Team:BostonU/Data

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Revision as of 20:18, 27 September 2013 by THaddock (Talk | contribs)



Data Collected

New Part Creation

Characterization of Level 1 MoClo Devices

    The Cytometer Setup and Tracking beads offered by BD Biosciences are utilized to set the laser delay and optimize the cytometer settings prior to running any samples through the Fortessa.

    We also utilize Spherotech's 8-peak particles (RCP-30-5A) in order to obtain standard MEFL units for the FITC channel. They are also used to measure the long term performance of the flow cytometer.

    Our results...

Datasheet Tool

    The Datasheet Tool was coded primarily in Java for the back-end server side and in HTML from the front-end client side. The app was coded in the NetBeans IDE and we stored all of our code on a private GitHub repository.

    Datasheet User Interface
    The code generates different sections for the user to complete. This sample section allows the user to fill out basic info about their part.

    This section allows the user to fill out specific design information.

Eugene Results

    We wrote Eugene scripts for our projects this summer. The wiki upload option does not allow .eug Eugene files so we uploaded our code as plain text files. To run our code in the Eugene Scriptor, simply save the code as .eug.

    The pConstitutive Library Eugene file shows all of the constitutive promoter and fluorescent protein permutations using the Anderson promoter library.

    The pRepressible Library Eugene file shows all of the possible repressible promoter and gene relationships based on our MoClo library.

    The Quorum Sensing Eugene file shows the permutations possible with the specified rules, such as the repressing relationship between certain promoters and genes and the small molecule arabinose inducing the pBad promoter.