Difference between revisions of "Team:Vilnius-Lithuania/Design"

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According to the obscure guidelines we split an unmodified neo gene sequence between 59 and 60 amino acid residues. Two subunits were termed a-neo and ß-neo. Furthermore, we added additional termination codon at the end of an a-neo fragment for the translation to stop. No other start codons were included into the ß-neo subunit as the gene was designed for toehold switch system. Despite the fact that ß-neo subunit had no start codon, the split antibiotic system worked perfectly when coupled with a standard promoter and a ribosome binding site (BBa_K608002). Consequently, a split antibiotic resistance gene provides a selection system to stably maintain two different plasmids.
 
According to the obscure guidelines we split an unmodified neo gene sequence between 59 and 60 amino acid residues. Two subunits were termed a-neo and ß-neo. Furthermore, we added additional termination codon at the end of an a-neo fragment for the translation to stop. No other start codons were included into the ß-neo subunit as the gene was designed for toehold switch system. Despite the fact that ß-neo subunit had no start codon, the split antibiotic system worked perfectly when coupled with a standard promoter and a ribosome binding site (BBa_K608002). Consequently, a split antibiotic resistance gene provides a selection system to stably maintain two different plasmids.
 
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             <img src="http://placehold.it/800x450" alt="img">
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             <img src="https://static.igem.org/mediawiki/2017/c/c4/1vln.png"img">
 
             <div class="img-label">Figure 1. Split neo gene principle scheme by M. Schmidt et al.
 
             <div class="img-label">Figure 1. Split neo gene principle scheme by M. Schmidt et al.
 
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Revision as of 21:59, 1 November 2017

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Determining the plasmid copy number

Design

Preparing for the framework: standard curve generation and plasmid copy number evaluation

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