Team:ETH Zurich/modeling/int

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m (Parameter fitting)
m (Parameter fitting)
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[[File:ETH Zurich Integrase SR1.png|center|800px|thumb|Parameter fitting of the dissociate rate constant of K<sub>SABxb1</sub>]]
[[File:ETH Zurich Integrase SR1.png|center|800px|thumb|Parameter fitting of the dissociate rate constant of K<sub>SABxb1</sub>]]
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;We assume that:
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We assume that:
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:d<sub>Bxb1</sub> corresponds to the order of magnitude of 10<sup>-2</sup> min<sup>-1</sup>, as most of the protein in ''E. coli'' <sup>[[Team:ETH_Zurich/project/references#refDegProtein|[17]]]</sup>.
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* d<sub>Bxb1</sub> corresponds to the order of magnitude of 10<sup>-2</sup> min<sup>-1</sup>, as most of the protein in ''E. coli'' <sup>[[Team:ETH_Zurich/project/references#refDegProtein|[17]]]</sup>.
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:k<sub>mRNA<sub>Bxb1</sub></sub> is of the order of magnitude 10<sup>-1</sup> min<sup>-1</sup> mRNA<sup>-1</sup>. We estimated to be a low value because the starting codon of Bxb1 is GTG (and not ATG) and this parameter also takes into account folding time.
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* k<sub>mRNA<sub>Bxb1</sub></sub> is of the order of magnitude 10<sup>-1</sup> min<sup>-1</sup> mRNA<sup>-1</sup>. We estimated to be a low value because the starting codon of Bxb1 is GTG (and not ATG) and this parameter also takes into account folding time.
Thus, K<sub>SABxb1</sub>'s order of magnitude is 10<sup>-6</sup> nM. The interpretation of this dissociation constant is that the DNA binding reaction is really specific, as it can be expected for integrases.
Thus, K<sub>SABxb1</sub>'s order of magnitude is 10<sup>-6</sup> nM. The interpretation of this dissociation constant is that the DNA binding reaction is really specific, as it can be expected for integrases.

Revision as of 16:08, 12 October 2014

iGEM ETH Zurich 2014