Preparation and application of enhanced serum avian adenovirus type 4 subunit vaccine
A technology of poultry adenovirus and vaccine composition, which is applied in the field of preparation of enhanced serum poultry adenovirus type 4 subunit vaccine, can solve the problems of uneven quality of inactivated virus, inappropriate attenuation method, expensive labor cost, etc.
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Embodiment 1
[0050] Embodiment 1, the construction of recombinant baculovirus
[0051] In the previous research of the present inventors, in order to reduce the cost of recombinant expression, they tried to express Fiber-2 in prokaryotic, using Escherichia coli. However, the expressed protein cannot be folded accurately. After selection of the expression system, it was determined to adopt the recombinant baculovirus expression system. In this embodiment, this expression method is provided.
[0052] 1. Obtaining the target gene
[0053] The construction and expression of Fiber-2 is based on the insect baculovirus expression system, and the target sequence encoding Fiber-2 (the gene sequence is optimized according to the insect cell expression system) is cloned into pFastBac TM 1 shuttle plasmid with 6 His-tags at its C-terminus, named pFastBac1-Fiber-2.
[0054] The amino acid sequence of the Fiber-2 protein is as follows (SEQ ID NO: 1):
[0055]
[0056]
[0057] 2. Construction...
Embodiment 2
[0066] Embodiment 2, the preparation of recombinant Fiber-2 protein
[0067] 1. Expression test of recombinant protein Fiber-2
[0068] The above-mentioned orifice plate prepared for the P3 generation virus was processed as follows: absorb 1ml of the culture supernatant from the well plate of the control group and the experimental group, centrifuge at 10000g for 15min at 4°C, and then take the centrifuged supernatant for sample preparation; Add 2ml of 1% TritonX-100 to the medium to lyse the cells. After the lysate is fully lysed, centrifuge the lysate at 10,000g for 15min at 4°C, take a sample from the centrifuged supernatant, suspend the precipitate with 2ml of PBS and take a sample, and detect the above sample by Western blot.
[0069] The result is as figure 2 , indicating that the target protein will not be secreted into the medium supernatant, and most of the target protein is located in the cell lysate supernatant in a soluble form after cell disruption.
[0070] 2. ...
Embodiment 3
[0077]Embodiment 3, expression and preparation of interleukin 2 and interferon gamma
[0078] 1. Obtaining the target gene
[0079] The sequences of chicken interleukin-2 (chIL-2) and chicken interferon gamma (chIFN-γ) were synthesized by Nanjing Jinsurui, and the target sequences encoding chIL-2 and chIFN-γ (gene sequences optimized by E. coli expression vector) were respectively cloned into pET28a (+), the recombinant plasmids pET28a-chIL-2 and pET28a-chIFN-γ were obtained respectively, and transformed into Escherichia coli BL21(DE3) for expression.
[0080] The amino acid sequence of chIL-2 is as follows (SEQ ID NO:2):
[0081]
[0082] The amino acid sequence of chIFN-γ is as follows (SEQ ID NO: 3):
[0083]
[0084] 2. Expression of recombinant chIL-2 and chIFN-γ
[0085] Inoculate the positive strain with 1% inoculum into the culture medium containing Kanna resistance, culture at 37°C until OD=0.6-0.8, add IPTG at a final concentration of 1mmol / L for induction, ...
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