Mythimna separata pupa ovary cell line capable of highly yielding baculovirus, and preparation method and applications thereof
A technology of baculovirus and ovarian cells, applied in the biological field, can solve the problem of cell lines without O. orientalis ovaries
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Embodiment 1
[0050] The establishment of embodiment 1 oriental armyworm pupal ovary cell line
[0051] The pupae of Oriental Armyworm at the final stage (raised in the Key Laboratory of Comprehensive Management of Agricultural Pests and Rodents, Institute of Zoology, Chinese Academy of Sciences) was immersed in an ethanol solution with a volume fraction of 75% for 10 minutes to carry out surface disinfection. The insect was dissected to remove the ovarian tissue, which was kept as intact as possible during the manipulation. Wash the tissue 2-3 times with physiological saline, then use cell culture medium (Insect-XPRESS, containing 100U / mL penicillin, 100U / mL streptomycin and 10% (v / v) fetal bovine serum, pH = 6.2) Wash 1-2 times, put into a 25cm 2 Cell culture flasks were placed in a dark cell culture incubator at 27°C for 24 hours. Then add 3mL of the above-mentioned cell culture medium, and culture under the same conditions. Note that the key to the successful establishment of cell ...
Embodiment 2I
[0052] Example 2. Observation and determination of biological characteristics of IOZCAS-Myse-1
[0053] (1) Morphological characteristics: Observed under a microscope, the cell line is usually suspended in the culture medium, and there are two types of cell shapes: round and spindle ( figure 2 ). In IOZCAS-Myse-1, round cells accounted for 77.09%, with an average diameter of 10.23±0.296 (mean±SD) μm; spindle cells accounted for 22.91%, with a length of 16.77±0.604 μm and a width of 9.33±0.226 μm.
[0054] (2) Cell growth: at 27°C, the 10th generation of the cell line was in TNM-FH medium containing 10% fetal bovine serum, 100U / mL penicillin, and 100U / mL streptomycin, and the cell population doubling time was 67.95 hours ( image 3 ). The highest cell density can reach about 3.61×10 6 cells / mL.
[0055] (3) DAF-PCR identification: the cell line IOZCAS-Myse-1 is indeed derived from oriental armyworm, not the pollution of other cell lines ( Figure 4 ). The DNA extracte...
Embodiment 3I
[0057] Example 3. Determination of IOZCAS-Myse-1 Sensitivity to Baculovirus
[0058] IOZCAS-Myse-1 against Oriental armyworm nuclear polyhedrosis virus (MyseNPV), Oriental armyworm granulosa virus (MyseGV), Autographa californica nuclear polyhedrosis virus (AcMNPV), cabbage armyworm nuclear polyhedrosis virus (MabrNPV), Spodoptera celery nucleopolyhedrosis virus (AnfaNPV) sensitive: inoculate IOZCAS-Myse-1 with AcMNPV, MabrNPV, AnfaNPV budding virion BV at a concentration of 0.001 larvae equivalent / ml, and after culturing for 10 days, the cells can be harvested and viral polyhedrons, under an inverted phase-contrast microscope, typical cytopathological features can be observed, that is, the nucleus is enlarged and contains a large number of polyhedron particles ( Figure 5-Figure 9 ). Each cell can produce 5-20 polyhedrons, comparable to commercial Sf21.
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