<p><b>cotz-aeBlue-CipA</b> a fusion protein sequencing consisting of a spore coat protein, cotZ (building off work done on Sporobeads by the LMU Munich 2012 iGEM team), and a cellulose binding domain (CIPA). Additionally, we decided to add aeBlue, a chromogenic protein, between cotZ and CIPA to be able to see with the naked eye whether <i>Bacillus</i> is in a vegetative or a spore state. </p>

           <p><b>Ptet + Luxl</b> Construct that was cloned to have P(3HB) producing <i>E. coli</i> cells lyse after reaching a certain population density using a quorum sensing promoter. This would greatly facilitate P(3HB) extraction. We are currently still testing and characterizing this part. </p>

           <p><b>Autolysis</b> Construct that was cloned to have P(3HB) producing <i>E. coli</i> cells lyse after reaching a certain population density using a quorum sensing promoter. The difference between this brick BBa_K1692023 is that the basic parts composing this gene are in a different order, which is part of our testing to optimize this system. This would greatly facilitate P(3HB) extraction. We are currently still testing and characterizing this part. </p>

           <p><b>CipA</b> Cellulose binding domain adapted from Imperial 2014 iGEM team. Last part of our composite part BBa_BBa_K1692028. We removed the illegal EcoR1 site that the Imperial 2014 iGEM team had in their construc. </p>

           <p><b>amilGFP yellow chromoprotein, RBS and promoter </b>This plasmid contains the amilGFP yellow chromoprotein gene from part BBa_K1033931 with the RBS and promoter from part BBa_K608002.</p>

           <p><b>meffBlue blue chromoprotein with RBS and promoter</b> This plasmid contains the meffBlue blue chromoprotein gene found in the BBa_K1033902 part, with the RBS and promoter from part BBa_K608002.</p>

           <p><b>amilCP blue chromoprotein with RBS and promoter</b> This plasmid contains the amilCP blue chromoprotein gene found in part BBa_K592009 and the RBS and promoter from part BBa_K608002.</p>