Development and Testing of a Low-Cost Inactivation Buffer That Allows for Direct SARS-CoV-2 Detection in Saliva

被引:2
|
作者
Bustos-Garcia, Brandon [1 ]
Garza-Manero, Sylvia [2 ]
Cano-Dominguez, Nallely [1 ]
Maria Lopez-Sanchez, Dulce [3 ]
Salgado-Montes de Oca, Gonzalo [3 ]
Salgado-Aguayo, Alfonso [4 ]
Recillas-Targa, Felix [2 ]
Avila-Rios, Santiago [3 ]
Julian Valdes, Victor [1 ]
机构
[1] Natl Autonomous Univ Mexico UNAM, Inst Cellular Physiol IFC, Dept Cell Biol & Dev, Mexico City 04510, DF, Mexico
[2] Natl Autonomous Univ Mexico UNAM, Inst Cellular Physiol IFC, Dept Mol Genet, Mexico City 04510, DF, Mexico
[3] Natl Inst Resp Dis CIENI INER, Ctr Res Infect Dis, Mexico City 14080, DF, Mexico
[4] Natl Inst Resp Dis INER, Lab Res Rheumat Dis, Mexico City 14080, DF, Mexico
关键词
SARS-CoV-2; COVID-19; testing; direct RT-qPCR; saliva; MEMBRANE-PROTEINS; DETERGENTS; LIPIDS; VIRUS;
D O I
10.3390/vaccines10050730
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Massive testing is a cornerstone in efforts to effectively track infections and stop COVID-19 transmission, including places with good vaccination coverage. However, SARS-CoV-2 testing by RT-qPCR requires specialized personnel, protection equipment, commercial kits, and dedicated facilities, which represent significant challenges for massive testing in resource-limited settings. It is therefore important to develop testing protocols that are inexpensive, fast, and sufficiently sensitive. Here, we optimized the composition of a buffer (PKTP), containing a protease, a detergent, and an RNase inhibitor, which is compatible with the RT-qPCR chemistry, allowing for direct SARS-CoV-2 detection from saliva without extracting RNA. PKTP is compatible with heat inactivation, reducing the biohazard risk of handling samples. We assessed the PKTP buffer performance in comparison to the RNA-extraction-based protocol of the US Centers for Disease Control and Prevention in saliva samples from 70 COVID-19 patients finding a good sensitivity (85.7% for the N1 and 87.1% for the N2 target) and correlations (R = 0.77, p < 0.001 for N1, and R = 0.78, p < 0.001 for N2). We also propose an auto-collection protocol for saliva samples and a multiplex reaction to minimize the PCR reaction number per patient and further reduce costs and processing time of several samples, while maintaining diagnostic standards in favor of massive testing.
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页数:17
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