Gene silencing technique based Laodelphax striatellus lethal gene fragment Alpha1-tubulin and dsRNA thereof
A technology of gene fragments and striatellus, applied in the field of agricultural biology, can solve the problems of poor chemical control effect and environmental pollution, and achieve the effects of reducing mechanical damage, convenient experimental operation, and low synthesis cost
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Embodiment 1
[0038] 1. Cloning method of Alpha1-tubulin gene fragment:
[0039] (1) Get 10-20 heads of SBPH, and use the TRIzol method to extract total RNA;
[0040] (2) Synthesizing the first strand of cDNA;
[0041] (3) Obtain the gene fragment sequence from the SBPH transcriptome. After homology comparison at http: / / www.ncbi.nlm.nih.gov / , it is predicted to be the SBPH Alpha1-tubulin gene, using Primer Premier 5.0 software designed P1 and P2, amplified by RT-PCR method;
[0042] Upstream primer (P1): 5'ACACCATCGGAAAGG 3'(SEQ ID NO.2),
[0043] Downstream primer (P2): 5'CACCGTCGAATCTCAATGA 3' (SEQ ID NO.3);
[0044] The PCR reaction program was: denaturation at 94°C for 2 min, 30 sec at 94°C, 30 sec at 55°C, 30 sec at 72°C, 35 cycles, and extension at 72°C.
[0045] PCR reaction system (50μL):
[0046]
[0047]
[0048] (4) The PCR product is separated by agarose gel electrophoresis, and the target DNA fragment is recovered;
[0049] (5) Insert the recovered target fragment i...
Embodiment 2
[0053] Embodiment 2.dsRNA synthesis and recovery
[0054] (1) According to the verified Alpha1-tubulin gene fragment sequence, use Primer Premier 5.0 software to design P3 and P4, and add the T7 promoter sequence TAATACGACTCACTATAGGG to the 5' end of the upstream and downstream primers;
[0055] Upstream primer (P4): 5' TAATACGACTCACTATAGGG ACACCATCGGAAAGG 3' (SEQ ID NO.5)
[0056] Upstream primer (P5): 5'TAATACGACTCACTATAGGG CACCGTCGAATCTCAATGA 3'(SEQ ID NO.6)
[0057]
[0058] PCR reaction program: denaturation at 94°C for 2min, 30sec at 94°C, 30sec at 60°C, 30sec at 72°C, 38 cycles, extension at 72°C.
[0059] (2) The PCR product was separated by electrophoresis on a low-melting point agarose gel with a concentration of 1% and observed under ultraviolet light. The results are shown in figure 1 , whose sequence is shown in SEQ ID NO.4.
[0060] (3) Using Promega's SV Gel and PCR Clean-Up System kit for recovery:
[0061] ① Cut the gel of the separated target fragmen...
Embodiment 3
[0071] Embodiment 3.dsRNA feeding experiment
[0072] (1) Seal one end of the glass tube with a parafilm, suck the second-instar SBPH into the glass tube with a sucker, and seal the other end with gauze;
[0073] (2) Gently pat the insects to one end with your hands, remove the gauze from the other end, put the prepared parafilm sticker up, pull evenly to both sides, pull it into a square, and then cover it on the glass On the nozzle of the tube, place the tube upright on the ultra-clean table;
[0074] (3) Draw 100 μl of feed with a pipette gun and drop it in the center of the parafilm, the control only adds feed (see Table 2 for formula), and the treatment group adds dsRNA of Alpha1-tubulin gene (see Table 1 for concentration) in the feed, and use a new The parafilm, with the side of the sticker facing down, is pasted on the opening of the glass tube, and the feed and dsRNA are sealed between the two layers of parafilm;
[0075] (4) Put the glass tube with feed and dsRNA b...
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