Rapid and High-Throughput Reverse Transcriptase Quantitative PCR (RT-qPCR) Assay for Identification and Differentiation between SARS-CoV-2 Variants B.1.1.7 and B.1.351

被引:19
|
作者
Erster, Oran [1 ]
Mendelson, Ella [1 ,2 ]
Levy, Virginia [1 ]
Kabat, Areej [1 ]
Mannasse, Batya [1 ]
Asraf, Hadar [1 ]
Azar, Roberto [1 ]
Ali, Yaniv [1 ]
Shirazi, Rachel [1 ]
Bucris, Efrat [1 ]
Bar-Ilan, Dana [1 ]
Mor, Orna [1 ,2 ]
Mandelboim, Michal [1 ,2 ]
Sofer, Danit [1 ]
Fleishon, Shai [1 ]
Zuckerman, Neta S. [1 ]
机构
[1] Chaim Sheba Med Ctr, Publ Hlth Serv, Cent Virol Lab, Minist Hlth, Ramat Gan, Israel
[2] Tel Aviv Univ, Sackler Fac Med, Sch Publ Hlth, Tel Aviv, Israel
来源
MICROBIOLOGY SPECTRUM | 2021年 / 9卷 / 02期
关键词
SARS-CoV-2; RT-qPCR; variant B.1.1.7; variant B.1.351; rapid diagnosis; differential PCR; Sanger sequencing; Illumina sequencing; Alpha variant; Beta variant; real-time PCR; SC-2; variants; molecular diagnostics; molecular virology; COVID-19;
D O I
10.1128/Spectrum.00506-21
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Emerging SARS-CoV-2 (SC-2) variants with increased infectivity and vaccine resistance are of major concern. Rapid identification of such variants is important for the public health decision making and to provide valuable data for epidemiological and policy decision making. We developed a multiplex reverse transcriptase quantitative PCR (RT-qPCR) assay that can specifically identify and differentiate between the emerging B.1.1.7 and B.1.351 SC-2 variants. In a single assay, we combined four reactions-one that detects SC-2 RNA independently of the strain, one that detects the D3L mutation, which is specific to variant B.1.1.7, one that detects the 242 to 244 deletion, which is specific to variant B.1.351, and the fourth reaction, which identifies the human RNAseP gene, serving as an endogenous control for RNA extraction integrity. We show that the strain-specific reactions target mutations that are strongly associated with the target variants and not with other major known variants. The assay's specificity was tested against a panel of respiratory pathogens (n = 16), showing high specificity toward SC-2 RNA. The assay's sensitivity was assessed using both in vitro transcribed RNA and clinical samples and was determined to be between 20 and 40 viral RNA copies per reaction. The assay performance was corroborated with Sanger and whole-genome sequencing, showing complete agreement with the sequencing results. The new assay is currently implemented in the routine diagnostic work at the Central Virology Laboratory, and may be used in other laboratories to facilitate the diagnosis of these major worldwide-circulating SC-2 variants. IMPORTANCE This study describes the design and utilization of a multiplex reverse transcriptase quantitative PCR (RT-qPCR) to identify SARS-COV-2 (SC2) RNA in general and, specifically, to detect whether it is of lineage B.1.1.7 or B.1.351. Implementation of this method in diagnostic and research laboratories worldwide may help the efforts to contain the COVID-19 pandemic. The method can be easily scaled up and be used in high-throughput laboratories, as well as small ones. In addition to immediate help in diagnostic efforts, this method may also help in epidemiological studies focused on the spread of emerging SC-2 lineages.
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页数:9
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