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New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene
New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene
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New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene
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New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene
New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene

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New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene
New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene
Journal Article

New and distinct chronic wasting disease strains associated with cervid polymorphism at codon 116 of the Prnp gene

2021
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Overview
Chronic wasting disease (CWD) is a prion disease affecting cervids. Polymorphisms in the prion protein gene can result in extended survival of CWD-infected animals. However, the impact of polymorphisms on cellular prion protein (PrP C ) and prion properties is less understood. Previously, we characterized the effects of a polymorphism at codon 116 (A>G) of the white-tailed deer (WTD) prion protein and determined that it destabilizes PrP C structure. Comparing CWD isolates from WTD expressing homozygous wild-type (116AA) or heterozygous (116AG) PrP, we found that 116AG-prions were conformationally less stable, more sensitive to proteases, with lower seeding activity in cell-free conversion and reduced infectivity. Here, we aimed to understand CWD strain emergence and adaptation. We show that the WTD-116AG isolate contains two different prion strains, distinguished by their host range, biochemical properties, and pathogenesis from WTD-116AA prions (Wisc-1). Serial passages of WTD-116AG prions in tg(CerPrP)1536 +/+ mice overexpressing wild-type deer-PrP C revealed two populations of mice with short and long incubation periods, respectively, and remarkably prolonged clinical phase upon inoculation with WTD-116AG prions. Inoculation of serially diluted brain homogenates confirmed the presence of two strains in the 116AG isolate with distinct pathology in the brain. Interestingly, deglycosylation revealed proteinase K-resistant fragments with different electrophoretic mobility in both tg(CerPrP)1536 +/+ mice and Syrian golden hamsters infected with WTD-116AG. Infection of tg60 mice expressing deer S96-PrP with 116AG, but not Wisc-1 prions induced clinical disease. On the contrary, bank voles resisted 116AG prions, but not Wisc-1 infection. Our data indicate that two strains co-existed in the WTD-116AG isolate, expanding the variety of CWD prion strains. We argue that the 116AG isolate does not contain Wisc-1 prions, indicating that the presence of 116G-PrP C diverted 116A-PrP C from adopting a Wisc-1 structure. This can have important implications for their possible distinct capacities to cross species barriers into both cervids and non-cervids.