Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.

Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.

In order to investigate the potential of voles to reproduce in vitro the efficiency of prion replication previously observed in vivo, we seeded protein misfolding cyclic amplification (PMCA) reactions with either rodent-adapted Transmissible Spongiform Encephalopathy (TSE) strains or natural TSE iso...

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Main Authors: Gian Mario Cosseddu, Romolo Nonno, Gabriele Vaccari, Cecilia Bucalossi, Natalia Fernandez-Borges, Michele Angelo Di Bari, Joaquin Castilla, Umberto Agrimi
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2011-11-01
Series:PLoS Pathogens
Online Access:http://europepmc.org/articles/PMC3219717?pdf=render
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spelling doaj-7f4ad1284e5148dfb859f66869e1a6072020-11-24T22:10:51ZengPublic Library of Science (PLoS)PLoS Pathogens1553-73661553-73742011-11-01711e100237010.1371/journal.ppat.1002370Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.Gian Mario CossedduRomolo NonnoGabriele VaccariCecilia BucalossiNatalia Fernandez-BorgesMichele Angelo Di BariJoaquin CastillaUmberto AgrimiIn order to investigate the potential of voles to reproduce in vitro the efficiency of prion replication previously observed in vivo, we seeded protein misfolding cyclic amplification (PMCA) reactions with either rodent-adapted Transmissible Spongiform Encephalopathy (TSE) strains or natural TSE isolates. Vole brain homogenates were shown to be a powerful substrate for both homologous or heterologous PMCA, sustaining the efficient amplification of prions from all the prion sources tested. However, after a few serial automated PMCA (saPMCA) rounds, we also observed the appearance of PK-resistant PrP(Sc) in samples containing exclusively unseeded substrate (negative controls), suggesting the possible spontaneous generation of infectious prions during PMCA reactions. As we could not definitively rule out cross-contamination through a posteriori biochemical and biological analyses of de novo generated prions, we decided to replicate the experiments in a different laboratory. Under rigorous prion-free conditions, we did not observe de novo appearance of PrP(Sc) in unseeded samples of M109M and I109I vole substrates, even after many consecutive rounds of saPMCA and working in different PMCA settings. Furthermore, when positive and negative samples were processed together, the appearance of spurious PrP(Sc) in unseeded negative controls suggested that the most likely explanation for the appearance of de novo PrP(Sc) was the occurrence of cross-contamination during saPMCA. Careful analysis of the PMCA process allowed us to identify critical points which are potentially responsible for contamination events. Appropriate technical improvements made it possible to overcome PMCA pitfalls, allowing PrP(Sc) to be reliably amplified up to extremely low dilutions of infected brain homogenate without any false positive results even after many consecutive rounds. Our findings underline the potential drawback of ultrasensitive in vitro prion replication and warn on cautious interpretation when assessing the spontaneous appearance of prions in vitro.http://europepmc.org/articles/PMC3219717?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Gian Mario Cosseddu
Romolo Nonno
Gabriele Vaccari
Cecilia Bucalossi
Natalia Fernandez-Borges
Michele Angelo Di Bari
Joaquin Castilla
Umberto Agrimi
spellingShingle Gian Mario Cosseddu
Romolo Nonno
Gabriele Vaccari
Cecilia Bucalossi
Natalia Fernandez-Borges
Michele Angelo Di Bari
Joaquin Castilla
Umberto Agrimi
Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.
PLoS Pathogens
author_facet Gian Mario Cosseddu
Romolo Nonno
Gabriele Vaccari
Cecilia Bucalossi
Natalia Fernandez-Borges
Michele Angelo Di Bari
Joaquin Castilla
Umberto Agrimi
author_sort Gian Mario Cosseddu
title Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.
title_short Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.
title_full Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.
title_fullStr Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.
title_full_unstemmed Ultra-efficient PrP(Sc) amplification highlights potentialities and pitfalls of PMCA technology.
title_sort ultra-efficient prp(sc) amplification highlights potentialities and pitfalls of pmca technology.
publisher Public Library of Science (PLoS)
series PLoS Pathogens
issn 1553-7366
1553-7374
publishDate 2011-11-01
description In order to investigate the potential of voles to reproduce in vitro the efficiency of prion replication previously observed in vivo, we seeded protein misfolding cyclic amplification (PMCA) reactions with either rodent-adapted Transmissible Spongiform Encephalopathy (TSE) strains or natural TSE isolates. Vole brain homogenates were shown to be a powerful substrate for both homologous or heterologous PMCA, sustaining the efficient amplification of prions from all the prion sources tested. However, after a few serial automated PMCA (saPMCA) rounds, we also observed the appearance of PK-resistant PrP(Sc) in samples containing exclusively unseeded substrate (negative controls), suggesting the possible spontaneous generation of infectious prions during PMCA reactions. As we could not definitively rule out cross-contamination through a posteriori biochemical and biological analyses of de novo generated prions, we decided to replicate the experiments in a different laboratory. Under rigorous prion-free conditions, we did not observe de novo appearance of PrP(Sc) in unseeded samples of M109M and I109I vole substrates, even after many consecutive rounds of saPMCA and working in different PMCA settings. Furthermore, when positive and negative samples were processed together, the appearance of spurious PrP(Sc) in unseeded negative controls suggested that the most likely explanation for the appearance of de novo PrP(Sc) was the occurrence of cross-contamination during saPMCA. Careful analysis of the PMCA process allowed us to identify critical points which are potentially responsible for contamination events. Appropriate technical improvements made it possible to overcome PMCA pitfalls, allowing PrP(Sc) to be reliably amplified up to extremely low dilutions of infected brain homogenate without any false positive results even after many consecutive rounds. Our findings underline the potential drawback of ultrasensitive in vitro prion replication and warn on cautious interpretation when assessing the spontaneous appearance of prions in vitro.
url http://europepmc.org/articles/PMC3219717?pdf=render
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