Primer and probe combination and kit for multiplex real-time fluorescence PCR detection of beta-thalassemia gene mutation

A thalassemia, real-time fluorescence technology, applied in the field of molecular biology detection, can solve problems such as inability to perform high-throughput detection

Active Publication Date: 2020-08-28
厦门安普利生物工程有限公司 +1
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  • Abstract
  • Description
  • Claims
  • Application Information

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Problems solved by technology

At present, some studies choose to use real-time fluorescent PCR technology for the detection of β-thalassemia gene mutations, but the

Method used

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  • Primer and probe combination and kit for multiplex real-time fluorescence PCR detection of beta-thalassemia gene mutation
  • Primer and probe combination and kit for multiplex real-time fluorescence PCR detection of beta-thalassemia gene mutation
  • Primer and probe combination and kit for multiplex real-time fluorescence PCR detection of beta-thalassemia gene mutation

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Embodiment 1

[0108] 1. The kit of the present invention contains the following components: 1 tube each of the 1st amplification solution to the 12th amplification solution (24 servings per tube), 4 tubes of reaction buffer solution (1.5mL / tube), and 3 tubes of enzyme mixture (50μL / bottle), 6 pieces of dilution buffer (1.5mL / bottle), 2 pieces of TE buffer solution (1.5mL / bottle), 5 pieces of paraffin oil (1.5mL / bottle), 1 piece of negative control substance (500μL / bottle ) and 1 positive control substance (500 μL / bottle).

[0109] Wherein the reaction buffer formulation: 50mM HEPES (4-hydroxyethylpiperazineethanesulfonic acid), 25mM (NH 4 ) 2 SO 4 , 125mM KCl, 7.5mM MgCl 2 , 2.50% formamide, 0.3 mM dNTPs. 0.6 mM dUTP.

[0110] Enzyme mixture formula: 4.0U / μL TaqDNA polymerase, 0.004U / μL UNG enzyme, enzyme storage solution A to make up to the prepared volume

[0111] Dilution buffer formulation: 1mM 9mM

[0112] TE buffer formulation: 5.6mM 4.4mM 1 mM EDTA·2Na

[0113] Negat...

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Abstract

The invention provides a primer and probe combination and a kit for multiplex real-time fluorescence PCR detection of beta-thalassemia gene mutation, and belongs to the technical field of molecular biology detection. The primer and probe combination comprises one or more of a first group of primer and probe combination to a twelfth group of primer and probe combination; each group of primer and probe combination comprises primers and probes for detecting two beta-thalassemia gene mutation types and two corresponding wild types; and conditions of the mutation types are indicated by an FAM fluorescence channel or an HEX fluorescence channel, and the wild types are indicated by an ROX fluorescence channel or a CY5 fluorescence channel. The primer and probe combination can simultaneously detect two or more sites in the mutation types and the wild types of a beta-thalassemia mutant gene, and reads information and a detection result through four different fluorescence channels, so that high-throughput and specific detection of beta-thalassemia is achieved.

Description

technical field [0001] The invention relates to the technical field of molecular biology detection, in particular to a combination of primers and probes and a kit for multiple real-time fluorescent PCR detection of beta-thalassemia gene mutation. Background technique [0002] β-thalassemia is a hemolytic anemia caused by the deletion or defect of the β-strain protein gene, which inhibits the synthesis of the β-strain protein chain. The main mutation method is point mutation, and a few are deletion mutations. Completely incapable of synthesizing β chains is called β0 thalassemia, can partially synthesize β chains and is called β+ thalassemia, which can be formed through different combinations: β0 thalassemia homozygote (β0 / β0), β0 thalassemia double heterozygote (β0 / β+ ), β0 heterozygous (β0 / βA), β+ thalassemia homozygous (β+ / β+) and β+ thalassemia heterozygous (β+ / βA). Among them, patients with β-thalassemia major are β+ thalassemia homozygotes, β0 thalassemia homozygotes, ...

Claims

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Application Information

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IPC IPC(8): C12Q1/6883C12Q1/6858C12N15/11
CPCC12Q1/6883C12Q1/6858C12Q2600/16C12Q2600/156C12Q2600/166C12Q2537/143C12Q2561/113C12Q2563/107C12Q2531/113C12Q2545/101Y02A50/30
Inventor 魏劭雷彩霞林培蕊魏超
Owner 厦门安普利生物工程有限公司
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