Artemisia carvifolia WRKY type transcription factor coding sequence and application
A technology for transcription factors and coding sequences, which is applied to the coding sequences and application fields of Qinghao WRKY transcription factors, can solve the problems of large-scale commercial production limitations, low feasibility and high cost of artemisinin
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Embodiment 1
[0034] Embodiment 1, cloning of Artemisia annua AaGSW1 gene
[0035] 1. Extraction of Total RNA from Artemisia annua Genome
[0036] Take the leaf tissue of Artemisia annua, grind it in liquid nitrogen, add it to a 1.5mL Eppendorf (EP) centrifuge tube filled with lysate, shake it fully, and extract total RNA according to the instructions of the TIANGEN kit. The quality of total RNA was identified by formaldehyde denaturing gel electrophoresis, and then the RNA content was determined on a spectrophotometer.
[0037] 2. Cloning of Artemisia annua AaGSW1 gene
[0038] Using the extracted total RNA as a template, cDNA was synthesized under the action of PowerScript reverse transcriptase; gene-specific primers (SEQ ID NO:3 and SEQ ID NO:4) were designed according to the sequence of the AaGSW1 gene, and the total cDNA was obtained by PCR. The AaGSW1 gene was amplified and sequenced.
[0039] Through the above steps, the full-length coding sequence (SEQ ID NO: 1) of the transcri...
Embodiment 2
[0040] Example 2, Construction of plant binary interference expression vector containing AaGSW1 gene
[0041] In order to study the effect of AaGSW1 gene on the development of secretory glandular hairs in Artemisia annua, an overexpression vector PHB-AaGSW1 was constructed to overexpress AaGSW1. In order to facilitate the construction of the expression vector, the restriction site of BamH1 was introduced into the forward primer, and the restriction site of Sac1 was introduced into the reverse primer. The primers are shown in Table 1;
[0042] Table 1 PCR primers constructed by PHB-AaGSW1 vector
[0043]
[0044] In this example, the Artemisia annua AaGSW1 gene is operably linked to the expression control sequence, and the vector can be used to regulate the content of artemisinin in Artemisia annua through a developmental regulation strategy.
Embodiment 3
[0045] Example 3. Agrobacterium tumefaciens-mediated AaGSW1 interference vector genetically transforms Artemisia annua to obtain transgenic Artemisia annua plants
[0046] 1. Acquisition of Agrobacterium tumefaciens Engineering Bacteria Containing AaGSW1 Overexpression Vector
[0047] The plant binary overexpression vector containing AaGSW1 in Example 2 was transformed into Agrobacterium tumefaciens (such as EHA105, which is a publicly available biological material in the market, which can be purchased from CAMBIA Company in Australia, and the strain number is Gambar 1 ), and validated by PCR. The results showed that the plant binary interference expression vector containing AaGSW1 had been successfully constructed into the Agrobacterium tumefaciens strain.
[0048] 2. Agrobacterium tumefaciens mediated AaGSW1 gene transformation of Artemisia annua
[0049] 2.1. Preculture of explants
[0050] Artemisia annua seeds were soaked in 75% ethanol for 1 min, then soaked in 20% Na...
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