A lily susceptibility fungal gene lrwrky-s1 and its application
A technology of lrwrky-s1 and fungus, applied in the fields of application, genetic engineering, plant gene improvement, etc., to achieve the effect of improving lily disease resistance and good application prospects
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Embodiment 1
[0024] Example 1 Cloning and Sequence Analysis of Laijiang Lily LRWRKY-S1 Gene
[0025] With the material of Lijiang lily blade, use Trizol TM Plus Rna Purification Kit (12183555, Invitrogen TM The total RNA is extracted according to the instruction step, and the residual micro DNA is removed by DNase I (18047019, InvitroGENTM), and the concentration of RNA is measured, and the concentration of RNA is measured.
[0026] Take the total RNA of the Lijiang Lancang Lijiang Lijiang Lani, synthesized the first chain cDNA according to the Primescript II First-Strand CDNASYNTHESIS KIT (6210A, TAKARA).
[0027] PCR amplification system: 2xFast PFU Master Max 10UL, forward primer (lrwrky-S1-1-F, 10 μm) 1 μL, reverse primer (lrwrky-S1-R, 10 μm) 1 μL, Template (cDNA) 1 μL, sterile DDH 2 O Adhesive to 20 μL.
[0028] The forward primers and reverse primers are:
[0029] LRWRKY-S1-F: 5'-gtccgaatatcatgggagag-3 '
[0030] LRWRKY-S1-R: 5'-ctacaacatttaaacgaagaaggcag-3 '
[0031] The PCR reaction pr...
Embodiment 2
[0035] Example 2GFP fusion expression vector construction and subcellular positioning analysis
[0036] (1) Construction of PTF101-P35S :: GFP-LRWRKY-S1 expression vector
[0037] According to the PTF101-GFP carrier sequence and the full length sequence (SEQ ID NO.1), the forward primer (lrwrky-S1-INF-F1) and the reverse primer (LRWRKY-S1-INF-R1) are designed. The positive cloned massage of the TA connected in Example 1 was a template, and the PCR amplification of the LRWRKY-S1 gene fragment was performed.
[0038] The primer sequence is as follows:
[0039] LRWRKY-S1-INF-F1:
[0040] 5'- ATGGACGGAGGCTGGGGAGAG-3 '
[0041] LRWRKY-S1-INF-R1:
[0042] 5 ' TTAAACGAGAGGCAGAGGCATCG-3 '
[0043] The underscore is a sequence of in-fusion cloned carrier joints, and the bold sequence is the enzyme sink.
[0044] PCR reaction system: High-fidelity expansion enzyme PrimeStarHS (R010 A, TAKARA) 0.5μL, 5XPrimesTarbuffer (Mg 2+ Plus) 10 μL, forward primer (10 μm) 1 μL, reverse primer (10 μm) ...
Embodiment 3
[0054] Example 3 LrWrky-S1 gene overduced vector constructs and genetic transformation of Arabidopsis
[0055] (1) Construction of PBI121-P35S :: lrwrky-S1 overexpression carrier
[0056] Depending on the PBI121 vector sequence and the Lrwrky-S1 gene sequence (SEQ ID NO.1), the primer lrwrky-S1-INF2 and LRWRKY-S1-INF-R2 are designed to introduce seamless cloned (in-fusion) carrier joint sequences. And the enzyme sequence sequence. The positive cloned massage of TA connection in Example 1 was a template, and the specific amplification of the LRWRKY-S1 gene fragment was performed.
[0057] The primer sequence is as follows:
[0058] LRWRKY-S1-INF-F2:
[0059] 5'- GGACTCTAGAGGATCC Gtccgaatatcatgggacgag-3 '
[0060]LRWRKY-S1-INF-R2:
[0061] 5'- GatcggGGAAATTCGAGCTC CTacaactttaaacgaagaaggcAg-3 '
[0062] Among them, the underscore is a sequence of the in-fusion cloned carrier joint.
[0063] The PCR reaction system is: high-fidelity expansion enzyme primestar HS (R010A, TAKARA) 0.5 μL...
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