Difference between revisions of "Team:Bulgaria/CONTRIBUTION"
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<h1>TITLE ONE</h1> | <h1>TITLE ONE</h1> | ||
<p> | <p> | ||
| − | + | In the initial stages of our work, we generated and tested the expression of 5 | |
| + | chromoprotein constructs to try our protocols. All of them were cloned into a pSB1C3 | ||
| + | vector with a strong promoter and a potent RBS site. Under these conditions, most of the | ||
| + | proteins showed as a severe metabolic burden to the host cells, leading to small sizes of | ||
| + | the colonies and color loss upon re-cultivation. The exception was the amilGFP protein - | ||
| + | was stable enough to be used under the control of a strong promoter and on a high copy | ||
| + | number vector. We also measured its growth kinetics in comparison with the standard | ||
| + | pSB1C3 vector with a red color device. All data could be viewed at the corresponding page | ||
| + | of the registry. | ||
</p> | </p> | ||
</div> | </div> | ||
Revision as of 14:59, 17 October 2018
TITLE ONE
In the initial stages of our work, we generated and tested the expression of 5 chromoprotein constructs to try our protocols. All of them were cloned into a pSB1C3 vector with a strong promoter and a potent RBS site. Under these conditions, most of the proteins showed as a severe metabolic burden to the host cells, leading to small sizes of the colonies and color loss upon re-cultivation. The exception was the amilGFP protein - was stable enough to be used under the control of a strong promoter and on a high copy number vector. We also measured its growth kinetics in comparison with the standard pSB1C3 vector with a red color device. All data could be viewed at the corresponding page of the registry.