High-temperature inducible promoter for specific expression of plant green tissues and application
A technology of green tissue and plant expression vector, which can be used in high temperature inducible promoters and application fields, and can solve problems such as energy consumption and dwarf plants
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Embodiment 1
[0026] Example 1: Real-time fluorescent quantitative PCR analysis of the expression characteristics of the RCA1 gene
[0027] 1. Use the RNAprep Pure Polysaccharide Polyphenol Plant Total RNA Extraction Kit (Tiangen Biochemical Technology Co., Ltd.) to extract the samples to be tested (young leaves, mature leaves, stems, and petals after three-year-old cutting seedlings of Rhododendron hainan treated at 37°C for 3 hours at high temperature , pistil, stamen) each sample RNA, agarose electrophoresis to detect the integrity, Nanodrop to determine the concentration.
[0028] 2. Take 1 μg RNA and use PrimeScript TM RT reagent Kit with gDNA Eraser (PerfectReal Time) kit (TaKaRa Company) was used to generate cDNA by reverse transcription, which was used as a template for quantitative PCR after dilution. Fluorescent quantitative PCR was carried out using the SYBR dye method, the instrument used was Roche LightCycler 480II, and 18S rRNA was used as an internal reference, according to...
Embodiment 2
[0034] Example 2: pRCA1 promotes the stable expression of the GUS gene
[0035] 1. Cloning of pRCA1
[0036] 1. Using the CTAB method to extract the genomic DNA of Rhododendron hainanensis.
[0037] 2. Using the Rhododendron hainanensis genomic DNA as a template, using the high-fidelity enzyme PrimeSTAR Max, the primer pair consisting of primers pRCA1-F1: 5'-ACTCGGCACAGCTACTACC-3' and pRCA1-R1: 5'-CAAAGGTGGAAACGGCAG-3' was used for PCR amplification , to obtain the PCR product.
[0038] The reaction system was 25 μL: 1 μL of upper and lower primers, 12.5 μL of Max mix, 1 μL of genomic DNA, 9.5 μL of ddH2O; the PCR reaction program was pre-denaturation at 98°C for 60 s; followed by denaturation at 98°C for 10 s, annealing at 57°C for 15 s, extension at 72°C for 60 s, and 30 cycle; 72°C extension for 10 min.
[0039]3. Carry out agarose gel electrophoresis to the PCR amplification product, reclaim the band similar to the size of the target promoter fragment with the DNA gel r...
Embodiment 3
[0060] Example 3: pRCA1 initiates transient expression of LUC gene
[0061] 1. Construction of recombinant plasmid pRCA1::LUC.
[0062] The schematic diagram of the recombinant plasmid pRCA1::LUC is shown in image 3 .
[0063] (1) Construction of plant expression vectors by seamless cloning method. The plant expression vector pGreenⅡ0800-LUC was single digested with Pst I, and the linearized vector fragment was recovered after agarose gel electrophoresis.
[0064] (2) Design the specific primer pRCA1-F5 containing the vector sequence according to the sequence at the gap after single restriction digestion of pGreenⅡ0800-LUC:
[0065] 5'-GCTTGATATCGAATTC CTGCAG CTACTACCAAGCACCTCCGC-3'
[0066] and pRCA1-R5:
[0067] 5'-GGATCCCCCGGG CTGCAG AGAAATCAAGGGTCTGTTTGGGA-3' (the underline is the recognition site of the restriction endonuclease PstI),
[0068] The promoter with vector sequences at both ends was amplified by the high-fidelity enzyme PrimeSTAR Max.
[0069] (3) ...
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