Team:UT Dallas/immunobot modeling

From 2011.igem.org

(Difference between revisions)

Latest revision as of 03:25, 29 September 2011

Model and simulation

The signaling network from the input of external ligand signal to the output of the tumbling state of a E coli cell can be quantitatively described by a modular model. The model is formulated based on the law of mass action and Michaelis-Menten mechanism and contains four relatively independent modules that are explained in detail below.

Module 1: Activation of ToxR receptor
In this module, the ligand signal activates the ToxR receptor into a dimerized complex formed with the ligand, which is the active state of the receptor. The biochemical reaction can be illustrated as:

where L, R, C and C2 represent the concentration of external ligand, free receptor, recptor-ligand complex, and the dimerized receptor-ligand complex. The first reaction represents the binding/unbinding between the free receptor and the ligand. The second reaction represents the dimerization/undimerization conversions between C and C2. The conservation of the total concentration of the receptor can be written as:

where R^T is the total receptor concentration. The governing differential equations of this module are:

The equations contain binding rate k_fL(R^T-C-2C₂ ), unbinding rate k_rC, dimerization rate k_dimC² and undimerization rate 2k_undimC₂, where k_f, k_r, k_dim and k_undim represent the rate constants for binding, unbinding, dimerization and undimerization reactions. The values of the parameters are obtained from (Forsten-Williams, Chua et al. 2005). Typical simulation results in response to L=1 µM are:

where the dissociation constant for receptor-ligand binding used in the right figure is 100 times than that in the left figure.

Module 2: Transcription/translation of CheZ
In this module, the dimerized complex C₂ activates the transcription of the cheZ mRNA. The reactions are the standard transcription and translation reactions illustrated as:

Where Zm and Zp represent the concentration of the mRNA and the protein product of CheZ. The formulation of the reactions follow the standard equations for transcription and translation.

Where k₀ represents the basal transcription rate of Z_m, k₁ represents the transcription rate activated by C₂, k₃ represents the translational rate of Z_p, and k₂ and k₄ represent the degradation rates of Z_m and Z_p. Typical simulation results are:

where the degradation rate for Zp in the right figure is 10 times than that in the left figure.

Module 3
In this module, the CheY protein is dephosphorylated by the CheZ protein and the reaction can be illustrated as:

The governing differential equation follows the format given in (Spiro, Parkinson et al. 1997)

Where Y^T is the total concentration of the CheY protein, and k_p and k_d are the phosphorylation and the dephosphorylation rate constants of CheY. The parameter values are obtained from (Spiro, Parkinson et al. 1997). Typical simulation results are:

where again the degradation rate for Zp in the right figure is 10 times than that in the left figure.

Module 4
In this module, the tumbling activity of E coli is characterized by the so-called “bias”, which is defined as the ratio of the time of directed movement and the total time. It is experimentally measured that the bias is a Hill function dependent on the concentration of phosphorylated CheY (Cluzel, Surette et al. 2000).

Using the steady-state value of Yp in the previous two figures, that is 4.08 µM or 14.25µM, the final bias is 6.6% or .01%.

References
Cluzel, P., M. Surette, et al. (2000). "An ultrasensitive bacterial motor revealed by monitoring signaling proteins in single cells." Science 287(5458): 1652-5.
Forsten-Williams, K., C. C. Chua, et al. (2005). "The kinetics of FGF-2 binding to heparan sulfate proteoglycans and MAP kinase signaling." J Theor Biol 233(4): 483-99.
Spiro, P. A., J. S. Parkinson, et al. (1997). "A model of excitation and adaptation in bacterial chemotaxis." Proc Natl Acad Sci U S A 94(14): 7263-8.

@@ Line 70: / Line 70: @@
 <div class="contents">
-<div id="container2">
+ <div id="container2">
-	<div id="container1">
+<div id="container1">
 		<div id="left">
 </html>{{:Team:UT_Dallas/Template:menu}}<html>
@@ Line 84: / Line 84: @@
 <img hight='30' src="https://static.igem.org/mediawiki/2011/c/c4/Equation1.png"><br>
 </center>
-where L, R, C and C2 represent the concentration of external ligand, free receptor, recptor-ligand complex, and the dimerized receptor-ligand complex. The first reaction represents the binding/unbinding between the free receptor and the ligand. The second reaction represents the dimerization /undimerization conversions between C and C2. The conservation of the total concentration of the receptor can be written as:
+where L, R, C and C2 represent the concentration of external ligand, free receptor, recptor-ligand complex, and the dimerized receptor-ligand complex. The first reaction represents the binding/unbinding between the free receptor and the ligand. The second reaction represents the dimerization/undimerization conversions between C and C2. The conservation of the total concentration of the receptor can be written as:
   <br>
 <center>
 <img hight='30' src="https://static.igem.org/mediawiki/2011/e/ea/Equation2.png"><br>
 </center>
-where R^T is the total receptor concentration. The governing differential equations of this module are:
+where R<sup>T</sup> is the total receptor concentration. The governing differential equations of this module are:
   <br>
 <center>
@@ Line 100: / Line 100: @@
 </center>
-The equations contain binding rate k_f L(R^T-C-2C_2 ), unbinding rate k_r C, dimerization rate k_dim C^2 and undimerization rate 2k_undim C_2, where k_f, k_r, k_dim and k_undim represent the rate constants for binding, unbinding, dimerization and undimerization reactions. The values of the parameters are obtained from (Forsten-Williams, Chua et al. 2005). Typical simulation results in response to L=1 µM are:
+The equations contain binding rate k<sub>f</sub>L(R<sup>T</sup>-C-2C<sub>2</sub> ), unbinding rate k<sub>r</sub>C, dimerization rate k<sub>dim</sub>C<sup>2</sup> and undimerization rate 2k<sub>undim</sub>C<sub>2</sub>, where k<sub>f</sub>, k<sub>r</sub>, k<sub>dim</sub> and k<sub>undim</sub> represent the rate constants for binding, unbinding, dimerization and undimerization reactions. The values of the parameters are obtained from (Forsten-Williams, Chua et al. 2005). Typical simulation results in response to L=1 µM are:
 <center>
@@ Line 120: / Line 120: @@
 <b>Module 2:</b> Transcription/translation of CheZ<br>
-In this module, the dimerized complex C_2 activates the transcription of the cheZ mRNA. The reactions are the standard transcription and translation reactions illustrated as:<br>
+In this module, the dimerized complex C<sub>2</sub> activates the transcription of the cheZ mRNA. The reactions are the standard transcription and translation reactions illustrated as:<br>
 <center>
 <img hight='30' src="https://static.igem.org/mediawiki/2011/0/0c/Equation5.jpg"><br>
@@ Line 136: / Line 136: @@
 </center>
-Where k_0 represents the basal transcription rate of Z_m, k_1 represents the transcription rate activated by C_2, k_3 represents the translational rate of Z_p, and k_2 and k_4 represent the degradation rates of Z_m and Z_p. Typical simulation results are:<br>
+Where k<sub>0</sub> represents the basal transcription rate of Z<sub>m</sub>, k<sub>1</sub> represents the transcription rate activated by C<sub>2</sub>, k<sub>3</sub> represents the translational rate of Z<sub>p</sub>, and k<sub>2</sub> and k<sub>4</sub> represent the degradation rates of Z<sub>m</sub> and Z<sub>p</sub>. Typical simulation results are:<br>
 <center>
@@ Line 162: / Line 162: @@
 <img hight='30' src="https://static.igem.org/mediawiki/2011/a/a1/Equation9.png"><br>
 </center>
-Where Y^Tis the total concentration of the CheY protein, and k_p and k_d are the phosphorylation and the dephosphorylation rate constants of CheY. The parameter values are obtained from (Spiro, Parkinson et al. 1997). Typical simulation results are:<br>
+Where Y<sup>T</sup> is the total concentration of the CheY protein, and k<sub>p</sub> and k<sub>d</sub> are the phosphorylation and the dephosphorylation rate constants of CheY. The parameter values are obtained from (Spiro, Parkinson et al. 1997). Typical simulation results are:<br>
 <center>
@@ Line 189: / Line 189: @@
 Cluzel, P., M. Surette, et al. (2000). "An ultrasensitive bacterial motor revealed by monitoring signaling proteins in single cells." Science 287(5458): 1652-5.<br>
 Forsten-Williams, K., C. C. Chua, et al. (2005). "The kinetics of FGF-2 binding to heparan sulfate proteoglycans and MAP kinase signaling." J Theor Biol 233(4): 483-99.<br>
-Spiro, P. A., J. S. Parkinson, et al. (1997). "A model of excitation and adaptation in bacterial chemotaxis." Proc Natl Acad Sci U S A 94(14): 7263-8.<br>
+Spiro, P. A., J. S. Parkinson, et al. (1997). "A model of excitation and adaptation in bacterial chemotaxis." Proc Natl Acad Sci U S A 94(14): 7263-8.<br><br><br>
 </div>