Team:Heidelberg/Notebook measure/NotebookFC
From 2009.igem.org
(Difference between revisions)
(→9-21-2009) |
(→10-14-2009) |
||
(35 intermediate revisions not shown) | |||
Line 1: | Line 1: | ||
__NOTOC__ | __NOTOC__ | ||
- | |||
{{Template_HD_3}} | {{Template_HD_3}} | ||
- | <html><body id=" | + | <html><body id="notebook"></body></html> |
{| | {| | ||
|-valign="top" border="0" | |-valign="top" border="0" | ||
|width="900px" style="padding: 0 20px 0 0; background-color:#ede8e2"| | |width="900px" style="padding: 0 20px 0 0; background-color:#ede8e2"| | ||
__NOTOC__ | __NOTOC__ | ||
- | |||
='''Notebook Flow Cytometry'''= | ='''Notebook Flow Cytometry'''= | ||
+ | |||
+ | == Contents == | ||
+ | |||
+ | {| class="wikitable centered" border="2" rules="rows" width="900px" style="border-color:white;" | ||
+ | |- | ||
+ | ! Week !! colspan="7" |Days | ||
+ | |- | ||
+ | |style="text-align:center"| 39 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#9-21-2009|9-21-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#9-24-2009|9-24-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#9-25-2009|9-25-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 40 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#9-28-2009|9-28-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#9-29-2009|9-29-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#9-30-2009|9-30-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-02-2009|10-02-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-03-2009|10-03-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |style="text-align:center"| 41 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-05-2009|10-05-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-07-2009|10-07-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-08-2009|10-08-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-09-2009|10-09-2009]] | ||
+ | |style="text-align:center"| | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-11-2009|10-11-2009]] | ||
+ | |- | ||
+ | |style="text-align:center"| 42 | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-12-2009|10-12-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-13-2009|10-13-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-14-2009|10-14-2009]] | ||
+ | |style="text-align:center"| [[Team:Heidelberg/Notebook_measure/NotebookFC#10-15-2009|10-15-2009]] | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |style="text-align:center"| - | ||
+ | |- | ||
+ | |} | ||
== 9-21-2009 == | == 9-21-2009 == | ||
* All cells for flow cytometry were transfected with the promoter of interest in front of GFP and the reference plasmid with JeT and mCherry in a 2:1 ratio. This ratio was chosen to ensure that we have GFP in every cell expressing mCherry and thereby increasing the number of double positive cells. | * All cells for flow cytometry were transfected with the promoter of interest in front of GFP and the reference plasmid with JeT and mCherry in a 2:1 ratio. This ratio was chosen to ensure that we have GFP in every cell expressing mCherry and thereby increasing the number of double positive cells. | ||
- | * Time course measurement of 24 and 96 well plate: Triplicates of cells transfected with the same promoter were loaded at different positions of the plates ( | + | * Time course measurement of 24 and 96 well plate (Fig. 1-2): Triplicates of cells transfected with the same promoter were loaded at different positions of the plates (Fig. 3-4) to ensure that the results do not change significantly over the time course of one flow cytometry measurement. |
{| | {| | ||
|-valign="top" border="0" | |-valign="top" border="0" | ||
|width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | |width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | ||
- | [[image:HD09_FACS_Time24well.PNG|center|400px|thumb|'''Figure 1: Time measurement 24 well.''' The bars indicate each triplicate | + | [[image:HD09_FACS_Time24well.PNG|center|400px|thumb|'''Figure 1: Time measurement 24 well.''' The bars indicate each triplicate located at a different position on the plate as shown in the scheme below. The standard deviations of the replicates are indicated by the error bars.]] |
- | |width=" | + | |width="400px"| |
- | [[image:HD09_FACS_Time96well2.PNG|center|400px|thumb|'''Figure 2: Time measurement 96 well.''' The bars indicate each triplicate | + | [[image:HD09_FACS_Time96well2.PNG|center|400px|thumb|'''Figure 2: Time measurement 96 well.''' The bars indicate each triplicate located at a different position on the plate as shown in the scheme below. The standard deviations of the replicates are indicated by the error bars.]] |
|} | |} | ||
Line 24: | Line 66: | ||
|-valign="top" border="0" | |-valign="top" border="0" | ||
|width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | |width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | ||
- | [[image:HD09_Hannah_24wellloadingscheme.JPG|center| | + | [[image:HD09_Hannah_24wellloadingscheme.JPG|center|200px|thumb|'''Table 1: 24 well loading scheme.''' The table represents the wells of a 24 well plate and the pink colored boxes indicating the loading wells.]] |
|width="450px"| | |width="450px"| | ||
- | [[image:HD09_Hannah_96wellloadingscheme.JPG|center| | + | [[image:HD09_Hannah_96wellloadingscheme.JPG|center|200px|thumb|'''Table 2: 96 well loading scheme.''' The table represents the wells of a 96 well plate and the pink colored boxes indicating the loading wells.]] |
|} | |} | ||
== 9-24-2009 == | == 9-24-2009 == | ||
- | * We performed standard measurements in HeLa, U2OS and MCF7 with our three standard promoters: CMV, JeT and JeT-CMV. These measurements were performed in 3 independent measurements. The initial results of U2OS standard are shown below, a standard measurement includes the constructs shown in table | + | * We performed standard measurements in HeLa, U2OS and MCF7 with our three standard promoters: CMV, JeT and JeT-CMV. These measurements were performed in 3 independent measurements. The initial results of U2OS standard are shown below (Fig. 3), a standard measurement includes the constructs shown in table 3. |
{| | {| | ||
Line 38: | Line 80: | ||
{| class="wikitable centered" style="margin: 1em auto 1em auto" | {| class="wikitable centered" style="margin: 1em auto 1em auto" | ||
|- style="background-color:#99cccc;" | |- style="background-color:#99cccc;" | ||
- | |style="text-align:center"|Sample | + | |style="text-align:center"|Table 3: Sample |
|- style="background-color:#9BDDFF;" | |- style="background-color:#9BDDFF;" | ||
|style="text-align:left"| negative control (transfection with a non-fluorescent plasmid p6) | |style="text-align:left"| negative control (transfection with a non-fluorescent plasmid p6) | ||
Line 62: | Line 104: | ||
|} | |} | ||
- | * We measured the constitutive promoters in the HeLa cell line. Unfortunately, the number of the viable cells are not enough for a reliable measurement. | + | * We measured the synthetic constitutive promoters in the HeLa cell line. Unfortunately, the number of the viable cells are not enough for a reliable measurement. |
== 9-25-2009 == | == 9-25-2009 == | ||
- | * Flow cytometric measurement of MCF-7 standard plate, which includes the same samples as above (see table | + | * Flow cytometric measurement of MCF-7 standard plate (Fig. 4), which includes the same samples as above (see table 3). |
[[image:HD09_2509_MCF7.png|center|440px|thumb|'''Figure 4: Flow cytometry results of the MCF-7 Standard plate (1st measurement).'''The three standard promoters CMV, JeT, and JeT_CMV were measured 20 hours after transfection of the MCF-7 cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above.The standard deviations of the replicates are also shown.]] | [[image:HD09_2509_MCF7.png|center|440px|thumb|'''Figure 4: Flow cytometry results of the MCF-7 Standard plate (1st measurement).'''The three standard promoters CMV, JeT, and JeT_CMV were measured 20 hours after transfection of the MCF-7 cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above.The standard deviations of the replicates are also shown.]] | ||
== 9-28-2009 == | == 9-28-2009 == | ||
- | * Second measurement of MCF-7 and U2-OS standard plates(same samples). | + | * Second measurement of MCF-7 (Fig. 6) and U2-OS (Fig. 5) standard plates(same samples). |
{| | {| | ||
Line 80: | Line 122: | ||
== 9-29-2009 == | == 9-29-2009 == | ||
- | * Third flow cytometry measurement of the MCF-7 and the U2-OS standard plates. Results are shown in the diagrams below. | + | * Third flow cytometry measurement of the MCF-7 (Fig. 8) and the U2-OS (Fig. 7) standard plates. Results are shown in the diagrams below. |
{| | {| | ||
Line 91: | Line 133: | ||
== 9-30-2009 == | == 9-30-2009 == | ||
- | * Second measurement of the constitutive promoters in HeLa. Results shown below. | + | * Second measurement of the synthetic constitutive promoters in HeLa. Results shown below (Fig. 9). |
[[image:HD09_3009_hela_const.png|center|800px|thumb|'''Figure 9: Flow cytometry results of the constitutive promoters in HeLa (1st measurement).'''The synthesized constitutive promoters of varying strength were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above.The standard deviations of the replicates are also shown .]] | [[image:HD09_3009_hela_const.png|center|800px|thumb|'''Figure 9: Flow cytometry results of the constitutive promoters in HeLa (1st measurement).'''The synthesized constitutive promoters of varying strength were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above.The standard deviations of the replicates are also shown .]] | ||
== 10-02-2009 == | == 10-02-2009 == | ||
- | * We measured the NFkB responsive promoter plate in U2-OS 10 hours | + | * We measured the synthetic NFkB responsive promoter plate in U2-OS after 10 hours of induction with TNF-alpha (Fig. 10). |
- | [[image:HD09_0210_U2os_nfkb.png|center|800px|thumb|'''Figure 10: Flow cytometry results of the NFkB responsive promoters in U2-OS (1st measurement).''' The .]] | + | [[image:HD09_0210_U2os_nfkb.png|center|800px|thumb|'''Figure 10: Flow cytometry results of the NFkB responsive promoters in U2-OS (1st measurement).''' The U2-OS cells were transfected with the different synthetic NFkB responsive promoters coupled to GFP. After 10 hours of induction with TNF-alpha the GFP fluorescence was measured by flow cytometry. The error bars represent the standard deviation.]] |
== 10-03-2009 == | == 10-03-2009 == | ||
- | * We measured the HIF responsive promoter in MCF-7. Unfortunately, the cell number was too low. | + | * We measured the synthetic HIF responsive promoter in MCF-7. Unfortunately, the cell number was too low. |
== 10-05-2009 == | == 10-05-2009 == | ||
- | * Three independent measurements of HeLa standard | + | * Three independent measurements of HeLa standard plates (Fig. 11-13), which include the same samples as above (see table 3) |
- | * We measured the constitutive promoters in the HeLa cell line again. Unfortunately, the number of the viable cells are not enough for a reliable measurement. | + | * We measured the synthetic constitutive promoters in the HeLa cell line again. Unfortunately, the number of the viable cells are not enough for a reliable measurement. |
- | * We measured the AhR responsive promoters and the natural promoter CYP1A1 (AhR responsive promoter) in HeLa. Unfortunately, the number of the viable cells are not enough for a reliable measurement. | + | * We measured the synthetic AhR responsive promoters and the natural promoter CYP1A1 (AhR responsive promoter) in HeLa. Unfortunately, the number of the viable cells are not enough for a reliable measurement. |
{| | {| | ||
Line 123: | Line 165: | ||
== 10-07-2009 == | == 10-07-2009 == | ||
- | * We measured the NFkB responsive promoter plate in U2-OS 10 hours | + | * We measured the synthetic NFkB responsive promoter plate in U2-OS after 10 hours of induction again (Fig. 14). |
- | [[image:HD09_0710_U2os_nfkb.png|center|700px|thumb|'''Figure 14: Flow cytometry results of the NFkB responsive promoters in U2-OS (2nd measurement).''' The .]] | + | [[image:HD09_0710_U2os_nfkb.png|center|700px|thumb|'''Figure 14: Flow cytometry results of the NFkB responsive promoters in U2-OS (2nd measurement).'''The U2-OS cells were transfected with the different synthetic NFkB responsive promoters coupled to GFP. After 10 hours of induction with TNF-alpha the GFP fluorescence was measured by flow cytometry. The error bars represent the standard deviation.]] |
== 10-08-2009 == | == 10-08-2009 == | ||
- | * We measured the Estrogen responsive promoter in MCF-7. Unfortunately, the number of the viable cells are not enough for a reliable measurement. | + | * We measured the synthetic Estrogen responsive promoter in MCF-7. Unfortunately, the number of the viable cells are not enough for a reliable measurement. |
== 10-09-2009 == | == 10-09-2009 == | ||
- | * Fourth measurement of the HeLa Standard plate. | + | * Fourth measurement of the HeLa Standard plate (Fig. 15). |
- | * We measured the SREBP responsive promoter in HeLa. | + | * We measured the synthetic SREBP responsive promoter in HeLa (induction with LDS). -> no successfull induction (Fig. 17). |
- | * Second measurement of the constitutive promoters in HeLa. | + | * Second measurement of the synthetic constitutive promoters in HeLa (Fig. 16). |
{| | {| | ||
Line 140: | Line 182: | ||
[[image:HD09_0910_Hela_stand.png|center|400px|thumb|'''Figure 15: Flow cytometry results of the HeLa Standard plate (4th measurement).''' The three standard promoters CMV, JeT, and JeT_CMV were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above. The standard deviations of the replicates are also shown.]] | [[image:HD09_0910_Hela_stand.png|center|400px|thumb|'''Figure 15: Flow cytometry results of the HeLa Standard plate (4th measurement).''' The three standard promoters CMV, JeT, and JeT_CMV were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above. The standard deviations of the replicates are also shown.]] | ||
|width="400px"| | |width="400px"| | ||
- | [[image:HD09_0910_Hela_const2.png|center|400px|thumb|'''Figure | + | [[image:HD09_0910_Hela_const2.png|center|400px|thumb|'''Figure 16: Flow cytometry results of the constitutive promoters in HeLa (2nd measurement).'''The synthesized constitutive promoters of varying strength were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above.The standard deviations of the replicates are also shown.]] |
|} | |} | ||
Line 146: | Line 188: | ||
|-valign="top" border="0" | |-valign="top" border="0" | ||
|width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | |width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | ||
- | [[image: | + | [[image:HD09_0910_Hela_srebp2.png|800px|center|thumb|'''Figure 17: Flow cytometry results of the SREBP responsive promoters in HeLa (1st measurement).''' The HeLa cells were transfected with different synthetic SREBP responsive promoters, which are coupled to the fluorescent protein GFP. The cells were measured with flow cytometry after induction with LDS (Lipoprotein Deficient Serum), full medium and Cholesterol + LDL. The induction substance LDS should activate the SREBP promoters and Cholesterol + LDL should inactivate the promoters. The error bars present the standard deviation.]] |
|} | |} | ||
== 10-11-2009 == | == 10-11-2009 == | ||
- | * We measured the natural promoter c-Jun (AP-1) in HeLa. | + | * We measured the natural promoter c-Jun (AP-1) in HeLa after induction with Epidermal Growth Factor (Fig. 18). |
- | + | ||
- | + | ||
+ | [[image:HD09_1110_c-jun.png|center|400px|thumb|'''Figure 18: Flow cytometry results of the natural promoter c-Jun (AP-1).''' The HeLa cells were transfected with the natural c-Jun promoter coupled to the fluorescent protein GFP. The c-Jun promoter is induced by Epidermal Growth Factor (diluted 1:2000 in DMEM++) for three hours. This GFP fluorescence is measured by flow cytometry. Besides, the standard deviation is also shown.]] | ||
== 10-12-2009 == | == 10-12-2009 == | ||
- | * Fifth measurement of the HeLa standard plate. Results shown below. | + | * Fifth measurement of the HeLa standard plate. Results shown below (Fig. 19). |
- | * Crossinduction of NF-kB responsive synthetic promoter NIIL10: We measured the promosing | + | * Crossinduction of NF-kB responsive synthetic promoter NIIL10 (Fig. 20): We measured the promosing NFkB responsive promoter NIIL10 (clone 31) in different media in U2-OS. Here, we want to see, if there is an induction of a nonspecific drug (Thiazolidinedione, 1:100 000) and how the different media affect the promoter activity. No significant change -> no influence/induction of the drug or medium. |
{| | {| | ||
Line 165: | Line 206: | ||
[[image:HD09_1210_Hela_stand.png|center|400px|thumb|'''Figure 19: Flow cytometry results of the HeLa Standard plate (5th measurement).''' The three standard promoters CMV, JeT, and JeT_CMV were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above. The standard deviations of the replicates are also shown.]] | [[image:HD09_1210_Hela_stand.png|center|400px|thumb|'''Figure 19: Flow cytometry results of the HeLa Standard plate (5th measurement).''' The three standard promoters CMV, JeT, and JeT_CMV were measured 20 hours after transfection of the HeLa cells and their Relative Expression Units (REU) normalized to the JeT promoter are shown above. The standard deviations of the replicates are also shown.]] | ||
|width="400px"| | |width="400px"| | ||
- | [[image: | + | [[image:HD09_U2os_cross.png|center|400px|thumb|'''Figure 20: Flow cytometry results of the NIIL10 (clone 31) promoter (NFkB responsive promoter) under different conditions in U2-OS.''' The U2-OS cells were transfected with the NIIL10 promoter (also clone 31), which is coupled to GFP. After induction with Thiazolidinedione (1:100 000) and different media the cells were measured by flow cytometry. The standard deviation is also shown.]] |
|} | |} | ||
== 10-13-2009 == | == 10-13-2009 == | ||
- | * We measured the p53 responsive promoter in MCF-7. Unfortunately, there were some problems with the flow cytometry analysis. | + | * We measured the synthetic p53 responsive promoter in MCF-7. Unfortunately, there were some problems with the flow cytometry analysis. |
== 10-14-2009 == | == 10-14-2009 == | ||
- | * We measured the standard CMV promoter under different conditions: full medium, minimal medium, and minimal medium + Erolimus. We wanted to check that CMV is comparable under different conditions. A fourth sample prepared at the same time will be measured after 50 hours to analyze the change of JeT and CMV over a long period of time. | + | * We measured the standard CMV promoter under different conditions (Fig. 21): full medium, minimal medium, and minimal medium + Erolimus. We wanted to check that CMV is comparable under different conditions. A fourth sample prepared at the same time will be measured after 50 hours to analyze the change of JeT and CMV over a long period of time. |
* Results of the first three measurements shown below. | * Results of the first three measurements shown below. | ||
- | [[image:HD09_FACS_cmv_medium_orange.PNG|center|400px|thumb|'''Figure 21: | + | [[image:HD09_FACS_cmv_medium_orange.PNG|center|400px|thumb|'''Figure 21: Flow cytometry results of the standard CMV promoter under different conditions''' The CMV promoter coupled to GFP was transfected into HeLa cells and its activity was tested under different conditionds: full medium, minimal medium, and minimal medium + Everolimus. The resulting GFP fluorescence were measured by flow cytometry. The standard deviations of the replicates are also shown.]] |
- | + | ||
- | + | ||
== 10-15-2009 == | == 10-15-2009 == | ||
- | * We measured the MCF-7 and U2-OS Standard plate (fourth measurements). | + | * We measured the MCF-7 (Fig. 22) and U2-OS (Fig. 23) Standard plate (fourth measurements). |
{| | {| | ||
Line 191: | Line 230: | ||
* We measured a second timepoint (after 50 hours) of the CMV promoter and added these results in the figure 21 (new figure 24, below). To check, if the GFP fluorescence changed after 50 hours. | * We measured a second timepoint (after 50 hours) of the CMV promoter and added these results in the figure 21 (new figure 24, below). To check, if the GFP fluorescence changed after 50 hours. | ||
+ | * Third measurement of NIIL10 (NFkb responsive) in U2-OS (Fig. 25). | ||
{| | {| | ||
|-valign="top" border="0" | |-valign="top" border="0" | ||
|width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | |width="400px" style="background-color:#ede8e5; padding: 0 20px 0 0;"| | ||
- | [[image:HD09_FACS_cmv_medium_with_time.PNG|center|400px|thumb|'''Figure 24: | + | [[image:HD09_FACS_cmv_medium_with_time.PNG|center|400px|thumb|'''Figure 24: Flow cytometry results of the standard CMV promoter under different conditions and time periods.''' The CMV promoter coupled to GFP was transfected into HeLa cells and its activity was tested under different conditionds: full medium, minimal medium, and minimal medium + Erolimus. Besides, its activity is measured after 50 hours by flow cytometry. The standard deviations of the replicates are also shown.]] |
|width="400px"| | |width="400px"| | ||
- | [[image:HD09_1510_u2os_nfkb.png|center|400px|thumb|Flow cytometry results of the NFkB responsive promoters in U2-OS ( | + | [[image:HD09_1510_u2os_nfkb.png|center|400px|thumb|'''Figure 25: Flow cytometry results of the synthetic NFkB responsive promoters in U2-OS (3nd measurement).''' The U2-OS cells were transfected with the NIIL10 promoter (also clone 31), which is coupled to GFP. After induction with TNF-alpha (10 hours) the cells were measured by flow cytometry. The standard deviations of the replicates are also shown.]] |
|} | |} |
Latest revision as of 23:35, 21 October 2009
Notebook Flow CytometryContents
9-21-2009
9-24-2009
9-25-2009
9-28-2009
9-29-2009
9-30-2009
10-02-2009
10-03-2009
10-05-2009
10-07-2009
10-08-2009
10-09-2009
10-11-2009
10-12-2009
10-13-2009
10-14-2009
10-15-2009
|