Recombinant human esoderma colyone adenovirus, and its preparing method and use
A technology of endostatin and adenovirus, which is applied in the field of genetic engineering, can solve the problems of complex and time-consuming protein purification process, large clinical application restrictions, and high cost, and achieve inhibition of growth and migration, inhibition of growth and metastasis, and increased administration time The effect of the interval
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Embodiment 1
[0060] Example 1 Preparation of human endostatin gene
[0061] In this example, the RT-PCR method was used to amplify the cDNA fragment of human endostatin from the total RNA of human liver.
[0062] Design and synthesize RT-PCR primers according to the human endostatin gene sequence, in order to directly insert the PCR product into the cloning vector—pUC18 (purchased from Invitrogen Company), the BamH I restriction site was designed in both the 5' primer and the 3' primer point, the primer sequences are as follows:
[0063] 5' Primer: 5'CGG GAT CCA CAG CCA CCG CGA CTT CCA GCC 3'
[0064] 3' Primer: 5'GCG GAT CCTACT TGG AGG CAG TCA TGA AGC 3'
[0065] RT-PCR conditions are as follows:
[0066] After the RT-PCR reaction mixture was denatured at 50°C for 30 minutes, the reaction was carried out according to the following conditions:
[0067] Reverse transcription reaction: denaturation at 94°C for 30 seconds; annealing at 50°C for 30 seconds; extension at 68°C for 1 minute. ...
Embodiment 2
[0070] Example 2 Preparation of human endostatin gene encoding human IL-2 gene signal peptide
[0071] With reference to the cDNA sequence of human IL-2 (GI: 28178860), PCR primers were designed and synthesized as follows:
[0072] 5’ Primer: 5’CGG ATC CAT GTA CAG GAT GCA ACT CCT GTC TTG CAT TGCACT AAG TCT TGC ACT TGT CAC GAA TTC GGC CCA CAG CCA CCG CGA CTTCCA GCC 3’
[0073] 3’ Primer: 5’GCG GAT CCT ACT TGG AGG CAG TCA TGA AGC 3’
[0074] Both the 5' primer and the 3' primer were designed with a BamH I restriction site, and were directly inserted into the shuttle vector pAdenovator-CMV5; the italic part of the 5' primer was the signal peptide sequence of human IL-2.
[0075] Then use pUC18-endo as a template to amplify the human endostatin DNA fragment containing the IL-2 gene signal peptide, and the PCR conditions are as follows:
[0076] Denaturation at 94°C for 30 seconds; annealing at 55°C for 30 seconds; extension at 72°C for 30 seconds. React for 30 cycles. This was...
Embodiment 3
[0078] Example 3 Construction and screening of recombinant adenovirus
[0079] 1. After constructing the cloned human endostatin gene containing human IL-2 signal peptide into the pAdenoVator-CMV5 shuttle vector, it was combined with the circular plasmid pAdenoVatorΔE1E3 (purchased from Qbiogene Corporation) containing the adenovirus genome (E1, E3 deletion) ) co-transform Escherichia coli BJ5183 (purchased from Qbiogene Company) by conventional electroporation method, and screen recombinant pAd-endo for identification. The results show that the recombinant pAd-endo (1) and pAd-endo (3) with two kinds of recombination sites have been screened respectively (see image 3 ). The homologous recombination site is located in the 3.0 kb cut out fragment of the left arm, and the recombination site is located in the 4.5 kb cut out fragment of the replicon.
[0080] 2. The linearized recombinant plasmid pAd-endo and liposome Lipofectamine (purchased from Invitrogen) were co-transfecte...
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