#TITLE_ALTERNATIVE#
Auto-inducible promoter usage is one of efficiency strategy for recombinant protein production <br /> <br /> <br /> without inducer. pMCD_sod plasmid is a gadA auto-inducible promoter based expression vector <br /> <br /> <br /> developed in Laboratory of Phar...
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| Format: | Final Project |
| Language: | Indonesia |
| Online Access: | https://digilib.itb.ac.id/gdl/view/31587 |
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| Institution: | Institut Teknologi Bandung |
| Language: | Indonesia |
| Summary: | Auto-inducible promoter usage is one of efficiency strategy for recombinant protein production <br />
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without inducer. pMCD_sod plasmid is a gadA auto-inducible promoter based expression vector <br />
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developed in Laboratory of Pharmaceutical Biotechnology ITB which has coding sequence of <br />
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superoxide dismutase from Staphyloccocus equorum (rMnSODSeq) for expression in Escherichia coli. <br />
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gadA promoter requires stationary phase, low pH, or salt stress to be activated. In previous research, <br />
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optimal protein production was accomplished by keeping the pH at 5.5 by adding HCl periodically. The <br />
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purpose of this research is to observe the effect of buffer and media modification in protein <br />
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production using pMCD_sod in Escherichia coli. pMCD_sod plasmid was confirmed by migration and <br />
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restriction analysis. rMnSODSeq protein production was analysed by SDS-PAGE method. Buffers that <br />
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had been used are succinate, acetate, and citrate buffer. The most suitable buffer was succinate <br />
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buffer and was used for overproduction of rMnSODSeq protein. Modification of Luria Bertani (LB) <br />
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media was performed by using LB media with ¼ of LB component. Effect of buffer to accelerate <br />
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protein production was observed by the presence of rMnSODSeqamount of protein produced at early <br />
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overproduction time. rMnSODSeq protein can be produced using succinate buffer at pH of 5.5 in LB <br />
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media with protein amount equal to LB media with HCl. The amount of protein produced with ¼LB <br />
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media was equal to overproduction with LB media. Optimal rMnSODSeq protein production can be <br />
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done with ¼ LB-succinate media for 11.5 hours resulting in 35.275±1.47% rMnSODSeq from total <br />
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protein with 4.05±0.69 mg rMnSODSeq in one g of wet cells and had activity of dismutasion. <br />
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