Similar biochemical signatures and prion protein genotypes in atypical scrapie and Nor98 cases, France and Norway.Isolates of atypical scrapie scrapie: see prion. recently identified in sheep and goats in France were compared with Nor98 isolates reported in Norway. Western blot Western blot A technique developed in 1979 that is used to confirm ELISA results. HIV antigen is purified by electrophoresis and attached by blotting to a nylon or nitrocellulose filter. methods for characterization of the protease-resistant prion prion (prī`ŏn), infectious agent thought to cause a group of diseases known as prion diseases or transmissible spongiform encephalopathies. protein showed that all these isolates shared a unique biochemical signature: 5 groups of bands, including a characteristic band of apparent low molecular weight (11 kDa). This pattern could originate from the presence of 3 different protease protease /pro·te·ase/ (pro´te-as) endopeptidase. pro·te·ase n. Any of various enzymes, including the proteinases and peptidases, that catalyze the hydrolytic breakdown of proteins. cleavage products, including the 11 kDa most likely cleaved cleaved (klevd) split or separated, as by cutting. at both N- and C-sides of the protein. Genetic data, which strongly suggested the higher susceptibility of AHQ AHQ Association des Hôpitaux du Québec AHQ Air Headquarters AHQ Army Headquarters AHQ Ad Hoc Query AHQ Acute Hazard Quotient AHQ Association Hypoglycémie Québec AHQ Audio High Quality and A[F.sub.141] RQ animals in French cases, resembled earlier data from Nor98 scrapie. ********** Transmissible spongiform encephalopathies (TSEs) are neurodegenerative disorders that occur in sheep and goats (scrapie), cattle (bovine spongiform encephalopathy bovine spongiform encephalopathy: see prion. [BSE See Bombay Stock Exchange. BSE See Boston Stock Exchange (BSE). ]), or humans (Creutzfeldt-Jakob disease Creutzfeldt-Jakob disease: see prion. Creutzfeldt-Jakob disease or CJD Rare fatal disease of the central nervous system. It destroys brain tissue, making it spongy and causing progressive loss of mental functioning and motor control. ). The biochemical marker of the disease is currently considered to be the accumulation of an abnormal isoform (PrPres) of the normal cellular prion protein (PrPc). PrPres can be identified by its partial resistance to proteases and insolubility in detergents. Classically, after pK treatment and Western blot (WB), PrPres exhibits a typical 3-band pattern comprising 18-30 kDa, whereas PrPc is totally digested (1,2). Ovine ovine pertaining to, characteristic of, or derived from sheep. ovine atopic dermatitis symmetrical erythema, alopecia, lichenification, excoriation on woolless areas; sporadic cases, recur each summer. susceptibility to scrapie is largely controlled by polymorphisms at the PrP gene (prnp). The major polymorphisms associated with susceptibility or resistance are located at codons 136 (A or V), 154 (R or H), and 171 (R, Q, of H) (3,4). [V.sup.136][R.sup.154][Q.sup.171]/VRQ, ARQ/VRQ, and ARQ/ ARQ (Automatic Repeat reQuest) A method of handling communications errors in which the receiving station requests retransmission if an error occurs. ARQ - Automatic Repeat Request PrP animals are considered the most susceptible to scrapie, whereas homozygous ho·mo·zy·gous adj. Having the same alleles at one or more gene loci on homologous chromosome segments. Homozygous Identical genes controlling a specified inherited trait. or heterozygous het·er·o·zy·gous adj. 1. Having different alleles at one or more corresponding chromosomal loci. 2. Of or relating to a heterozygote. AHQ and heterozygous ARR ARR See: Average rate of return animals show only marginal susceptibility (5). ARR/ARR sheep are considered to be the more resistant (4,6), but after oral challenge with BSE agent they can accumulate PrPres in the spleen (7). In 1998, a novel and unusual TSE See Tokyo Stock Exchange. TSE 1. See Tokyo Stock Exchange (TSE). 2. See Toronto Stock Exchange (TSE). type (called Nor98) was identified in sheep in Norway (8). A large proportion of animals were carriers of AHQ and A[F.sub.141]RQ alleles (9). The PrP WB signature in these cases differed from the known scrapie profile; the classic 3-band WB pattern was replaced by a multiband pattern with a prominent band of low molecular mass ([approximately equal to] 12 kDa). Since 2002, an active surveillance program for TSE has been implemented in small ruminants in European Union European Union (EU), name given since the ratification (Nov., 1993) of the Treaty of European Union, or Maastricht Treaty, to the European Community (EU) countries. As a result of this program, unusual TSE isolates were rapidly identified in sheep and goats in France, Germany (10,11), and Great Britain Great Britain, officially United Kingdom of Great Britain and Northern Ireland, constitutional monarchy (2005 est. pop. 60,441,000), 94,226 sq mi (244,044 sq km), on the British Isles, off W Europe. The country is often referred to simply as Britain. (12). These atypical TSE isolates had the following characteristics: 1) they carne from sheep carrying PrP alleles reportedly associated with resistance to TSEs; 2) their rapid diagnostic test results based on PrPres detection showed discrepancies; and 3) they could not be readily confirmed by recommended Office International des Epizooties diagnostic methods (10). In this study we investigated a panel of 54 French atypical isolates from sheep (n = 51) and goats (n = 3) and compared their PrP genotypes and advanced PrPres biochemical signatures (WB electrophoretic mobility, epitope mapping Epitope mapping is the process of identification and characterization of the minimum molecular structures that are able to be recognized by the Immune System elements, mainly T and B cells. A collection of in vivo and in vitromethodologies are used for epitope mapping. , and PrPres deglycosylation pattern) with those of Nor98 cases. Materials and Methods Small Ruminant ruminant, any of a group of hooved mammals that chew their cud, i.e., that regurgitate and chew again food that has already been swallowed. Ruminants have an even number of toes on each foot and a stomach with either three or four chambers. Isolates The biologic samples (Table) consisted of 54 brain stems from 51 sheep from France and 3 goats previously classified as having atypical scrapie and collected during the active surveillance program between 2002 and 2004. These samples were compared with Nor98 samples from 4 Norwegian sheep. The prnp polymorphisms from these atypical cases were compared with a panel from animals with classic scrapie (74 clinically affected sheep obtained from 60 flocks between 2000 and 2002 and 60 scrapie-positive goats obtained from 13 flocks between 2002 and 2004. The animals with classic scrapie were not matched for age, breed, or flock structure with animals with atypical scrapie. prnp ORF Sequencing In each case, DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. was directly recovered from brain stem (30 mg) by using a commercial DNA extraction DNA extraction is a routine procedure to collect DNA for subsequent molecular or forensic analysis. Outline of a DNA extraction There are three basic steps in a DNA extraction, the details of which may vary depending on the type of sample and any substances that may kit (Qiaprep DNeasy Minikit (QIAGEN, Courtaboeuf, France) according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. manufacturer's recommendations. The complete open reading frame (ORF) sequence of the prnp gene was determined by sequencing both strands of 2 overlapping PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) fragments covering the complete ovine prnp ORF (primer 1F: GTGGGCATTTGATGCTGACAC, primer 1R: TGGTTGGGGTAACGGTACATG, Tml 59[degrees]C, primer 2F: TCAGCCCCATGGTGGTGGCT, primer 2R: CTGCAGGTAGACACTCCCTCC, Tm2 61 [degrees]C). The same primers were used for the goat samples. The PCR products were amplified for 35 cycles (extension time 45 s) and allowed to migrate on 1% agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gel. They were then purified, and both strands were sequenced. The appropriate software (SemanII, DNAstar, Monlucon, France) was then used to reconstitute re·con·sti·tute tr.v. re·con·sti·tut·ed, re·con·sti·tut·ing, re·con·sti·tutes 1. To provide with a new structure: The parks commission has been reconstituted. 2. the ORF sequence and align it with reference sequences from both ovine and caprine cap·rine n. See norleucine. caprine pertaining to or emanating from goats. caprine arthritis-encephalitis (CAE) species. PrPres Purification and Western Blotting Samples were examined by TeSeE WB (Bio-Rad, Marnes la Coquette, France), according to manufacturer's recommendations. Briefly, 20% brain homogenate homogenate /ho·mog·e·nate/ (ho-moj´in-at) material obtained by homogenization. homogenate material obtained by homogenization. was incubated with pK and detergent solution for 10 min at 37[degrees]C before buffer B was added. Samples were then centrifuged at 15,000x g for 7 min and the pellet solubilized by incubation at 100[degrees]C for 5 min in 100 [micro] L Laemmli solution completed (Bio-Rad) with 5% (v/v) [beta]-mercaptoethanol and 2% (w/v) sodium dodecyl sulfate Sodium dodecyl sulfate (or sulphate) (SDS or NaDS) (C12H25NaO4S),is an anionic surfactant that is used in household products such as toothpastes, shampoos, shaving foams and bubble baths for its thickening effect and its ability to (SDS 1. (company) SDS - Scientific Data Systems. 2. (tool) SDS - Schema Definition Set. ). Samples were centrifuged at 15,000x g for 15 min. The supernatants were then heated at 100[degrees]C for 5 min and subjected to electrophoresis. The undiluted sample (equivalent to 15 mg of tissue) was loaded onto homemade acrylamide acrylamide /acryl·a·mide/ (ah-kril´ah-mid) a vinyl monomer used in the production of polymers with many industrial and research uses; the monomeric form is a neurotoxin. SDS-polyacrylamide gels. Gels (15% resolving gel and 4% stacking gel) were subjected to electrophoresis for 60 min at 200 V. The proteins were transferred onto a polyvinylidene difluoride membrane at 115 V for 60 min. The membrane was soaked successively with phosphate-buffered saline (PBS PBS in full Public Broadcasting Service Private, nonprofit U.S. corporation of public television stations. PBS provides its member stations, which are supported by public funds and private contributions rather than by commercials, with educational, cultural, ), ethanol, and distilled water Noun 1. distilled water - water that has been purified by distillation H2O, water - binary compound that occurs at room temperature as a clear colorless odorless tasteless liquid; freezes into ice below 0 degrees centigrade and boils above 100 degrees centigrade; ; saturated with blocking solution A blocking solution is especially useful in immunostaining for reducing background staining. Blocking solutions bind to any open protein binding sites that do not have antibodies or antigens attached. [1] for 30 min; and then incubated for 30 min at room temperature with Sha 31 (4 gg/mL in PBS-Tween [PBST]) against the YEDRYYRE (148-155) ovine PrP sequence (13). The membrane was then washed with PBST and incubated for 20 min with goat anti-mouse immunoglobulin G immunoglobulin G n. Abbr. IgG The most abundant class of antibodies found in blood serum and lymph and active against bacteria, fungi, viruses, and foreign particles. Immunoglobulin G antibodies trigger action of the complement system. (IgG) antibody conjugated conjugated adj. Conjugate. estrogens, conjugated Warning - Hazardous drug! C.E.S. with horseradish peroxidase horse·rad·ish peroxidase n. An enzyme used in immunohistochemistry to label the antigen-antibody complex. diluted 1:10 in PBST. It was the subjected to the enhanced chemiluminescence chemiluminescence /chemi·lu·mi·nes·cence/ (kem?i-loo?mi-nes´ens) luminescence produced by direct transformation of chemical energy into light energy. WB detection (Amersham or Supersignal, Pierce, Orsay, France) and visualized by using the Versa Versa Versatile System Architecture (Genrad) Doc image analysis system (Bio-Rad). MW Determination A panel of 20 of these samples from 17 French sheep with atypical cases, 2 French goats with atypical cases, and a Norwegian sheep with Nor98 (Table) were selected for detailed molecular characterization. The apparent molecular weights (MWs) were determined with a protein standard (B2787; Sigma, Saint Louis Saint Louis (l  `ĭs), city (1990 pop. 396,685), independent and in no county, E Mo., on the Mississippi River below the mouth of the Missouri; inc. as a city 1822. St. , MO, USA). Each band was measured (apparent
MWs and proportions) by using Quantity One software (Bio-Rad).Epitope Mapping Different monoclonal antibodies This is a list of monoclonal antibodies, antibodies which are clones of a single parent cell. When used as medications, the generic names end in -mab (see "Nomenclature of monoclonal antibodies"). (MAbs) were used for detection of PrPres fragments: Sha 31 (4 [micro]g/mL in PBST), P4 (1/2,500 in PBST) (R-Biopharm, Saint-Didier Au Mont d'Or, France), 4F2 (1/2,500 in PBST), and 99/97.6.1 (1/2,500 in PBST). They recognized the following respective ovine sequences: YEDRYYRE (148-155) (13), WGQGGSH (93-99) (14),QPHGGGW (62-93), and 99/97.6.1 YQRE (221-224) (J. Langeveld, unpub. Pepscan data). The membranes were washed and then incubated with peroxidase-labeled conjugates against mouse Ig (1/2,500 in PBST) (Ozyme, Saint Quentin/Yvelines, France). Deglycosylation Experiments Deglycosylation experiments were performed on 6 French and 1 Nor98 isolates with PNGaseF, following the Ozyme manufacturer's instructions (P0704S) and TeSeE WB protocol for sample purification. Briefly, after PrPres purification, the pellet was solubilized by incubating at 100[degrees]C for 10 ruin in glycoprotein glycoprotein (glī'kōprō`tēn), organic compound composed of both a protein and a carbohydrate joined together in covalent chemical linkage. denaturing buffer 1x instead of Laemmli (Bio-Rad) solution. Samples were treated with PNGase F for 1 h at 37[degrees]C (reaction buffer 1x, 10% NP-40, PNGase F); buffer B was then added. Samples were centrifuged at 15,000x g for 7 min, and the pellets were solubilized in 100 [micro]L completed Laemmli solution by incubation at 100[degrees]C for 5 min. Samples were then centrifuged at 15,000x g for 15 min, and the supernatants were heated at 100[degrees]C for 5 min before electrophoresis. Results All the atypical cases detected in France by the surveillance program were initially identified by an ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. rapid diagnosis test (TeSeE Bio-Rad). The brain stem samples in our atypical scrapie panel (n = 54) invariably in·var·i·a·ble adj. Not changing or subject to change; constant. in·var  i·a·bil gave negative results with modified SAF SAF SafetySAF Society of American Foresters SAF Society of American Florists SAF Secretary of the Air Force SAF Second Amendment Foundation SAF Singapore Armed Forces SAF Students for Academic Freedom SAF Store And Forward (Scrapie-associated fibrils) Immunoblot (10,15). However, the 51 sheep and 3 goat isolates analyzed gave positive results with the highly sensitive Adj. 1. highly sensitive - readily affected by various agents; "a highly sensitive explosive is easily exploded by a shock"; "a sensitive colloid is readily coagulated" WB method (TeSeE Bio-Rad), which used the classic pK concentration for sample digestion and Sha31 MAb for PrPres detection. PrP Genetics of Classie and Atypical Cases The prnp genotypes at codons 136, 141,154, and 171 are shown in the Table. Most (87.8%) samples from sheep with classic scrapie were observed in genotypes with combinations of the ARQ, ARH ARH Agence Régionale de l'Hospitalisation ARH Art History ARH Armed Reconnaissance Helicopter ARH Adolescent Reproductive Health ARH Autosomal Recessive Hypercholesterolemia ARH Appalachian Regional Hospital ARH Appalachian Regional Healthcare, Inc. , and VRQ VRQ Valorisation-Recherche Québec (Canada) VRQ Vocationally-Related Qualification (UK) alleles. A small proportion (12%) of classic scrapie cases were observed in AF[I.sub.141] RQ carriers, but no classic scrapie was found in animals carrying the AHQ or ARR allele allele (əlēl`): see genetics. allele Any one of two or more alternative forms of a gene that may occur alternatively at a given site on a chromosome. . A large proportion (82.3%) of animals in the atypical sheep scrapie group carried the AF[I.sub.141]RQ (n = 35, 68.6%) or AHQ (n = 7, 13.7%) allele. An unusually high proportion of atypical cases were ARR heterozygous (n = 20, 39.2%), but in 16 cases the ARR allele was associated with either the AF[I.sub.141]RQ or AHQ allele. Six of the atypical cases were ARR/ARR homozygous (11.8%). Only 3 of the atypical cases had genotypes combining the ARQ, ARH, and VRQ alleles association, which was strikingly different from the group of classic sheep scrapie cases. Similarly, only 4 animals (7.8%) carried the highly susceptible VRQ allele, and in all cases this was associated with the AF[I.sub.141]RQ allele. Two of the 3 goats with atypical cases carried the AHQ allele (1 homozygous and 1 heterozygous), whereas none of the 60 sheep with cases of classic scrapie carried the AHQ allele (Table). Taken together, these data strongly suggest that AHQ and AF[I.sub.141]RQ animals are more susceptibile to atypical scrapie than to classic scrapie. PrPres WB Pattern of Atypical Scrapie and Nor98 Isolates All the atypical isolates showed a complex multiband pattern that differed dramatically from the 3-band pattern observed in classic scrapie (Figure 1A, B). Five major bands (designated I to V according to increasing electromobility) could be distinguished in all atypical cases, irrespective of irrespective of prep. Without consideration of; regardless of. irrespective of preposition despite genotype or species (sheep or goat); in all 54 cases, a V band was clearly observed around 11 kDa. [FIGURE 1 OMITTED] Twenty isolates, from 17 sheep with various genotypes, 2 goats, and 1 Nor98 sheep (Table), were subjected to repeated electrophoresis to measure the bands' apparent form. According to our measurements, the patterns from the 19 French atypical cases were very similar to each other and indistinguishable from those from the Norwegian Nor98 isolate (Figure 1C). However, a slight variability could be observed in the apparent MWs between cases. Variations of the WB method were further examined in repeated runs of PrPres isolated from a classic scrapie isolate to assess their possible significance. The analysis of 15 different runs of such a sample showed a variation coefficient (standard deviation In statistics, the average amount a number varies from the average number in a series of numbers. (statistics) standard deviation - (SD) A measure of the range of values in a set of numbers. divided by mean) of 2.1% ([+ or -] 0.1%) for the 3 bands. The observed variations in the individual measures for atypical scrapie samples were 2.0% ([+ or -] 1.0%) for bands I to IV and 4.5% ([+ or -] 3.0%) for band V. These findings strongly suggest that the observed variations between the different samples were probably due to the method rather than to significant differences between samples. The proportion of total PrPres WB signal represented by each band in the same panel of 19 French atypical cases was measured (Figure 1D). Band II was significantly more intense (mean 35%) than band III Band III is the name of a radio frequency range within the very high frequency part of the electromagnetic spectrum. Band III ranges from 174 to 230 MHz, and it is primarily used for radio and television broadcasting. (mean 20%) or bands I, IV, and V (means 10%-15%). Two individual peaks could be identified in bands II and III in runs and lanes with the highest resolution. These 2 peaks were located at 28.5 ([+ or -]50.6) and 26.6 ([+ or -]0.55) kDa in band II and at 22.5 ([+ or -]0.8) and 20.9 ([+ or -]0.4) kDa in band III (Figure 2, small arrows). PrPres Deglycosylation and Epitope Mapping Deglycosylations experiments with PNGase before WB analysis were then conducted to investigate the origin of this complex banding pattern. Because of the limited amount of field-collected material (brain stem only) and their low PrPres levels, only 6 atypical sheep isolates and 1 Nor98 isolate could be investigated. A similar pattern of 3 bands at 23.0 ([+ or -]0.5), 17.8 ([+ or -]0.7), and 10.9 ([+ or -]0.4) kDa (referred to as A, B, and C forms, respectively) (Figure 1E) was observed in all 7 samples. PNGase treatment of classic scrapie cases resulted in a single band at 19.2 ([+ or -]0.4) kDa (Figure 1F), which is consistent with already published data. The biochemical pattern was characterized by epitope mapping of PrPres using 4F2 (62-93), P4 (93-99), Sha 31 (148-155), and 99/97.6.1 (221-224) (Figure 2). Bands I to III were strongly recognized by all 4 MAbs in our panel, which indicated that the 3 bands at least contained the 85-to 155-amino acid sequence. Band IV was clearly recognized by P4 and Sha31 antibodies and faintly by 4F2 and 99/97.6.1. Band V was not recognized by the more C-terminal 99/97.6.1 antibody, which suggests that this band corresponds to a C-terminal cleaved PrPres fragment but was labeled by the 3 other MAbs, although more weakly by the 4F2 antibody. Discussion In this study, we characterized a series of TSE isolates from French sheep and goats originally classified as having atypical scrapie cases (10) on the basis of discrepancies between rapid diagnostic tests and confirmatory methods used to detect PrPres in brain stem samples. Similar discrepancies had been observed in the early description of so-called Nor98 scrapie isolates (8). The long-debated hypothesis that atypical cases and Nor98 cases could be only artifacts artifacts see specimen artifacts. and not true TSE was recently ruled out by the successful transmission of 10 of these French atypical isolates and 3 Nor98 isolates to transgenic mice over-expressing the ovine PrP ([V.sub.136] [R.sub.154] [Q.sub.171] allele) (16). Similarly, PrPres could be detected by using the TeSeE Bio-Rad WB method for all the French atypical and Nor98 cases studied here. Original PrPres WB Signature We found that PrPres showed a unique biochemical signature in all cases (54 French atypical and 4 Nor98 isolates) in comparison to classic scrapie, with 1) a multiband pattern with a characteristic band of low MW (11 kDa) and 2) 3 distinct deglycosylated PrPres forms of 23, 18, and 11 kDa (A, B, and C fragments, respectively). Given the theoretical MW of [approximately equal to] 22.8 kDa of the mature ovine PrP protein, the results obtained with all 4 antibodies in our panel, and the C-terminal 99/97.6.1 epitope epitope: see immunity. undetected from only band V, the following hypothetical sequences of the A, B, and C fragments can be inferred (Figure 3A; [17]). The PrPres fragment A (23 kDa) might correspond to a native (uncleaved or marginally cleaved by pK treatment) PrP fragment. The PrPres fragment B could be N terminally cleaved (nearby 4F2 epitope), as in classic scrapie, although cleavage of the C-terminal end cannot be fully excluded. While this scenario is already suggested by the faint labeling with 99/97.6.1 antibody, it would also be consistent with the observation that, despite the presence of the P4 epitope, PrPres B apparently has a lower mass than PrPres in ovine BSE (18). The C fragment (11 kDa) could correspond to an N (nearby 4F2 epitope) and C terminally cleaved PrPres protein. [FIGURE 3 OMITTED] If one assumes that the PrPres glycosylation process could be similar in classic (+3.8 or +7.9 for monoglycosylation and biglycosylation, respectively) and atypical scrapie cases, the theoretical MWs of the unglycosylated, monoglycosylated, and biglycosylated forms that could be derived from A, B, and C fragments can be reconstituted and compared with the banding pattern observed with different antibodies, such as Sha31 MAb (Figure 3B). Glycosylations of the 23-kDa A form would result in bands at 26.8 kDa and 30.9 kDa and those of the 18-kDa B form in bands at 21.6 and 25.7 kDa. These forms are consistent with bands I to IV, as well as with the presence of 2 distinct PrP forms detectable in both band II and band III in WB with the highest resolution (Figure 3B). The absence of detectable bands at 15 kDa and 19 kDa with any of the antibodies tested could suggest that the C form would only be present in the unglycosylated form. This lack of glycosylation would be consistent with a C-terminal cleavage of this PrP from upstream from the N-glycosylation sites (amino acids 184 and 200). Taken together, these hypotheses could explain the unique WB pattern identified in all the French atypical and Nor98 isolates studied here (Figure 3B). However, other hypotheses, such as the existence of random pK-digested fragments resulting in 3 major PrPres with variable sequences after deglycosylation, cannot be fully excluded. These hypotheses need to be considered in the light of results recently published by Klingeborn et al. (19). After purification of PrPres, including a pK treatment at 100 [micro]g/mL for 1 h at 37[degrees]C, and concentration by precipitation with trichloroacetic acid trichloroacetic acid /tri·chlo·ro·ace·tic ac·id/ (tri-klor?o-ah-se´tik) an extremely caustic acid, used in clinical chemistry to precipitate proteins and applied topically in chemabrasion and to remove warts. , these authors detected 2 PrPres products at 7 kDa (Nor98-PrP7) and 14 kDa (PrP-CTF14) in Nor98 case isolates from Swedish sheep. Importantly, 1 of these Swedish Nor98 cases was investigated in a laboratory taking part in this study (that of S.L. Benestad) and showed the same pattern with the band of low MW at 11 kDa with TeSeE Bio-Rad WB. Differences in the apparent molecular masses between the isolates from the 2 studies could result, at least in part, from the different methods used for PrPres purification and concentration, when one considers the high pK sensitivity of PrPres in atypical scrapie (10,12). The choice of antibodies could also contribute to the observed differences. For instance, in our study, band V consistently showed an apparently lower molecular mass (9-10 kDa), with P4 antibody (antibody used in the Klingeborn et al. study). Therefore, fragments C (11 kDa) and B (18 kDa) could correspond to Nor98-PrP7 and PrP-CTF14, respectively, in the harsher pK conditions used by Klingeborn et al. PrPres fragment A (23 kDa) was not observed by Klingeborn et al., which suggests that this PrPres form might be completely digested or transformed into fragments of Nor98-PrP7, PrPCTF14, or both. Despite minor differences, the results of the 2 studies in regard to the particular molecular features of atypical scrapie/Nor98 isolates are consistent. The presence of a PrPres fragment with an apparently low molecular mass, which is a salient feature of atypical and Nor98 cases, has already been reported in several human diseases. N terminally truncated PrPres migrating to either 12 kDa or 13 kDa have been reported in some sporadic Creutzfeldt-Jakob disease cases (20). The identification of a low-MW fragment cleaved at both C- and N-terminal ends of the prion protein has even been described as the hallmark of Gerstmann-Straussler-Scheinker syndrome in humans (2,21-24). However, even if these atypical isolates appear to have similarities with those from rare human prion diseases, atypical cases of scrapie are not rare in sheep and goats and, in some countries, are more frequent than the classic disease. Biodiversity in Atypical Cases The isolates from the 54 atypical cases we investigated here, which included a large panel of different PrP genotypes and 2 species (sheep and goat), possessed a unique biochemical signature, indistinguishable from that of the Nor98 isolates. All of the isolates from the French atypical and Nor98 cases that were transmitted to Tg338 ovine transgenic mice also shared the same biologic signature, with comparable incubation periods, clinical signs, lesion profiles, and PrPres deposits patterns in the central nervous system (16). Moreover, the PrPres biochemical signature in the inoculated Tg338 was strikingly comparable to that observed in the present study. Taken together, these data strongly suggest that the prions involved in atypical (sheep and goat) and Nor98 cases are in fact a unique TSE agent. However, because our cases were obtained from only 2 countries, whereas atypical cases have been identified throughout Europe (12,25-29), further studies are required before definitive conclusions can be drawn. Nevertheless, the lack of diversity in our panel, combined with the identity with Nor98 cases, suggests that the biodiversity of the TSE agents of atypical scrapie is not large. Allelic al·lele n. One member of a pair or series of genes that occupy a specific position on a specific chromosome. [German Allel, short for Allelomorph, allelomorph, from English Tropism tropism (trōp`ĭzəm), involuntary response of an organism, or part of an organism, involving orientation toward (positive tropism) or away from (negative tropism) one or more external stimuli. in Atypical Cases Although polymorphisms associated with classic scrapie have been widely documented (4,6), both the atypical and Nor98 cases (9) seemed to deviate from the established concepts of classic scrapie. In our panel, an obviously high susceptibility seemed to be associated with the AHQ and A[F.sub.141]RQ alleles, whereas the VRQ allele was poorly represented. Similar observations were reported for Nor98 cases (8,9). However, a proper analysis of the risk associated with each genotype in atypical cases will require much more data than those presented here. Indeed, all our atypical case data were collected through active surveillance network, by using a particular rapid diagnosis test. These affected animals would need to be matched for breed, age, and population (detection within the same active surveillance program with similar tests) to permitan appropriate risk factor analysis and comparison of susceptibility with animals with classic scrapie. Moreover, the distribution of A[F.sub.141] within each breed is currently unknown. This work is ongoing in France, and results should be presented soon. The involvement of ARR/ARR genotype animals not only in our study (6 cases) but also in several EU countries (11,30) is also of some concern. Based on the observed resistance to TSE in homozygous ARR animals, a breeding program A breeding program is the planned breeding of a group of animals or plants, usually involving at least several individuals and extending over several generations. Breeding programs are commonly employed in several fields where humans wish to manage the characteristics of their for resistance to scrapie and BSE has been implemented in several EU countries to control human exposure to TSE risk. This unusual susceptibility of small ruminants believed to be genetically resistant to TSE could lead to a reevaluation of such a policy. In this context, determining the distribution of infectivity in different tissues of affected animals and whether or not atypical scrapie is naturally transmissible transmissible /trans·mis·si·ble/ (trans-mis´i-b'l) capable of being transmitted. trans·mis·si·ble adj. Capable of being conveyed from one person to another. between animals within affected flocks would also be helpful. Conclusion Our data provide new information about the recently described atypical cases of TSE. These cases appear to be associated with a novel PrPres biochemical pattern; they shared similarities with some rare prion diseases in humans and were clearly distinct from classic scrapie or BSE. This potential similarity in PrPres formation mechanisms with some other rare prion diseases in humans is intriguing. However, the unusual properties of these atypical cases illustrate our decades of underestimating the biodiversity of TSEs in small ruminants and the consequences. This finding should lead to a general re-examination of our conceptual approach in the control of TSEs in small ruminants. Acknowledgments We gratefully acknowledge technical assistance from Joel Delphin, Jonathan Blachier, Dominique Canal, and Jeremy Verchere. MAbs were kindly provided by J. Grassi and K. O'Rourke. This work was partly supported by the NEUROPRION European network of excellence (EUROSTRAINS project). References (1.) McKinley MP, Bolton DC, Prusiner SB. A protease-resistant protein is a structural component of the scrapie prion. Cell. 1983;35:57-62. (2.) Tagliavini F, Lievens PM, Tranchant C, Warter JM, Mohr M, Giaccone G, et al. A 7-kDa prion protein (PrP) fragment, an integral component of the PrP region required for infectivity, is the major amyloid amyloid /am·y·loid/ (am´i-loid) 1. starchlike; amylaceous. 2. the pathologic, extracellular, waxy, amorphous substance deposited in amyloidosis, being composed of fibrils in bundles or in a meshwork of polypeptide protein in Gerstmann-Straussler-Scheinker disease A 117V. J Biol Chem. 2001;276:6009-15. (3.) Clouscard C, Beaudry P, Elsen JM, Milan D, Dussaucy M, Bounneau C, et al. Different allelic effects of the codons 136 and 171 of the prion protein gene in sheep with natural scrapie. J Gen Virol. 1995;76:2097-101. (4.) Hunter N, Foster JD, Goldmann W, Stear MJ, Hope J, Bostock C. Natural scrapie in a closed flock of Cheviot sheep The Cheviot is a breed of white faced sheep which gets its name from a range of hills in the Scottish Borders. It is still common in this area of the United Kingdom, but also in north west Scotland, Wales and the south west of England (especially Dartmoor and Exmoor) as well as occurs only in specific PrP genotypes. Arch Virol. 1996;141:809-24. (5.) Baylis M, Chihota C, Stevenson E, Goldmann W, Smith A, Sivam K, et al. Risk of scrapie in British sheep of different prion protein genotype. J Gen Virol. 2004;85:2735-40. (6.) Hunter N, Goldmann W, Foster JD, Cairns Cairns, city (1991 pop. 64,463), Queensland, NE Australia, on Trinity Bay. It is a principal sugar port of Australia; lumber and other agricultural products are also exported. The city's proximity to the Great Barrier Reef has made it a tourist center. D, Smith G. Natural scrapie and PrP genotype: case-control studies in British sheep. Ver Rec. 1997;141:137-40. (7.) Andreoletti O, Morel morel Any of various species of edible mushrooms in the genera Morchella and Verpa. Morels have a convoluted or pitted head, or cap, vary in shape, and occur in diverse habitats. The edible M. N, Lacroux C, Rouillon V, Barc C, Tabouret tab·o·ret also tab·ou·ret n. 1. A low stool without a back or arms. 2. A low stand or cabinet. 3. An embroidery frame. G, et al. Bovine spongiform encephalopathy agent in spleen from an ARR/ARR orally exposed sheep. J Gen Virol. 2006;87:1043-6. (8.) Benestad SL, Sarradin P, Thu B, Schonheit J, Tranulis MA, Bratberg B. Cases of scrapie with unusual features in Norway and designation of a new type, Nor98. Vet Rec. 2003;153:202-8. (9.) Moum T, Olsaker I, Hopp P, Moldal T, Valheim M, Benestad SL. Polymorphisms at codons 141 and 154 in the ovine prion protein gene are associated with scrapie Nor98 cases. J Gen Virol. 2005;86:231-5. (10.) Buschmann A, Biacabe AG, Ziegler U, Bencsik A, Madec JY, Erhardt G, et al. Atypical scrapie cases in Germany and France are identified by discrepant dis·crep·ant adj. Marked by discrepancy; disagreeing. [Middle English discrepaunt, from Latin discrep reaction patterns in BSE rapid tests. J Virol Methods. 2004; 117:27-36. (11.) Buschmann A, Luhken G, Schultz J, Erhardt G, Groschup MH. Neuronal accumulation of abnormal prion protein in sheep carrying a scrapie-resistant genotype (PrPARR/ARR). J Gen Virol. 2004; 85:2727-33. (12.) Everest SJ, Thorne L, Barnicle DA, Edwards JC, Elliott H, Jackman R, et al. Atypical prion protein in sheep brain collected during the British scrapie-surveillance programme. J Gen Virol. 2006;87:471-7. (13.) Feraudet C, Morel N, Simon S, Volland H, Frobert Y, Creminon C, et al. Screening of 145 anti-PrP monoclonal antibodies for their capacity to inhibit PrPSc replication in infected cells. J Biol Chem. 2005;280:11247-58. (14.) Thuring CM, van Keulen LJ, Langeveld JP, Vromans ME, van Zijderveld FG, Sweeney T. Immunohistochemical distinction between preclinical bovine spongiform encephalopathy and scrapie infection in sheep. J Comp Pathol. 2005; 132:59-69. (15.) Madec JY, Belli P, Calavas D, Baron T. Efficiency of Western blotting for the specific immunodetection of proteinase proteinase /pro·tein·ase/ (pro´ten-as?) endopeptidase. pro·tein·ase n. A protease that begins the hydrolytic breakdown of proteins usually by splitting them into polypeptide chains. K--resistant prion protein in BSE diagnosis in France. Vet Rec. 2000;146:74-6. (16.) Le Dur A, Beringue V, Andreoletti O, Reine F, Lai TL, Baron T, et al. A newly identified type of scrapie agent can naturally infect sheep with resistant PrP genotypes. Proc Natl Acad Sci U S A. 2005;102:16031-6. (17.) Sambrook J, Russell DW. Codons and amino acids. Molecular cloning-laboratory manuals. 3rd edition. Cold Spring Harbor (NY): Cold Spfing Harbor Press; 2001. p. A7-9. (18.) Stack MJ, Chaplin MJ, Clark J. Differentiation of prion protein glycoforms from naturally occurring sheep scrapie, sheep-passaged scrapie strains (CH1641 and SSBP SSBP Society for the Study of Behavioural Phenotypes (UK) SSBP Supplemental Survivor Benefit Plan 1), bovine spongiform encephalopathy (BSE) cases and Romney and Cheviot breed sheep experimentally inoculated with BSE using two monoclonal antibodies. Acta Neuropathol (Berl). 2002;104:279 86. (19.) Klingebom M, Wik L, Simonsson M, Renstrom LH, Ottinger T, Linne T. Characterization of proteinase K-resistant N- and C-terminally truncated PrP in Nor98 atypical scrapie. J Gen Virol. 2006;87:1751-60. (20.) Zou WQ, Capellari S, Parchi P, Sy MS, Gambetti P, Chen SG. Identification of novel proteinase K-resistant C-terminal fragments of PrP in Creutzfeldt-Jakob disease. J Biol Chem. 2003;278:40429-36. (21.) Tagliavini F, Prelli F, Ghiso J, Bugiani O, Serban D, Prusiner SB, et al. Amyloid protein of Gerstmann-Straussler-Scheinker disease (Indiana kindred) is an 11 kd fragment of prion protein with an N-terminal glycine glycine (glī`sēn), organic compound, one of the 20 amino acids commonly found in animal proteins. Glycine is the only one of these amino acids that is not optically active, i.e. at codon codon: see nucleic acid. 58. EMBO J. 1991 ; 10:513-9. (22.) Parchi P, Chen SG, Brown P, Zou W, Capellari S, Budka H, et al. Different patterns of truncated prion protein fragments correlate with distinct phenotypes in P 102L Gerstmann-Straussler-Scheinker disease. Proc Natl Acad Sci U S A. 1998;95:8322-7. (23.) Ghetti B, Piccardo P, Spillantini MG, ichimiya Y, Porro M, Perini F, et al. Vascular variant of prion protein cerebral amyloidosis Amyloidosis Definition Amyloidosis is a progressive, incurable, metabolic disease characterized by abnormal deposits of protein in one or more organs or body systems. with tau-positive neurofibrillary tangles Neurofibrillary tangles Abnormal structures, composed of twisted masses of protein fibers within nerve cells, found in the brains of people with Alzheimer's disease. Mentioned in: Dementia : the phenotype of the stop codon stop codon n. Any of three codons, UAA, UAG, or UGA, that signal the termination of the synthesis of a protein. Also called chain termination codon. 145 mutation in PRNE Proc Natl Acad Sci U S A. 1996;93:744-8. (24.) Ghetti B, Piccardo P, Frangione B, Bugiani O, Giaccone G, Young K, et al. Prion protein amyloidosis. Brain Pathol. 1996;6:127-45. (25.) Orge L, Galo A, Machado C, Lima C, Ochoa C, Silva J, et al. Identification of putative atypical scrapie in sheep in Portugal. J Gen Virol. 2004;85:3487-91. (26.) Gavier-Widen D, Noremark M, Benestad S, Simmons M, Renstrom L, Bratberg B, et al. Recognition of the Nor98 variant of scrapie in the Swedish sheep population. J Vet Diagn Invest. 2004;16:562-7. (27.) Epstein V, Pointing S, Halfacre S. Atypical scrapie in the Falkland Islands. Vet Rec. 2005;157:667-8. (28.) De Bosschere H, Roels S, Benestad SL, Vanopdenbosch E. Scrapie case similar to Nor98 diagnosed in Belgium via active surveillance. Vet Rec. 2004; 155:707-8. (29.) Onnasch H, Gunn HM, Bradshaw BJ, Benestad SL, Bassett HF. Two Irish cases of scrapie resembling Nor98. Ver Rec. 2004; 155:636-7. (30.) De Bosschere H, Roels S, Dechamps P, Vanopdenbosch E. TSE detected in a Belgian ARR-homozygous sheep via active surveillance. Vet J. 2005; [Epub ahead of print]. Address for correspondence: Thierry Baron, AFSSA-Lyon, Unite ATNC ATNC Apparent Total N-Nitroso Compound , 31 Ave Tony Garnier, 69364 Lyon Cedex 07, France; email: t.baron@lyon.afssa.fr Jean-Noel Arsac, * Olivier Andreoletti, ([dagger]) Jean-Marc Bilheude, ([doubledagger]) Caroline Lacroux, ([dagger]) Sylvie L. Benestad, ([section]) and Thierry Baron * * Agence Francaise de Securite Sanitaire des Aliments ALIMENTS. In the Roman and French law this word signifies the food and other things necessary to the support of life, as clothing and the like. The same name is given to the money allowed for aliments. Dig. 50, 16, 43. 2. , Lyon, France; ([dagger]) Ecole Nationale Veterinaire de Toulouse, Toulouse, France; ([doubledagger]) Bio-Rad, Marnes-la-Coquette, France; and ([section]) National Veterinary Institute, Oslo, Norway Mr Arsac is a doctoral student researching the diagnosis and characterization of prion diseases in ruminants. His research interests include molecular characterization of prion diseases from small ruminants in their natural host and in experimental mouse models.
Table. Atypical, Nor98, and classic scrapie isolates from sheep and
goats and distribution of genotypes *
Sheep isolates
Atypical, n = 51
(no. of fully
characterized Nor98, Classic,
Genotype isolates) n = 4 n = 74
A[F.sub.141]RQ/ ARR 16 (3) 1 (0) --
ARQ 9 (3) -- 5
A[F.sub.141]RQ 7 (3) 1 (0) --
VRQ 3 (0) -- 4
AHQ/ ARR 2 (1) -- --
AHQ 2 (0) 2 (1) --
ARQ 1 (0) -- --
ARH 1 (1) -- --
VRQ 1 (0) -- --
ARR/ ARR 6 (3) -- --
ARQ/ ARR 2 (2) -- --
ARQ -- -- 29
ARH -- -- 13
ARH/ ARH 1 (1) -- 3
VRQ/ ARQ -- -- 10
VRQ -- -- 9
ARH -- -- 1
Goat isolates
Atypical, Classic,
Genotype n = 3 n = 60
A[F.sub.141]RQ/ ARR -- --
ARQ -- --
A[F.sub.141]RQ -- --
VRQ -- --
AHQ/ ARR -- --
AHQ 1 (1) --
ARQ 1 (1) --
ARH -- --
VRQ -- --
ARR/ ARR -- --
ARQ/ ARR -- --
ARQ 1 (0) 60
ARH -- --
ARH/ ARH -- --
VRQ/ ARQ -- --
VRQ -- --
ARH -- --
* Amino acids encoded at positions 136, 141, 154, and 171 are
indicated.
Figure 2. Western blot profiles of PrPres in an atypical scrapie
isolate (lane 2) detected by using N-terminal (4F2, P4), central
(Sha31), or C-terminal (99/97.6.1) monoclonal antibodies. Molecular
weight (MW) standard (lane 1). Immunoreactivities obtained with each
anti-body on 10 different atypical scrapie isolates are indicated
(+, strong, [+ or -], low, -, absent).
Biochemical
pattern 4F2 P4 Sha31 99/97.6.1
Band I + + + +
Band II + + + +
Band III + + + +
Band IV (*) +/- + + +/-
Band V (**) +/- + + -
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