Method for transient expression of wheat leaf single cell based on efficient gene gun conversion and application of method
A biolistic transformation, single-cell technology, applied in biochemical equipment and methods, applications, botanical equipment and methods, etc., can solve the problems of low efficiency, lack of biolistic transformation parameters, and unstable expression efficiency of reporter gene selection. to increase resistance
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Embodiment 1
[0026] Example 1 Establishment of High Gene Gun Transformation Wheat Detached Leaf System
[0027] 1.1 Materials and methods
[0028] Expression vectors with different reporter genes: reporter gene anthocyanin synthesis regulatory gene C1-Lc expression vector pBecks400.Red (McCormac AC, Wu HX, Bao MZ, Wang YB, Xu RJ, Elliott MC, Chen DF. The use of visual marker genes as cell-specific reporters of Agrobacterium-mediated T-DNA delivery towheat (Triticum aes tivum L.) and barley (Hordeum vulgare L.). Euphytica, 1998, 99 (1): 17-25.). The expression vector psGFP of the green fluorescent protein gene GFP (Takashi Tamura, KojiroHara, Yube Yamaguchi, Nozomu Koizumi and Hiroshi Sano. Osmotic stress tolerance of transgenic tobacco expressing a gene encoding a membrane-located receptor-likeprotein from tobacco plants. PlantPhysiol, 2003, 131: 454-462.). The expression vector pAHC25 of β-1,3-glucuronidase gene GUS (Christensen A H, Quail P H, Ubiquitin promoter-based vectors for high-...
Embodiment 2
[0045] Example 2 Construction of overexpression vector of SGT1 gene Hv-SGT1
[0046] The SGT1 gene cDNA (SEQ ID NO.1) was used as a template, and the primer pair SGT1ATG-BamHIF (TT GGATCC TCGACGCAGACATGG, SEQ ID NO.2) and SGT1-TGA-KpnI-R (GC GGTACC TCATTAATACTCCCAC, SEQ ID NO.3) was amplified by PCR, and the amplified fragment was recovered. The amplified product was double digested with BamHI and KpnI, and the digested product was inserted into the vector pBI220 (Jefferson RA, Kavanagh TA, Bevan MW. GUS fusions: beta-glucuronidase as a sensitive and versatile gene fusion marker in higher plants.EMBO J.1987,6:3901-3907.)), put Hv-SGT1 at the multiple cloning site behind the 35S promoter. Thus, the target gene Hv-SGT1 was cloned to the downstream of the strong promoter 35S to obtain the expression vector pBI220:Hv-SGT1 ( Figure 4 ). It was verified by sequencing that the vector was constructed successfully.
Embodiment 3
[0047] Example 3 Transition of Hv-SGT1 gene into susceptible wheat leaves by transient expression method to study its interaction with wheat powdery mildew
[0048] 3.1 Materials and methods
[0049] The expression vector of the target gene Hv-SGT1 and the GUS expression vector pAHC25 (Christensen A H, Quail P H. Ubiquitin promoter-based vectors for high-level expression of selectable and / orscreenable marker genes in monocotyledonous plants. Transgenic Research, 1996, 5: 213-218.) Plasmid DNA was mixed and coated with tungsten powder (the molar ratio of the target gene carrier to the GUS gene carrier concentration was 2:1), and the wheat leaves were bombarded with a gene gun for co-transformation.
[0050] The powdery mildew spores were inoculated 4 hours after the leaves were bombarded. Inoculation method: roll a plastic sheet into a drum shape and place it on a porcelain plate, and evenly shake off fresh powdery mildew spores from above. The inoculation density should be hi...
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