An Upgrade on the Surveillance System of SARS-CoV-2: Deployment of New Methods for Genetic Inspection |
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Authors: | José Francisco Muñ oz-Valle,Alberto Antony Venancio-Landeros,Rocí o Sá nchez-Sá nchez,Karen Reyes-Dí az,Byron Galindo-Ornelas,Wendy Susana Hé rnandez-Monjaraz,Alejandra Garcí a-Rí os,Luis Fernando Garcí a-Ortega,Jorge Herná ndez-Bello,Marcela Peñ a-Rodrí guez,Natali Vega-Magañ a,Luis Delaye,Mauricio Dí az-Sá nchez,Octavio Patricio Garcí a-Gonzá lez |
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Abstract: | SARS-CoV-2 variants surveillance is a worldwide task that has been approached with techniques such as Next Generation Sequencing (NGS); however, this technology is not widely available in developing countries because of the lack of equipment and limited funding in science. An option is to deploy a RT-qPCR screening test which aids in the analysis of a higher number of samples, in a shorter time and at a lower cost. In this study, variants present in samples positive for SARS-CoV-2 were identified with a RT-qPCR mutation screening kit and were later confirmed by NGS. A sample with an abnormal result was found with the screening test, suggesting the simultaneous presence of two viral populations with different mutations. The DRAGEN Lineage analysis identified the Delta variant, but there was no information about the other three mutations previously detected. When the sequenced data was deeply analyzed, there were reads with differential mutation patterns, that could be identified and classified in terms of relative abundance, whereas only the dominant population was reported by DRAGEN software. Since most of the software developed to analyze SARS-CoV-2 sequences was aimed at obtaining the consensus sequence quickly, the information about viral populations within a sample is scarce. Here, we present a faster and deeper SARS-CoV-2 surveillance method, from RT-qPCR screening to NGS analysis. |
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Keywords: | qPCR variant screening SARS-CoV-2 variant identification SARS-CoV-2 epidemiology genetic surveillance |
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