Combined methylmalonic acidemia gene mutation detection kit
A technology of methylmalonic acidemia and detection kits, which is applied to the determination/testing of microorganisms, DNA/RNA fragments, recombinant DNA technology, etc., to achieve the effects of poor long-term prognosis, short time period and high precision
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[0025] The present invention establishes a primer and a kit for detecting the hotspot mutation region of human MMAHCC gene by using multiplex PCR-sanger sequencing technology, which is simple, fast, accurate and high-throughput, so as to provide a reference for the detection of MMAHC gene mutation. The kit is stored in -20°C. Kit specifications: 50 servings / box, see Table 1 for specific components.
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[0034] Kit Performance Verification
[0035] 1. Sample processing
[0036] Enterprise reference products were selected for kit performance verification. All samples were subjected to nucleic acid extraction kit (Product No.: IVD4173) from Biogene, and the obtained DNA samples were stored at 2-8°C; if the samples were not used for a long time, they could be stored at -20°C.
[0037] 2. PCR amplification
[0038] Configure the PCR amplification reaction solution as shown in the table ...
experiment example
[0074] 60 clinical samples were tested.
[0075] 1.1 Sample processing
[0076] Blood samples were collected from 20 combined MMA subjects and 40 healthy subjects.
[0077] Key points for sample collection: Use purple cranial tubes (blood collection tubes containing ethylenediaminetetraacetic acid and its salts) to collect venous blood, and store it at 4°C for later use.
[0078] Take 200 µL from each sample, and extract DNA according to the DNA extraction kit (product number: IVD4173) of Biogene Biotechnology.
[0079] 1.2 PCR amplification
[0080] Configure the PCR amplification reaction solution as shown in the table below (45 μL for each reaction)
[0081] .
[0082] Aliquot the configured PCR amplification reaction solution into 45 μL of each reaction space. Add 5 μL each of the processed sample DNA, positive control DNA, and negative control DNA to the corresponding reaction wells, and perform PCR amplification on the machine.
[0083] 1.3 Amplification procedur...
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