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<h2 class="title" id="s1">Improved Part </h2> | <h2 class="title" id="s1">Improved Part </h2> | ||
− | <p>According to the problem we mentioned in the demonstration, the expression of the <i>NicA2</i> protein may be toxic to<latin>E. coli</latin>so that its gene cannot be stably present in<latin> E. coli.</latin> Similarly, genes that are toxic to<latin>E. coli</latin>are difficult to achieve genetic manipulation in it, especially using replication-dependent recombination methods such as <i>Red/ET</i> homologous recombination. However, many proteins that are toxic to<latin>E. coli</latin>are normally present in <latin>Pseudomonas</latin>, and during the establishment of the <latin>P.fluorescens pf-5 </latin> promoter library of <latin>Pseudomonas fluorescens</latin>, we found that most of the promoters of<latin> P.fluorescens pf-5</latin> cannot work in<latin> E. coli.</latin><p> | + | <p>According to the problem we mentioned in the demonstration, the expression of the <i>NicA2</i> protein may be toxic to<latin>E. coli</latin>so that its gene cannot be stably present in<latin> E. coli.</latin> Similarly, genes that are toxic to<latin>E. coli</latin>are difficult to achieve genetic manipulation in it, especially using replication-dependent recombination methods such as <i>Red/ET</i> homologous recombination. However, many proteins that are toxic to<latin>E. coli</latin>are normally present in <latin>Pseudomonas</latin>, and during the establishment of the <latin>P.fluorescens pf-5</latin> promoter library of <latin>Pseudomonas fluorescens</latin>, we found that most of the promoters of<latin> P.fluorescens pf-5</latin> cannot work in<latin> E. coli.</latin><p> |
− | <p>Therefore, in addition to the transformation of <latin>P.fluorescens pf-5 </latin>into a new chassis for heterologous expression, we are also interested in directly implementing genetic manipulation in <latin>Pseudomonas</latin>. The genetic manipulation of <latin>Pseudomonas</latin> was carried out earlier. The early genetic manipulation method was to use the homologous recombination of the endogenous RecA recombinase, but the efficiency was very low and it was prone to off target. In 2017, Zheng Wenzhao et al<sup>[1]</sup>. studied the construction of the <latin>Pseudomonas</latin> <i>Red/ET</i> recombination system and achieved preliminary results in <latin>Pseudomonas putida</latin>, <latin>Pseudomonas aeruginosa</latin>, <latin>Pseudomonas syringae</latin> and <latin>Pseudomonas fluorescens. </latin></p> | + | <p>Therefore, in addition to the transformation of <latin>P.fluorescens pf-5 </latin> into a new chassis for heterologous expression, we are also interested in directly implementing genetic manipulation in <latin>Pseudomonas</latin>. The genetic manipulation of <latin>Pseudomonas</latin> was carried out earlier. The early genetic manipulation method was to use the homologous recombination of the endogenous RecA recombinase, but the efficiency was very low and it was prone to off target. In 2017, Zheng Wenzhao et al<sup>[1]</sup>. studied the construction of the <latin>Pseudomonas</latin> <i>Red/ET</i> recombination system and achieved preliminary results in <latin>Pseudomonas putida</latin>, <latin>Pseudomonas aeruginosa</latin>, <latin>Pseudomonas syringae</latin> and <latin>Pseudomonas fluorescens. </latin></p> |
− | <p>Regardless of the type of cloning, screening markers are indispensable, and our part <a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K2569032">BBa_K2569032</a> have improved one of the most widely used parts <a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_J04450">BBa_J04450</a> in iGEM. < | + | <p>Regardless of the type of cloning, screening markers are indispensable, and our part <a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K2569032">BBa_K2569032</a> have improved one of the most widely used parts <a href="http://parts.igem.org/wiki/index.php?title=Part:BBa_J04450">BBa_J04450</a> in iGEM. <i>lacI</i> is present on the genome of many host cells, which suggests that he normal expression of <I>RFP</I> requires the induction of IPTG and need 18 hours of waiting. We replaced the lac promoter in front of the <i>RFP</i> gene with the strong pf-5 promoter <i>PampC</i>. And hope that <i>RFP</i>, as a visible marker for the naked eye, can be expressed more pronouncedly and faster in <latin>Pseudomonas fluorescens pf-5</latin>.</p> |
</div> | </div> |
Latest revision as of 18:26, 17 October 2018
Improved Part
According to the problem we mentioned in the demonstration, the expression of the NicA2 protein may be toxic to
Therefore, in addition to the transformation of
Regardless of the type of cloning, screening markers are indispensable, and our part BBa_K2569032 have improved one of the most widely used parts BBa_J04450 in iGEM. lacI is present on the genome of many host cells, which suggests that he normal expression of RFP requires the induction of IPTG and need 18 hours of waiting. We replaced the lac promoter in front of the RFP gene with the strong pf-5 promoter PampC. And hope that RFP, as a visible marker for the naked eye, can be expressed more pronouncedly and faster in
Reference
[1] Zheng Wenzhao. Construction and application of Red/ET recombination system in