Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.

Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.

<h4>Background</h4>Variant Creutzfeldt-Jakob disease (vCJD) is a neurodegenerative infectious disorder, characterized by a prominent accumulation of pathological isoforms of the prion protein (PrP(TSE)) in the brain and lymphoid tissues. Since the publication in the United Kingdom of fou...

Full description

Bibliographic Details
Main Authors: Christiane Segarra, Daisy Bougard, Mohammed Moudjou, Hubert Laude, Vincent Béringue, Joliette Coste
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23894513/?tool=EBI
id doaj-32c156f7feb248f1a9805fb7b607648e
record_format Article
spelling doaj-32c156f7feb248f1a9805fb7b607648e2021-03-03T23:05:56ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-0187e6963210.1371/journal.pone.0069632Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.Christiane SegarraDaisy BougardMohammed MoudjouHubert LaudeVincent BéringueJoliette Coste<h4>Background</h4>Variant Creutzfeldt-Jakob disease (vCJD) is a neurodegenerative infectious disorder, characterized by a prominent accumulation of pathological isoforms of the prion protein (PrP(TSE)) in the brain and lymphoid tissues. Since the publication in the United Kingdom of four apparent vCJD cases following transfusion of red blood cells and one apparent case following treatment with factor VIII, the presence of vCJD infectivity in the blood seems highly probable. For effective blood testing of vCJD individuals in the preclinical or clinical phase of infection, it is considered necessary that assays detect PrP(TSE) concentrations in the femtomolar range.<h4>Methodology/principal findings</h4>We have developed a three-step assay that firstly captures PrP(TSE) from infected blood using a plasminogen-coated magnetic-nanobead method prior to its serial amplification via protein misfolding cyclic amplification (PMCA) and specific PrP(TSE) detection by western blot. We achieved a PrP(TSE) capture yield of 95% from scrapie-infected material. We demonstrated the possibility of detecting PrP(TSE) in white blood cells, in buffy coat and in plasma isolated from the blood of scrapie-infected sheep collected at the pre-clinical stage of the disease. The test also allowed the detection of PrP(TSE) in human plasma spiked with a 10(-8) dilution of vCJD-infected brain homogenate corresponding to the level of sensitivity (femtogram) required for the detection of the PrP(TSE) in asymptomatic carriers. The 100% specificity of the test was revealed using a blinded panel comprising 96 human plasma samples.<h4>Conclusion/significance</h4>We have developed a sensitive and specific amplification assay allowing the detection of PrP(TSE) in the plasma and buffy coat fractions of blood collected at the pre-clinical phase of the disease. This assay represents a good candidate as a confirmatory assay for the presence of PrP(TSE) in blood of patients displaying positivity in large scale screening tests.https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23894513/?tool=EBI
collection DOAJ
language English
format Article
sources DOAJ
author Christiane Segarra
Daisy Bougard
Mohammed Moudjou
Hubert Laude
Vincent Béringue
Joliette Coste
spellingShingle Christiane Segarra
Daisy Bougard
Mohammed Moudjou
Hubert Laude
Vincent Béringue
Joliette Coste
Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.
PLoS ONE
author_facet Christiane Segarra
Daisy Bougard
Mohammed Moudjou
Hubert Laude
Vincent Béringue
Joliette Coste
author_sort Christiane Segarra
title Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.
title_short Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.
title_full Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.
title_fullStr Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.
title_full_unstemmed Plasminogen-based capture combined with amplification technology for the detection of PrP(TSE) in the pre-clinical phase of infection.
title_sort plasminogen-based capture combined with amplification technology for the detection of prp(tse) in the pre-clinical phase of infection.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description <h4>Background</h4>Variant Creutzfeldt-Jakob disease (vCJD) is a neurodegenerative infectious disorder, characterized by a prominent accumulation of pathological isoforms of the prion protein (PrP(TSE)) in the brain and lymphoid tissues. Since the publication in the United Kingdom of four apparent vCJD cases following transfusion of red blood cells and one apparent case following treatment with factor VIII, the presence of vCJD infectivity in the blood seems highly probable. For effective blood testing of vCJD individuals in the preclinical or clinical phase of infection, it is considered necessary that assays detect PrP(TSE) concentrations in the femtomolar range.<h4>Methodology/principal findings</h4>We have developed a three-step assay that firstly captures PrP(TSE) from infected blood using a plasminogen-coated magnetic-nanobead method prior to its serial amplification via protein misfolding cyclic amplification (PMCA) and specific PrP(TSE) detection by western blot. We achieved a PrP(TSE) capture yield of 95% from scrapie-infected material. We demonstrated the possibility of detecting PrP(TSE) in white blood cells, in buffy coat and in plasma isolated from the blood of scrapie-infected sheep collected at the pre-clinical stage of the disease. The test also allowed the detection of PrP(TSE) in human plasma spiked with a 10(-8) dilution of vCJD-infected brain homogenate corresponding to the level of sensitivity (femtogram) required for the detection of the PrP(TSE) in asymptomatic carriers. The 100% specificity of the test was revealed using a blinded panel comprising 96 human plasma samples.<h4>Conclusion/significance</h4>We have developed a sensitive and specific amplification assay allowing the detection of PrP(TSE) in the plasma and buffy coat fractions of blood collected at the pre-clinical phase of the disease. This assay represents a good candidate as a confirmatory assay for the presence of PrP(TSE) in blood of patients displaying positivity in large scale screening tests.
url https://www.ncbi.nlm.nih.gov/pmc/articles/pmid/23894513/?tool=EBI
work_keys_str_mv AT christianesegarra plasminogenbasedcapturecombinedwithamplificationtechnologyforthedetectionofprptseinthepreclinicalphaseofinfection
AT daisybougard plasminogenbasedcapturecombinedwithamplificationtechnologyforthedetectionofprptseinthepreclinicalphaseofinfection
AT mohammedmoudjou plasminogenbasedcapturecombinedwithamplificationtechnologyforthedetectionofprptseinthepreclinicalphaseofinfection
AT hubertlaude plasminogenbasedcapturecombinedwithamplificationtechnologyforthedetectionofprptseinthepreclinicalphaseofinfection
AT vincentberingue plasminogenbasedcapturecombinedwithamplificationtechnologyforthedetectionofprptseinthepreclinicalphaseofinfection
AT joliettecoste plasminogenbasedcapturecombinedwithamplificationtechnologyforthedetectionofprptseinthepreclinicalphaseofinfection
_version_ 1714811863201480704

Similar Items