A Novel Salt Tolerance Gene zmubp in Zoysia rugosa and Its Expression Vector and Application
A technology of Zoysia grove and salt tolerance gene, applied in the field of molecular biology, can solve the problem that salt tolerance function has not been reported, and achieve the effect of improving salt tolerance
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Embodiment 1
[0028] Example 1 Zoysia folium BYZGR clone of ( figure 1 ).
[0029] Choose Zoysia ditch leaves ( Zoysia matrella ) as materials, select healthy turf pieces, place them in a cup filled with quartz sand, and culture them in 1 / 2 Hongland nutrient solution for 20 days, then transfer them to 1 / 2 Hongland nutrient solution containing 300mM NaCl for 7 days, take 0.1g of young leaves, according to the instructions of the Trizol RNA extraction kit (TaKaRa), extract the total RNA of the leaves, take 1 µg of total RNA according to the M-MLV reverse transcription kit (TaKaRa), reverse transcribe into cDNA, and digest the cDNA product with RNase , design primers to amplify BYZGR ;
[0030] Upstream primer ZmUBP-F: 5′-ATGCCAAAGGACAGGAGC-3′ (SEQ ID NO.2);
[0031] Downstream primer ZmUBP-R: 5′-TTGTGCAGGGTCACCGTC-3′ (SEQ ID NO.3).
[0032] Using the extracted leaf cDNA as a template, carry out PCR reaction, 20 μL reaction system: 2×LA RCR Mix 10 μL, ZmUBP-F, ZmUBP-R primers 1.0 μL ea...
Embodiment 2
[0033] Example 2. Plant expression vector pEarleyGate103- BYZGR build ( figure 1 , figure 2 ).
[0034] Design primers for PCR reaction in target gene BYZGR Respectively introduce enzyme cutting sites upstream and downstream Bam H I and not Ⅰ. The PCR product was connected to the pMD19-T Simple vector, transformed into TOP10 competent cells, and the positive plasmid was extracted. Bam H I and not Ⅰ double digested BYZGR fragment with Bam H I and not Ⅰ The double-digested pENTR1A connection was transformed into Escherichia coli, and the extracted positive plasmid was Nsi ⅠAfter linearization by single enzyme digestion, carry out LR recombination reaction (Invitrogen) with pEarleyGate103 vector plasmid, transform, extract positive plasmid, electrophoresis detection and sequencing verification as SEQ ID NO.1;
[0035] Upstream primer ZmUBP-BamHI-F: 5′-GGATCCGGATGCCAAAGGACAGGAGC-3′ (SEQ ID NO.4);
[0036]Downstream primer ZmUBP-NotI-R: 5'-GCGGCCGCGATTGTGCAGGGTC...
Embodiment 3
[0040] Example 3 Plant expression vector pEarleyGate103- BYZGR Genetic transformation of Arabidopsis thaliana and identification of its salt tolerance ( image 3 , Figure 4 ).
[0041] ①Competent preparation of Agrobacterium strain EHA105 and transformation by freeze-thaw method: Pick a single colony of EHA105 from a YEB (50 µg / mL rifampicin) plate and inoculate it in 50 mL of YEB liquid medium containing 50 µg / mL rifampicin medium, 220 rpm, 28°C to OD value 0.6, then ice-bathed the bacteria solution for 30 min, centrifuged to collect the bacteria, suspended in 2 mL of pre-cooled 100mM CaCl 2 (20% glycerol) solution, aliquot 200 µL / tube for use. Take 5 µL of pEarleyGate103- BYZGR Add 100 µL of competent cells to the vector plasmid, ice bath for 30 min, freeze in liquid nitrogen for 5 min, 37°C for 5 min, add 800 µL of YEB liquid medium, pre-culture for 3 h at 28°C and 200 rpm, and smear the bacterial solution on YEB ( 50 µg / mL rifampicin + 50 µg / mL kanamycin) solid mediu...
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