Pig myostatin gene promoter and its applications
A molecular and DNA molecular technology, applied in the field of porcine myostatin gene promoter and its application, to achieve the effect of valuable gene resources
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Embodiment 1
[0037] Embodiment 1, cloning and verification of porcine myostatin gene promoter
[0038] 1. Experimental materials
[0039] Table 1 Experimental materials
[0040]
[0041]
[0042] 2. Instruments and equipment
[0043] Table 2 Instruments and equipment
[0044]
[0045]
[0046] 3. Experimental method
[0047] 1) Pig genomic DNA extraction
[0048] Take 0.1 g of isolated pig ear muscle tissue samples from piglets, wash them, and cut them into pieces.
[0049] Add 300μl DNA extraction buffer (Tris-Hcl 10mM, EDTA 10mM, SDS 2%, NaCl 300mM, pH8.0), 8μl proteinase K (10mg / ml) to each sample, and digest at 55°C for 6 hours.
[0050] Extract twice with phenol, centrifuge at 10,000rpm for 10 minutes to get the supernatant, and remove the protein and phenol in the lower layer.
[0051] Extract again with chloroform / isoamyl alcohol and phenol, and centrifuge at 10,000 rpm for 10 minutes to get the supernatant.
[0052] Add 30 μl 3M NaAC and 600 μl absolute ethanol t...
Embodiment 2
[0074] The plasmid identified as positive by PCR and enzyme digestion was sent for sequencing. The result was that the plasmid was obtained by inserting sequence 1 in the sequence table between the MluI and BglII restriction sites of pGL3-bai sc, and the plasmid was named pGL3-MSTN. Embodiment 2, functional identification of porcine myostatin gene promoter
[0075] 1. Detection of transcriptional activity of porcine myostatin gene promoter
[0076] A. Preparation and verification of mutation vector of porcine myostatin gene promoter reporter system
[0077] 1. Experimental materials
[0078] Table 5 Experimental materials
[0079]
[0080]
[0081] 2. Instruments and equipment
[0082] Table 6 Instruments and equipment
[0083]
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