Method for constructing recombinant bombyx mori cypovirus for expressing red fluorescence protein
A technology of red fluorescent protein and plastid polyhedrosis, which is applied in the field of virus genetic engineering and can solve the problems of constructing recombinant silkworm plastid polyhedrosis virus in vitro, expressing foreign genes, constructing recombination, etc.
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Embodiment 1
[0077] Example 1: Construction and performance testing of recombinant silkworm plasmopolyhedrosis virus expressing red fluorescent protein.
[0078] 1. Virus construction:
[0079] (1) Extract the silkworm plasmopolyhedrosis virus genome:
[0080] Collect the midgut tissue of silkworm diseased polyhedrosis silkworm, add double distilled water according to the ratio of 1g midgut tissue: 10mL double distilled water (self-made, Chengdu Ultrapure Technology Co., Ltd., UPT-Ⅲ-5T ultrapure water machine) , after homogenization, it was filtered with gauze, and the filtrate was centrifuged at a differential speed by a CF15D2 centrifuge (KuBoTa Company, Japan) to obtain pure silkworm polyhedron; the pure silkworm polyhedron was added with water (self-made, Chengdu Chaopure Technology Co., Ltd. company, UPT-Ⅲ-5T ultrapure water machine) suspension, adjust the concentration to contain at least 10 per mL of water 8 For each polyhedron, take 0.5 mL of the polyhedron suspension, add an equ...
Embodiment 2
[0145] Example 2: Construction of recombinant silkworm plasmopolyhedrosis virus expressing red fluorescent protein.
[0146] (1) Extracting the silkworm plasmopolyhedrosis virus genome: the same as step (1) in Example 1.
[0147] (2) Design and synthesis of primers: same as step (2) in Example 1.
[0148] (3) Reverse transcription to obtain cDNA of S1 to S10 fragments: same as step (3) in Example 1.
[0149] (4) PCR amplification of the full-length cDNA of S1 to S10 fragments: same as step (4) in Example 1.
[0150] (5) Construction of recombinant plasmid: same as step (5) in Example 1.
[0151] (6) Preparation of RNA from S1 to S9 fragments: Take the PCR-amplified full-length cDNA from S1 to S9 fragments in step 4 as templates, use mMESSAGE mMACHINE T7 Ultra Kit (Ambion Company) to transcribe in vitro according to the product instructions, and in vitro transcribe products The DNA template was removed by RNase-free DNase digestion, the in vitro transcribed RNA was precipita...
Embodiment 3
[0154] Example 3: Construction of recombinant silkworm plasmopolyhedrosis virus expressing red fluorescent protein.
[0155] (1) Extracting the silkworm plasmopolyhedrosis virus genome: the same as step (1) in Example 1.
[0156] (2) Design and synthesis of primers: same as step (2) in Example 1.
[0157] (3) Reverse transcription to obtain cDNA of S1 to S10 fragments: same as step (3) in Example 1.
[0158] (4) PCR amplification of the full-length cDNA of S1 to S10 fragments: same as step (4) in Example 1.
[0159] (5) Construction of recombinant plasmid: same as step (5) in Example 1.
[0160] (6) Preparation of RNA fragments from S1 to S9: use the recombinant plasmids pT-S1 to pT-S9 obtained in step (5) as templates, and use the 9 pairs of primers synthesized in step (2) for PCR amplification, that is, recombinant Plasmid pT-S1 uses primers to amplify PS1F / PS1R, recombinant plasmid pT-S2 uses primers to amplify PS2F / PS2R, and so on. Then use each amplified product as an...
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