Barley α-amylase and its coding gene and application
A technology of amylase and barley, applied in application, genetic engineering, plant genetic improvement, etc., can solve the problems of insufficient starch accumulation, lower pollen energy metabolism level, abortion, etc., and achieve the elimination of artificial detasseling steps, gene expression Precise regulation to control the effect of transgene spread
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Embodiment 1
[0050] Example 1 Barley α-amylase acquisition
[0051] 1. Extraction of barley RNA
[0052] Use the Biozol Reagent method to extract barley RNA: Weigh 0.1g fresh young ear tissue of barley, add 1ml Biozol Reagent to mix, let stand at room temperature for 5min; Let stand at room temperature for 5 minutes, centrifuge at 12,000 rpm, 4°C for 15 minutes; carefully remove 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 turn the centrifuge tube upside down After fully mixing, let 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 (made with RNase-free water) to wash, invert and mix well, Centrifuge at 10,000rpm at 4°C for 5min; repeat once, dry at low temperature to evaporate ethanol; add 50μl of RNase-free water to dissolve th...
Embodiment 2
[0070] Example 2 Construction of pollen abortion gene plant binary expression vector DX2182-HVAA1
[0071] See the build process figure 1, the amplified product of Example 1, i.e. primer SEQ ID NO: 7-8 amplified PCR product 1% agarose gel electrophoresis reclaims about 1300bp product, inserts DX2182 (disclosed in Chinese patent CN106434673A, invention name: a kind of plant Anther-specific promoter PCHF15 and its application) in the linear restriction vector of MluI and SacI. The DX2182 vector already contains the pG47-optimized promoter and terminator, and is located on both sides of the MluI and SacI restriction sites, so MluI and SacI digest the vector DX2182, recover the linear restriction vector, and amplify as in Example 1 The PCR products were connected in a certain ratio, and finally a binary vector containing the pollen-specific expression cassette of HVAA1 was constructed.
[0072] 2X ligation kit ligates abortion gene to DX2182, 10μl system is as follows:
[0073]...
Embodiment 3
[0078] Embodiment 3 HVAA1 transgenic rice creation
[0079] Agrobacterium EHA105 stored at -70°C was streaked on a YEP plate containing Rif (25 μg / ml) + streptomycin (50 μg / ml), and cultured at 28°C. Pick a single colony and inoculate it in 50ml of YEP liquid medium containing the above antibiotics, and shake at 220rpm at 28°C for 12-16h. Take 2ml of the bacterial liquid and transfer it to 100ml (containing the above antibiotics) YEP liquid medium, shake and culture at 28°C and 220rpm until OD 600 = 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% glycerol. Take 100 μl of competent cells and add 1 μl of the DX2182-HVAA1 plasmid obtained in Example 2, and transform by electroporation at 2.5KV. Culture on a YEP culture plate containing kanamycin, rifampicin and streptomycin, select positive clones, and verify by PCR with...
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