Preparation method of anti-tobacco potato Y virus vaccine
A virus vaccine, potato technology, applied in the directions of botanical equipment and methods, disinfectants, chemicals for biological control, etc., can solve problems such as environmental biosafety hazards, pesticide residues, PVY virus prevention and control, etc. Reduced duplication, easy and fast effects
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Embodiment 1
[0036] 1. Preparation of c-DNA template
[0037] RNeasyPlantMinikit from QIAGEN was used to extract RNA from tobacco LJ925 fresh leaves, and c-DNA was synthesized by reverse transcription using TaKaRaRNAPCRKitVer.3.0 kit as a template. For specific operations, refer to the instructions of the kit.
[0038] 2. Amplification of eIF4E-6 gene
[0039] Add 2.5 μL of 10×PCR buffer (Buffer), 0.5 μL of 10 pmol / μL PVX-BF and PVX-MR primers, 0.5 μL of 2.5 U / μL pfuDNA polymerase, and dNTPs (each dNTP (10 mM) 1 μL, c-DNA template 2 μL, ultrapure water 18 μL. The PCR amplification program is shown in Table 1:
[0040] Table 1: PCR reaction conditions
[0041]
[0042] 3. Construction of pMD18-T-eIF4E-6 plasmid
[0043] The amplified product of 25 μL IF4E-6 gene was separated by 1.5% agarose electrophoresis, and the target fragment was recovered by cutting the gel in the ultraviolet analyzer; the target fragment was recovered and purified, cloned into pMD18-TSimpleVector (Dalian Bao...
Embodiment 2
[0048] Example 2: Amplification of Vaccines Against Tobacco Potato Virus Y
[0049] Take 50 μL of the anti-tobacco potato virus Y vaccine prepared in Example 1, respectively, and add it to 50 mL of YEP liquid medium (containing 50 mg / mL of kanamycin, take 10 mL after each bacterial solution is shaken), shake the bacteria at 28°C until logarithmic growth During the period, after centrifugation at 8000rpm for 5 minutes, the cells were osmotic medium buffer (10mmol / LMES, 10mmol / LMgCl 2 , 100 μmol / L acetosyringone) was suspended, the concentration of the bacterial solution was adjusted to OD600 = 1.5, and stood at 28°C for 3 hours for use.
Embodiment 3
[0050] Embodiment 3: the inoculation method of tobacco potato virus Y and the use of anti-tobacco potato virus Y vaccine
[0051] The anti-tobacco potato virus Y vaccine suspension in embodiment 3 is diluted 50 times, before tobacco seedlings are transplanted, spray tobacco kind LJ911 (sensitivity to PVY) seedling (5 true leaf stage) twice, spray interval 5 days, as test Group. At the same time, no inoculation and inoculation of PVX empty vector controls were set. Nine pots were planted in each treatment, and the PVY virus was inoculated by rubbing when the tobacco seedlings grew to the group tree stage (12 true leaf stage). The inoculation method is: take the fresh PVY diseased leaves bred by LJ912 (anti-TMV) tobacco seedlings, put them into a mortar and mash them, add phosphate buffer solution equal to the weight of the diseased leaves twice as much (0.5 g of sodium sulfite, 5 g of potassium dihydrogen phosphate , dissolved in 500ml of water) ground and smashed into a past...
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