IGEM:IMPERIAL/2009/4Sep/System Overview/Mod3

=Module 3=

Module function in overall design
This module serves to remove the genetic material from the bacteria after both protein production and encapsulation have been completed. This serves to allay any genetically modified organism concerns, and is useful as a reusable module for other projects.
 * High level description

2 main parts: 1) Thermoinduction 2) Restriction Enzyme killing

Temperature increase to 42 degrees Celsius will trigger Module 3
 * Input

Restriction Enzyme DpnII and TaqI activity leads to cell death
 * Output(s)

Testing Construct Design
Definite constructs: 2 Possible constructs: 3 (depending on if Harvard GFP works)
 * Total Number of testing constructs

For all the constructs currently being designed - see here

To test how temperature will affect either the GFP expression, or the efficiency of killing.
 * Rationale behind testing constructs

Progress

 * Current status in terms of cloning for each assembly




 * The Harvard-GFP is the main ligation, from which testing can start.
 * For the second testing construct, we are awaiting DpnII and TaqI from MrGene
 * To save time, the self-synthesized cI and pLambda will not be constructed until after Harvard-GFP has been tested

What can be completed in time for Jamboree
 * Will definitely finish the Harvard-GFP testing, but the rest will depend on when Resriction enzymes come and ligation success

Data we hope to get from this
NO DNA construct To test how the concentration of restriction enzymes and methylases affects the cutting of genomic DNA. - will get a Yes/No answer for each set concentration of restriction enzymes and methylases.

Importance:
 * in showing that the restriction enzymes work and that there is a balance with the methylases (the concentration can be experimentally determined)

Assay:
 * Genomic preparation assay to test if it can be cut

How essential in whole project: 4

To test how the GFP fluorescence will vary with the temperature - will get fluorescence output(A.U.) over time for 28 degrees and 42 degrees

In addition, since GFP is temp sensitive, need to also find out how GFP fluorescence varies with temperature use - test GFP fluorescence varying with temperature using any promoter with GFP eg CRP promoter

Importance:
 * in showing that the thermoinduction system works- trigger for killing

Assay:
 * Promoter characterisation assay and the effect of increasing temperature
 * Essentially just monitering GFP fluorescence over time at different temperatures

How essential in whole project: 6

To test the effect of temperature on the killing efficiency of the restriction enzymes Importance:
 * In showing that the thermoinduction system and the killing strategy works- trigger for killing

Assay:
 * Staining Assay which gives the percentage of viable and dead cells over time
 * Important for modelling killing rate

How essential in whole project: 8

Ready for testing construct
GFP fluorescence and Harvard YES Staining Assay YES Restriction Enzyme and Genomic Assay YES
 * Protocols written and reviewed ?

Multiplate reader
 * Any expertise needed? Acces to specific equipment needed ?

Modelling for the killing: YES - ready for data from the staining assay
 * Modelling done ? Ready to analyse experimental data ?