Team:ESBS-Strasbourg/measurements

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Revision as of 07:21, 21 August 2008

<= back

In general

BD means the four DNA binding proteins: LexA, LacI, CI and TetR
The promoter consists of a repeat of the binding sequence of the DBP and the minimal Promoter (containing TATA box and the Kozak sequence)
There is a glycin linker between every protein fused
The IRES also contains already a Kozak sequence
The used colors are
- Blue for the self activator
- Yellow for the cross activator
- Red for the (cross) repressor

Line 0: Functionality of basic Biobricks

Test whether EYFP is working at all

Line 1: Activity and functionality of the single activator constructs

Here we are going to test two things:

The functionality of the inducer construct in regard to the position of the XFP. This will first be tested for one construct and then later on be transfered to the others. The thing to measure is the amount of CFP under same inducer conditions for the three constructs.
The strength of the promoters for the different DNA Binding Proteins. Therefore we will induce our system with different time steps and measure the outcome of the CFP. Then we'll try to find couples of DBP with similar activities/Kds by changing the number of operons. The thing to measure is the ratio between YFP and CFP under different inducer conditions and different operon numbers and the total amount of CFP.

1.2 Reporter construct

Line 2: Stability of the self activator

Here we are going to test if the self activation of the constructs is sufficiently strong to keep the signal through several cell divisions. The thing to measure is the CFP amount after induction and after several (~10) cell divisions.
2.1 Inducer

Same as under 1.1

2.2 Reporter construct

Line 3: Effect of the repressor

Here we can measure two things:

the efficiency of the repressor. The thing to measure is the CFP amount.

3.1 Inducer

3.1 Reporter construct

Same as under 1.1

Line 4: Tag-testing

Here first of all the efficiency of our tags are tested with XFP before we can test out at which position to put them into the BD-VP16-XFP-NLS-PEST-APC construct. The thing to measure is the development of the XFP.

@@ Line 17: / Line 17: @@
 ** Yellow for the cross activator
 ** Red for the (cross) repressor<br>
-==Functionality of basic Biobricks==
+==Line 0: Functionality of basic Biobricks==
 *Test whether EYFP is working at all
 [[Image:ESBS-tester1.JPG]]<br>
-==Activity and functionality of the single activator constructs==
+==Line 1: Activity and functionality of the single activator constructs==
 Here we are going to test two things:
 * The functionality of the inducer construct in regard to the position of the XFP. This will first be tested for one construct and then later on be transfered to the others. '''The thing to measure''' is the amount of CFP under same inducer conditions for the three constructs.
@@ Line 32: / Line 32: @@
 [[Image:ESBS-tester14.JPG]]<br>
-==Stability of the self activator==
+==Line 2: Stability of the self activator==
 Here we are going to test if the self activation of the constructs is sufficiently strong to keep the signal through several cell divisions. '''The thing to measure''' is the CFP amount after induction and after several (~10) cell divisions.<br>
 <big> '''2.1 Inducer''' </big><br><br>
@@ Line 39: / Line 39: @@
 [[Image:ESBS-tester21.JPG]]<br>
-==Effect of the repressor==
+==Line 3: Effect of the repressor==
 Here we can measure two things:
 * the efficiency of the repressor. '''The thing to measure''' is the CFP amount.<br>
@@ Line 48: / Line 48: @@
 Same as under 1.1<br><br>
-==Tag-testing==
+==Line 4: Tag-testing==
 Here first of all the efficiency of our tags are tested with XFP before we can test out at which position to put them into the BD-VP16-XFP-NLS-PEST-APC construct. '''The thing to measure''' is the development of the XFP.<br>
 [[Image:ESBS-tester41.JPG]]<br>