A kind of recombinant vector and its construction method and application
A technology for recombining vectors and constructing methods, which is applied in the direction of vectors, applications, nucleic acid vectors, etc., to achieve the effect of easy operation, simple operation and accurate results
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Embodiment 1
[0050] Preparation of the 3'UTR region fragment of Ccdc124 gene of brown planthopper:
[0051] Extraction and Detection of Total RNA from Brown Planthopper Tissue
[0052] Trizol reagent (purchased from Invitrogen) was used to extract the total RNA of the brown planthopper (provided by Wuhan University). For the specific extraction steps, refer to the instruction manual of the Trizol reagent. The dissolved RNA was detected by electrophoresis on a 1.5% agarose gel containing ethidium bromide (EB), and the concentration was measured on an RNA concentration analyzer at the same time.
[0053] Design of primers for the 3'UTR region of Ccdc124 gene in brown planthopper
[0054] According to the 3'UTR region of the brown planthopper Ccdc124 gene sequence (ID: XM_022350855.1) in GenBank, PCR primers were designed using PrimerPremier5.0 software, and the Ccdc124 gene amplification primer sequences were as follows:
[0055] Ccdc124-3'UTR-F:5'-ccggctcgagcaaatcacccgagaacccta-3' (SEQ ID...
Embodiment 2
[0074] Example 2 Application of psi-CHECK2-Ccdc124-3'UTR luciferase reporter carrier
[0075] Artificially synthesized candidate miRNAs
[0076] Synthetic miR-8: 5'-ucuguuucagcagugcgagcgg-3' (SEQ ID No.4) and NC negative control: 5'-ugacaaagucgucugcgagcgg-3' (SEQ ID No.5). The above miRNAs and NC controls were synthesized by Shanghai Gemma Pharmaceutical Technology Co., Ltd.
[0077] Recovery and passaging of Drosophila cells
[0078] Hold the cryopreservation tube containing 1mL of Drosophila cell suspension and quickly put it into a 37°C water bath (the water level should be lower than the cap of the cryopreservation tube) to shake and thaw, transfer it into a 15mL glass core tube containing 4mL of medium prepared in advance and mix well . Centrifuge at 1000rpm for 4min, discard the supernatant, add 1mL medium and blow evenly. Then all cell suspensions were transferred to culture flasks containing 5 mL of dark medium and cultured overnight. Change the medium the next da...
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