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Team:Tsinghua-E/Part1
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| - | + | <h2>[[File:4_1s.png|68px|left]] '''Part 1: THU-E Mutation Part''' </h2> | |
| - | [[File: | + | [[File:Plasmid1.png|446px|right]] |
| - | A plasmid used for the construction of high-diversity library in vivo ingenome level. In this vector, highly error-prone <em>dnaQ</em> mutant, <em>mutD</em><html><a href="#_ENREF_1" title="Lou, 2012 #499">1</a></html>was cloned downstream of <em>araBAD</em> promoter to control the mutation rate of the target genome by the concentration of <em>araBAD</em> promoter’s inducer, L-arabinose, in a strict manner.<em>E. Coli</em> JM109 carrying different vectors of pBAD_B0030-<em>mutD</em>-<em>sfGFP</em>, pBAD_B0032-<em>mutD</em>-<em>sfGFP</em> and pBAD_SDA_RBS-<em>mutD-sfGFP</em>(this RBS sequence was derived from the RBS sequence upstream of sfGFP in original AraC_pBAD_CI_OR222-sfGFP vector<html><a href="#_ENREF_2" title="Lou, 2012 #499">2</a></html>)were constructed. By detecting the induced fluorescence intensity, we found that pBAD_B0030-<em>mutD</em>-<em>sfGFP</em>, andpBAD_SDA_RBS-<em>mutD- sfGFP</em>have relatively higher <em>mutD</em> expression. The increaseof mutation rate induced by our mutation part was measured by quantifying the reversion of rifampinresistance caused by mutation in genome.pBAD_SDA_RBS-<em>mutD- sfGFP</em>could increase the genome mutation rate up to 10 times compared with negative control with 1g/L induction concentration of L-arabinose. <br /> | + | A plasmid used for the construction of high-diversity library in vivo ingenome level. In this vector, highly error-prone <em>dnaQ</em> mutant, <em>mutD</em><html><a href="#_ENREF_1" title="Lou, 2012 #499">[1]</a></html>was cloned downstream of <em>araBAD</em> promoter to control the mutation rate of the target genome by the concentration of <em>araBAD</em> promoter’s inducer, L-arabinose, in a strict manner.<em>E. Coli</em> JM109 carrying different vectors of pBAD_B0030-<em>mutD</em>-<em>sfGFP</em>, pBAD_B0032-<em>mutD</em>-<em>sfGFP</em> and pBAD_SDA_RBS-<em>mutD-sfGFP</em>(this RBS sequence was derived from the RBS sequence upstream of sfGFP in original AraC_pBAD_CI_OR222-sfGFP vector<html><a href="#_ENREF_2" title="Lou, 2012 #499">[2]</a></html>)were constructed. By detecting the induced fluorescence intensity, we found that pBAD_B0030-<em>mutD</em>-<em>sfGFP</em>, andpBAD_SDA_RBS-<em>mutD- sfGFP</em>have relatively higher <em>mutD</em> expression. The increaseof mutation rate induced by our mutation part was measured by quantifying the reversion of rifampinresistance caused by mutation in genome.pBAD_SDA_RBS-<em>mutD- sfGFP</em>could increase the genome mutation rate up to 10 times compared with negative control with 1g/L induction concentration of L-arabinose. <br /> |
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<img border="0" width="446" src="/wiki/images/a/a3/Part1II.png" /> <br /> | <img border="0" width="446" src="/wiki/images/a/a3/Part1II.png" /> <br /> | ||
| - | Figure.1 Conception illustration of the working mechanism of <em>mutD</em | + | Figure.1 Conception illustration of the working mechanism of <em>mutD</em> |
<img border="0" width="446" src="/wiki/images/7/70/Part1I.png" /> <br /> | <img border="0" width="446" src="/wiki/images/7/70/Part1I.png" /> <br /> | ||
Figure.2 rifampicin reversion mutants caused by <em>mutD</em> expression and the counts by agar plate<br /> | Figure.2 rifampicin reversion mutants caused by <em>mutD</em> expression and the counts by agar plate<br /> | ||
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| - | + | <p><font style="font-size: 12px">[1] Schaaper, R. M. Mechanisms of mutagenesis in the Escherichia-Coli mutator mutd5 - role of DNA mismatch repair. <em>Proc. Natl. Acad. Sci. U. S. A.</em> 85, 8126-8130,doi:10.1073/pnas.85.21.8126 (1988).</font></p> | |
| - | + | <p><font style="font-size: 12px">[2] Lou, C. B., Stanton, B., Chen, Y. J., Munsky, B. & Voigt, C. A. Ribozyme-based insulator parts buffer synthetic circuits from genetic context. <em>Nature Biotechnology</em> 30, 1137-+, doi:10.1038/nbt.2401 (2012).</font></p> | |
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Latest revision as of 03:07, 28 September 2013
Part 1: THU-E Mutation Part
A plasmid used for the construction of high-diversity library in vivo ingenome level. In this vector, highly error-prone dnaQ mutant, mutD[1]was cloned downstream of araBAD promoter to control the mutation rate of the target genome by the concentration of araBAD promoter’s inducer, L-arabinose, in a strict manner.E. Coli JM109 carrying different vectors of pBAD_B0030-mutD-sfGFP, pBAD_B0032-mutD-sfGFP and pBAD_SDA_RBS-mutD-sfGFP(this RBS sequence was derived from the RBS sequence upstream of sfGFP in original AraC_pBAD_CI_OR222-sfGFP vector[2])were constructed. By detecting the induced fluorescence intensity, we found that pBAD_B0030-mutD-sfGFP, andpBAD_SDA_RBS-mutD- sfGFPhave relatively higher mutD expression. The increaseof mutation rate induced by our mutation part was measured by quantifying the reversion of rifampinresistance caused by mutation in genome.pBAD_SDA_RBS-mutD- sfGFPcould increase the genome mutation rate up to 10 times compared with negative control with 1g/L induction concentration of L-arabinose.
Figure.1 Conception illustration of the working mechanism of mutD
Figure.2 rifampicin reversion mutants caused by mutD expression and the counts by agar plate
[1] Schaaper, R. M. Mechanisms of mutagenesis in the Escherichia-Coli mutator mutd5 - role of DNA mismatch repair. Proc. Natl. Acad. Sci. U. S. A. 85, 8126-8130,doi:10.1073/pnas.85.21.8126 (1988).
[2] Lou, C. B., Stanton, B., Chen, Y. J., Munsky, B. & Voigt, C. A. Ribozyme-based insulator parts buffer synthetic circuits from genetic context. Nature Biotechnology 30, 1137-+, doi:10.1038/nbt.2401 (2012).
