Fusion protein with protein transduction structure field TAT-PTD and application thereof
A fusion protein and sequence technology, applied in the field of genetic engineering, can solve problems such as reducing application value, and achieve the effects of improving antioxidant capacity, high-efficiency antioxidant drugs, and high application value
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Embodiment 1
[0037] Example 1 Expression of HIV-TAT-SOD-1 fusion protein in Escherichia coli
[0038] 1. Construction of recombinant TAT-SOD-1 fusion protein gene
[0039] 1) Amplify the SOD-1 gene with RT-pCR
[0040]The total RNA of the liver was extracted with TRIzol, and PCR amplification was performed with primers P1 and P2 (synthesized by Shanghai Sangon Bioengineering Technology Service Co., Ltd.), P1: 5'-CTCGAGGCGACGAAGGCCGTGTGCGTG-3' (SEQ ID NO: 8), and P2 : 5'-GGATCCTTATTGGGCGATCCCAATTAC-3' (eg, SEQ ID NO: 9). The PCR amplification reaction was carried out in a 50 microliter system, and the conditions were denaturation at 94°C for 5 min, 30 s at 94°C, 1 min at 54°C, Imim at 72°C, 30 cycles, and 5 min at 72°C. After the reaction was completed, the entire PCR reaction solution was added to 1% agarose for electrophoresis, and a 500 bp band was recovered by tapping the gel (the recovery reaction used Saibaisheng Company's recovery kit). The recovered product was connected to the T...
Embodiment 2
[0047] Example 2 Detection of TAT-SOD-1 fusion protein antioxidant effect in Hela cells
[0048] In the culture medium of Hela cells cultured in vitro, 0.1-2 μl of purified TAT-SOD-1 protein was added to the test group, and 0.1-2 μl of purified SOD-1 protein was added to the control group, and the medium was replaced two hours later. Methyl viologen (Paraquat) was added at a final concentration of 5 mM to generate superoxide anion. Cell viability was measured 12 hours later by colorimetry. Colorimetric method adopts MTT (3-(4,5-dimethylthiazol-2-yl)-2,5-dip-henyltetrazolium bromide, Sigma) to measure. The results show that the cell survival rate of the test group adding TAT-SOD-1 protein is obvious increased, confirming that the TAT-SOD-1 fusion protein has entered the cell and has obvious antioxidant capacity ( Figure 4 shown).
Embodiment 3
[0049] Example 3 Detection of TAT-SOD-1 fusion protein's antioxidant effect in keratinocytes
[0050] In the culture medium of primary cultured mouse skin keratinocytes, add 0.5-2 μl purified TAT-SOD-1 protein to the test group, add 0.5-2 μl purified SOD-1 protein to the control group, and use trypsin after two hours Digest the cells with EDTA mixture, centrifuge to remove the supernatant, add phosphate buffer solution, place on a vortex mixer for vigorous mixing, and centrifuge again, the supernatant is the SOD-1 extract. Adding NaOH to dimethyl sulfoxide can generate oxygen free radicals under aerobic conditions. At this time, adding chemiluminescent agent luminol will emit cold chemiluminescence. Add 0.1ml of SOD-1 extract to the luminescence solution, and calculate the luminescence inhibition rate. The higher the inhibition rate, the higher the concentration of SOD-1. The results showed that the SOD-1 concentration of the test group was significantly higher than that of ...
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Abstract
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