Pretreatment method, pretreatment solution and kit for virus nucleic acid detection, and application of pretreatment solution
A technology of pretreatment solution and viral nucleic acid, which is applied in microorganism-based methods, biochemical equipment and methods, and microbial determination/inspection, etc. Conducive to long-term storage and detection, easy degradation, and improved detection efficiency
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Embodiment 1
[0053] Example 1 The present invention is used for the pretreatment and rapid detection of respiratory syncytial virus (RSV) oropharyngeal swab samples
[0054] In order to evaluate the virus pretreatment solution in this invention, the virus pretreatment solution of this invention (the concentration of Tris-HCl is 100mM, the concentration of EDTA-2Na is 10mM, the concentration of sodium chloride is 0.9% (w / v), The concentration of RNasin was 20U / mL, and the concentration of Proclin950 was 0.04% (v / v)) were compared with normal saline and commercial virus pretreatment solution. The method for comparison is pretreatment with a clinically diagnosed positive respiratory syncytial virus (RSV) throat swab sample diluted (1:9, v / v). Hours / 24 hours / 48 hours and 72 hours were used for direct amplification of samples, and the detection efficiency of real-time qPCR (real-time qPCR) under room temperature pretreatment conditions was compared by Ct value to evaluate the effect of differen...
Embodiment 2
[0059] Example 2 The present invention is used for nucleic acid pretreatment and rapid detection after purification of 2019 novel coronavirus (2019-nCoV) samples
[0060] In order to evaluate the virus pretreatment solution in this invention, the virus pretreatment solution of this invention (the concentration of Tris-HCl is 100mM, the concentration of EDTA-2Na is 10mM, the concentration of sodium chloride is 0.9% (w / v), The concentration of RNasin was 20U / mL, and the concentration of Proclin 300 was 0.01% (v / v)) were compared with normal saline and commercial virus pretreatment solution. The method for comparison is to dilute (1:9, v / v) pretreatment with the nucleic acid of the 2019 novel coronavirus (2019-nCoV) that is clinically diagnosed as positive. hours / 24 hours / 48 hours and 72 hours for direct amplification of samples, and by comparing the detection efficiency of real-time fluorescent quantitative PCR (real-timeqPCR) under room temperature pretreatment conditions by Ct...
Embodiment 3
[0063] Example 3 The present invention is used for pretreatment and rapid detection of enterovirus versatility (EV) throat swab samples
[0064] In order to evaluate the virus pretreatment solution in this invention, the virus pretreatment solution of this invention (the concentration of Tris-HCl is 100mM, the concentration of EDTA-2Na is 10mM, the concentration of sodium chloride is 0.9% (w / v), The concentration of SDS was 0.1%, and the concentration of Proclin950 was 0.04% (v / v)) were compared with normal saline and commercial virus pretreatment solution. The method for comparison is pretreatment with the common enterovirus (EV) throat swab samples clinically diagnosed as positive (1:9, v / v). The pretreatment condition is room temperature 25°C. Samples were directly amplified at 0 hours / 24 hours / 48 hours and 72 hours, and the detection efficiency of real-time qPCR (real-time qPCR) under room temperature pretreatment conditions was compared by Ct value to evaluate the effect ...
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