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Team:Hong Kong HKUST/pneumosensor/characterization
From 2014.igem.org
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<p><br><b><u>Introduction</u></b> <br><br> | <p><br><b><u>Introduction</u></b> <br><br> | ||
| - | <p class="first_letter_enhanced">To test the functionality of σ<sup>X</sup>, we first enable constitutive expression of σ<sup>X</sup> in the σ<sup>X</sup> Generator, <a href= "http://parts.igem.org/Part:BBa_K1379006">BBa_K1379006</a>.The generator was then assembled with the standard promoter measurement kit <a href= "http://parts.igem.org/Part:BBa_E0240">BBa_E0240</a>, with either promoter P<sub> | + | <p class="first_letter_enhanced">To test the functionality of σ<sup>X</sup>, we first enable constitutive expression of σ<sup>X</sup> in the σ<sup>X</sup> Generator, <a href= "http://parts.igem.org/Part:BBa_K1379006">BBa_K1379006</a>.The generator was then assembled with the standard promoter measurement kit <a href= "http://parts.igem.org/Part:BBa_E0240">BBa_E0240</a>, with either promoter P<sub>celA</sub> (Promoter only: <a href= "http://parts.igem.org/Part:BBa_K1379000">BBa_K1379000</a>, w/ <a href= "http://parts.igem.org/Part:BBa_E0240">BBa_E0240</a>: <a href= "http://parts.igem.org/Part:BBa_K1379002">BBa_K1379002</a>) and P<sub>comFA</sub> (Promoter only: <a href= "http://parts.igem.org/Part:BBa_K1379001">BBa_K1379001</a>, w/ <a href= "http://parts.igem.org/Part:BBa_E0240">BBa_E0240</a>: <a href= "http://parts.igem.org/Part:BBa_K1379003">BBa_K1379003</a>). <i>E. coli</i> colonies holding the resulting constructs in pSB3K3 were observed under fluorescent macroscope with UV filter. Measurement kit for standard reference promoter <a href= "http://parts.igem.org/Part:BBa_J23101">BBa_J23101</a>, which is <a href= "http://parts.igem.org/Part:BBa_I20260">BBa_I20260</a> was used as a positive control; <a href= "http://parts.igem.org/Part:BBa_E0240">BBa_E0240</a> was used as the general negative control. for background fluorescence. Measurement kits for P<sub>celA</sub> P<sub>comFA</sub> without σ<sup>X</sup> Generator were used as negative controls for function of σ<sup>X</sup>. |
<br> | <br> | ||
</p><br><br> | </p><br><br> | ||
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<div class="content_image"> | <div class="content_image"> | ||
<img src= "https://static.igem.org/mediawiki/2014/4/43/PxhvV%26PcomFA_WIKI_copy.png"/> | <img src= "https://static.igem.org/mediawiki/2014/4/43/PxhvV%26PcomFA_WIKI_copy.png"/> | ||
| - | <h5 style="font-size: 13px">Figure 1. P<sub> | + | <h5 style="font-size: 13px">Figure 1. P<sub>celA</sub> and P<sub>comFA</sub> promoters activated in presence of σ<sup>X</sup>.</h5> |
| - | <h6 style= "font-size: 13px"> Only in the presence of σ<sup>X</sup> would P<sub> | + | <h6 style= "font-size: 13px"> Only in the presence of σ<sup>X</sup> would P<sub>celA</sub> and P<sub>comFA</sub> be turned on, as GFP expression could be seen when σ<sup>X</sup> present. Therefore, σ<sup>X</sup> is functional. P<sub>celA</sub> and P<sub>comFA</sub> gave little GFP signal in the absence of σ<sup>X</sup> but has comparable activity as reference promoter BBa_J23101 in presence of σ<sup>X</sup>. Scale bar = 5mm.</h6> |
</div> | </div> | ||
</div> | </div> | ||
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| - | <div class='content_1'><h3> <a href= "http://parts.igem.org/Part:BBa_K1379000">P<sub> | + | <div class='content_1'><h3> <a href= "http://parts.igem.org/Part:BBa_K1379000">P<sub>celA</sub> (BBa_K1379000) </a></h3> |
<table class="content_table" align= "center" > | <table class="content_table" align= "center" > | ||
<tr class= "content_row"> | <tr class= "content_row"> | ||
<td class= "content_cell"> | <td class= "content_cell"> | ||
<div class= "content_area_one_row"> | <div class= "content_area_one_row"> | ||
| - | <p class="first_letter_enhanced">To measure the R.P.U (Relative Promoter Unit) of P<sub> | + | <p class="first_letter_enhanced">To measure the R.P.U (Relative Promoter Unit) of P<sub>celA</sub> promoter, we adopted the method described by Kelly et al. in “Measuring the activity of BioBrick promoters using an in vivo reference standard” (Kelly et al., 2009). By linking P<sub>celA</sub> promoter with GFP generator (BBa_E0240), the promoter activity was represented by the GFP synthesis rate. Fluorescence was measured using EnVision multilabel reader from Perkin Elmer Company, when the cells are in the mid-log phase. OD595 values were measured and converted to OD600 to obtain the R.P.U of the promoter. The σ<sup>x</sup> gene and P<sub>celA</sub> promoter used in the construct are both cloned from <i>E. coli</i> NCTC 7465 strain. The experimental construct used was BBa_K1379005, which contain σ<sup>x</sup> generator, P<sub>celA</sub>, and GFP generator. The positive control used in this characterization is BBa_I20260 which is a constitutive promoter containing GFP generator, while the negative control used in this characterization is BBa_K1379002 which is P<sub>celA</sub> promoter with GFP generator but without σ<sup>x</sup> generator.<br> </p> |
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<div class="content_image"> | <div class="content_image"> | ||
<img src= "https://static.igem.org/mediawiki/2014/6/6d/PchbB_prism_Large.png"/><br> | <img src= "https://static.igem.org/mediawiki/2014/6/6d/PchbB_prism_Large.png"/><br> | ||
| - | <h5 style="font-size: 13px">Figure 2. P<sub> | + | <h5 style="font-size: 13px">Figure 2. P<sub>celA</sub> promoter Relative Promoter Unit (RPU) is measured with reference to J23101 constitutive promoter.</h5> |
| - | <h6 style= "font-size: 13px"> P<sub> | + | <h6 style= "font-size: 13px"> P<sub>celA</sub> promoter induced by σ<sup>x</sup> gave GFP signals. This fluorescence expression was measured over time, and divided by the OD of the cells. In the end, it was standardized based on J23101 promoter strength. Measurement was done by using 3 replicas.</h6> |
</div> | </div> | ||
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| - | <div class='content_1'><h3>P<sub> | + | <div class='content_1'><h3>P<sub>celA</sub> Characterization Method</a></h3> |
<table class="content_table" align= "center" > | <table class="content_table" align= "center" > | ||
<tr class= "content_row"> | <tr class= "content_row"> | ||
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<p><br><u><b>Characterization Procedure</b></u><br><br> | <p><br><u><b>Characterization Procedure</b></u><br><br> | ||
| - | 1. Constructing BBa_K1379005-pSB3K3 (σ<sup>x</sup> Generator (BBa_K1379006)-P<sub> | + | 1. Constructing BBa_K1379005-pSB3K3 (σ<sup>x</sup> Generator (BBa_K1379006)-P<sub>celA</sub>-BBa_E0240-pSB3K3) ,Transforming BBa_K1379002-pSB3K3 (P<sub>celA</sub>-BBa_E0240-pSB3K3), Transforming BBa_I20260-pSB3K3 (Standard Constitutive Promoter/Reference Promoter) from the 2014 Distribution Kit, Transforming BBa_E0240-pSB3K3 (GFP generator) from the 2014 Distribution Kit.<br><br> |
2. Preparing supplemented M9 medium (M9 Minimal salt medium protocols could be seen on the protocols page) <br><br> | 2. Preparing supplemented M9 medium (M9 Minimal salt medium protocols could be seen on the protocols page) <br><br> | ||
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3. GFP synthesis rate was then obtained by calculating the slope of the above mentioned curve; <br><br> | 3. GFP synthesis rate was then obtained by calculating the slope of the above mentioned curve; <br><br> | ||
| - | 4. Absolute promoter activity of P<sub> | + | 4. Absolute promoter activity of P<sub>celA</sub> and I20260 were calculated by dividing the GFP synthesis rate of BBa_K1379005-pSB3K3, BBa_K1379002-PSB3K3, and BBa_I20260-pSB3K3 over the average OD600 value; <br><br> |
5. Averaged absolute promoter activity was then obtained by averaging the respective 3 sets of absolute promoter activity values; <br><br> | 5. Averaged absolute promoter activity was then obtained by averaging the respective 3 sets of absolute promoter activity values; <br><br> | ||
| - | 6. Finally, R.P.U was calculated by dividing the averaged P<sub> | + | 6. Finally, R.P.U was calculated by dividing the averaged P<sub>celA</sub> absolute promoter activity over the averaged I20260 absolute promoter activity. R.P.U value of BBa_K1379005-pSB3K3 reflect the maximum GFP expression of PcelA promoter in the presence of σ<sup>x</sup>. Leakage could be analyzed according to the R.P.U value of BBa_K1379002-PSB3K3 which shows the GFP expression of P<sub>celA</sub> promoter without σ<sup>x</sup>.<br><br> |
</p> | </p> | ||
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<td class= "content_cell"> | <td class= "content_cell"> | ||
<div class= "content_area_one_row"> | <div class= "content_area_one_row"> | ||
| - | <p class="first_letter_enhanced">The method of measuring RPU (Relative Promoter Unit) of P<sub>comFA</sub> promoter is similar to measuring RPU of P<sub> | + | <p class="first_letter_enhanced">The method of measuring RPU (Relative Promoter Unit) of P<sub>comFA</sub> promoter is similar to measuring RPU of P<sub>celA</sub> which adopted the method described by Kelly et al. in “Measuring the activity of BioBrick promoters using an in vivo reference standard” (Kelly et al., 2009). There are no difference in measurement condition of measuring P<sub>comFA</sub> and P<sub>celA</sub>. Fluorescence and absorbance are measured in the same time period. The experimental construct used was BBa_K1379007, which contain σ<sup>x</sup> generator, P<sub>comFA</sub>, and GFP generator. The positive control used in this characterization is BBa_I20260 which is a constitutive promoter containing GFP generator, while the negative control used in this characterization is BBa_K1379002 which is P<sub>comFA</sub> promoter with GFP generator but without σ<sup>x</sup> generator. </p> |
</div> | </div> | ||
</td> | </td> | ||
Revision as of 12:29, 10 October 2014
Pneumosensor Characterization
σx(BBa_K1379004)
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To test the functionality of σX, we first enable constitutive expression of σX in the σX Generator, BBa_K1379006.The generator was then assembled with the standard promoter measurement kit BBa_E0240, with either promoter PcelA (Promoter only: BBa_K1379000, w/ BBa_E0240: BBa_K1379002) and PcomFA (Promoter only: BBa_K1379001, w/ BBa_E0240: BBa_K1379003). E. coli colonies holding the resulting constructs in pSB3K3 were observed under fluorescent macroscope with UV filter. Measurement kit for standard reference promoter BBa_J23101, which is BBa_I20260 was used as a positive control; BBa_E0240 was used as the general negative control. for background fluorescence. Measurement kits for PcelA PcomFA without σX Generator were used as negative controls for function of σX.
Figure 1. PcelA and PcomFA promoters activated in presence of σX.Only in the presence of σX would PcelA and PcomFA be turned on, as GFP expression could be seen when σX present. Therefore, σX is functional. PcelA and PcomFA gave little GFP signal in the absence of σX but has comparable activity as reference promoter BBa_J23101 in presence of σX. Scale bar = 5mm. |
PcelA (BBa_K1379000)
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To measure the R.P.U (Relative Promoter Unit) of PcelA promoter, we adopted the method described by Kelly et al. in “Measuring the activity of BioBrick promoters using an in vivo reference standard” (Kelly et al., 2009). By linking PcelA promoter with GFP generator (BBa_E0240), the promoter activity was represented by the GFP synthesis rate. Fluorescence was measured using EnVision multilabel reader from Perkin Elmer Company, when the cells are in the mid-log phase. OD595 values were measured and converted to OD600 to obtain the R.P.U of the promoter. The σx gene and PcelA promoter used in the construct are both cloned from E. coli NCTC 7465 strain. The experimental construct used was BBa_K1379005, which contain σx generator, PcelA, and GFP generator. The positive control used in this characterization is BBa_I20260 which is a constitutive promoter containing GFP generator, while the negative control used in this characterization is BBa_K1379002 which is PcelA promoter with GFP generator but without σx generator. |
 Figure 2. PcelA promoter Relative Promoter Unit (RPU) is measured with reference to J23101 constitutive promoter.PcelA promoter induced by σx gave GFP signals. This fluorescence expression was measured over time, and divided by the OD of the cells. In the end, it was standardized based on J23101 promoter strength. Measurement was done by using 3 replicas. |
PcelA Characterization Method
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PcomFA(BBa_K1379001)
Figure 3. PcomFA promoter Relative Promoter Unit (RPU) is measured with reference to J23101 constitutive promoter.Phelicase promoter induced by σx gave GFP signals. This fluorescence expression was measured over time, and divided by the OD of the cells. In the end, it was standardized based on J23101 promoter strength. Measurement was done by using 3 replicas. |
The method of measuring RPU (Relative Promoter Unit) of PcomFA promoter is similar to measuring RPU of PcelA which adopted the method described by Kelly et al. in “Measuring the activity of BioBrick promoters using an in vivo reference standard” (Kelly et al., 2009). There are no difference in measurement condition of measuring PcomFA and PcelA. Fluorescence and absorbance are measured in the same time period. The experimental construct used was BBa_K1379007, which contain σx generator, PcomFA, and GFP generator. The positive control used in this characterization is BBa_I20260 which is a constitutive promoter containing GFP generator, while the negative control used in this characterization is BBa_K1379002 which is PcomFA promoter with GFP generator but without σx generator. |
PcomFA Characterization Method
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J. R. Kelly, A. J. Rubin, J. H. Davis, J. Cumbers, M. J. Czar, ..., D. Endy. (2009). Measuring the activity of BioBrick promoters using an in vivo reference standard. Journal of Biological Engineering, 3, 4. doi: 10.1186/1754-1611-3-4 |
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