have been generated. Interestingly, it has been shown that anti-PrP monoclonal antibodies are able to inhibit prion propagation in vitro and in vivo, presumably by stabilizing the PrPC conformation. Therefore, passive immunization with anti-PrP antibodies presents a promising therapeutic approach against TSEs[11]. We recently reported that an anti-PrP camelid heavy chain antibody or nanobody (Nb), namely Nb484, inhibits prion conversion in cultured mouse neuronal cells in a dose-dependent manner[12].

To understand the structural basis of Nb484 mediated inhibition, here we report two new X-ray crystal structures of mouse (Mo) PrP•Nb484 complexes at pH 6.0 and pH 8.0 resolved with a resolution of 2.1 Å and 1.2 Å, respectively; and the crystal structure of the nanobody Nb484 alone (at 1.2 Å resolution). Similar to a previous report on the human prion protein[12], our current study reveals that Nb484 allows the crystallization of MoPrP polypeptide from residues 118 to 226 and that the hydrophobic region folds into a stable three-stranded antiparallel β-sheet arrangement. In both structures at different pH, Nb484 stabilizes residues 120–122 of MoPrP into a β-strand, termed β0, which folds into a three-stranded antiparallel β-sheet with β1 and β2. We further demonstrate the prion inhibitory effect of Nb484 on the mouse PrP in Protein Misfolding Cyclic Amplification (PMCA) reactions. Together, our study provides convincing structure-function evidence for the critical role of the hydrophobic region in converting normal PrPC to pathogenic PrPSc.

Results

Crystal structures of MoPrP•Nb484 complexes

Using a nanobody as a crystallization chaperone, we obtained well diffracting crystals of MoPrP(89–230) in complex with Nb484 at different pH. In these complexes, the total amount of structured polypeptide (125 amino acids of antibody and 108 amino acids of the prion protein) rises to 71% in contrast to 52% for free PrP, thus providing a much better starting point for crystallization. The first high-resolution MoPrP(89–230)•Nb484 crystal was obtained at pH 6.0, and the structure was refined to 2.1 Å resolution. The second complex was crystallized at pH 8.0 and determined to 1.2 Å resolution. Both structures contain residues from 118–226 and the average backbone root-mean-square distance between them is only 0.609 Å, indicating that both structures are almost identical. X-ray data-collection and crystal structure-refinement statistics are summarized in Table 1.

Tab. 1. Statistics of X-ray diffraction data collection and atomic refinement of MoPrP•Nb484 complexes and free Nb484.
Statistics of X-ray diffraction data collection and atomic refinement of MoPrP•Nb484 complexes and free Nb484.

The overall structure of the MoPrP(89–230) in complex with Nb484 consists of three antiparallel β-strands (β0: residues 120–122, β1: residues 125–130 and β2: residues 161–163, human numbering, for the convenience of direct comparison between Mouse PrP and Human PrP) and three α-helices (α1: residues 144–153, α2: residues 172–190 and α3: residues 200–226) (Fig 1A and 1C). Similar to the human protein, the palindromic motif, AGAAAAGA, of MoPrP (residues 113–120) adopts a stable β-hairpin fold to form a three-stranded antiparallel β-sheet with the β1 and β2 strands (Fig 1B). It thus appears that the MoPrP structure also adopts a more elaborate β0-β1-α1-β2-α2-α3 fold than the canonical PrPC fold[12]. MoPrP(89–230) interacts with Nb484 through a discontinuous binding epitope comprising residues 123 and 125 of the β0-β1 loop; residue 128 of β1 strand; residues 164, 167, 168, and169 of the β2-α2 loop; and residues 173, 174, 177, 178, 182, 185 and 189 of the α2-helix. A detailed overview of all the interactions occurring between the folded domain of MoPrP and Nb484 is shown in S1 Fig and S1 Table.

Fig. 1. Crystal structure of the MoPrP(89–230) in complex with Nb484 at pH 8.0.
Crystal structure of the MoPrP(89–230) in complex with Nb484 at pH 8.0.
(A) Ribbon representation of the MoPrP•Nb484 complex shown in two orientations, the MoPrP is shown in green and Nb484 highlighted in cyan. (B) Cartoon representation of the three-stranded antiparallel β-sheet shown in red. (C) The β0-β1-α1-β2-α2-α3 topology of MoPrP(89–230).

In both MoPrP structures, Nb484 binds the hydrophobic domain at Gly123 and Leu125 to stabilize a third β-strand (β0), which forms a three-stranded anti-parallel β-sheet with the extended strands β1 and β2. The β0 strand in both MoPrP structures (residues 120–122) is shorter than in the one reported in human structure (residues 118–122)[12] (S2 Fig).

We also crystallized Nb484 alone and solved its structure to a high resolution (1.2 Å) by X-ray crystallography. Nb484 contains three complementarity determining regions (CDRs), each noncontiguous with the others (termed CDR1, CDR2, CDR3) (S3A and S3F Fig). These regions account for the specificity of the antibody for a particular antigenic determinant. Remarkably, the structure of the free Nb484 changes in the CDR3 from the same nanobody in complex with the MoPrP (S3A and S3B Fig). More specifically, the orientation of the CDR3 changes upon binding with the MoPrP, thus interacting with β0-β1 loop and β2-α2 loop. The B-factors indicate that the CDR3 of the Nb484 is significantly more rigid in the MoPrP•Nb484 complex as compared to the nanobody alone (S3C and S3D Fig). Specifically, Ile102 and Tyr103 of the Nb484 undergo major structural rearrangement towards Gly123 and stabilize the β0-β1 loop of MoPrP. In addition, Arg106 stabilizes α2 of MoPrP by binding to Asn174, His177 and Asp178, while Ala107 stabilizes the β2-α2 loop of MoPrP by binding to Gln168 and Tyr169 (S3E Fig). It thus appears that Nb484 undergoes structural changes in the CDR3 to enable a greater complementarity between the nanobody and MoPrP (S3E and S4 Figs).

The inhibitory effect on prion conversion by Nb484 is epitope-specific

We previously reported that Nb484 inhibits prion propagation in a scrapie-infected GT1 mouse hypothalamic (ScGT1) cell line in a dose-dependent manner and cures the scrapie-infected cells[12]. Here, we tested the ability of Nb484 to inhibit prion conversion in our recently developed recombinant prion propagation system, in which the non-infectious, α-helical recombinant mouse PrP (recPrP) is converted into the highly infectious recombinant prion (recPrPSc) by PMCA reaction supplemented with two auxiliary cofactors, phospholipid POPG and RNA molecules[13]. In the PMCA reactions seeded with recPrPSc, robust recombinant prion amplification was observed in the absence of Nb484 (Fig 2A), while in the presence of Nb484 (1, 2, 4 and 8 μM Nb484), the propagation of recPrPSc was blocked depending on the concentration of Nb484 (Fig 2A). To further evaluate the inhibitory effect of Nb484 on prion infectivity, we collected PMCA products from the 6th round and performed the cell-based prion infectivity assay[14]. Our results revealed that Nb484 inhibits the propagation of mouse prion infectivity as well (Fig 2B). ELISA was performed to evaluate the binding of Nb484 to recPrP and recPrPSc. Our result confirmed that Nb484 has a high affinity for recPrP, as previously reported (Kd = 40 nM)[12], but revealed that its binding to the infectious recPrPSc is minimal (S5A Fig, Nb484), indicating that Nb484 exerts its inhibitory effect on prion propagation through binding to the non-infectious recPrP (Fig 2A and 2B).

Fig. 2. Effect of nanobodies on the prion amplification.
Effect of nanobodies on the prion amplification.
(A) Inhibition of prion propagation by different concentrations (1, 2, 4 and 8 μM) of Nb484 in Protein Misfolding Cyclic amplification (PMCA) for six consecutive rounds. (B) Elispot cell culture assay of prion infectivity from PMCA samples (round 6) for Nb484. (C) Inhibition of prion propagation by different concentrations (1, 2, 4 and 8 μM) of Nb862 in PMCA. (D) Elispot cell culture assay of prion infectivity from PMCA samples (round 6) for Nb862. CAD5 cells were infected with serial 10-fold dilutions of round six of PMCA products.

It has been suggested that the inhibitory efficacy of conventional antibodies on prion conversion positively correlates with their binding affinity for PrPC, i.e. higher affinity, stronger inhibition[11]. To evaluate whether such correlation exists for nanobodies, we tested the inhibitory abilities of two extra nanobodies, Nb862 and Nb486, which have higher and lower binding affinity for MoPrP, respectively, compared to Nb484 (S2 Table and ref.[12]). Interestingly, neither Nb862 nor Nb486 inhibits the prion propagation of MoPrP in the seeded PMCA reactions (Fig 2C and 2D and S5B Fig), suggesting Nb484 inhibits prion conversion in an epitope-specific manner.

Nb484 inhibits recombinant prion conversion by competitively binding to the hydrophobic region of MoPrP

Structure-function studies have shown that anti-PrP monoclonal antibody ICSM18, a therapeutic antibody, blocks prion amplification through binding to and stabilizing the α-helix 1 of PrP[11]. The crystal structure of MoPrP(89–230)•Nb484 complex clearly reveals the stabilization of β0-β1 loop and β2-α2 loop (Fig 1 and S1 and S2 Figs). To investigate the underlying mechanism of the inhibitory effect of Nb484 on mouse recombinant prion propagation, we started with the lipid binding and PK-digestion assay.

We have previously shown that anionic phospholipid POPG, one of the cofactors that facilitate the propagation of recombinant prion, can bind to recPrP and induce conformational changes and C-terminal Proteinase K (PK)-resistance of recPrP[13]. The recPrP-POPG interaction is initiated by the electrostatic interaction between the positively charged residues of PrP and the negatively charged head groups of POPG and followed by the hydrophobic interactions between the hydrophobic region of PrP (112–135, human numbering) and the hydrophobic acyl chains of POPG, and such hydrophobic interaction is essential for the POPG-induced C-terminal PK-resistance[15, 16]. Since the novel β0 strand (120–122) and β0-β1 loop (123–125) stabilized by Nb484 locate within the MoPrP hydrophobic region (112–135), we tested if Nb484 can block the access of POPG to the hydrophobic region of MoPrP and then if it can inhibit POPG-induced recPrP prion-like conversion. Increased amounts of Nb484 were incubated with either the recPrP•POPG mixture or recPrP alone prior to the addition of POPG, and the development of the C-terminal PK-resistance was used to track the conformational change of recPrP. As previously reported[15], recPrP underwent structural changes and acquired the C-terminal PK-resistance when incubated with POPG alone (Fig 3A, 0 μM Nb484). Interestingly, the addition of Nb484 at various concentrations to the recPrP•POPG mixture had no effect on the lipid-induced C-terminal PK-resistance (Fig 3A, 7.8, 15.6, 31.2 and 62.4 μM Nb484). However, when Nb484 was allowed to interact with recPrP prior to being mixed with POPG, a dose-dependent inhibition of POPG-induced PK-resistance of recPrP was found (Fig 3A and S6 Fig), suggesting a competition between Nb484 and POPG for binding to the hydrophobic region of MoPrP.

Fig. 3. Nb484 interacting with the hydrophobic region of PrPC.
Nb484 interacting with the hydrophobic region of PrP<sup>C</sup>.
(A) Influence of Nb484 on the interaction of PrP and POPG synthetic lipid. For rPrP+POPG+Nb484, recombinant mouse PrP was incubated with POPG before mixed with Nb484 at different molar ratios (Nb484:recPrP = 0, 1, 2, 4, or 8:1). For rPrP+Nb484+POPG, recombinant mouse PrP was incubated with Nb484 at different molar ratios (Nb484:recPrP = 0, 1, 2, 4, or 8:1) before mixed with POPG. PK-resistant PrP was detected using POM1 antibody. (B) Representative ELISA results show that both Nb484 and Nb862 bind strongly to rPrP. Nb484 has very week binding to ΔHC, but Nb862 shows strong binding signal to ΔHC. POM1 antibody was used as a primary antibody to determine the binding signal. POM1 displayed similar binding for both rPrP and ΔHC. All results are the average of 3 replicates.rPrP: MoPrP(23–230), ΔHC: MoPrPΔHC.

The competitive binding of Nb484 or POPG to recPrP was further supported by results of the discontinuous iodixanol density gradient floatation assay (S7 Fig). In this assay, various mixtures composed of recPrP, Nb484 and/or POPG were loaded at the bottom fraction of the density gradient and subjected to ultracentrifugation. If the sample contains lipids and there is an interaction between lipids and other components, the lipid-bound components will migrate along with the lipids to the top fractions of the gradient due to the low density of lipids; otherwise the non-lipid components will remain at the bottom fractions. As previously reported[15, 16], recPrP alone stayed at the bottom fractions and recPrP•POPG mixture migrated to the top fractions (S7A Fig). When recPrP was first incubated with POPG and then mixed with Nb484, recPrP floated to the top fractions, but most of Nb484 was left at the bottom fractions (S7B Fig, [recPrP•POPG]+Nb484), showing recPrP-POPG interaction prohibited Nb484 binding to recPrP. Interestingly, when the recPrP•Nb484 mixture was incubated with POPG, both recPrP and most of Nb484 were found in the top fractions (S7B Fig, [recPrP•Nb484]+POPG). It is most likely that recPrP in the mixture of [recPrP•Nb484]+POPG binds to POPG through its positively charged residues instead of the hydrophobic region that is occupied by Nb484.

To evaluate if the availability of the hydrophobic region of MoPrP for conformational change is indeed involved in forming an infectious prion, we generated a recPrP mutant, in which a segment (from amino acid 112 to 132, human numbering) of the hydrophobic region was deleted (designated as MoPrPΔHC). This mutant does not support recPrPSc-seeded prion propagation in PMCA (S8 Fig). Relative to the full-length recPrP, binding of MoPrPΔHC to Nb484 dramatically decreases (Fig 3B, Nb484), indicating that the β0-β1 loop is the major contributor to the interactions between recPrP and Nb484. In contrast, Nb862, the nanobody that does not inhibit prion propagation, binds to both full-length recPrP and MoPrPΔHC similarly (Fig 3B, Nb862), indicating that the epitope for Nb862 does not include residues within the hydrophobic region of PrP. The epitope for a conformational anti-PrP monoclonal antibody POM1 has been determined, via a structural study, to include residues 138–147, which encompass the β1-α1 loop and part of α-helix 1 and are just outside of the hydrophobic region, and three discontinuous residues 204, 208 and 212 on α-helix 3[17, 18]. The ELISA result shows that the binding of POM1 to full-length recPrP and MoPrPΔHC are essentially the same (Fig 3B, POM1). Together with the recPrPSc propagation inhibition results, the ELISA data strongly suggests that Nb484 binds to recPrP hydrophobic region, blocks the interactions between recPrP and cofactor molecules, and inhibits PrP conversion and prion propagation.

To assess the effects of β2-α2 loop stabilization by Nb484 on recPrP conformational change and prion conversion, we generated a “rigid loop” MoPrP variant by introducing both S170N and N174T mutations (human numbering)[19] (designated as MoPrPS170N/N174T) and subjected the mutant MoPrP to both lipid interaction and PMCA assays. Interestingly, the stabilized β2-α2 loop does not affect the interaction between MoPrPS170N/N174T and POPG (S10A Fig, molar ratio of Nb484:PrP = 0:1), and the competition binding assay reveals that MoPrPS170N/N174T behaves like wild-type MoPrP (S10A Fig, in comparison with S6 Fig and Fig 3A). Furthermore, MoPrPS170N/N174Tcan be readily converted to prion in our recombinant PMCA assay (S10B Fig), indicating that stabilization of β2-α2 loop would not inhibit recombinant prion propagation. Taken together, our results support that Nb484 inhibits recombinant prion conversion by competitively binding to the hydrophobic region of MoPrP.

Nb484 does not induce neurotoxicity in organotypic cultured slices

It has been shown that certain antibodies (including POM1) that bind to the C-terminal globular domain of MoPrP (residues 124–230) induce strong neurotoxicity in mice and cerebellar organotypic cultured slices[18]. To evaluate whether Nb484, which binds discontinuous epitopes involving both the hydrophobic region and C-terminal domain of PrP, causes neurotoxicity in PrPC expressing cells, we cultured cerebellar organotypic cultured slices from tga20 transgenic mice and treated slices with either POM1 or Nb484. Consistent with previous report, POM1 at 270 nM induced rapid neurotoxicity in the cultured slices in two weeks (Fig 4). In contrast, Nb484 at concentration of 270 nM or 2700 nM did not elicit any obvious neurotoxicity (Fig 4 and S11 Fig), revealing that Nb484 binding to the hydrophobic region does not cause neurotoxicity and confirming that the neurotoxicity induced by globular domain-ligand binding- is mediated through specific regions of PrP[18].

Fig. 4. Nb484 did not induce neurotoxicity in Tga20 mice organotypic slices comparing to POM1 antibody.
Nb484 did not induce neurotoxicity in Tga20 mice organotypic slices comparing to POM1 antibody.
NeuN staining showing that POM1 has strong toxicity similar to the pervious results obtained by Aguzzi group [18]. Nb484 shows no neurotoxicity in Tga20 mice organotypic slices similar to the slices treated with PBS. Slices were stained with IgG1 antibodies to NeuN. The white bar is 100 μm.

Discussion

Despite great advances in understanding prion propagation, the molecular mechanism underlying the conformational conversion from normal PrPC to the infectious PrPSc remains largely unknown. We previously reported that Nb484, an anti-PrP nanobody, could inhibit such PrPC-to-PrPSc conversion in chronically prion infected mouse hypothalamic cells (scrapie-infected GT1 mouse hypothalamic (ScGT1) cell line)[12]. To better understand how Nb484 recognizes MoPrP and inhibits prion propagation in vitro, crystal structures of the MoPrP(89–230)•Nb484 complexes and Nb484 alone were determined in current study. The discontinuous epitope of MoPrP that interacts with Nb484 includes residues 123–125 in the β0- β1 loop, residues 164–170 in the β2–α2 loop and residues 174–185 in the α2-helix.

The structure of MoPrP•Nb484 complex confirms structural insights into the folding of the hydrophobic region from residues 118 to 135. Similar to the HuPrP•Nb484 complex, the C-terminus of the palindromic segment participates in the formation of an additional β-strand (residues 120–122, designated as β0), which packs with β1 and β2 into three anti-parallel β-sheets. Remarkably, Nb484 binds to Y128 between G127 and M129, which leads to an extended β1 strand (residues 125–130). The β0 and β1 strands are connected with a defined loop, termed β0-β1 loop (Fig 1), which forms a 2:2 IP type β-hairpin between β0 and β1 strands (S9 Fig). In this loop, Gly123 and Gly124 occupy a type I′ β-turn and are stabilized by H-bonds located between Val122 and Leu125. In addition, the formation of this β-hairpin exposes several backbone hydrogen donors and acceptors to solvent (S4 Fig). These amino acids are prone to stacking with other β-strands in parallel or anti-parallel fashion to build β-sheeted amyloid fibers (S4 Fig). Our findings suggest that the binding of Nb484 to this region not only stabilizes the PrP hydrophobic region, but also prevents the amyloid fiber formation.

The MoPrP-Nb484 interactions also significantly stabilize the β2–α2 loop at the C-terminal domain, leading to a rigid β2–α2 loop (S3G Fig). The rigidity of this loop was initially linked to the efficiency of the interspecies prion transmission, that is, PrP of a species with a rigid β2–α2 loop will be susceptible to infection by prions from another species with a similar rigid β2–α2 loop[19]. However, in an elegant follow-up transmission study, it has been shown that the efficiency of prion conversion correlates with primary sequence homology rather than the rigidity of β2–α2 loop in different PrP species[20]. In our hands, the stabilized β2–α2 loop, resulting from amino acid substitutions, namely S170N and N174T, does not affect the binding between the MoPrP and POPG (S10A Fig), which is not surprising since we have shown previously that POPG binds to the positively charged residues and the hydrophobic region of MoPrP, but not the folded C-terminus[16]. Interestingly, the rigid β2–α2 loop in MoPrPS170N/N174T does not prevent its conversion to recombinant prion (S10B Fig). Therefore, it is unlikely that the β2–α2 loop, stabilized by Nb484, accounts for the inhibitory effect of Nb484 on prion conversion.

On the other hand, the β0 strand (120–122) and β0-β1 loop (123–125), stabilized by Nb484, locate within the PrP hydrophobic region (112–135), which is the most conserved motif of PrP among all species[21]. PrP-null mice expressing PrPΔ94–134 or PrPΔ105–125, both of which lack the hydrophobic region, spontaneously developed rapid and lethal neurodegenerative illnesses[22, 23]. Although such neurodegenerations are distinct from those observed in prion infected mice and can be rescued by co-expression of wild-type PrPC, these observations suggest that the alteration of the hydrophobic region may affect its binding to a ligand and leads to neurotoxicity[22, 23]. The hydrophobic region also harbors multiple mutation sites that are associated with inherited human prion disease, such as G114V and A117V mutations in the palindromic sequence AGAAAAGA (113–120), which cause early onset Gerstmann-Straussler-Scheinker disease (GSS)[24, 25]. Removing this palindromic sequence in PrP led to failed PrPSc conversion in prion-infected ScN2a cells and altered PrP aggregation in yeast, suggesting that the AGAAAAGA sequence is not only required for forming a prion but also likely involves in the PrPSc-PrPC interaction to initiate the conformational conversion[26]. It has been shown that the hydrophobicity of the palindromic region is critical for the neurotoxicity and fibrillogenicity of the PrP106-126 peptide[27, 28]. Low-resolution spectroscopy data also indicate that the hydrophobic AGAAAAGA motif may adopt multiple discrete conformations, suggesting this region is metastable, and depending on intermolecular interactions, forms various structures[29, 30]. Consistent with this idea, the Eisenberg and Yee groups have identified that multiple segments in the hydrophobic region could form different steric zipper structures, including 113AGAAAA118, 119GAVVGG124, 126GGYMLG131, 127GYMLGS132, 126GGYVLG131 and 127GYVLGS132 with class 7, 4, 7, 8, 8 and 8, respectively[3133].

The therapeutic anti-PrP monoclonal antibody ICSM18 inhibits prion conversion by binding strongly to the whole α-helix 1 and the binding affinity of an antibody for PrP has been suggested to correlate with its ability to inhibit PrPSc propagation[11]. Interestingly, we found that Nb862, which has a much higher binding affinity for MoPrP (0.158 nM vs. 40 nM of Nb484), does not affect recPrPSc propagation at all (Fig 2C and 2D), suggesting that, for a nanobody that is much smaller compared to the conventional antibody, the binding epitope is more critical for its inhibitory effect. Among the different epitopes of Nb484, the hydrophobic region plays the most critical role in forming an infectious prion. Using the recombinant prion propagation system with defined components, Nb484 inhibits recPrPSc propagation in a dose-dependent fashion (Fig 2A and 2B). We have also found that the hydrophobic region is required for an effective binding of Nb484 to PrP (Fig 3B) and Nb484 blocks the hydrophobic interactions between PrP and POPG (Fig 3A and S6 and S7 Figs). These data demonstrate that Nb484 inhibits prion conversion through a competitive inhibitory mechanism.

The conversion of PrPC to PrPSc involves major conformational rearrangements[8, 34]. However, it is unlikely that the whole C-terminal region of PrPC undergoes dramatic conformational changes simultaneously, and the conversion is likely initiated at one or a few parts of PrPC in contact with PrPSc directly or through certain ligands[4]. The hydrophobic region has been suggested to be involved in the PrPC-PrPSc interaction during prion conversion[21]. Moreover, an anti-prion phenothiazine compound has been shown to bind to a “hydrophobic pocket” that encompasses part of the hydrophobic region and stabilize the PrP molecule[35]. Our previous study found that the hydrophobic region is indispensable to the formation of POPG-induced C-terminal PK-resistance[16]. Our current data reveal that the hydrophobic region is also critical for the inhibitory nanobody Nb484 to bind PrP (Fig 3B). Therefore, it is reasonable to speculate that the hydrophobic region represents one of the misfolding initiation sites for the prion conversion.

Many anti-prion compounds have been identified to inhibit prion replications in cell cultures and cell free conversion assays, such as polyanions[36], iododoxorubicin[37], tetracycline[37], Congo Red[38], polyene antibiotics[39] and quinacrine[39]. However, these compounds have limited applications in treating human prion diseases mainly due to their limited ability to cross the blood brain barrier (BBB)[40, 41]. It has been reported that an anti-prion nanobody is able to cross BBB in vitro and in vivo, making them particularly interesting for therapeutic application[40]. As mentioned above, passive immunotherapy with anti-PrP antibodies is a promising therapeutic approach against prion disease, but the observations that some anti-PrP antibodies induce rapid neurotoxicity cause some concerns about this strategy[18, 42]. Interestingly, the inhibitory Nb484 does not elicit any toxicity in cultured cerebellar organotypic slices (Fig 4 and S11 Fig). Structural superimposition of MoPrP bound to Nb484 with MoPrP•POM1 Fab[35], huPrP•ICSM18 Fab[17] and ovPrP•VRQ14 Fab[43] clearly reveals the distinct binding orientations of each antibody (Fig 5 and S3 Table), which may be implicated in the antibody-induced neurotoxicity and warrants further investigations.

Fig. 5. Superimposition of different MoPrP, HuPrP and ovine PrP structures in complex with Fab and Nb484.
Superimposition of different MoPrP, HuPrP and ovine PrP structures in complex with Fab and Nb484.
(A) Front view, all prion proteins are shown in green, heavy and light chains of POM1 Fab (PDB 4H88) are shown in yellow, ICSM18 (PDB 2W9E) in pink, VRQ14 Fab (PDB 1TPX) in cyan and Nb484 in brown. (B) Top view of the superposition.

In summary, we have determined the structure of the MoPrP•Nb484 complexes, providing new structure-function evidence to support a critical role of the hydrophobic region of PrP in the formation of an infectious prion. Moreover, our data indicate an epitope-dependent inhibitory or neurotoxic mechanism for each individual antibody/nanobody. With this work we have identified a PrPC region likely to be responsible for prion conversion and discovered a new potential therapeutic nanobody for prion diseases.

Materials and methods

Cloning, expression and purification of recombinant MoPrP(89–230)

Cloning of MoPrP(89–230) into pET-28a (Novagen) was performed as described previously[44]. Protein expression and purification was achieved according to our protocol[45]. In this method, MoPrP(89–230) was co-expressed with QSOX in E. coli Rosetta (DE3) pLysS. 10 mL of pre-culture supplemented with the appreciate antibiotics (100 μg/mL ampicillin and 25 μg/mL kanamycin) and were used to inoculate 1L of L.B medium. Cells were growing at 37 °C and induced at A600 = 0.7 by adding 1 mM isopropyl-b-D-thiogalactopyranoside (IPTG) and temperature was shifted to 15 °C for 16 h. Cells were collected by centrifugation (15 min at 15,000g). Next, pellets were re-suspended to a density of 0.1 g of cell paste/mL in lysing buffer (50 mM potassium phosphate, pH 7.5, 300 mM NaCl supplemented with 0.1 mg/mL lysozyme, 0.1 mg/mL AEBSF and 1 μg/mL leupeptin). Cells were lysed using a French press (10,000 psi) and followed by centrifugation at 4 °C for 60 min at 20,000 rpm. The collected supernatant was loaded on a 5 mL Histrap Ni-NTA column (GE-healthcare) previously equilibrated with equilibration buffer (50 mM potassium phosphate pH 7.5, 300 mM NaCl, 10 mM imidazole). The column was washed with five column volumes (CV) of washing buffer: 50 mM potassium phosphate pH 7.5, 1 M NaCl, 50 mM imidazole, followed by ten CV of 50 mM potassium phosphate pH 6.0, 1 M NaCl, 50 mM imidazole. The protein was eluted with a gradient of imidazole from 50 mM to 500 mM in 50 mM potassium phosphate pH 7.5. The eluted MoPrP(89–230) fractions were loaded on a SDS/PAGE to evaluate purity, then pooled, and concentrated for a second purification step. The concentrated pool was applied onto a Superdex75 HR 10/30 column (GE Healthcare) and eluted with 20 mM Tris-HCl pH 7.5 containing 150 mM NaCl. The elution peak was again loaded on SDS/PAGE. The fraction containing only MoPrP(89–230) was collected for a dialysis against 10 mM sodium acetate pH 4.6, 1 mM EDTA followed by the final dialysis buffer of 10 mM sodium acetate pH 4.6. Protein aliquots were stored at -80 °C until further usage.

Expression and purification of recPrP23-230 and MoPrPΔHC

Full-length recPrP23-230 was expressed in E. coli BL21 (DE3) and purified according to the previous reported protocols[46, 47]. MoPrPΔHC is a mutant with deletion of the hydrophobic domain (amino acids 112–132 deletion, human numbering). MoPrPΔHC was constructed, expressed and purified according to the previous reported protocol[16].

Construction, expression and purification of MoPrPS170N/N174T

Mutations S170N and N174T in MoPrP were generated using the QuikChange site-directed mutagenesis kit (Stratagene) from pPROEX-HT-b vector containing mouse PrP23–230. The mutant was expressed in E. coli BL21 (DE3) and the purification was carried out as previously described[16].

Generation, expression and purification of nanobodies

Nb484 and Nb486 were generated from llama immunized 6 times bi-weekly with 200 μg of purified recombinant MoPrP(23–230). Nb484 and Nb486 were generated and selected according to our protocol[48]. Nb862 were generated by immunizing llama 6 times bi-weekly with approximately 200 μg of PrPSc chemically purified from ScGT1 cell[12]. Nb484, Nb486 and Nb862 were cloned into (pHEN6) vector bearing a C-terminal His6 tag and a pelB signal peptide for periplasmic protein expression. The plasmid was transformed into E. coli WK6 cells and a single colony was grown overnight in LB medium 100 μg ml−1 ampicillin. Next, 10 ml of pre-culture was used to inoculate 1 L TB medium containing 100 μg ml−1 ampicillin, 2 mM MgCl2 and 0.1% glucose and grown overnight at 37 °C. Cultures were grown to A600 = 0.7 and induced with 1mM IPTG followed by shifting the growing temperature to 28 °C overnight. Cells were harvested by centrifugation and lysed in ice-cold buffer (50 mM Tris pH 8.0, 12.5 mM EDTA and 0.125 M sucrose), then centrifuged to remove cell debris. The periplasmic extract of the nanobody was applied to Ni-NTA column and washed with buffer: 50 mM Na2HPO4, 1 M NaCl pH 7 followed by 50 mM NaH2PO4, 1 M NaCl pH 6.0. The purified nanobody with eluted using 10 ml of 50 mM sodium acetate pH 4.7, 1 M NaCl and neutralized with 2 ml 1 M Tris–HCl pH 7.5. Next, the collected fraction was concentrated and applied for another purification step using gel filtration on a Superdex 75 HR 10/30 column equilibrated in 20 mM Tris–HCl pH 7.5, 150 mM NaCl. Fractions were collected, concentrated and applied for SDS PAGE and showed 99% pure nanobody.

Purification and crystallization of MoPrP(89–230)•Nb484 complex

MoPrP(89–230) and Nb484 were mixed in an equimolar ratio in order to form the protein complex. Presence of a stable complex was monitored by analytical SEC using a Superdex 75 HR 10/30 column (GE Healthcare Life Sciences) in a buffer running containing 20 mM Tris-HCl pH 7.5, 150 mM NaCl. Two crystals of MoPrP(89–230)•Nb484 complexes were grown after using several commercial screening conditions (MD-proplex, Index, Crystal Screen, Crystal Screen 2, PACT, JCSG, JBScreen Classic 1–4 HTS, JBScreen Classic 5–8 HTS and JBScreen Basic HTS) in 96-well Intelli-plates (Hampton research). The first complex crystal was grown at 20 mg/mL complex in MD-proplex screen in B10 (0.15 M ammonium sulfate, 0.1 M MES pH6.0, 15% w/v PEG 4000) within 2 weeks. The second complex crystal was grown at concentration 68 mg/mL complex in MD-proplex screen in G1 (0.1 M Tris pH 8, 1.5 M ammonium sulfate) within one year. Nb484 has crystallized and diffracted to 1.2 Å resolution as described previously[49]. All crystals were grown at 20 °C and cryoprotected using 15% glycerol.

Data collection and structure determination

The MoPrP(89–230)•Nb484 complex crystal diffracted to 2.1 Å resolution and a complete dataset was collected at X06DA beamline at SLS, Paul Scherer institute, Switzerland as described previously[44]. The second crystal diffracted to 1.2 Å resolution and a complete dataset was collected at X06DA beamline at SLS, Paul Scherer institute. Both Mouse PrP structures data were processed using XDS[50]. The structures of the different MoPrP•Nb484 complexes were determined by molecular replacement (PHASER)[51] using the HuPrP•Nb484 crystal structure (PDB entry 4KML)[12]. Nb484 was processed using iMOSFLM as described previously[49]. The Nb484 structure was solved by molecular replacement using PDB entry 1OL0 as search model.

The data collection details and refinement statics are shown in Table 1. Models were built manually using the Crystallographic Object-Oriented Toolkit (Coot)[52] and multiple refinement rounds were performed using Refmac5[53] and Phenix[54]. Structural analyses were performed using Ligplot[55], Promotif[56], and Pisa[57].

Protein misfolding cyclic amplification (PMCA)

To prepare substrate for propagation of recPrPSc, 38.5 μL of soluble recPrP (0.75 mg/mL in deionized H2O) was mixed thoroughly with 81.5 μL of RNase free water (Invitrogen) in a 1.5-ml siliconized microcentrifuge tube (Midsci, St. Louis). In the presence of Nb484 or Nb862, serial concentrations of (1, 2, 4 and 8 μM) or Nb462 (4 and 8 μM) was mixed with recPrP and incubated for 10 min at RT. Then, 10.7 μL of POPG (2.5 mg/mL in 20 mM Tris-HCl, pH 7.4) were added to each tube and mixtures were incubated at room temperature for 10 minutes. During the incubation, 848.36 μL of deionized H2O, 66.64 μL of 5% Triton X-100 and 120 μL of 10 x TN buffer (1.5 M NaCl, 100 mM Tris-HCl, pH 7.5) was added into another 1.5-ml siliconized microcentrifuge tube and mix thoroughly. The recPrP-POPG mixture was transferred to the 1.5-mL tube containing the buffer and mixed thoroughly. The mixture was incubated at room temperature for 5 minutes. Then, 45 μL of liver RNA (10 mg/mL in Nuclease Free Water) was added and the substrate mixture was thoroughly mixed, aliquoted (90 μL per tube), and stored at -80°C. All PMCA experiments were repeated twice.

The enzyme-linked immunospot (Elispot) cell infection assay

The Elispot cell infection assay was performed according to previous studies[58] with minor modifications. Briefly, 200 μL of PMCA products at round 6 were collected and centrifuged at 100,000 × g, 4 °C for 1 hour and the pellets were washed twice with 200 μL PBS, followed by centrifugation at 100,000 × g, 4 °C for 1 hour after each wash. After the final wash, the pellets were resuspended in 200 μL of CAD5 growth media (OPTI-MEM, 5% BGS and 1% penicillin and streptomycin) and sonicated for 30 seconds with 50% output (Misonic Sonicator XL2020). Each sample was serially diluted 10, 100, and 1,000 times and 60 μL of undiluted and diluted samples were used to infect CAD5 cells. After two 1:10 splits, 20,000 CAD5 cells/well were transferred to the Millipore 96-well Elispot plates (MSIPN4W) and subjected to the Elispot assay (42). The images were taken by S6 Micro Analyzer (CTL Analyzers, LLC) and processed by the ImmunoSpot software (CTL Analyzers, LLC). The graph was generated using GraphPad Prism (GraphPad Software, Inc.).

Enzyme-linked immunosorbent assay (ELISA)

Maxisorp 96-well plates (Nunc) were coated overnight at 4 °C with purified 2 μg/mL of Nb484 in sodium bicarbonate buffer pH 8.2. Residual protein binding sites in the wells were blocked with 2% milk in PBS for two hours at room temperature. 50 ng of recPrP23-230, PrPSc (-PK) and PrPSc (+PK) were incubated for 2 hours with the nanobody at room temperature. Then plate was incubated with 1:2500 dilution of POM1 anti-PrP antibody[59] for 2 hours. Wells were then incubated with 1:2000 dilution of goat anti-mouse HRP (Bio-Rad) for 1 hour. Absorption at 405 nm was measured 30 min after adding 100 μL of ultra TMB-ELISA (Thermo-Scientific, Product no. 34028).

Surface Plasmon Resonance (SPR)

MoPrP(23–230) was immobilized on a CM5 chip (GE Healthcare) with Surface Plasmon Resonance (SPR) on a Biacore 3000 according to our previous reported protocol[12]. Nb862 and Nb486 used as analytes and all binding isothermes were fitted to 1 to 1 Langmuir binding model.

Binding of Nb484 or Nb862 to MoPrP(23–230) and MoPrPΔHC

Maxisorp 96-well ELISA plates were coated overnight at 4 °C with purified 2 μg/mL of Nb484 or Nb862 in sodium bicarbonate buffer pH 8.2. Residual protein binding site was blocked as above mentions. Serial concentrations (250 nM, 100 nM, 10 nM and 1 nM) of MoPrP(23–230) or MoPrPΔHC incubated 2 hours with nanobodies. POM1 anti-PrP antibody was used as a primary antibody followed by goat anti-mouse HRP as secondary antibody as previous descried. In the same time a control experiment was performed using Serial concentrations (250 nM, 100 nM, 10 nM and 1 nM) of MoPrP(23–230) or MoPrPΔHC coated in 96-well ELISA plates. The control experiment was probed by POM1 anti-PrP antibody followed by secondary antibody as described early. ELISA signal was recorded by measuring the absorption at 405 nm after adding TMB-ELISA substrate.

PrP lipid interaction and PK digestion

15 μL recPrP (7.8 μM) was incubated for 1 hour with 10 μL of POPG (2.5 mg/mL) and 1.2 μL NaCL (5M) with the final volume of 40 μL, either before or after mixing with Nb484 in different concentrations (7.8, 15.6, 31.2 and 62.4 μM) for 10 minutes.

The PK digestions were performed by incubating 10 μL of samples with 10 μL PK (100 μg/mL) at 37 °C for 30 minutes. The reaction was stopped by adding 5 mM phenylmethyl-sulfonylfluoride (PMSF) and kept on ice for 5 minutes. The PK digested samples were separated by SDS-PAGE and the PrP was detected by immunoblot analyses with the POM1 anti-PrP antibody[59].

Gradient floatation assay

In order to perform the discontinuous iodixanol density gradient floatation assay, we incubated recPrP or recPrP plus Nb484 with POPG for 10 minutes and the high-density phase of the iodixanol gradient was applied as previously described[15, 16]. Twelve fractions (200 μL/fraction) were collected from top to bottom of the gradient as indicated.

Organotypic cultured slices

Cerebellar organotypic cultured slices were prepared using a vibratome from 12-day-old mice according to previously reported protocols[18, 60, 61]. Tga20 mice cerebellar organotypic cultured slices were exposed for two weeks to 270 nM and 2.7 μM of anti-PrP monoclonal antibody POM1[18] and Nb484, respectively. A control experiment was performed by exposing cerebellar organotypic cultured slices to PBS buffer.

Accession numbers

The structures have deposited in the protein data bank as

Nb484: 6HEQ

PrP•Nb484 (at 1.2 Å resolution): 6HER

PrP•Nb484 (at 2.1 Å resolution): 6HHD

Supporting information

S1 Fig [a]
Intermolecular contacts at the MoPrP•Nb484 interface.

S2 Fig [a]
Comparison of MoPrP and HuPrP protein.

S3 Fig [a]
Binding of MoPrP to Nb484 leads to structural changes in the nanobody CDR3.

S4 Fig [a]
Structure of the β0-β1 hairpin in MoPrP structure.

S5 Fig [a]
Nb484 or Nb862 binds PrP but not PrP.

S6 Fig [tif]
Effect of Nb484 on the interaction of PrP and POPG synthetic lipid.

S7 Fig [a]
Effect of Nb484 on the interaction of rPrP with anionic lipid.

S8 Fig [a]
The propagation of MoPrPΔ in PMCA.

S9 Fig [a]
Structural analysis of the β0-β1 hairpin according to Promotif.

S10 Fig [a]
Effect of Nb484 on the interaction of MoPrP with POPG.

S11 Fig [tif]
Nb484 is not toxic to organotypic slices at higher concentration.

S1 Table [docx]
Intermolecular interactions between MoPrP(89–230) and Nb484 in the crystal structure of the complex.

S2 Table [docx]
Binding kinetics of Nb862 and Nb486 for MoPrP(23–230).

S3 Table [docx]
Comparison of backbone superposition root-mean-square deviation values (RMSD, Å) of multiple PrP-antibody complexes.


Zdroje

1. Prusiner SB. Prions. Proceedings of the National Academy of Sciences of the United States of America. 1998;95(23):13363–83. doi: 10.1073/pnas.95.23.13363 9811807

2. Pan KM, Baldwin M, Nguyen J, Gasset M, Serban A, Groth D, et al. Conversion of alpha-helices into beta-sheets features in the formation of the scrapie prion proteins. Proc Natl Acad Sci U S A. 1993;90(23):10962–6. doi: 10.1073/pnas.90.23.10962 7902575.

3. Wille H, Requena JR. The Structure of PrP(Sc) Prions. Pathogens. 2018;7(1). doi: 10.3390/pathogens7010020 29414853.

4. Aguzzi A, Sigurdson C, Heikenwaelder M. Molecular mechanisms of prion pathogenesis. Annu Rev Pathol. 2008;3:11–40. doi: 10.1146/annurev.pathmechdis.3.121806.154326 18233951.

5. Knaus KJ, Morillas M, Swietnicki W, Malone M, Surewicz WK, Yee VC. Crystal structure of the human prion protein reveals a mechanism for oligomerization. Nat Struct Biol. 2001;8(9):770–4. doi: 10.1038/nsb0901-770 11524679.

6. Haire LF, Whyte SM, Vasisht N, Gill AC, Verma C, Dodson EJ, et al. The crystal structure of the globular domain of sheep prion protein. J Mol Biol. 2004;336(5):1175–83. Epub 2004/03/24. doi: 10.1016/j.jmb.2003.12.059 15037077.

7. Khan MQ, Sweeting B, Mulligan VK, Arslan PE, Cashman NR, Pai EF, et al. Prion disease susceptibility is affected by beta-structure folding propensity and local side-chain interactions in PrP. Proceedings of the National Academy of Sciences of the United States of America. 2010;107(46):19808–13. doi: 10.1073/pnas.1005267107 21041683.

8. Vazquez-Fernandez E, Vos MR, Afanasyev P, Cebey L, Sevillano AM, Vidal E, et al. The Structural Architecture of an Infectious Mammalian Prion Using Electron Cryomicroscopy. PLoS pathogens. 2016;12(9):e1005835. doi: 10.1371/journal.ppat.1005835 27606840 alter our adherence to all PLoS Pathogens policies on sharing data and materials.

9. Garnier J, Osguthorpe DJ, Robson B. Analysis of the accuracy and implications of simple methods for predicting the secondary structure of globular proteins. J Mol Biol. 1978;120(1):97–120. doi: 10.1016/0022-2836(78)90297-8 642007.

10. Zhang J, Zhang Y. Molecular dynamics studies on 3D structures of the hydrophobic region PrP(109–136). Acta Biochim Biophys Sin (Shanghai). 2013;45(6):509–19. doi: 10.1093/abbs/gmt031 23563221.

11. Antonyuk SV, Trevitt CR, Strange RW, Jackson GS, Sangar D, Batchelor M, et al. Crystal structure of human prion protein bound to a therapeutic antibody. Proceedings of the National Academy of Sciences of the United States of America. 2009;106(8):2554–8. doi: 10.1073/pnas.0809170106 19204296.

12. Abskharon RN, Giachin G, Wohlkonig A, Soror SH, Pardon E, Legname G, et al. Probing the N-terminal beta-sheet conversion in the crystal structure of the human prion protein bound to a nanobody. Journal of the American Chemical Society. 2014;136(3):937–44. doi: 10.1021/ja407527p 24400836.

13. Wang F, Wang X, Yuan CG, Ma J. Generating a prion with bacterially expressed recombinant prion protein. Science. 2010;327(5969):1132–5. doi: 10.1126/science.1183748 20110469.

14. Wang F, Wang X, Abskharon R, Ma J. Prion infectivity is encoded exclusively within the structure of proteinase K-resistant fragments of synthetically generated recombinant PrP(Sc). Acta Neuropathol Commun. 2018;6(1):30. doi: 10.1186/s40478-018-0534-0 29699569.

15. Wang F, Yang F, Hu Y, Wang X, Jin C, Ma J. Lipid interaction converts prion protein to a PrPSc-like proteinase K-resistant conformation under physiological conditions. Biochemistry. 2007;46(23):7045–53. doi: 10.1021/bi700299h 17503780.

16. Wang F, Yin S, Wang X, Zha L, Sy MS, Ma J. Role of the highly conserved middle region of prion protein (PrP) in PrP-lipid interaction. Biochemistry. 2010;49(37):8169–76. doi: 10.1021/bi101146v 20718504.

17. Baral PK, Wieland B, Swayampakula M, Polymenidou M, Rahman MH, Kav NN, et al. Structural studies on the folded domain of the human prion protein bound to the Fab fragment of the antibody POM1. Acta Crystallogr D Biol Crystallogr. 2012;68(Pt 11):1501–12. Epub 2012/10/24. doi: 10.1107/S0907444912037328 23090399.

18. Sonati T, Reimann RR, Falsig J, Baral PK, O’Connor T, Hornemann S, et al. The toxicity of antiprion antibodies is mediated by the flexible tail of the prion protein. Nature. 2013;501(7465):102–6. doi: 10.1038/nature12402 23903654.

19. Sigurdson CJ, Nilsson KP, Hornemann S, Manco G, Fernandez-Borges N, Schwarz P, et al. A molecular switch controls interspecies prion disease transmission in mice. J Clin Invest. 2010;120(7):2590–9. doi: 10.1172/JCI42051 20551516.

20. Bett C, Fernandez-Borges N, Kurt TD, Lucero M, Nilsson KP, Castilla J, et al. Structure of the beta2-alpha2 loop and interspecies prion transmission. FASEB journal: official publication of the Federation of American Societies for Experimental Biology. 2012;26(7):2868–76. doi: 10.1096/fj.11-200923 22490928.

21. Aguzzi A, Baumann F, Bremer J. The prion’s elusive reason for being. Annu Rev Neurosci. 2008;31:439–77. Epub 2008/06/19. doi: 10.1146/annurev.neuro.31.060407.125620 18558863.

22. Baumann F, Tolnay M, Brabeck C, Pahnke J, Kloz U, Niemann HH, et al. Lethal recessive myelin toxicity of prion protein lacking its central domain. The EMBO journal. 2007;26(2):538–47. doi: 10.1038/sj.emboj.7601510 17245436.

23. Li A, Christensen HM, Stewart LR, Roth KA, Chiesa R, Harris DA. Neonatal lethality in transgenic mice expressing prion protein with a deletion of residues 105–125. The EMBO journal. 2007;26(2):548–58. doi: 10.1038/sj.emboj.7601507 17245437.

24. Rodriguez MM, Peoc’h K, Haik S, Bouchet C, Vernengo L, Manana G, et al. A novel mutation (G114V) in the prion protein gene in a family with inherited prion disease. Neurology. 2005;64(8):1455–7. doi: 10.1212/01.WNL.0000158618.39527.93 15851745.

25. Schmitz M, Dittmar K, Llorens F, Gelpi E, Ferrer I, Schulz-Schaeffer WJ, et al. Hereditary Human Prion Diseases: an Update. Molecular neurobiology. 2017;54(6):4138–49. doi: 10.1007/s12035-016-9918-y 27324792.

26. Norstrom EM, Mastrianni JA. The AGAAAAGA palindrome in PrP is required to generate a productive PrPSc-PrPC complex that leads to prion propagation. J Biol Chem. 2005;280(29):27236–43. Epub 2005/05/27. doi: 10.1074/jbc.M413441200 15917252.

27. Forloni G, Angeretti N, Chiesa R, Monzani E, Salmona M, Bugiani O, et al. Neurotoxicity of a prion protein fragment. Nature. 1993;362(6420):543–6. doi: 10.1038/362543a0 8464494.

28. Jobling MF, Stewart LR, White AR, McLean C, Friedhuber A, Maher F, et al. The hydrophobic core sequence modulates the neurotoxic and secondary structure properties of the prion peptide 106–126. Journal of neurochemistry. 1999;73(4):1557–65. doi: 10.1046/j.1471-4159.1999.0731557.x 10501201.

29. Kuwata K, Matumoto T, Cheng H, Nagayama K, James TL, Roder H. NMR-detected hydrogen exchange and molecular dynamics simulations provide structural insight into fibril formation of prion protein fragment 106–126. Proceedings of the National Academy of Sciences of the United States of America. 2003;100(25):14790–5. doi: 10.1073/pnas.2433563100 14657385.

30. Lim KH, Nguyen TN, Damo SM, Mazur T, Ball HL, Prusiner SB, et al. Solid-state NMR structural studies of the fibril form of a mutant mouse prion peptide PrP89-143(P101L). Solid State Nucl Magn Reson. 2006;29(1–3):183–90. doi: 10.1016/j.ssnmr.2005.09.017 16256316.

31. Rodriguez JA, Jiang L, Eisenberg DS. Toward the Atomic Structure of PrP(Sc). Cold Spring Harb Perspect Biol. 2017;9(9). doi: 10.1101/cshperspect.a031336 28096267.

32. Yu L, Lee SJ, Yee VC. Crystal Structures of Polymorphic Prion Protein beta1 Peptides Reveal Variable Steric Zipper Conformations. Biochemistry. 2015;54(23):3640–8. doi: 10.1021/acs.biochem.5b00425

33. Apostol MI, Sawaya MR, Cascio D, Eisenberg D. Crystallographic studies of prion protein (PrP) segments suggest how structural changes encoded by polymorphism at residue 129 modulate susceptibility to human prion disease. J Biol Chem. 2010;285(39):29671–5. doi: 10.1074/jbc.C110.158303 20685658.

34. Smirnovas V, Baron GS, Offerdahl DK, Raymond GJ, Caughey B, Surewicz WK. Structural organization of brain-derived mammalian prions examined by hydrogen-deuterium exchange. Nat Struct Mol Biol. 2011;18(4):504–6. doi: 10.1038/nsmb.2035 21441913.

35. Baral PK, Swayampakula M, Rout MK, Kav NN, Spyracopoulos L, Aguzzi A, et al. Structural basis of prion inhibition by phenothiazine compounds. Structure. 2014;22(2):291–303. doi: 10.1016/j.str.2013.11.009 24373770.

36. Diringer H, Ehlers B. Chemoprophylaxis of scrapie in mice. J Gen Virol. 1991;72 (Pt 2):457–60. Epub 1991/02/01. doi: 10.1099/0022-1317-72-2-457 1704414.

37. Forloni G, Iussich S, Awan T, Colombo L, Angeretti N, Girola L, et al. Tetracyclines affect prion infectivity. Proc Natl Acad Sci U S A. 2002;99(16):10849–54. Epub 2002/08/01. doi: 10.1073/pnas.162195499 12149459.

38. Caspi S, Halimi M, Yanai A, Sasson SB, Taraboulos A, Gabizon R. The anti-prion activity of Congo red. Putative mechanism. J Biol Chem. 1998;273(6):3484–9. Epub 1998/03/07. doi: 10.1074/jbc.273.6.3484 9452472.

39. Adjou KT, Privat N, Demart S, Deslys JP, Seman M, Hauw JJ, et al. MS-8209, an amphotericin B analogue, delays the appearance of spongiosis, astrogliosis and PrPres accumulation in the brain of scrapie-infected hamsters. J Comp Pathol. 2000;122(1):3–8. Epub 2000/01/11. doi: 10.1053/jcpa.1999.0338 10627386.

40. Jones DR, Taylor WA, Bate C, David M, Tayebi M. A camelid anti-PrP antibody abrogates PrP replication in prion-permissive neuroblastoma cell lines. PloS one. 2010;5(3):e9804. doi: 10.1371/journal.pone.0009804 20339552.

41. Brazier MW, Wall VA, Brazier BW, Masters CL, Collins SJ. Therapeutic interventions ameliorating prion disease. Expert review of anti-infective therapy. 2009;7(1):83–105. doi: 10.1586/14787210.7.1.83 19622059.

42. Aguzzi A, Lakkaraju AKK, Frontzek K. Toward Therapy of Human Prion Diseases. Annual review of pharmacology and toxicology. 2018;58:331–51. doi: 10.1146/annurev-pharmtox-010617-052745 28961066.

43. Eghiaian F, Grosclaude J, Lesceu S, Debey P, Doublet B, Treguer E, et al. Insight into the PrPC—>PrPSc conversion from the structures of antibody-bound ovine prion scrapie-susceptibility variants. Proceedings of the National Academy of Sciences of the United States of America. 2004;101(28):10254–9. doi: 10.1073/pnas.0400014101 15240887.

44. Abskharon RN, Soror SH, Pardon E, El Hassan H, Legname G, Steyaert J, et al. Combining in-situ proteolysis and microseed matrix screening to promote crystallization of PrPc-nanobody complexes. Protein Eng Des Sel. 2011;24(9):737–41. Epub 2011/05/04. doi: 10.1093/protein/gzr017 21536542.

45. Abskharon RN, Ramboarina S, El Hassan H, Gad W, Apostol MI, Giachin G, et al. A novel expression system for production of soluble prion proteins in E. coli. Microb Cell Fact. 2012;11:6. doi: 10.1186/1475-2859-11-6 22233534.

46. Zahn R, von Schroetter C, Wuthrich K. Human prion proteins expressed in Escherichia coli and purified by high-affinity column refolding. FEBS letters. 1997;417(3):400–4. doi: 10.1016/s0014-5793(97)01330-6 9409760.

47. Abskharon R, Wang F, Vander Stel KJ, Sinniah K, Ma J. The role of the unusual threonine string in the conversion of prion protein. Scientific reports. 2016;6:38877. doi: 10.1038/srep38877 27982059.

48. Pardon E, Laeremans T, Triest S, Rasmussen SG, Wohlkonig A, Ruf A, et al. A general protocol for the generation of Nanobodies for structural biology. Nature protocols. 2014;9(3):674–93. doi: 10.1038/nprot.2014.039 24577359.

49. Abskharon RN, Soror SH, Pardon E, El Hassan H, Legname G, Steyaert J, et al. Crystallization and preliminary X-ray diffraction analysis of a specific VHH domain against mouse prion protein. Acta Crystallogr Sect F Struct Biol Cryst Commun. 2010;66(Pt 12):1644–6. doi: 10.1107/S1744309110042168 21139215.

50. Kabsch W. Integration, scaling, space-group assignment and post-refinement. Acta Crystallogr D Biol Crystallogr. 2010;66(Pt 2):133–44. doi: 10.1107/S0907444909047374 20124693.

51. McCoy AJ. Solving structures of protein complexes by molecular replacement with Phaser. Acta Crystallogr D Biol Crystallogr. 2007;63(Pt 1):32–41. doi: 10.1107/S0907444906045975 17164524.

52. Emsley P, Cowtan K. Coot: model-building tools for molecular graphics. Acta Crystallogr D Biol Crystallogr. 2004;60(Pt 12 Pt 1):2126–32. doi: 10.1107/S0907444904019158 15572765.

53. Vagin AA, Steiner RA, Lebedev AA, Potterton L, McNicholas S, Long F, et al. REFMAC5 dictionary: organization of prior chemical knowledge and guidelines for its use. Acta Crystallogr D Biol Crystallogr. 2004;60(Pt 12 Pt 1):2184–95. doi: 10.1107/S0907444904023510 15572771.

54. Afonine PV, Grosse-Kunstleve RW, Echols N, Headd JJ, Moriarty NW, Mustyakimov M, et al. Towards automated crystallographic structure refinement with phenix.refine. Acta Crystallogr D Biol Crystallogr. 2012;68(Pt 4):352–67. Epub 2012/04/17. doi: 10.1107/S0907444912001308 22505256.

55. Wallace AC, Laskowski RA, Thornton JM. LIGPLOT: a program to generate schematic diagrams of protein-ligand interactions. Protein Eng. 1995;8(2):127–34. doi: 10.1093/protein/8.2.127 7630882.

56. Hutchinson EG, Thornton JM. PROMOTIF—a program to identify and analyze structural motifs in proteins. Protein science: a publication of the Protein Society. 1996;5(2):212–20. doi: 10.1002/pro.5560050204 8745398.

57. Krissinel E, Henrick K. Inference of macromolecular assemblies from crystalline state. J Mol Biol. 2007;372(3):774–97. doi: 10.1016/j.jmb.2007.05.022 17681537.

58. Mahal SP, Baker CA, Demczyk CA, Smith EW, Julius C, Weissmann C. Prion strain discrimination in cell culture: the cell panel assay. Proc Natl Acad Sci U S A. 2007;104(52):20908–13. doi: 10.1073/pnas.0710054104 18077360.

59. Polymenidou M, Moos R, Scott M, Sigurdson C, Shi YZ, Yajima B, et al. The POM monoclonals: a comprehensive set of antibodies to non-overlapping prion protein epitopes. PloS one. 2008;3(12):e3872. doi: 10.1371/journal.pone.0003872 19060956.

60. Falsig J, Aguzzi A. The prion organotypic slice culture assay—POSCA. Nature protocols. 2008;3(4):555–62. doi: 10.1038/nprot.2008.13 18388937.

61. Hurtado de Mendoza T, Balana B, Slesinger PA, Verma IM. Organotypic cerebellar cultures: apoptotic challenges and detection. J Vis Exp. 2011;(51). doi: 10.3791/2564 21633327.

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