A kind of Pseudomonas syringae bacteriophage and its composition, test kit and application
A technology of pseudomonas and phage, applied in the field of phage, can solve the problems affecting the titer of phage, and achieve good biological control effect, high specificity and lysis, and wide host range
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Embodiment 1
[0059] Example 1: Isolation, preparation and purification of Pseudomonas syringae pseudomonas kiwifruit pathogenic variant phage PSA-P1
[0060] In the present invention, the source sample of Pseudomonas syringae kiwifruit pathogenic variant bacteriophage PSA-P1 is collected from the sewage of Zhongcai farmer's market in Jiangning District, Nanjing City, Jiangsu Province, filtered by double-layer filter paper, centrifuged at low speed and normal temperature, and then filtered with a 0.22 μm filter membrane supernatant.
[0061] Phage Isolation:
[0062] (1) Take 10 mL of the filtered supernatant, add it to 10 mL of 2 times TSB liquid medium, and add 1 mL of the bacteriophage host Psa-1 logarithmic phase bacterial liquid at the same time, and place it at 28°C for overnight cultivation;
[0063] (2) Take the above culture, centrifuge at 8000rpm for 10min, filter the supernatant with a 0.22μm filter membrane, and set aside;
[0064] (3) Take 0.5 mL of the bacteriophage host bac...
Embodiment 2
[0073] Example 2: Electron microscope observation of Pseudomonas syringae pv. Absorb excess liquid from the side, add 1 drop of 2% phosphotungstic acid to the copper grid, dye for 10 minutes, use filter paper to absorb the dye solution from the side, and observe with electron microscope after drying.
[0074] The result is as figure 2 As shown, observing the morphology of Pseudomonas syringae pv. The length of the tail is 15-20nm, and the diameter of the tail is 6-10nm. Pseudomonas syringae pv. kiwifruit bacteriophage PSA-P1 belongs to the family Autographiviridae.
Embodiment 3
[0075] Example 3: Preparation of Pseudomonas syringae pv. kiwifruit phage PSA-P1 particles and genome extraction and sequencing
[0076] (1) Take 100 mL of the purified phage solution prepared in Example 1, add 20 μL of DNaseI and 20 μL of RNaseA at a concentration of 5 mg / mL in turn, incubate at 37° C. for 60 minutes, add 5.84 g of NaCl, and place it in an ice bath for 1 hour after dissolving;
[0077](2) Centrifuge at 11,000rpm for 10min at 4°C, transfer the centrifuged supernatant to a new centrifuge tube, add solid PEG8000 to make the final concentration 10% (w / v), and after the PEG8000 is completely dissolved, Ice bath for 1h;
[0078] (3) Centrifuge at 11,000 rpm for 20 minutes at 4°C, add 1 mL of SM solution to resuspend the precipitate, and obtain a phage particle concentrate, which is stored at 4°C until use.
[0079] Phage nucleic acid was extracted and sequenced using λ phage genomic DNA kit. After nucleotide sequencing, the Pseudomonas syringae pv. Actinidiaephag...
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