Evaluation of sample pooling for screening of SARS CoV-2.

Evaluation of sample pooling for screening of SARS CoV-2.

<h4>Background</h4>The coronavirus disease 2019 (COVID-19) pandemic has revealed the global public health importance of robust diagnostic testing. To overcome the challenge of nucleic acid (NA) extraction and testing kit availability, an efficient method is urgently needed.<h4>Obje...

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Main Authors: Andargachew Mulu, Dawit Hailu Alemayehu, Fekadu Alemu, Dessalegn Abeje Tefera, Sinknesh Wolde, Gebeyehu Aseffa, Tamrayehu Seyoum, Meseret Habtamu, Alemseged Abdissa, Abebe Genetu Bayih, Getachew Tesfaye Beyene
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.0247767
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spelling doaj-a11d4d1740a6459baabae372ad84ee1e2021-03-12T05:31:30ZengPublic Library of Science (PLoS)PLoS ONE1932-62032021-01-01162e024776710.1371/journal.pone.0247767Evaluation of sample pooling for screening of SARS CoV-2.Andargachew MuluDawit Hailu AlemayehuFekadu AlemuDessalegn Abeje TeferaSinknesh WoldeGebeyehu AseffaTamrayehu SeyoumMeseret HabtamuAlemseged AbdissaAbebe Genetu BayihGetachew Tesfaye Beyene<h4>Background</h4>The coronavirus disease 2019 (COVID-19) pandemic has revealed the global public health importance of robust diagnostic testing. To overcome the challenge of nucleic acid (NA) extraction and testing kit availability, an efficient method is urgently needed.<h4>Objectives</h4>To establish an efficient, time and resource-saving and cost-effective methods, and to propose an ad hoc pooling approach for mass screening of SARS-CoV-2.<h4>Methods</h4>We evaluated pooling approach on both direct clinical and NA samples. The standard reverse transcriptase polymerase chain reaction (RT-PCR) test of the SARS CoV-2 was employed targeting the nucleocapsid (N) and open reading frame (ORF1ab) genomic region of the virus. The experimental pools were created using SARS CoV-2 positive clinical samples and extracted RNA spiked with up to 9 negative samples. For the direct clinical samples viral NA was extracted from each pool to a final extraction volume of 200μL, and subsequently both samples tested using the SARS CoV-2 RT-PCR assay.<h4>Results</h4>We found that a single positive sample can be amplified and detected in pools of up to 7 samples depending on the cycle threshold (Ct) value of the original sample, corresponding to high, and low SARS CoV-2 viral copies per reaction. However, to minimize false negativity of the assay with pooling strategies and with unknown false negativity rate of the assay under validation, we recommend pooling of 4/5 in 1 using the standard protocols of the assay, reagents and equipment. The predictive algorithm indicated a pooling ratio of 5 in 1 was expected to retain accuracy of the test irrespective of the Ct value samples spiked, and result in a 137% increase in testing efficiency.<h4>Conclusions</h4>The approaches showed its concept in easily customized and resource-saving manner and would allow expanding of current screening capacities and enable the expansion of detection in the community. We recommend clinical sample pooling of 4 or 5 in 1. However, we don't advise pooling of clinical samples when disease prevalence is greater than 7%; particularly when sample size is large.https://doi.org/10.1371/journal.pone.0247767
collection DOAJ
language English
format Article
sources DOAJ
author Andargachew Mulu
Dawit Hailu Alemayehu
Fekadu Alemu
Dessalegn Abeje Tefera
Sinknesh Wolde
Gebeyehu Aseffa
Tamrayehu Seyoum
Meseret Habtamu
Alemseged Abdissa
Abebe Genetu Bayih
Getachew Tesfaye Beyene
spellingShingle Andargachew Mulu
Dawit Hailu Alemayehu
Fekadu Alemu
Dessalegn Abeje Tefera
Sinknesh Wolde
Gebeyehu Aseffa
Tamrayehu Seyoum
Meseret Habtamu
Alemseged Abdissa
Abebe Genetu Bayih
Getachew Tesfaye Beyene
Evaluation of sample pooling for screening of SARS CoV-2.
PLoS ONE
author_facet Andargachew Mulu
Dawit Hailu Alemayehu
Fekadu Alemu
Dessalegn Abeje Tefera
Sinknesh Wolde
Gebeyehu Aseffa
Tamrayehu Seyoum
Meseret Habtamu
Alemseged Abdissa
Abebe Genetu Bayih
Getachew Tesfaye Beyene
author_sort Andargachew Mulu
title Evaluation of sample pooling for screening of SARS CoV-2.
title_short Evaluation of sample pooling for screening of SARS CoV-2.
title_full Evaluation of sample pooling for screening of SARS CoV-2.
title_fullStr Evaluation of sample pooling for screening of SARS CoV-2.
title_full_unstemmed Evaluation of sample pooling for screening of SARS CoV-2.
title_sort evaluation of sample pooling for screening of sars cov-2.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2021-01-01
description <h4>Background</h4>The coronavirus disease 2019 (COVID-19) pandemic has revealed the global public health importance of robust diagnostic testing. To overcome the challenge of nucleic acid (NA) extraction and testing kit availability, an efficient method is urgently needed.<h4>Objectives</h4>To establish an efficient, time and resource-saving and cost-effective methods, and to propose an ad hoc pooling approach for mass screening of SARS-CoV-2.<h4>Methods</h4>We evaluated pooling approach on both direct clinical and NA samples. The standard reverse transcriptase polymerase chain reaction (RT-PCR) test of the SARS CoV-2 was employed targeting the nucleocapsid (N) and open reading frame (ORF1ab) genomic region of the virus. The experimental pools were created using SARS CoV-2 positive clinical samples and extracted RNA spiked with up to 9 negative samples. For the direct clinical samples viral NA was extracted from each pool to a final extraction volume of 200μL, and subsequently both samples tested using the SARS CoV-2 RT-PCR assay.<h4>Results</h4>We found that a single positive sample can be amplified and detected in pools of up to 7 samples depending on the cycle threshold (Ct) value of the original sample, corresponding to high, and low SARS CoV-2 viral copies per reaction. However, to minimize false negativity of the assay with pooling strategies and with unknown false negativity rate of the assay under validation, we recommend pooling of 4/5 in 1 using the standard protocols of the assay, reagents and equipment. The predictive algorithm indicated a pooling ratio of 5 in 1 was expected to retain accuracy of the test irrespective of the Ct value samples spiked, and result in a 137% increase in testing efficiency.<h4>Conclusions</h4>The approaches showed its concept in easily customized and resource-saving manner and would allow expanding of current screening capacities and enable the expansion of detection in the community. We recommend clinical sample pooling of 4 or 5 in 1. However, we don't advise pooling of clinical samples when disease prevalence is greater than 7%; particularly when sample size is large.
url https://doi.org/10.1371/journal.pone.0247767
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