Pseudobagrus-fulvidraco-richardson-origin transgenic vectors constructed with elements of pseudobagrus fulvidraco richardson [beta]-actin promoter and growth hormone gene, and application thereof
A technology of actin and growth hormone, applied in the field of genetic engineering
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Embodiment 1
[0033] The cloning of embodiment 1 yellow catfish β-actin promoter
[0034] 1. Primer design: compare the β-actin promoter sequences of fish such as stingcatfish and tilapia published on GenBank, and design an upstream primer P1 in the homologous conserved region, whose position is near the CAAT box . Afterwards, the sequences of the exons were compared, and a downstream primer P2 was designed in the conserved region of exon 3 of β-actin, and the β-actin promoter of the yellow catfish was cloned through this pair of primers .
[0035] P1: 5'-GTGWGTGACGCMGGACCAATC-3' (W=A+T, M=T+C)
[0036] P2: 5'-CCATXTCXTCCCAGTTGGTYACAAT-3' (X=A+G, Y=G+C)
[0037] 2. Genomic DNA extraction: Take the adult yellow catfish pituitary gland and cut it into 1.5ml sterilized centrifuge tube, add a certain amount (m / v=1 / 10, preferably 10ml per g tissue) of digestion buffer (10mM Tris-Cl, pH 8.0, 1% SDS, 100μg / ml proteinase K) and placed in a water bath at 37°C for 5 hours with slight shaking from...
Embodiment 2
[0052] Example 2 Identification of the activity of the yellow catfish β-actin promoter
[0053] 1. The connection of the promoter and the yellow fluorescent protein YFP carrier: in order to prove the activity of the yellow catfish β-actin promoter, the plasmid (pActin proexon-T) constructed in Example 1 is extracted, the promoter is separated, and inserted into In the yellow fluorescent protein carrier, see if it can drive the expression of fluorescent protein. In the pActin proexon-T plasmid, the pMD18-T vector has its own BamHI site; and at the end of the inserted yellow catfish β-actin promoter, it is the beginning of encoding β-actin At the codon (ATG), it has an Nco I site. Double digestion with BamH I and Nco I can obtain a complete promoter fragment without actin sequence. In addition, the pCYP26A1-2.5keYFP plasmid was digested with BamH I and Nco I to obtain the yellow fluorescent protein vector. The digestion system is: 10×buffer 2.5μl, plasmid 4μl, BamH I and Nco ...
Embodiment 3
[0055] Cloning of the open reading frame (ORF) of embodiment 3 yellow catfish growth hormone gene
[0056] 1. Primer design: Design a pair of degenerate primers (P3 and P4) in the homologous conserved region with reference to the growth hormone gene cDNA sequences of fish sting catfish (AF147792), giant catfish (L27835) and channel catfish (AF267989) published in GenBank ) amplifies the open reading frame (ORF) sequence of the gene.
[0057] P3: 5'ATGGCTXGAGYYTTMGTG 3' (X=A,C; Y=G,T; M=G,A);
[0058] P4: 5' CTACAGPGTGCAGTTGGAATC 3' (P = G, A).
[0059] 2. Reverse transcription reaction: Take about 1 gram of brain tissue of yellow catfish and extract total RNA. For specific steps, refer to the instructions of Qiagen RNA extraction kit. The obtained total RNA was detected by 0.8% agarose gel electrophoresis and stored at -20°C for future use. The reverse transcription of RNA was carried out according to the instructions of Promega's M-MLV reverse transcriptase, and the first-...
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