Team:UNIPV-Pavia/Project/Motivation2

From 2011.igem.org

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<table class='data' width='100%'>
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<tr>
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<td class="row"><b>RBS</b></td>
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<td class="row"><b>&alpha;<sub>p<sub>Lux</sub></sub> [(AUr/min)/cell]</b></td>
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<td class="row"><b>&delta;<sub>p<sub>Lux</sub></sub> [-]</b></td>
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<td class="row"><b>&eta;<sub>p<sub>Lux</sub></sub> [-]</b></td>
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<td class="row"><b>k<sub>p<sub>Lux</sub></sub> [ng/ml]</b></td>
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</tr>
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<tr><td class="row">BBa_B0030</td>
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<td class="row">438 [10]</td>
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<td class="row">0.05 [>100]</td>
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<td class="row">2 [47]</td>
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<td class="row">1.88 [27]</td>
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</tr>
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<tr><td class="row">BBa_B0031</td>
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<td class="row">9.8 [7]</td>
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<td class="row">0.11 [57]</td>
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<td class="row">1.2 [29]</td>
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<td class="row">1.5 [26]</td>
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</tr>
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<tr><td class="row">BBa_B0032</td>
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<td class="row">206 [3]</td>
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<td class="row">0 [>>100]</td>
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<td class="row">1.36 [10]</td>
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<td class="row">1.87 [9]</td>
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</tr>
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<tr><td class="row">BBa_B0034</td>
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<td class="row">1105 [6]</td>
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<td class="row">0.02 [>100]</td>
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<td class="row">1.33 [19]</td>
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<td class="row">2.34 [18]</td>
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</tr>
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</table>
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<div align="center">Data are provided as average [CV%].</div><br>
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Revision as of 19:40, 21 September 2011

UNIPV TEAM 2011

Results


Contents

NB: unless differently specified, all tests were performed in E. coli MGZ1 in M9 supplemented medium at 37°C. For the cloning of the parts, E. coli TOP10 was used.

Parts assembly

All the parts have been cloned with success. The part name, plasmids and quality controls are reported in the Freezer section.

Characterization of basic modules

Characterization of promoters pTet and pLux

Inducible and constitutive promoters were assembled upstream of different coding sequences containing an RBS from the Community collection.

The assembled RBSs are:


BioBrick code Declared efficiency
BBa_B0030 0,6
BBa_B0031 0,07
BBa_B0032 0,3
BBa_B0034 1

For an inducible device, the RBS variation has the purpose to stretch the induction curve, thus modulating its PoPs-OUT range.

The complex RBS-promoter acts as a whole regulatory element and determines the amount of translated protein. RBSs have been reported to have an un-modular behavior, since the translational efficiency is not independent on the coding sequences, but variates as an effect of different mRNA structure stability [Salis et al., Nat Biotec, 2009]. It is not possible to separate the effects of the sole promoter and of the sole RBS on the total amount/activity of gene product (in this case study, mRFP).

For this reason, every combination 'Promoter+RBS' was studied as a different regulatory element. Regulatory elements were characterized using mRFP reporter protein for different RBSs in terms of Synthesis rate per Cell (Scell) and R.P.U.s (Relative Promoter Units) as explained in measurements section.

Operative parameters of the promoter are derived from the estimated Hill equations obtained by nonlinear least squares fitting (lsqnonlin Matlab routine) of the Hill function expressed in RPUs:

    • RPUmax is equal to the α and represents the maximum promoter activity

    • RPUmin is equal to the α * δ represents the minimum promoter activity

    • Switch point is computed as the abscissa of the inflection point of the Hill curve and it is representative of the position of linear region

    • Linearity boundaries are determined as the intersection between the tangent line to the inflection point and the upper and lower horizontal boundaries of the Hill curve.

The estimated parameters for the Hill functions of pLux are summarized in the table below. For more details on parameter estimation, see the model section.

RBS αpLux [(AUr/min)/cell] δpLux [-] ηpLux [-] kpLux [ng/ml]
BBa_B0030 438 [10] 0.05 [>100] 2 [47] 1.88 [27]
BBa_B0031 9.8 [7] 0.11 [57] 1.2 [29] 1.5 [26]
BBa_B0032 206 [3] 0 [>>100] 1.36 [10] 1.87 [9]
BBa_B0034 1105 [6] 0.02 [>100] 1.33 [19] 2.34 [18]
Data are provided as average [CV%].

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