Bactrocera dorsalis Taiman gene as well as qRT-PCR (quantitative Reverse Transcription-Polymerase Chain Reaction) detection method and siRNA (small interference Ribonucleic Acid) thereof
A kind of fruit fly, gene technology, applied in its siRNA field, can solve the problems such as unseen, achieve the effect of high silencing efficiency and good application prospect
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Embodiment 1
[0025] Embodiment 1, Bacteralis dorsalis Taiman gene alternative splice body sequence cloning
[0026] Follow the steps below:
[0027] 1) Use the RNA extraction kit RNeasy Plus Micro Kit to extract the total RNA of B. dorsalis according to the instructions, and then use the reverse transcription kit Perfectreal time RT reagent to reverse transcribe 1 μg of total RNA into cDNA according to the instructions.
[0028] 2) Using the cDNA obtained above as a template, according to the Bacteralis dorsalis Taiman gene sequence predicted on NCBI and the conserved structural sequence of the gene, the full-length amplification primers were designed in segments, and a total of 5 pairs of segmented amplification primers were designed for full-length amplification. Long amplification: BdTaiS1-F / BdTaiS1-R, BdTaiS2-F / BdTaiS2-R, BdTaiS3-F / BdTaiS3-R, BdTaiS4-F / BdTaiS4-R, BdTaiS5-F / BdTaiS5-R. The PCR conditions were: pre-denaturation at 98°C for 3 min; denaturation at 98°C for 30 s, annealing ...
Embodiment 2
[0043] Embodiment two, the dsRNA of Bactrocera dorsalis Taiman gene
[0044] 1) According to the Bacteralis dorsalis Taiman gene sequence obtained by cloning, design the upstream and downstream primers (sequence containing the T7 promoter) for amplifying the Taiman gene: T7-Tai-core-F (as shown in SEQ ID NO: 16) , T7-Tai-core-R (as shown in SEQID NO: 17), the primer sequences are respectively:
[0045] T7-Tai-core-F: 5'-TAATACGACTCACTATAGGGGCTCTCAATTCGACGACACC-3';
[0046] T7-Tai-core-R: 5'-TAATACGACTCACTATAGGGACCTGACCGTTAAGCAGTGA-3'.
[0047] Use the RNA extraction kit RNeasy Plus Micro Kit to extract the total RNA of Bacteralis dorsalis according to the instructions, and then use the reverse transcription kit Perfect real time RT reagent to reverse transcribe 1 μg of total RNA into cDNA according to the instructions. The reverse transcription system 20 μl, including: total RNA 1 μl (about 1 μg), 5×PrimeScriptBuffer 4 μl, PrimeScriptRT Enzyme Mix I 1 μl, Oligo dT Primer (50...
Embodiment 3
[0055] Embodiment 3, the siRNA of Bactrocera dorsalis Taiman gene
[0056] According to the 5 alternative splicing forms of the Bacteralis dorsalis Taiman gene obtained in Example 1, for the Taiman genes Taiman-A, Taiman-B, Taiman-C, Taiman-D, Taiman-E gene, correspondingly designed 5 specific siRNA sequences and sent them to Guangzhou Ruibo Biological Co., Ltd. for synthesis. The siRNA sequences are as follows:
[0057] siTaiman-A: 5'-GUGUAUCUGCACUACUUAAUA-3', as shown in SEQ ID NO:21;
[0058] siTaiman-B: 5'-UCUAAUGUCGGUCCUGGCGGU-3', as shown in SEQ ID NO:22;
[0059] siTaiman-C: 5'-AAUUCUUUUCAAGGUGGCGGC-3', as shown in SEQ ID NO:23;
[0060] siTaiman-D: 5'-UCAACAUUUACCUGCAGGUAA-3', as shown in SEQ ID NO:24;
[0061] siTaiman-E: 5'-GUAUUGUUGGCUUUGGUGGCA-3', as shown in SEQ ID NO:25;
[0062] siGFP: 5'-GCCACAACGUCUAUAUCAUGG-3', as shown in SEQ ID NO:26.
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