Team:Freiburg Transfection and Synthetic Receptor

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<font face="Arial Rounded MT Bold" style="color:#010369">_transfection and synthetic receptor activation  </font></div>
<font face="Arial Rounded MT Bold" style="color:#010369">_transfection and synthetic receptor activation  </font></div>
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<br><br>
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==Introduction==
+
<h2>Introduction</h2>
-
The functionality of our parts was analyzed in three steps. First, we tested the transfection protocol and checked the utility of the transfectionvector-CMV construct for expressing proteins in eucaryotic cells. Second, we analyzed protein expression level and cellular localization. Third, cotransfections were performed to show that clustering of two receptors leads to an assembly of the intracellular splitfluorophores/-enzymes resulting in a functional protein.
+
The functionality of our parts was analyzed in three steps. First, we tested the transfection protocol and checked the utility of the transfection vector CMV construct for expressing proteins in eucaryotic cells. Second, we analyzed protein expression level and cellular localization. Third, cotransfections were performed to show that clustering of two receptors leads to an assembly of the intracellular split fluorophores/-enzymes resulting in a functional protein.<br>  
-
==Methods==
+
-
'''Transfection of 293T cells'''<br>
+
-
One day before transfection cells were counted in the Neubauer chamber and 6*10^4 cells/cm² were seeded in 6 well plates. Approximately 1 hour before transfection cells were washed with 1xPBS and fresh DMEM medium was added. For transfection 2µg of DNA were mixed with 25µl CaCl2 and ddH2O was filled up to 250µl. After an incubation on ice for 20 min 250µl BBS (2x) were added. This mixture was given to the cells and after 4-12 hours cells were washed and fresh medium was added.<br>
+
<br>
<br>
-
'''ONPG Test'''<br>
+
<h2>Methods</h2>
-
Transfection was performed with a lac z gene using the transfection protocol described above. After 48h one part of the cells was harvested by washing them in PBS and scraping them off. Then the cells were centrifuged at 13000rpm for 2 min and the PBS was replaced by 500µl lysisbuffer (1x). Incubation took place at -80°C for 20min. After thawing the solution was vortexed, spun down and the supernatant was frozen at -20°C. The same procedure was done with the rest of the cells one day later (68h). Then 20µl of each lysate was given to 130µl reactionbuffer (incl. ONPG) letting the mixture incubate for 1h at 37°C. Measurement was done using the ELISA-reader at 405nm.<br>
+
<h4>Transfection of 293T cells</h4>
 +
One day before transfection cells were counted in the Neubauer chamber and 6*10^4 cells/cm² were seeded in 6 well plates. Approximately 1 hour before transfection cells were washed with 1xPBS and fresh DMEM medium was added. For transfection 2 µg of DNA were mixed with 25 µl CaCl2 and ddH2O was filled up to 250 µl. After an incubation on ice for 20 min 250 µl BBS (2x) were added. This mixture was given to the cells and after 4-12 hours cells were washed and fresh medium was added.<br>
 +
<h4>ONPG (o-Nitrophenyl-ß-D-galactopyranosid) Test</h4>
 +
Transfection was performed with a lac Z gene using the transfection protocol described above. After 48h one part of the cells was harvested by washing them in PBS and scraping them off. Then the cells were centrifuged at 13000 rpm for 2 min and the PBS was replaced by 500µl lysis buffer (1x). Incubation took place at -80°C for 20 min. After thawing, the solution was vortexed, spun down and the supernatant was frozen at -20°C. The same procedure was done with the rest of the cells one day later (68h). Then 20 µl of each lysate was given to 130 µl reaction buffer (incl. ONPG) letting the mixture incubate for 1h at 37°C. Measurement was done using the ELISA-reader at 405 nm.<br>
<br>
<br>
-
==Results==
+
<h2>Results and discussion</h2>
-
<h4>'''Testing the transfection protocol'''</h4>
+
<h3>Testing the transfection protocol</h3>
-
In order to check if the transfection protocol (Ca2+ precipitation) is suitable to transfect 293T cells a 'test'transfection with a lac z gene (Test-vector from Katja Arndt's lab) was done and the β-galactosidase was detected with an ONPG test.<br>
+
In order to check if the transfection protocol (Ca2+ precipitation) is suitable to transfect 293T cells a 'test'transfection with a lac Z gene (Test-vector from Katja Arndt's lab) was done and the β-galactosidase was detected with an ONPG test.<br>
<br>
<br>
ONPG-assay: <br>
ONPG-assay: <br>
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''Graph 1_Transfection: Absorbance of o-Nitrophenol produced by the β-galactosidase (Control was done with untransfected cells using the same procedure)''<br>
''Graph 1_Transfection: Absorbance of o-Nitrophenol produced by the β-galactosidase (Control was done with untransfected cells using the same procedure)''<br>
<br>
<br>
-
Due to the results of the ONPG assay the Ca2+ precipitation proofed to be a very simple and effective method to transfect the 293t cells.<br>
+
Due to the results of the ONPG assay, the Ca2+ precipitation proved to be a very simple and effective method to transfect the 293T cells.<br>
<br>
<br>
-
<h4>'''Testing the transfectionvector-CMV promoter construct'''</h4>
+
<h3>Testing the transfection vector CMV promoter construct</h3>
-
To test the functionality of the transfectionvector and the CMV-promoter (BBa_K157040), YFP was cloned behind the promoter and the plasmid was brought into 293T cells. The detection of YFP took place 1 day later under a microscope with YFP filter.<br>
+
To test the functionality of the transfection vector and the CMV-promoter (BBa_K157040), YFP was cloned downstream of the promoter and the plasmid was brought into 293T cells. The detection of YFP took place 1 day later under a microscope with YFP filter.<br>
-
The transfected cells show fluorescence  by excitation of 510-520nm while the untransfected remain dark at this wavelength demonstrating the capability of the transfectionvector-CMV construct to induce protein expression in eucaryotic cells.<br>
+
The transfected cells show fluorescence  by excitation of 510-520nm while the untransfected remain dark at this wavelength demonstrating the capability of the transfection vector CMV construct to induce protein expression in eucaryotic cells.<br>
<br>
<br>
[[Image:Freiburg2008_150%_293Tzvi.jpg]]  [[Image:Freiburg2008_Kontrolle.jpg]]  [[Image:Freiburg2008_Kontrolle_Durchlicht.jpg]]<br>
[[Image:Freiburg2008_150%_293Tzvi.jpg]]  [[Image:Freiburg2008_Kontrolle.jpg]]  [[Image:Freiburg2008_Kontrolle_Durchlicht.jpg]]<br>
''Figure 1_Transfection: Transfected 293T cells (left), untransfected cells (middle) and transfected cells transmitted light (right)''<br>
''Figure 1_Transfection: Transfected 293T cells (left), untransfected cells (middle) and transfected cells transmitted light (right)''<br>
<br>
<br>
-
<h4>'''Localization at the cell membrane'''</h4>
+
<h3>Localization at the cell membrane</h3>
-
To show the localization of the constructs at the cell membrane transfection of the construct signalpeptide-Lipocalin-transmembraneregion-betaLactamase1-YFP was performed.<br>
+
To show the localization of the constructs at the cell membrane transfection of the construct signal_peptide-Lipocalin-transmembrane_region-betaLactamase1-YFP was performed.<br>
-
Figure 2_Transfection shows the model of the protein structure based on PDB files. Anti-fluorescein Anticalin (BBa_K157004) is the extracellular part of the construct. The transmembrane region is identical to that of the EGF-receptor erbb1 (BBa_K157002). Split-beta-Lactamase (BBa_I757011), the intracellular part is labeled to the yellow fluorescent protein to detect membrane localization.<br>
+
Figure 2_Transfection shows the model of the protein structure based on PDB files. Anti-fluorescein Anticalin (BBa_K157004) is the extracellular part of the construct. The transmembrane region is identical to that of the EGF-receptor erbb1 (BBa_K157002). Split beta-Lactamase (BBa_I757011), the intracellular part is fused to the yellow fluorescent protein to detect membrane localization.<br>
<br>
<br>
[[Image:Freiburg2008_Lipo_bla1+YFP.jpg|500px]]
[[Image:Freiburg2008_Lipo_bla1+YFP.jpg|500px]]
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'''Figure 2_Transfection: Structure of the signalpeptide-Lipocalin-transmembraneregion-betaLactamase1-YFP construct. Extracellular: Lipocalin, GGGSlinker; Transmembrane: transmembraneregion of the EGF-receptor; Intracellular: Split-beta-Lactamase1, YFP.'''<br>
'''Figure 2_Transfection: Structure of the signalpeptide-Lipocalin-transmembraneregion-betaLactamase1-YFP construct. Extracellular: Lipocalin, GGGSlinker; Transmembrane: transmembraneregion of the EGF-receptor; Intracellular: Split-beta-Lactamase1, YFP.'''<br>
<br>
<br>
-
Membranelocalization of the construct signalpeptide-Lipocalin-transmembraneregion-betaLactamase1-YFP is visible in transfected 293T cells (Figure 3_Transfection). The fluorescence of the cells is most likely restricted to the cellmembrane as evident by the strong signal at the surface of the cell spheres confirming the assembly of the construct in the cytoplasmamembrane.<br>
+
Membrane localization of the construct signal_peptide-Lipocalin-transmembrane_region-betaLactamase1-YFP is visible in transfected 293T cells (Figure 3_Transfection). The fluorescence of the cells is most likely restricted to the cell membrane as evident by the strong signal at the surface of the cell spheres confirming the assembly of the construct in the cytoplasma membrane.<br>
-
In comparison, 293T cells transfected with the construct transfectionvector-CMV-YFP show a uniformly distributed fluorescence all over the cell (Figure 4_Transfection A and B).<br>
+
In comparison, 293T cells transfected with the construct transfection vector-CMV-YFP show a uniformly distributed fluorescence all over the cell (Figure 4_Transfection A and B).<br>
-
Transfection with the construct transfectionvector-CMV-CFP (BBa_K157041), i.e. without membrane targeting as well results in completely fluorescent cells (Figure 4_Transfection C and D).<br>  
+
Transfection with the construct transfection vector-CMV-CFP (BBa_K157041), i.e. without membrane targeting as well results in completely fluorescent cells (Figure 4_Transfection C and D).<br>  
<br>   
<br>   
[[Image:Freiburg2008_SP_LIPO_GGGS_TM_bla1_YFP_1.jpg|710px]]<br>
[[Image:Freiburg2008_SP_LIPO_GGGS_TM_bla1_YFP_1.jpg|710px]]<br>
-
'''Figure 3_Transfection: 293T cells transfected with signalpeptide-Lipocalin-transmembraneregion-betaLactamase1-YFP.<br> This picture demonstrates the high expression level of the fusionprotein and the localization at the cellmembrane obvious by the strong fluorescent signal at the cell surface'''<br>
+
'''Figure 3_Transfection: 293T cells transfected with signal_peptide-Lipocalin-transmembrane_region-betaLactamase1-YFP.<br> This picture demonstrates the high expression level of the fusion protein and the localization at the cell membrane obvious by the strong fluorescent signal at the cell surface'''<br>
<br>
<br>
[[Image:Freiburg2008_TV_CMV_YFP___CFP_loeslich.jpg|700px]]<br>
[[Image:Freiburg2008_TV_CMV_YFP___CFP_loeslich.jpg|700px]]<br>
-
'''Figure 4_Transfection: 293T cells transfected with transfectionvector-CMV-YFP (A and B); 293T cells transfected with transfectionvector-CMV-CFP (C and D)<br>Fluorescence is uniformly distributed all over the cell and not restricted to the cell membrane'''<br>
+
'''Figure 4_Transfection: 293T cells transfected with transfection vector-CMV-YFP (A and B); 293T cells transfected with transfection vector-CMV-CFP (C and D)<br>Fluorescence is uniformly distributed all over the cell and not restricted to the cell membrane'''<br>
<br>
<br>
-
<h4>'''Cotransfections with Splitfluorophor-/Splitenzyme-constructs'''</h4>
+
<h3>Cotransfections with Splitfluorophor-/Splitenzyme-constructs</h3>
-
Figure 5_Transfection gives the model of the Anticalin fused to the GGGSlinker, the transmembrane domain and the N-terminal part of Cerulean CFP or the C-terminal part of Cerulean CFP. To achieve more flexibility and to support the assembly of the two splitfluorophore parts a fluolinker is fused in between the transmembrane region and the C-terminal part of the splitfluorophores. The signalpeptide is not displayed. <br>
+
Figure 5_Transfection gives the model of the Anticalin fused to the GGGSlinker, the transmembrane domain and the N-terminal part of Cerulean CFP or the C-terminal part of Cerulean CFP. To achieve more flexibility and to support the assembly of the two split fluorophore parts a fluolinker is fused in between the transmembrane region and the C-terminal part of the split fluorophores. The signal peptide is not displayed. <br>
<br>
<br>
[[Image:Freiburg2008_Lipo+Split_CFP.jpg|450px]]<br>
[[Image:Freiburg2008_Lipo+Split_CFP.jpg|450px]]<br>
-
'''Figure 5_Transfection: Structures of the signalpeptide-Lipocalin-transmembraneregion-nCFP and signalpeptide-Lipocalin-transmembraneregion-fluolinker-cCFP constructs'''<br>
+
'''Figure 5_Transfection: Structures of the signal_peptide-Lipocalin-transmembrane_region-nCFP and signal_peptide-Lipocalin-transmembrane_region-fluolinker-cCFP constructs'''<br>
<br>
<br>
We hypothesize that adding fluorescein-coupled molecules leads to a clustering of the Lipocalin constructs due to the fluorescein-Lipocalin-binding.
We hypothesize that adding fluorescein-coupled molecules leads to a clustering of the Lipocalin constructs due to the fluorescein-Lipocalin-binding.
-
The clustering of the constructs in turn results in an assembly of the splitfluorophores or splitenzymes and therefore creates a functional protein (Figure 6_Transfection).<br>
+
The clustering of the constructs in turn results in an assembly of the split fluorophores or split enzymes and therefore creates a functional protein (Figure 6_Transfection).<br>
<br>
<br>
<br>
<br>
-
[[Image:Freiburg2008_Lipo+Split_YFP.jpg|450px]]<br>
+
[[Image:Korrektur_Freiburg2008_Lipo+Split_YFP.jpg|450px]]<br><br>
-
'''Figure 6_Transfection: Clustering and assembly of the signalpeptide-Lipocalin-transmembraneregion-nYFP and signalpeptide-Lipocalin-transmembraneregion-fluolinker-cYFP constructs'''<br>
+
'''Figure 6_Transfection: Clustering and assembly of the signal_peptide-Lipocalin-transmembrane_region-nYFP and signal_peptide-Lipocalin-transmembrane_region-fluolinker-cYFP constructs'''<br>
<br>
<br>
<br>
<br>

Latest revision as of 23:04, 29 October 2008


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_transfection and synthetic receptor activation



Contents

Introduction

The functionality of our parts was analyzed in three steps. First, we tested the transfection protocol and checked the utility of the transfection vector CMV construct for expressing proteins in eucaryotic cells. Second, we analyzed protein expression level and cellular localization. Third, cotransfections were performed to show that clustering of two receptors leads to an assembly of the intracellular split fluorophores/-enzymes resulting in a functional protein.

Methods

Transfection of 293T cells

One day before transfection cells were counted in the Neubauer chamber and 6*10^4 cells/cm² were seeded in 6 well plates. Approximately 1 hour before transfection cells were washed with 1xPBS and fresh DMEM medium was added. For transfection 2 µg of DNA were mixed with 25 µl CaCl2 and ddH2O was filled up to 250 µl. After an incubation on ice for 20 min 250 µl BBS (2x) were added. This mixture was given to the cells and after 4-12 hours cells were washed and fresh medium was added.

ONPG (o-Nitrophenyl-ß-D-galactopyranosid) Test

Transfection was performed with a lac Z gene using the transfection protocol described above. After 48h one part of the cells was harvested by washing them in PBS and scraping them off. Then the cells were centrifuged at 13000 rpm for 2 min and the PBS was replaced by 500µl lysis buffer (1x). Incubation took place at -80°C for 20 min. After thawing, the solution was vortexed, spun down and the supernatant was frozen at -20°C. The same procedure was done with the rest of the cells one day later (68h). Then 20 µl of each lysate was given to 130 µl reaction buffer (incl. ONPG) letting the mixture incubate for 1h at 37°C. Measurement was done using the ELISA-reader at 405 nm.

Results and discussion

Testing the transfection protocol

In order to check if the transfection protocol (Ca2+ precipitation) is suitable to transfect 293T cells a 'test'transfection with a lac Z gene (Test-vector from Katja Arndt's lab) was done and the β-galactosidase was detected with an ONPG test.

ONPG-assay:

FreiGEMTable3onpg.JPG
Table 1_Transfection: Absorbance of o-Nitrophenol produced by the β-galactosidase
Graph2onpg.JPG
Graph 1_Transfection: Absorbance of o-Nitrophenol produced by the β-galactosidase (Control was done with untransfected cells using the same procedure)

Due to the results of the ONPG assay, the Ca2+ precipitation proved to be a very simple and effective method to transfect the 293T cells.

Testing the transfection vector CMV promoter construct

To test the functionality of the transfection vector and the CMV-promoter (BBa_K157040), YFP was cloned downstream of the promoter and the plasmid was brought into 293T cells. The detection of YFP took place 1 day later under a microscope with YFP filter.
The transfected cells show fluorescence by excitation of 510-520nm while the untransfected remain dark at this wavelength demonstrating the capability of the transfection vector CMV construct to induce protein expression in eucaryotic cells.

Freiburg2008 150% 293Tzvi.jpg Freiburg2008 Kontrolle.jpg Freiburg2008 Kontrolle Durchlicht.jpg
Figure 1_Transfection: Transfected 293T cells (left), untransfected cells (middle) and transfected cells transmitted light (right)

Localization at the cell membrane

To show the localization of the constructs at the cell membrane transfection of the construct signal_peptide-Lipocalin-transmembrane_region-betaLactamase1-YFP was performed.
Figure 2_Transfection shows the model of the protein structure based on PDB files. Anti-fluorescein Anticalin (BBa_K157004) is the extracellular part of the construct. The transmembrane region is identical to that of the EGF-receptor erbb1 (BBa_K157002). Split beta-Lactamase (BBa_I757011), the intracellular part is fused to the yellow fluorescent protein to detect membrane localization.

Freiburg2008 Lipo bla1+YFP.jpg
Figure 2_Transfection: Structure of the signalpeptide-Lipocalin-transmembraneregion-betaLactamase1-YFP construct. Extracellular: Lipocalin, GGGSlinker; Transmembrane: transmembraneregion of the EGF-receptor; Intracellular: Split-beta-Lactamase1, YFP.

Membrane localization of the construct signal_peptide-Lipocalin-transmembrane_region-betaLactamase1-YFP is visible in transfected 293T cells (Figure 3_Transfection). The fluorescence of the cells is most likely restricted to the cell membrane as evident by the strong signal at the surface of the cell spheres confirming the assembly of the construct in the cytoplasma membrane.
In comparison, 293T cells transfected with the construct transfection vector-CMV-YFP show a uniformly distributed fluorescence all over the cell (Figure 4_Transfection A and B).
Transfection with the construct transfection vector-CMV-CFP (BBa_K157041), i.e. without membrane targeting as well results in completely fluorescent cells (Figure 4_Transfection C and D).

Freiburg2008 SP LIPO GGGS TM bla1 YFP 1.jpg
Figure 3_Transfection: 293T cells transfected with signal_peptide-Lipocalin-transmembrane_region-betaLactamase1-YFP.
This picture demonstrates the high expression level of the fusion protein and the localization at the cell membrane obvious by the strong fluorescent signal at the cell surface

Freiburg2008 TV CMV YFP CFP loeslich.jpg
Figure 4_Transfection: 293T cells transfected with transfection vector-CMV-YFP (A and B); 293T cells transfected with transfection vector-CMV-CFP (C and D)
Fluorescence is uniformly distributed all over the cell and not restricted to the cell membrane

Cotransfections with Splitfluorophor-/Splitenzyme-constructs

Figure 5_Transfection gives the model of the Anticalin fused to the GGGSlinker, the transmembrane domain and the N-terminal part of Cerulean CFP or the C-terminal part of Cerulean CFP. To achieve more flexibility and to support the assembly of the two split fluorophore parts a fluolinker is fused in between the transmembrane region and the C-terminal part of the split fluorophores. The signal peptide is not displayed.

Freiburg2008 Lipo+Split CFP.jpg
Figure 5_Transfection: Structures of the signal_peptide-Lipocalin-transmembrane_region-nCFP and signal_peptide-Lipocalin-transmembrane_region-fluolinker-cCFP constructs

We hypothesize that adding fluorescein-coupled molecules leads to a clustering of the Lipocalin constructs due to the fluorescein-Lipocalin-binding. The clustering of the constructs in turn results in an assembly of the split fluorophores or split enzymes and therefore creates a functional protein (Figure 6_Transfection).


Korrektur Freiburg2008 Lipo+Split YFP.jpg

Figure 6_Transfection: Clustering and assembly of the signal_peptide-Lipocalin-transmembrane_region-nYFP and signal_peptide-Lipocalin-transmembrane_region-fluolinker-cYFP constructs


Freiburg08 FT3.png

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