Real-time fluorescent nucleic acid constant-temperature amplification and detection kit for human seasonal influenza viruses H1N1 (HuH1N1)
A seasonal influenza and H1N1 technology, applied in fluorescence/phosphorescence, microbial measurement/inspection, biochemical equipment and methods, etc., can solve problems such as complicated operation, hindering large-scale promotion and use, and contamination of amplicons
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Embodiment 1
[0099] Example 1. Design of special primers and probes for real-time fluorescent nucleic acid constant temperature amplification detection of human seasonal influenza virus H1N1 (HuH1N1)
[0100] The present invention selects the non-secondary structure and highly conserved segment in the HuH1N1 virus HA gene as the amplified target sequence region (its nucleotide sequence is shown in sequence 1 in the sequence table), according to the principle of primer probe design, using DNAATAR, DNAman Software and artificially designed special primers and probe sequences for real-time fluorescent nucleic acid constant temperature amplification detection of human seasonal influenza virus H1N1 (HuH1N1), and obtained the following specific sequences:
[0101] (1) a capture probe (TCO, Target Capture Oligo) that can specifically combine with the target nucleic acid (HuH1N1 RNA) sequence of human seasonal influenza virus H1N1 (HuH1N1) as shown in Sequence 1 in the sequence listing, the capture...
Embodiment 2
[0105] Example 2, Preparation of Human Seasonal Influenza Virus H1N1 (HuH1N1) Real-time Fluorescent Nucleic Acid Constant Temperature Amplification Detection Kit
[0106] Using the special primers and probes provided in Example 1, the human seasonal influenza virus H1N1 (HuH1N1) real-time fluorescent nucleic acid constant temperature amplification detection kit of the present invention was obtained. The kit contains capture probes (TCO, Target Capture Oligo), T7 primers, nT7 primers, HuH1N1 detection probes, M-MLV reverse transcriptase and T7 RNA polymerase; when there is an internal standard in the kit, it also includes Labeled detection probes.
[0107] The capture probe exists in the nucleic acid extraction solution, the T7 primer, nT7 primer, HuH1N1 detection probe, and internal standard detection probe exist in the HuH1N1 detection solution, and the M-MLV reverse transcriptase and T7 RNA polymerase The enzyme exists in the SAT enzyme solution. Specifically, the kit is di...
Embodiment 3
[0140] Embodiment 3, detection sensitivity of real-time fluorescent nucleic acid constant temperature amplification of human seasonal influenza virus H1N1 (HuH1N1)
[0141] With the kit of the present invention (see Example 2 for the composition, there is no HuH1N1 internal standard in the kit, and there is no internal standard detection probe in the detection solution) the measured concentration is 1 × 10 4 copies / reaction, 1×10 3 copies / reaction, 1×10 2 Copies / reaction, 10copies / reaction of human seasonal influenza virus positive control RNA, determine the lower limit of sensitivity. Specific steps are as follows:
[0142] (1) dilution
[0143] Will 1×10 4 Copies / reaction of human seasonal influenza virus positive reference RNA, 10-fold serial dilution to 1×10 3 copies / reaction, 1×10 2 copies / reaction, 10copies / reaction.
[0144] (2) Nucleic acid extraction
[0145] 2.1 Add 200 μl lysate (containing HEPES 35mM, (NH 4 ) 2 SO 4 20mM), 200 μl influenza virus positive...
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