Team:BCCS-Bristol/Modeling-Parameters

From 2008.igem.org

(Difference between revisions)
(Run Tumble Motion)
(GRN Modelling)
 
(16 intermediate revisions not shown)
Line 20: Line 20:
* [[Team:BCCS-Bristol/Modeling-Parameters#Bacteria|'''Bacteria''']]
* [[Team:BCCS-Bristol/Modeling-Parameters#Bacteria|'''Bacteria''']]
-
* [[Team:BCCS-Bristol/Modeling-Parameters#Run_and_Tumble|'''Run and tumble motion''']]
+
* [[Team:BCCS-Bristol/Modeling-Parameters#Run_Tumble_Motion|'''Run Tumble motion''']]
-
* [[Team:BCCS-Bristol/Modeling-Parameters#Properties of the media|'''Properties of the Media''']]
+
* [[Team:BCCS-Bristol/Modeling-Parameters#GRN_Modelling|'''GRN Modelling''']]
-
* [[Team:BCCS-Bristol/Modeling-Parameters#Intracellular modelling|'''Intracellular Modelling''']]
+
=== Bacteria ===
=== Bacteria ===
Line 88: Line 87:
|}
|}
-
=== Intracellular Modelling ===
+
=== GRN Modelling ===
{| class="bccstable"
{| class="bccstable"
-
| align="center" width="10%" style="background:#f0f0f0;"|'''Attribute'''
+
| align="center" width="10%" style="background:#f0f0f0;"|'''Parameter'''
-
| align="center" width="10%" style="background:#f0f0f0;"|'''Value'''
+
| align="center" width="20%" style="background:#f0f0f0;"|'''Value'''
-
| align="center" width="10%" style="background:#f0f0f0;"|'''Strain'''
+
| align="center" width="40%" style="background:#f0f0f0;"|'''Description'''
-
| align="center" width="40%" style="background:#f0f0f0;"|'''Justification'''
+
| align="center" width="30%" style="background:#f0f0f0;"|'''Reference'''
| align="center" width="30%" style="background:#f0f0f0;"|'''Reference'''
|-
|-
-
| T||taxis receptor MW (kDa) = 58-60||RP437||Receptor (total) = 15000±1700, Tsr + Tar = 14000±1700, Trg = 440±70. Value was determined in RP437 strain in rich medium. Note that cellular amounts vary 10 fold but the stiochiometric ratios only vary 30%. Segall et al. 1986 assumed that there was 600 Tar receptors per cell (determined in RP437- a strain often used in chemotaxis studies)||[http://jb.asm.org/cgi/reprint/186/12/3687?maxtoshow=&HITS=10&hits=10&RESULTFORMAT=&author1=hazelbauer&searchid=1&FIRSTINDEX=0&resourcetype=HWCIT Cellular Stoichiometry of the Components of the Chemotaxis Signaling Complex], [http://www.pdn.cam.ac.uk/groups/comp-cell/Rates.html Bray Computer Modelling group], [http://www.pubmedcentral.nih.gov/picrender.fcgi?artid=387059&blobtype=pdf Temporal comparisons in bacterial chemotaxis ]
+
| C<sub>pMax<sub> ||Unknown (varied in the program)||Maximal CpxR protein concentration||||
 +
|-
 +
| k<sub>Cp<sub> ||0.075min<sup>-1<sup> <br> ESTIMATED ||Maximal transcription rate of pCpxR promoter || [http://www.pubmedcentral.nih.gov/articlerender.fcgi?tool=pubmed&pubmedid=11830644 Surface Sensing and Adhesion of Escherichia Coli controlled by the cpx-signalling pathway.]
 +
|-
 +
| theta<sub>Cpx<sub> ||1 x 10<sup>-9</sup> M <br> ESTIMATED ||Threshold for pCpxR promoter Hill Function || [https://2008.igem.org/team:kuleuven iGEM 2008 KULeuven ]||
 +
|-
 +
| m<sub>Cpx<sub> ||1.0 || Co-operativity of pCpxR promoter Hill function ||||
 +
|-
 +
| d<sub>Im<sub> || 3.6 x 10<sup>-1</sup>  min<sup>-1<sup> || Degradation rate of GFP mRNA ||[http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| k<sub>Ip<sub> || 9.6 x 10<sup>-1</sup>  min<sup>-1<sup> || Rate of LuxI protein translation || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| d<sub>Ip<sub> || 1.67 x 10<sup>-2</sup>  min<sup>-1<sup> || Degradation rate of LuxI protein || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| d<sub>Gm<sub> || 1.65 x 10<sup>-3</sup> min<sup>-1<sup> || Degradation rate of GFP protein || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T36-42HFN5W-11&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_acct=C000010018&_version=1&_urlVersion=0&_userid=121739&md5=38be996fd7eb7dc4e71179e9d721b298 Efficient GFP mutations profoundly affect mRNA transcription and translation rates ]
 +
|-
 +
| k<sub>Gp<sub> || 2.4 x 10<sup>-1</sup> min<sup>-1<sup> || Rate of GFP protein translation || [http://www.springerlink.com/content/p14488p56p37n602/  Quantitative measurement of green fluorescent protein expression]
 +
|-
 +
| d<sub>Gp<sub> || 2.14 x 10<sup>-4</sup> min<sup>-1<sup> || Degradation rate of GFP protein || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| A<sub>prod<sub> || 3.6 min<sup>-1<sup> || AHL production rate per LuxI enzyme ||[[http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| d<sub>A<sub> || 1 x 10<sup>-2</sup> min<sup>-1<sup> || Degradation rate of AHL molecule ||[http://www.nature.com/nature/journal/v434/n7037/full/nature03461.html A synthetic multicellular system for programmed pattern formation ]
 +
|-
 +
| D<sub>A<sub> || 0.23s<sup>-1<sup> || Diffusion coefficient of AHL || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| k<sub>Tp<sub> || 0.08min<sup>-1<sup> || Maximal Transcription rate of ptetR promoter || [https://2007.igem.org/Imperial/imperial/cell-free/characterisation iGEM 2007Imperial College London]
 +
|-
 +
| d<sub>Rm<sub> || 3.6 x 10<sup>-1</sup> min<sup>-1<sup> || Degradation rate of LuxR mRNA || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| k<sub>Rp<sub> || 9.6 x 10<sup>-1</sup> min<sup>-1<sup> || Rate of Lux protein translation || [http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
 +
|-
 +
| d<sub>Rp<sub> || 2.31 x 10<sup>-2</sup> min<sup>-1<sup> || Degration rate of LuxR protein ||[http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6T2K-4H4T39N-1&_user=121739&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_version=1&_urlVersion=0&_userid=121739&md5=08a37acb41420b0e80d3cde6ead4a347      Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.]
|-
|-
-
| R||CheR MW (kDa) = 33||RP437||140 ± 10. Value was determined in RP437 strain in rich medium.||[http://jb.asm.org/cgi/reprint/186/12/3687?maxtoshow=&HITS=10&hits=10&RESULTFORMAT=&author1=hazelbauer&searchid=1&FIRSTINDEX=0&resourcetype=HWCIT Cellular Stoichiometry of the Components of the Chemotaxis Signaling], [http://www.pdn.cam.ac.uk/groups/comp-cell/Rates.html Bray Computer Modelling Group]  
+
| k<sub>LuxR<sub> || 0.11 min<sup>-1<sup> || Maximal transcription rate of LuxR promoter || [https://2008.igem.org/team:kuleuven iGEM 2008 KULeuven ]
|-
|-
-
| B||CheB MW (kDa) = 37||RP437||240 ± 10,  Value was determined in RP437 strain in rich medium.||[http://jb.asm.org/cgi/reprint/186/12/3687?maxtoshow=&HITS=10&hits=10&RESULTFORMAT=&author1=hazelbauer&searchid=1&FIRSTINDEX=0&resourcetype=HWCIT Cellular Stoichiometry of the Components of the Chemotaxis Signaling], [http://www.pdn.cam.ac.uk/groups/comp-cell/Rates.html Bray Computer Modelling Group]  
+
| theta<sub>LuxR<sub> || 1.5 x 10<sup>-9</sup> M || Threshold for LuxR pR promoter Hill function || [https://2008.igem.org/team:kuleuven iGEM 2008 KULeuven ]
|-
|-
-
| W||CheW MW (kDa) = 18||RP437||6700 ± 890,  Value was determined in RP437 strain in rich medium.||[http://jb.asm.org/cgi/reprint/186/12/3687?maxtoshow=&HITS=10&hits=10&RESULTFORMAT=&author1=hazelbauer&searchid=1&FIRSTINDEX=0&resourcetype=HWCIT Cellular Stoichiometry of the Components of the Chemotaxis Signaling], [http://www.pdn.cam.ac.uk/groups/comp-cell/Rates.html Bray Computer Modelling Group]
+
| m<sub>LuxR<sub> || 1.6 || Co-operativity of LuxpR promoter Hill function || [https://2008.igem.org/team:kuleuven iGEM 2008 KULeuven ]
|-
|-
-
| A||CheA MW (kDa) = 71||RP437||CheA (total) =6700±1100, CheA (long) 4500±940, CheA (short) = 2200±520. The “short” form of kinase CheA results from an alternative translational start site in E. coli approximately 90 codons interior to the start site that generates the “long” form, CheAL. CheZ does still bind CheAs protein. Modest differences in growth phase can have significant effects on cellular content of chemotaxis components, as previously documented by Wang and Matsumura for CheAL and CheAS ||[http://jb.asm.org/cgi/reprint/186/12/3687?maxtoshow=&HITS=10&hits=10&RESULTFORMAT=&author1=hazelbauer&searchid=1&FIRSTINDEX=0&resourcetype=HWCIT Cellular Stoichiometry of the Components of the Chemotaxis Signaling], [http://www.pdn.cam.ac.uk/groups/comp-cell/Rates.html Bray Computer Modelling Group]
+
| rho<sub>C<sub> || 0.5 micro M<sup>-3</sup> min<sup>-1</sup> || LuxR/AHL dimerisation ||[http://www.nature.com/nature/journal/v434/n7037/full/nature03461.html A synthetic multicellular system for programmed pattern formation ]
|-
|-
-
| Y||CheY MW (kDa) = 14||Ratio of CheY:CheZ =2.3:1 ||Values for AW405 6850±1300 molecules/cell (or 27.2±5.2µM) for RP437 2750±275 (or 9.1±0.9µM). Tethering and swimming assays suggest ~30% of CheY is phosphorylated (Alon et al., 1998). Values in the literature for the same and different strains differ greatly but the ratios of CheY:CheZ are very similar (2.3:1). As the swarming ability between AW405 and RP347 are very similar it shows that the ratio rather than the actual numerical value of molecules per cell is the deciding factor. The different values between papers for the same species can be attributed to differences in protein expression and cell volume (this is very dependant on how the cells are grown). The lack of regulated conditions for cell growth mean that any value used in modelling will not be accurate. As the majority of values for molecules per cell are for RP347 use values for RP437|| [http://jb.asm.org/cgi/reprint/180/19/5123 CheZ Has No Effect on Flagellar Motors Activated by CheY13DK106YW ], [http://www.pdn.cam.ac.uk/groups/comp-cell/Rates.html Bray Computer Modelling Group], [http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=1170757 Response regulator output in bacterial chemotaxis]
+
| d<sub>C<sub> || 0.0231 min<sup>-1<sup> || Degradation rate of mCherry  mRNA ||[http://www.nature.com/nature/journal/v434/n7037/full/nature03461.html A synthetic multicellular system for programmed pattern formation ]
|-
|-
-
| Z||CheZ MW (kDa) = 24||24||3050 ±580 (12.1±2.3µM) (AW405), 1170 ± 170 (3.9±0.5µM) (RP437) the different values between papers for the same species can be attributed to differences in protein expression and cell volume (this is very dependant on how the cells are grown). The lack of regulated conditions for cell growth mean that any value used in modelling will not be accurate. As the majority of values for molecules per cell are for RP347 use values for RP437||[http://jb.asm.org/cgi/reprint/180/19/5123 CheZ Has No Effect on Flagellar Motors Activated by CheY13DK106YW ]
+
| d<sub>Mm<sub> || 1.65 x 10<sup>-3</sup> min<sup>-1<sup> || Degradation rate of LuxR/AHL complex ||Due to difficulty in finding mCherry modelling parameters, exsisting GFP parameters have been used. ||
|-
|-
-
| M||FliM MW (kDa) = 38||38||37±13 copies per flagella. Determined in salmonella but the value has be used by other groups when referring to E. coli||[http://jb.asm.org/cgi/content/abstract/178/1/258?ijkey=b6d6fd8a1c8564ac118449c4acdff535727e46d6&keytype2=tf_ipsecsha FliG and FliM distribution in the Salmonella typhimurium cell and flagellar basal bodies]
+
| k<sub>Mp<sub> || 2.4 x 10<sup>-1</sup> min<sup>-1<sup> || Rate of mCherry protein translation || Due to difficulty in finding mCherry modelling parameters, exsisting GFP parameters have been used. ||
|-
|-
-
| a||aspartate||N/A||N/A||
+
| d<sub>Mp<sub> || 2.14 x 10<sup>-4</sup> min<sup>-1<sup> || Degradation rate of mCherry protein || Due to difficulty in finding mCherry modelling parameters, exsisting GFP parameters have been used. ||
|}
|}

Latest revision as of 15:38, 26 September 2008

Modelling Parameters

Bacteria

Attribute Value Strain Justification Reference
Length2μmMG1655Values come from the University of Alberta’s datasheet on MG1655, produced to aid modelling. There is variability in size between strains - for instance, AW405 length varies between 1.5±0.2μm. But University of Alberta datasheet is specifically for MG1655.University of Alberta
Diameter0.8μmMG1655University of Alberta
ShapeCircle r =0.714μmMG1655Actually rod-like. A circle with r= 0.714μm will have equivalent surface area to rod-like.University of Alberta
Mass1.02x10-13gMG1655Given 1x10-12g for cell wet weight. Dividing this by gravity (=9.81) gives mass. University of Alberta
Swimming Speed50μms-1MG1655University Alberta's datasheet gives 50μms-1. However, Swimming speed is affected by:
  • Viscosity (as viscosity increases the speed increases to some maximum, then decreases as the viscosity increases further. E.coli (strain:KL227 of length: 1.0μm and diameter: 0.5μm) maximum speed occurs at viscosity 8cp.
  • Temperature
  • Culture medium
  • Vary strain to strain.
  • Experimental methods

Various papers give different speeds for E. coli (most papers provide information on AW405 with a speed of ~20μms-1). The speed itself is nearly uniform during the run. The wet lab may need to measure this experimentally as we are unaware of the conditions that the speed for MG1655 was obtained. Alberta's value is higher than other values, but this probably because MG1655 is a motile strain.

University of Alberta
A Method for Measuring Bacterial Chemotaxis Parameters in a Microcapillary

Run Tumble Motion

Attribute Value Strain Justification Reference
Aspartate concentration detected by E. coliOver ~5 orders of magnitude, 10nM up to 10mM. Can detect changes of as little as ~0.1%N/AE. coli detect small changes in concentration of 0.1% via temporal comparisons (4s) over a large range ( 10-8 to 10-3 ). Most computer simulations of chemotaxis are based on experimentally determined rates and concentrations. As a result they predict that the minimum detectable concentration of Aspartate is at ~200 nM. Experiments performed by Segall et al. in 1986, exposed tethered E. coli cells to iontophoretically delivered quantities of chemoattractant. These experiments indicated that a change in receptor occupancy of as little as 1/600 could produce an detectable change in swimming behaviour. With a Kd of 1 µM, this corresponds to a minimum detectable concentration of about 2 nM Aspartate. Wild type E. coli cells can detect <10nM of Asp and respond to Asp concentrations of upto 1mM,(responding to over ~5 orders of magnitude). M)Competitive and Cooperative Interactions in Receptor Signalling Complexes
Temporal comparison of chemotactic gradient4 secondsN/AThe past second has positive weighting, the previous 3 seconds have negative weighting. E coli compares past and present concentrations by comparing the average occupancy of the receptors over the 4s. Models reflecting this system have been developed by Segall et al and Schnitzer, cells compare their average receptor occupancy between 4 and 1 s ago c1-4 to the average receptor occupancy during the last second c0-1 . Hence b= c0-1 - c1-4 . If b>0, the cell reduces the tumbling rate to Ttumbling from the ambient value T0 , 1s-1 e.g. b>0 don't tumble. b< 0, tumble at a rate of 1s-1 Temporal comparisons in bacterial chemotaxis
Quantitative analysis of signalling networks
Motility of Escherichia coli cells in clusters formed by chemotactic aggregation
Tumbling angleShape parameter 4 Scale parameter 18.32 Location parameter -4.6AW405The tumble angle appears not to be dependant on the concentration gradient of chemoattractants/repellents. Nor is there correlation between the length of the run and the change in direction. The program uses a gamma distribution that fits the data collected by Berg and Brown. Several groups though, have observed that the tumble angle is not noramlly distributed but suggest that non-normality was only due to the experimental methods used e.g. in the capillary tube. Tumbling can cause a change in direction when as few as one flagella moves out of the bundle. Chemotaxis in E. coli anaylsed by three-dimensions
AgentCell: a digital single-cell assay for bacterial chemotaxis
On Torque and tumbling in swimming Escherichia coli
Tumble angle directionBidirectionalAW405Personal communication with Howard Berg. 'The direction is random, more or less, but there is a slight forward bias. It varies from tumble to tumble. The turn-angle distribution peaks at 68° rather than 90°. Tumbles turn out to be more complex than believed in 1972. Motors switch independently, and a tumble can occur if one or just a few motors change their directions of rotation. Tumbles are short, as judged by the tracking microscope, because they involve filament physics rather than motor physics: a transformation in polymorphic form, following motor reversal, from normal to semi-coiled. See Darnton, N.C., Turner, L., Rojevsky, S. and Berg, H.C. On torque and tumbling in swimming Escherichia coli, J. Bacteriol. 189, 1756-1764 (2007).'
Tumbling time0.14±0.19sAW405Exponential distribution fitted (stated to be exponential by Berg and Brown) using only the mean tumble length (not STDEV).Chemotaxis in E. Coli anaylsed by three-dimensional tracking
Relationship between tumbling angle and time
Speed while Tumbling0μm.s-1AW405Berg and Brown noted that AW405 slowed/stopped while tumbling.Chemotaxis in E. Coli anaylsed by three-dimensional tracking
Drift during run23±23°AW405Drift was observed. It is what would be expected from rotational diffusion. (at 2.7cp at 32ºC drift was 23±23°). Rotational Brownian motion cause the cell to veer off course, so that in between tumbles the probability density function f of the swimming direction e evolves according to the Fokker-Planck equation. Drift velocity in steep gradient of attractant ~7 µm.s-1(Berg & Turner, 1990. Note our model did not include the effects of driftChemotaxis in E. Coli anaylsed by three-dimensional tracking
Persistence of direction increases the drift velocity of run and tumble chemotaxis
Bray computer modelling
ThrustDown an Asp gradient 0.41pN, Up an Asp gradient 0.4387pN AW405Average thrust =0.41pN. In the Berg and Brown paper it states that the speed of the bacteria up an aspartate chemotactic gradient increases by 7%. Therefore in our model we shall use the following; thrust DOWN the Asp gradient =0.41pN, up the Asp gradient = 0.4387pN. Data was obtained from 32 AW405s, a strain which has provided the majority of our previous parameters but is not as motile as MG1655. The value was obtained at 23ºC in viscosity 0.93 and 3.07 cP for motility buffer and motility buffer with 0.18% methylcellulose, respectively. The standard deviation is not used as the speed is fixed at 50µm.s-1 . 0.57pN is the average thrust generated in strain HCB30 (a non tumbling strain). The thrust value was obtained when the imposed flow (U) U=0 at 23ºC. O.41pN was calculated using the resistance force theory treating the flagellar bundle as a single filament. The body was assumed to be prolate elipsoid using values roughly similar to ours, 2μm for length and 0.86μm for diameter. Chemotaxis in E. Coli anaylsed by three-dimensional tracking
On Torque and Tumbling in Swimming E. coli
Swimming efficiency of bacterium E. coli.
Isotropic run lengths0.86±1.18sAW405Exponential distribution fitted, this is only an approximate and does not fit exactly (see fig.4 Berg and Brown) The standard deviation is the standard deviation of the mean and has not been used in the exponential distributionChemotaxis in E. Coli anaylsed by three-dimensional tracking
Run length UP Aspartate gradient1.07±1.80sAW405Exponential distribution fitted, this is only an approximate and does not fit exactly (see fig.6, Berg and Brown). The standard deviation is the standard deviation of the mean and has not been used in the exponential distribution. Chemotaxis in E. Coli anaylsed by three-dimensional tracking
UCSF wiki
Run length DOWN Aspartate gradient0.8±1.38sAW405Exponential distribution fitted, this is only an approximate and does not fit exactly (see fig.6, Berg and Brown) The standard deviation is the standard deviation of the mean and has not been used in the exponential distributionChemotaxis in E. Coli anaylsed by three-dimensional tracking
ViscosityViscosity of water is 1.002cP at 20°CN/AAt present the medium being used by the lab is still be discussed. Currently though the medium most resembles water and therefore the water's viscosity value can be used. This allows us to assume that the medium is Newtonian (dilute aqueous medium that doesn’t contain long unbranched molecules such as methylcellulose or polyvinylpyrrolidone. Note that methlycellulose does not alter the run and tumble statistics, only bundle and motor rotation rates are affected by the addition of methylcellulose). If agar were to be used then the medium would be Non-Newtonian. Even though it would be Non- Newtonian John Hogan in passing said that we could assume it is Newtonian.The rotary motor of bacterial flagella., On Torque and Tumbling in swimming Escherichia coli

GRN Modelling

Parameter Value Description Reference
CpMax Unknown (varied in the program)Maximal CpxR protein concentration
kCp 0.075min-1
ESTIMATED
Maximal transcription rate of pCpxR promoter Surface Sensing and Adhesion of Escherichia Coli controlled by the cpx-signalling pathway.
thetaCpx 1 x 10-9 M
ESTIMATED
Threshold for pCpxR promoter Hill Function iGEM 2008 KULeuven
mCpx 1.0 Co-operativity of pCpxR promoter Hill function
dIm 3.6 x 10-1 min-1 Degradation rate of GFP mRNA Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
kIp 9.6 x 10-1 min-1 Rate of LuxI protein translation Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
dIp 1.67 x 10-2 min-1 Degradation rate of LuxI protein Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
dGm 1.65 x 10-3 min-1 Degradation rate of GFP protein Efficient GFP mutations profoundly affect mRNA transcription and translation rates
kGp 2.4 x 10-1 min-1 Rate of GFP protein translation Quantitative measurement of green fluorescent protein expression
dGp 2.14 x 10-4 min-1 Degradation rate of GFP protein Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
Aprod 3.6 min-1 AHL production rate per LuxI enzyme [Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
dA 1 x 10-2 min-1 Degradation rate of AHL molecule A synthetic multicellular system for programmed pattern formation
DA 0.23s-1 Diffusion coefficient of AHL Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
kTp 0.08min-1 Maximal Transcription rate of ptetR promoter iGEM 2007Imperial College London
dRm 3.6 x 10-1 min-1 Degradation rate of LuxR mRNA Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
kRp 9.6 x 10-1 min-1 Rate of Lux protein translation Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
dRp 2.31 x 10-2 min-1 Degration rate of LuxR protein Systems Analysis of a quorum sensing network: Design constraints imposed by the functional requirements, network topology and kinetic constants.
kLuxR 0.11 min-1 Maximal transcription rate of LuxR promoter iGEM 2008 KULeuven
thetaLuxR 1.5 x 10-9 M Threshold for LuxR pR promoter Hill function iGEM 2008 KULeuven
mLuxR 1.6 Co-operativity of LuxpR promoter Hill function iGEM 2008 KULeuven
rhoC 0.5 micro M-3 min-1 LuxR/AHL dimerisation A synthetic multicellular system for programmed pattern formation
dC 0.0231 min-1 Degradation rate of mCherry mRNA A synthetic multicellular system for programmed pattern formation
dMm 1.65 x 10-3 min-1 Degradation rate of LuxR/AHL complex Due to difficulty in finding mCherry modelling parameters, exsisting GFP parameters have been used.
kMp 2.4 x 10-1 min-1 Rate of mCherry protein translation Due to difficulty in finding mCherry modelling parameters, exsisting GFP parameters have been used.
dMp 2.14 x 10-4 min-1 Degradation rate of mCherry protein Due to difficulty in finding mCherry modelling parameters, exsisting GFP parameters have been used.