Virus nucleic acid extraction or preservation reagent, primer probe combination, virus amplification reagent, kit and application thereof

A technology for virus nucleic acid and preservation reagents, applied in the field of virus nucleic acid extraction or preservation reagents, virus amplification reagents, can solve problems such as poor repeatability, long time, health hazards, etc.

Active Publication Date: 2021-01-26
CAPITALBIO CORP +1
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0005] (1) At present, the commonly used nucleic acid extraction technology has complex extraction process, long time and low nucleic acid extraction efficiency, which cannot meet the needs of clinical testing; commonly used viral nucleic acid extraction and purification technologies include Trizol method, spin column method, magnetic bead method, etc.
The Trizol method separates proteins and nucleic acids by using the difference in the distribution positions of DNA, RNA, and proteins in the organic layer and the aqueous layer. In the process of obtaining nucleic acids, phenol, chloroform, isoamyl alcohol, isopropanol, and ethanol are used, which are harmful to the human body. The volatile organic solvents present great health hazards to operators, and the Trizol method for nucleic acid extraction is cumbersome, and the reproducibility of different sample extraction results is not good. It takes at least 1.5 hours from sample lysis to nucleic acid acquisition. Time-consuming, not suitable for clinical testing
Conventional centrifugal adsorption column and magnetic bead method need to use ethanol or isopropanol for binding when extracting nucleic acid, and need to add ethanol for cleaning. This method of adding alcohol for cleaning makes the operation of nucleic acid extraction reagents relatively complicated and time-consuming. , if ethanol is not removed cleanly, it will also inhibit the subsequent reaction
[0006] (2) The amplification efficiency of the isothermal amplification system is extremely high. During the amplification process of the target, unnecessary non-specific amplification is inevitably introduced, making it difficult to judge the result. For non-specific amplification, non-specific fluorescent dyes The incorporation method can't do anything about the specificity of the product, and further analysis of the product is required, such as cas enzyme digestion identification, etc.
However, it involves opening the cover, which can easily cause environmental pollution such as aerosol pollution, which is not conducive to clinical testing.

Method used

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  • Virus nucleic acid extraction or preservation reagent, primer probe combination, virus amplification reagent, kit and application thereof
  • Virus nucleic acid extraction or preservation reagent, primer probe combination, virus amplification reagent, kit and application thereof
  • Virus nucleic acid extraction or preservation reagent, primer probe combination, virus amplification reagent, kit and application thereof

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Experimental program
Comparison scheme
Effect test

Embodiment 1

[0113] Embodiment 1: the extraction reagent of viral nucleic acid

[0114] The specific component configuration can be composed as follows:

[0115] Component 1 is containing oligodT 14-20 magnetic beads.

[0116] Component 2 is the lysis preservation solution, which consists of: lithium dodecyl sulfate (final concentration 0.016%), TritonX-100 (final concentration 1.64%), guanidine isothiocyanate (final concentration 1.03M), Tris pH= 8.0 (final concentration 0.042M), NaCl (final concentration 0.21M).

[0117] (3) Component 3 is a cleaning solution, and its composition is: TritonX-100 (final concentration 0.1%), KCl (0.1M).

[0118] (4) Component 4 is the eluent, and its composition is: the final concentration of Tris is 100 mM, and the final concentration of EDTA is 10 mM.

Embodiment 2

[0119] Embodiment 2: the extraction reagent of viral nucleic acid

[0120] The specific component configuration can be composed as follows:

[0121] Component 1 is containing oligodT 14-20 magnetic beads.

[0122] Component 2 is the lysis preservation solution, and its composition is: lithium dodecyl sulfate (0.01%), TritonX-100 (3%), guanidine isothiocyanate (0.5M), Tris (0.1M), NaCl (0.1 M).

[0123] (3) Component 3 is a cleaning solution, which consists of TritonX-100 (0.05%) and KCl (0.2M).

[0124] (4) Component 4 is the eluent, which consists of Tris (10 mM) and EDTA (10 mM).

Embodiment 3

[0125] Embodiment 3: the extraction reagent of viral nucleic acid

[0126] The specific component configuration can be composed as follows:

[0127] Component 1 is containing oligodT 14-20 magnetic beads.

[0128] Component 2 is the lysis preservation solution, which consists of lithium dodecyl sulfate (0.05%), TritonX-100 (0.5%), guanidine isothiocyanate (1.5M), Tris (0.01), NaCl (0.2M) .

[0129] (3) Component 3 is a cleaning solution, which consists of TritonX-100 (0.2%) and KCl (0.05M).

[0130] (4) Component 4 is the eluent, which consists of Tris (100 mM) and EDTA (1 mM).

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Abstract

The invention relates to the field of virus detection, and particularly relates to a virus nucleic acid extraction or preservation reagent, a primer probe combination, a virus amplification reagent, akit and application thereof. A virus detection device provides a simple and feasible virus nucleic acid extraction method, the whole process is about 5-15 minutes, and purified nucleic acid is recovered and can be used for detecting virus nucleic acid. The method comprises PCR, NASBA, LAMP, RPA and the like. Compared with a traditional virus extraction method, the method is high in virus nucleicacid recovery rate, short in time, convenient to operate and easy to clinically popularize. The invention relates to an isothermal amplification primer, a probe combination sequence and a reaction buffer solution for simultaneously detecting novel coronavirus COVID-19N and ORF genes and human-derived reference genes through a single tube. The system is good in specificity, high in sensitivity (50cp / mL) and high in specificity, only needs 20min of detection time, and can report positive within about 10 min at the soonest.

Description

technical field [0001] The invention relates to the field of virus detection, in particular to virus nucleic acid extraction or preservation reagents, primer probe combinations, virus amplification reagents, kits and applications thereof. Background technique [0002] The new coronavirus is the third to appear in humans in the past 20 years after the severe acute respiratory syndrome coronavirus (SARS-CoV) that broke out in 2002 and the Middle East respiratory syndrome coronavirus (MERS-CoV) that broke out in 2012 Highly pathogenic coronavirus. Nucleic acid detection is a basis for pathogen diagnosis, and it is also an important basis for the current diagnosis of new crown infection. Therefore, carrying out nucleic acid virus detection is also an important means for virus infection screening and virus disease prevention and control. In the process of clinical and practical application, not only the specificity, sensitivity and accuracy of the virus detection method have hi...

Claims

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Application Information

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IPC IPC(8): C12Q1/70C12Q1/6806C12Q1/6844C12N15/11C12R1/93
CPCC12Q1/6806C12Q1/6844C12Q1/701C12Q2600/166C12Q2523/308C12Q2527/125C12Q2531/119C12Q2545/101C12Q2563/107
Inventor 郭弘妍王辉毛沁心陈翔徐友春王会丽邓浩浩李雅婷程京
Owner CAPITALBIO CORP
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