Real-time fluorescent quantitative PCR probe detection method and reaction solution and kit thereof

A real-time fluorescence quantitative and probe detection technology, applied in the field of biochemical detection, can solve the problems of low content, affect the detection results, long reaction time, etc., and achieve the effects of improving yield and efficiency, high amplification efficiency, and improving specificity

Inactive Publication Date: 2018-11-02
GUANGDONG SHUNDE IND DESIGN INST GUANGDONG SHUNDE INNOVATIVE DESIGN INST
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Problems solved by technology

In applications using real-time fluorescent quantitative PCR, samples are often precious and low in content, and the length of reaction time has a great impact on stability and detection sensitivity. Short reaction time is conducive to ensuring stability and improving detection sensitivity, and vice versa. Test results
However, mos...

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  • Real-time fluorescent quantitative PCR probe detection method and reaction solution and kit thereof
  • Real-time fluorescent quantitative PCR probe detection method and reaction solution and kit thereof
  • Real-time fluorescent quantitative PCR probe detection method and reaction solution and kit thereof

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Embodiment 1

[0033] 1. Description of the main reagents involved

[0034] Betaine (Bet) and trehalose (Tre) were analytically pure, purchased from sigma; tetramethylammonium chloride and magnesium chloride were analytically pure, purchased from Shanghai Bioengineering Technology Service Co., Ltd.; micro sample genomic DNA extraction kit (spin column Type) was purchased from Tiangen Biochemical Technology Co., Ltd.; TAKARA Ex Taq HS was purchased from Shanghai Bao Biological Engineering Co., Ltd.; Genstar qPCRprobe Mix was purchased from Beijing Kangrun Biotechnology Co., Ltd.

[0035] TAKARA Ex Taq HS hot-start enzyme is used in the reaction solution of real-time fluorescent quantitative PCR probe detection method, the enzyme dosage is 0.025~0.05U / μL, the concentration of dNTP is 0.2~0.25mM, and 20~55mM pH8.0 ~9.0 Tris-HCl, 2.0~2.5mM magnesium chloride and 250~750mM potassium chloride PCR buffer; on the basis of this embodiment, a certain amount of PCR enhancer is added through the control...

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Abstract

The invention discloses a real-time fluorescent quantitative PCR probe detection method and a reaction solution and a kit thereof. The reaction solution comprises a PCR buffer solution, a Taq hot start enzyme, dNTP, betaine with the final concentration of 0.04-0.05M, trehalose with the final concentration being not higher than 0.05M and tetramethylammonium chloride with the final concentration of30-40mM, and in the reaction solution, magnesium chloride is further added till the final concentration of the magnesium chloride is 3.0-5.0mM. The normal activity of the Taq hot start enzyme can be protected at high temperature through addition of the betaine and the trehalose with the specific concentrations into the reaction solution, the specificity of a PCR reaction can be improved through addition of the tetramethylammonium chloride with the specific concentration, and the concentration of the magnesium chloride in the reaction solution is further increased, so that the yield and the efficiency of amplification are significantly improved and the time required for the amplification can be effectively shortened while no influence on the specificity of the amplification is guaranteed.

Description

technical field [0001] The invention relates to the technical field of biochemical detection, in particular to a real-time fluorescence quantitative PCR probe detection method, a reaction solution and a kit thereof. Background technique [0002] Real-time fluorescent quantitative PCR (Real-time fluorescent quantitative PCR, qPCR) was first launched by Applied Biosystems in 1996, and has been widely used in gene expression differential analysis, nucleic acid copy number detection, single nucleotide polymorphism analysis , tumor gene detection, prenatal diagnosis and other basic scientific research, as well as clinical diagnosis, detection of pathogenic microorganisms, disease research and drug development and other fields. This technology can be divided into non-specific fluorescent dye method and specific fluorescent probe detection method. In terms of specific gene detection and quantification, Taqman and MGB probe detection methods are the most widely used, and there are c...

Claims

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Application Information

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IPC IPC(8): C12Q1/6851
CPCC12Q1/6851C12Q2531/113C12Q2527/125
Inventor 刘倩张琳高秋芳李家玉
Owner GUANGDONG SHUNDE IND DESIGN INST GUANGDONG SHUNDE INNOVATIVE DESIGN INST
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