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Real-time fluorescent PCR (polymerase chain reaction) detection kit for non-deletion type alpha thalassemia

A technology of thalassemia and detection kit, which is applied in the field of biomedicine, can solve the problems that affect the application of TaqMan fluorescent PCR method, the number of users of fluorescent PCR instruments, and the long detection process, so as to reduce the probability of cross-contamination, and the operation is simple and fast , the effect of short detection time

Active Publication Date: 2013-09-11
深圳益生堂生物企业有限公司 +1
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  • Application Information

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Problems solved by technology

These two methods involve many operational steps, and the results cannot be directly interpreted after PCR. Subsequent analysis of the PCR products is required. The operation of opening the tube is prone to contamination, and the detection process takes a long time.
[0014] However, when using the TaqMan probe fluorescent PCR method, the design is relatively difficult, especially the design of the TaqMan probe, which must not only ensure specificity but also satisfy effective and efficient amplification, and at the same time need to solve the gap between channels in single-tube multi-channel detection. The problem of signal interference, as well as the problem that there were not many users of fluorescent PCR instruments before, have affected the application of TaqMan fluorescent PCR method.

Method used

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  • Real-time fluorescent PCR (polymerase chain reaction) detection kit for non-deletion type alpha thalassemia
  • Real-time fluorescent PCR (polymerase chain reaction) detection kit for non-deletion type alpha thalassemia
  • Real-time fluorescent PCR (polymerase chain reaction) detection kit for non-deletion type alpha thalassemia

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Experimental program
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Embodiment 1

[0088] 1. Preparation of sample genomic DNA

[0089] This kit has no specified requirements for the extraction method of human genomic DNA. Human genomic DNA can be extracted by routine laboratory methods (phenol chloroform extraction method) or kits. It is recommended to use blood / cell / Organize the genomic DNA extraction kit and operate according to the kit instructions. Blood samples were anticoagulated with EDTA or sodium citrate.

[0090] 2. Preparation of PCR reaction solutions Ⅰ and Ⅱ

[0091] 1) The preparation of PCR reaction solution I is shown in Table 5.

[0092]

[0093] table 5

[0094] 2) The preparation of PCR reaction solution II is shown in Table 6.

[0095]

[0096] Table 6

[0097] Mix the prepared PCR reaction solutions I and II evenly, centrifuge briefly for 5 seconds, and dispense them into PCR tubes.

[0098] 3. Add 2 μL of the extracted genomic DNA template to the PCR reaction tubes containing PCR reaction solutions I and II, centrifuge at ...

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Abstract

The invention relates to the field of a biological medicine, and particularly relates to a real-time fluorescent PCR (polymerase chain reaction) detection kit for non-deletion type alpha thalassemia. The kit comprises two PCR reagents, namely a PCR reagent I and CPR reagent II, wherein each PCR reagent comprises a primer, a probe, PCR Buffer, dNTPs, MgCl2, DNA (deoxyribonucleic acid) polymerase, UNG (unguentum) enzyme and glycine betaine. By adopting the kit, QS (quality safety) and CS mutant types of the non-deletion type alpha-thalassemia can be simultaneously detected by a single test. The real-time fluorescent PCR detection kit has the characteristics of short detection time, high sensitivity and strong specificity, and is simple to operate; the result can be judged and read after fluorescent PCR is finished; the problem of carrying out complicated operations of hybridization, sequencing and solubility curve analysis on a PCR product in the prior art is overcome.

Description

technical field [0001] The invention relates to the field of biomedicine, in particular to a real-time fluorescent PCR detection kit for non-deletion type α-thalassemia. Background technique [0002] Thalassemia, also known as thalassemia, is an inherited hemolytic anemia. Its pathogenesis is the reduction or loss of globin chains in the synthesis of hemoglobin, resulting in abnormal structure of hemoglobin. Thalassemias are classified according to the amino acid chains involved, and thalassemias are usually divided into 4 types: α, β, δβ, and δ, among which β and α thalassemias are more common. [0003] In foreign countries, thalassemia is more common in Mediterranean countries (hence the name thalassemia) and Southeast Asian countries. The vast area south of the Yangtze River in my country is a high incidence area of ​​thalassemia, especially in the three provinces (regions) of Guangxi, Guangdong, and Hainan, and other provinces (regions) such as Hong Kong, Taiwan, Fujia...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/68
Inventor 刘红光陈立炎张文
Owner 深圳益生堂生物企业有限公司
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