Application of plant alpha diastase
An alpha amylase and pollen abortion technology, applied in the fields of plant molecular biology and genetic engineering, can solve the problems of reducing the level of pollen energy metabolism, insufficient starch accumulation, few reports, etc. The effect of precise expression levels, retention and reproduction
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Embodiment 1
[0056] Embodiment 1 Rice α-amylase gene acquisition
[0057] 1. Extraction of rice Nipponbare RNA
[0058] Use the Biozol Reagent method to extract rice Nipponbare RNA: Weigh 0.1g Nipponbare fresh young ear tissue and mix it with 1ml Biozol Reagent, and let it stand at room temperature for 5 minutes; add 0.2ml chloroform for every 1ml Biozol Reagent, shake vigorously for 15s, and wait until the solution is fully emulsified, Let stand at room temperature for 5 minutes, centrifuge at 12000rmp, 4°C for 15 minutes; carefully take out the centrifuge tube from the centrifuge, absorb the supernatant and transfer it to another new centrifuge tube; add an equal volume of isopropanol to the supernatant, and centrifuge upside down After the tube is fully mixed, let it stand at room temperature for 10 minutes, centrifuge at 12000 rpm for 10 minutes at 4°C; discard the supernatant, a white precipitate may appear on the tube wall, add 0.5ml of 75% ethanol (prepared with sterilized DEPC wate...
Embodiment 2
[0073] Example 2 Constructing the recombinant expression vector DX2182-α-Amylase of rice α-amylase
[0074] See the build process figure 1 , Insert the amplified product of Example 1 into the DX2182 vector Mlu1 and Sac1 restriction sites.
[0075] Primers SEQ ID NO: 5 and SEQ ID NO: 6 amplify the PCR product and recover a product of about 1300 bp by electrophoresis on 1% agarose gel. The vector DX2182 was digested with Mlu1 and Sac1, and the linearized vector was recovered.
[0076] 2X ligation kit connects the abortion gene to DX2182, the 10ul system is as follows:
[0077] 2.5 μl of α-amylase PCR product (50 ng), 2.5 μl of enzyme-cut vector (100 ng), 5 μl of Ligation Mix, ligation procedure: 50°C for 60 minutes.
[0078] Transformation: Take 2 μl of the above ligation product and transform Escherichia coli competent cells by electroporation. Select positive clones for sequencing. Named DX2182-α-Amylase. The DX2182-α-Amylase vector contains a hygromycin resistance gene, ...
Embodiment 3
[0079] The acquisition of embodiment 3 transgenic rice plants
[0080] Agrobacterium EHA105 stored at -70°C was streaked on a plate containing Kan (50 μg / ml) + Rif (25 μg / ml) + streptomycin (50 μg / ml) and cultured at 28°C. Pick a single colony and inoculate it in 50ml of YEB liquid medium, shake it at 220rpm at 28°C for 12-16hr. Take 2ml of the bacterial liquid and transfer it to 100ml (containing antibiotics) YEB liquid medium, shake and cultivate at 28°C and 220rpm until OD600=0.5. Pre-cool on ice for 10 minutes, 5000rpm 10min (refrigerated centrifuge pre-cooled to 4°C). Wash twice with sterile deionized water (10ml each time), wash once with 10% glycerol and dissolve in 3ml 10% glycerin. Take 100 μl of competent cells and add 1 μl of the DX2182-α-Amylase plasmid obtained in Example 1, and transform by electroporation at 2.5KV. Culture at 28°C on a YEB culture plate containing kanamycin and rifampicin, select positive clones, and verify by PCR with DX2182-α-Amylase vector...
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