Team:Paris/Modeling/f3

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[[Image:f3omp.jpg|thumb]]
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{{Paris/Menu}}
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We have [OmpR<sup>*</sup>] = {coef<sub>omp</sub>}''expr(pTet)'' = {coef<sub>omp</sub>} &#131;1([aTc]<sub>i</sub>)
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{{Paris/Header|Method & Algorithm : &#131;3}}
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<center> = act_''pFlhDC'' </center>
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<br>
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and [FliA] = {coef<sub>FliA</sub>}''expr(pBad)'' = {coef<sub>FliA</sub>} &#131;2([arab]<sub>i</sub>)
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[[Image:f3omp.jpg|thumb|Specific Plasmid Characterisation for &#131;3]]
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So, at steady-states,
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According to the characterization plasmid (see right) and to our modeling, in the '''exponential phase of growth''', at the steady state,
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[[Image:F3ompfinal.jpg|center]]
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we have ''' [''OmpR<sup>*</sup>'']<sub>''real''</sub> = {coef<sub>''ompR''</sub>} &#131;1([aTc]<sub>i</sub>) '''
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and ''' [FliA]<sub>''real''</sub> = {coef<sub>FliA</sub>} &#131;2([arab]<sub>i</sub>) '''
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<br><br>
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but we use ''' [aTc]<sub>i</sub> = Inv_&#131;1( [OmpR<sup>*</sup>] ) '''
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and        ''' [arab]<sub>i</sub> = Inv_&#131;2( [FliA] ) '''
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{|border="1" style="text-align: center"
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So, at steady-states,
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|param
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|signification
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|unit
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|value
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|comments
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|-
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|[expr(pFlhDC)]
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|expression rate of <br> pFlhDC '''with RBS E0032'''
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|nM.min<sup>-1</sup>
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|need for 20 mesures with well choosen values of [aTc]<sub>i</sub> <br> and for 20 mesures with well choosen values of [arab]<sub>i</sub> <br> and 5x5 measures for the relation below?
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|-
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|γ<sub>GFP</sub>
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|dilution-degradation rate <br> of GFP(mut3b)
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|min<sup>-1</sup>
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|0.0198
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|[GFP]
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|GFP concentration at steady-state
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|nM
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|need for 20 + 20 measures <br> and 5x5 measures for the relation below?
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|-
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|(''fluorescence'')
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|value of the observed fluorescence
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|au
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|need for 20 + 20 measures <br> and 5x5 measures for the relation below?
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|''conversion''
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|conversion ratio between <br> fluorescence and concentration
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|nM.au<sup>-1</sup>
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|(1/79.429)
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|}
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<br><br>
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[[Image:F3ompfinal.jpg|center]]
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{|border="1" style="text-align: center"
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we use this analytical expression to determine the parameters :
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|param
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|signification <br> corresponding parameters in the [[Team:Paris/Modeling/Oscillations#Resulting_Equations|equations]]
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|unit
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|value
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|comments
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|-
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|β<sub>13</sub>
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|production rate of FliA-pFlhDC '''with RBS E0032''' <br> β<sub>13</sub>
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|nM.min<sup>-1</sup>
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|(K<sub>12</sub>/{coef<sub>fliA</sub>})
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|activation constant of FliA-pFlhDC <br> K<sub>12</sub>
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|nM
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|n<sub>12</sub>
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|complexation order of FliA-pFlhDC <br> n<sub>12</sub>
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|no dimension
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|β<sub>2</sub>
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|production rate of OmpR-pFlhDC '''with RBS E0032''' <br> β<sub>2</sub>
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|nM.min<sup>-1</sup>
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|(K<sub>22</sub>/{coef<sub>omp</sub>})
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|activation constant of OmpR-pFlhDC <br> K<sub>22</sub>
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|nM
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|n<sub>22</sub>
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|complexation order of OmpR-pFlhDC <br> n<sub>22</sub>
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|no dimension
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|}
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<br><br>
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<div style="text-align: center">
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{{Paris/Toggle|Table of Values|Team:Paris/Modeling/More_f3_Table}}
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</div>
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<div style="text-align: center">
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{{Paris/Toggle|Algorithm|Team:Paris/Modeling/More_f3_Algo}}
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</div>
Then, if we have time, we want to verify the expected relation
Then, if we have time, we want to verify the expected relation
[[Image:SumFlhDC1.jpg|center]]
[[Image:SumFlhDC1.jpg|center]]
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<br>
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<center>
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[[Team:Paris/Modeling/Implementation| <Back - to "Implementation" ]]| <br>
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[[Team:Paris/Modeling/Protocol_Of_Characterization| <Back - to "Protocol Of Characterization" ]]|
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</center>

Latest revision as of 02:12, 30 October 2008

Method & Algorithm : ƒ3


= act_pFlhDC


Specific Plasmid Characterisation for ƒ3

According to the characterization plasmid (see right) and to our modeling, in the exponential phase of growth, at the steady state,

we have [OmpR*]real = {coefompR} ƒ1([aTc]i) and [FliA]real = {coefFliA} ƒ2([arab]i)

but we use [aTc]i = Inv_ƒ1( [OmpR*] ) and [arab]i = Inv_ƒ2( [FliA] )

So, at steady-states,

F3ompfinal.jpg

we use this analytical expression to determine the parameters :

↓ Table of Values ↑


param signification unit value comments
(fluorescence) value of the observed fluorescence au need for 20 mesures with well choosen values of [aTc]i
and for 20 mesures with well choosen values of [arab]i
and 5x5 measures for the relation below?
conversion conversion ratio between
fluorescence and concentration
↓ gives ↓
nM.au-1 (1/79.429)
[GFP] GFP concentration at steady-state nM
γGFP dilution-degradation rate
of GFP(mut3b)
↓ gives ↓
min-1 0.0198 Time Cell Division : 35 min.
ƒ3 activity of
pFlhDC with RBS E0032
nM.min-1



param signification
corresponding parameters in the equations
unit value comments
β22 total transcription rate of
FliA><pFlhDC with RBS B0034
β22
nM.min-1
(K6/{coeffliA}) activation constant of FliA><pFlhDC
K6
nM
n6 complexation order of FliA><pFlhDC
n6
no dimension
β17 basal activity of
pFlhDC with RBS B0034
β17
nM.min-1
(K15/{coefompR}) activation constant of OmpR><pFlhDC
K15
nM
n15 complexation order of OmpR><pFlhDC
n15
no dimension
↓ Algorithm ↑


find_ƒ3 ( FliA )

function optimal_parameters = find_f3_FliA(X_data, Y_data, initial_parameters)
% gives the 'best parameters' involved in f3 with OmpR = 0 by least-square optimisation
% -> USE IT AFTER find_f3_OmpR
 
% X_data = vector of given values of ( [FliA]i ) (experimentally
% controled)
% Y_data = vector of experimentally measured values f3 corresponding of
% the X_data
% initial_parameters = values of the parameters proposed by the literature
%                       or simply guessed
%                    = [beta22, K6 -> (K6)/(coefOmp), n6]
 
global beta17; % parameter GIVEN BY find_f3_OmpR
 
     function output = act_pFlhDC(parameters, X_data)
         for k = 1:length(X_data)
                 output(k) = beta17*(1 - hill( X_data(k), parameters(2), parameters(3))) ...
                     + parameters(1)*hill(X_data(k), parameters(2), parameters(3));
         end
     end
 
options=optimset('LevenbergMarquardt','on','TolX',1e-10,'MaxFunEvals',1e10,'TolFun',1e-10,'MaxIter',1e4);
% options for the function lsqcurvefit
 
optimal_parameters = lsqcurvefit( @(parameters, X_data) act_pFlhDC(parameters, X_data), ...
     initial_parameters, X_data, Y_data, options );
% search for the fittest parameters, between 1/10 and 10 times the initial
% parameters
 
end

find_ƒ3 ( OmpR* )

function optimal_parameters = find_f3_OmpR(X_data, Y_data, initial_parameters)
% gives the 'best parameters' involved in f3 with FliA = 0 by least-square optimisation
% -> USE IT BEFORE find_f3_FliA
 
% X_data = vector of given values of ( [OmpR]i ) (experimentally
% controled)
% Y_data = vector of experimentally measured values f3 corresponding of
% the X_data
% initial_parameters = values of the parameters proposed by the literature
%                       or simply guessed
%                    = [beta17, K15 -> (K15)/(coefOmp), n15]
 
     function output = act_pFlhDC(parameters, X_data)
         for k = 1:length(X_data)
                 output(k) =(1 - hill( X_data(k), parameters(2), parameters(3) )) * parameters(1);
         end
     end
 
options=optimset('LevenbergMarquardt','on','TolX',1e-10,'MaxFunEvals',1e10,'TolFun',1e-10,'MaxIter',1e4);
% options for the function lsqcurvefit
 
optimal_parameters = lsqcurvefit( @(parameters, X_data) act_pFlhDC(parameters, X_data), ...
    initial_parameters, X_data, Y_data, options );
% search for the fittest parameters, between 1/10 and 10 times the initial
% parameters
 
end

Then, if we have time, we want to verify the expected relation

SumFlhDC1.jpg


<Back - to "Implementation" |
<Back - to "Protocol Of Characterization" |