Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.

Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.

<h4>Introduction</h4>Toxoplasma-PCR is essential to diagnose ocular, cerebral, disseminated and congenital toxoplasmosis. This multicenter study evaluated the impact of sample storage duration at +4°C on PCR assay performances in order to propose guidelines for the storage of samples dur...

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Main Authors: Marie-Pierre Brenier-Pinchart, Emmanuelle Varlet-Marie, Florence Robert-Gangneux, Denis Filisetti, Juliette Guitard, Yvon Sterkers, Hélène Yera, Hervé Pelloux, Patrick Bastien
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2021-01-01
Series:PLoS ONE
Online Access:https://doi.org/10.1371/journal.pone.0246802
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spelling doaj-f132e8c475314383b900de6034effcf92021-08-05T04:30:55ZengPublic Library of Science (PLoS)PLoS ONE1932-62032021-01-01162e024680210.1371/journal.pone.0246802Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.Marie-Pierre Brenier-PinchartEmmanuelle Varlet-MarieFlorence Robert-GangneuxDenis FilisettiJuliette GuitardYvon SterkersHélène YeraHervé PellouxPatrick Bastien<h4>Introduction</h4>Toxoplasma-PCR is essential to diagnose ocular, cerebral, disseminated and congenital toxoplasmosis. This multicenter study evaluated the impact of sample storage duration at +4°C on PCR assay performances in order to propose guidelines for the storage of samples during shipment or/and before PCR.<h4>Materials and methods</h4>Five matrices, amniotic (AF), cerebrospinal (CSF), and bronchoalveolar lavage fluids (BALF), whole blood (WB) and buffy coat (BC), were artificially spiked with different amounts of Toxoplasma gondii (20, 100, 500 tachyzoites per mL of sample) or with previously infected THP1 cells. DNA extractions were performed at day 0 and after 2, 4 and 7 days of storage at +4°C. Each extract was amplified at least twice by real-time PCR.<h4>Results</h4>A total of 252 spiked samples was studied. No increase of crossing point was observed and all samples were positive for AF, BALF, BC and infected THP1-spiked WB after up to 7 days at 4°C. For CSF spiked with 20 parasites/mL, only 50% of PCR reactions were positive at D7 (p<0.05). For WB spiked with type II parasites, all reactions remained positive at D7 but amplifications were significantly delayed from D2; and for WB spiked with RH strain, the proportion of positive reactions decreased at D7.<h4>Conclusion</h4>The storage of clinical samples at +4°C is compatible with the molecular detection of T. gondii parasites. Provided that PCR assays are performed in duplicate, storage of samples is possible up to 7 days. However, from the fifth day onwards, and for samples susceptible to contain low parasitic loads, we recommend to perform the PCR in multiplicate.https://doi.org/10.1371/journal.pone.0246802
collection DOAJ
language English
format Article
sources DOAJ
author Marie-Pierre Brenier-Pinchart
Emmanuelle Varlet-Marie
Florence Robert-Gangneux
Denis Filisetti
Juliette Guitard
Yvon Sterkers
Hélène Yera
Hervé Pelloux
Patrick Bastien
spellingShingle Marie-Pierre Brenier-Pinchart
Emmanuelle Varlet-Marie
Florence Robert-Gangneux
Denis Filisetti
Juliette Guitard
Yvon Sterkers
Hélène Yera
Hervé Pelloux
Patrick Bastien
Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
PLoS ONE
author_facet Marie-Pierre Brenier-Pinchart
Emmanuelle Varlet-Marie
Florence Robert-Gangneux
Denis Filisetti
Juliette Guitard
Yvon Sterkers
Hélène Yera
Hervé Pelloux
Patrick Bastien
author_sort Marie-Pierre Brenier-Pinchart
title Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
title_short Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
title_full Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
title_fullStr Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
title_full_unstemmed Impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
title_sort impact of pre-analytic step duration on molecular diagnosis of toxoplasmosis for five types of biological samples.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2021-01-01
description <h4>Introduction</h4>Toxoplasma-PCR is essential to diagnose ocular, cerebral, disseminated and congenital toxoplasmosis. This multicenter study evaluated the impact of sample storage duration at +4°C on PCR assay performances in order to propose guidelines for the storage of samples during shipment or/and before PCR.<h4>Materials and methods</h4>Five matrices, amniotic (AF), cerebrospinal (CSF), and bronchoalveolar lavage fluids (BALF), whole blood (WB) and buffy coat (BC), were artificially spiked with different amounts of Toxoplasma gondii (20, 100, 500 tachyzoites per mL of sample) or with previously infected THP1 cells. DNA extractions were performed at day 0 and after 2, 4 and 7 days of storage at +4°C. Each extract was amplified at least twice by real-time PCR.<h4>Results</h4>A total of 252 spiked samples was studied. No increase of crossing point was observed and all samples were positive for AF, BALF, BC and infected THP1-spiked WB after up to 7 days at 4°C. For CSF spiked with 20 parasites/mL, only 50% of PCR reactions were positive at D7 (p<0.05). For WB spiked with type II parasites, all reactions remained positive at D7 but amplifications were significantly delayed from D2; and for WB spiked with RH strain, the proportion of positive reactions decreased at D7.<h4>Conclusion</h4>The storage of clinical samples at +4°C is compatible with the molecular detection of T. gondii parasites. Provided that PCR assays are performed in duplicate, storage of samples is possible up to 7 days. However, from the fifth day onwards, and for samples susceptible to contain low parasitic loads, we recommend to perform the PCR in multiplicate.
url https://doi.org/10.1371/journal.pone.0246802
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