Difference between revisions of "Part:BBa K2365048"

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(Characterization & Improvement by AFCM-Egypt 2021)
 
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Coding sequence of Bax mutant form1 protein which releases cytochrome C and leads to apoptosis  in the most broadly used eukaryotic chassis. This year we choose Saccharomyces cerevisiae as our chassis fungal, so we use this gene as the key gene in our biosafety device. It worked well when we detected it's function.We submitted as a improvement of already exist hbax biobrick. The link of original biobrick is here:https://parts.igem.org/Part:BBa_K364202
 
Coding sequence of Bax mutant form1 protein which releases cytochrome C and leads to apoptosis  in the most broadly used eukaryotic chassis. This year we choose Saccharomyces cerevisiae as our chassis fungal, so we use this gene as the key gene in our biosafety device. It worked well when we detected it's function.We submitted as a improvement of already exist hbax biobrick. The link of original biobrick is here:https://parts.igem.org/Part:BBa_K364202
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=='''Characterization & Improvement by <html><a href="https://2021.igem.org/Team:AFCM-Egypt">AFCM-Egypt 2021</a></html>'''==
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===Characterization Of Mutational Landscape===
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Team:<html><a href="https://2021.igem.org/Team:AFCM-Egypt">AFCM-Egypt 2021</a></html>has characterized & improved this part As shown in <html><a href="https://parts.igem.org/wiki/index.php?title=Part:BBa_K3743013">BBa_K3743013</a></html> by performing mutagenesis prediction of mutational landscape of Bax mutant and testing the effect of these mutations on the evolutionary fitness of the protein after generating multiple sequence alignment of the protein sequence and predict mutational landscapes. As shown in the chart, the (G36E) mutation showed the highest score compared to other mutations. On the contrary, we can see that the (G36K) contributed to the lowest evolutionary fitness to Bax mutant. As shown in Figure (1), That's why we changed the sequence according to the highest positive mutation.
 +
[[File:T--AFCM-EGYPT--HBAX2.PNG|thumb|left|Figure 1.shows the positive fit mutants upon saturation mutagenesis prediction of mutational landscape of BAX mutant]]
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===Improvement of RFC [21] Assembly compatibility===
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We improved BAX sequence by performing codon optimization on parts of the sequence that would be a target of restriction enzyme BamHI making it a better fit for assembly as shown in part <html><a href="https://parts.igem.org/wiki/index.php?title=Part:BBa_K3743013">BBa_K3743013</a></html>
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<partinfo>BBa_K2365048 parameters</partinfo>
 
<partinfo>BBa_K2365048 parameters</partinfo>
 
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===[[File:Bax.png|300px|center]]===
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Figure1: Picture of gel electrophoresis (PCR validated products of Bax mutant form1 ; 579bp)
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===Introduction:===
 +
 
 +
Coding sequence of Bax mutant form1 protein.
 +
[[File:Bax.png|300px|center]]
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Figure1: Picture of gel electrophoresis (PCR validated products of Bax mutant form1 ; 579bp).
 
Function:We use Bax protein to kill our engineered yeast when the fungal has finished its mission.
 
Function:We use Bax protein to kill our engineered yeast when the fungal has finished its mission.
  
===[[File:图片3.png|300px|center]]===
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 +
===Improved design:===
 +
[[File:图片3.png|300px|center]]
 
The 579bp fragment was cloned under the GAL1 promoter, followed by CYC1 terminator. The pYES2 vector is designed for native expression of protein of interest in S. cerevisiae. It contains the URA3 gene for selection in yeast and 2µ origin for high-copy maintenance. After verifying the right constructs by restriction enzyme digestions and sequencing, the plasmids were transformed into S. cerevisiae SEY6210.
 
The 579bp fragment was cloned under the GAL1 promoter, followed by CYC1 terminator. The pYES2 vector is designed for native expression of protein of interest in S. cerevisiae. It contains the URA3 gene for selection in yeast and 2µ origin for high-copy maintenance. After verifying the right constructs by restriction enzyme digestions and sequencing, the plasmids were transformed into S. cerevisiae SEY6210.
  
===[[File:图片4.png|300px|center]]===
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 +
===Characterization:===
 +
[[File:图片4.png|400px|center]]
 
Figure 2: Yeast growth curve induced by galactose.  
 
Figure 2: Yeast growth curve induced by galactose.  
 
The expression of Bax protein was activated by inducer-2% galactose.  
 
The expression of Bax protein was activated by inducer-2% galactose.  
 
The cells were washed and diluted 1:1000 into fresh medium to induce the GAL promoter. We use the microplate reader to test the value of OD600. By comparing pYES2-Bax’s growth-inhibiting effect with the control, we can see from the picture that the inhibition level of Bax mutant form1 induced by 2% galactose is significantly higher than the control. It is remarkable that expression of the proapoptotic protein Bax conferred a lethal phenotype in the yeast.
 
The cells were washed and diluted 1:1000 into fresh medium to induce the GAL promoter. We use the microplate reader to test the value of OD600. By comparing pYES2-Bax’s growth-inhibiting effect with the control, we can see from the picture that the inhibition level of Bax mutant form1 induced by 2% galactose is significantly higher than the control. It is remarkable that expression of the proapoptotic protein Bax conferred a lethal phenotype in the yeast.
  
===[[File:图片5.png|300px|center]]===
+
[[File:图片5.png|400px|center]]
 
Figure 3: Yeast growth curve (with glucose as carbon source).  
 
Figure 3: Yeast growth curve (with glucose as carbon source).  
 
In theory, when there is glucose, Bax protein is not expressed. However, from the picture we can be seen that there is a certain leakage.
 
In theory, when there is glucose, Bax protein is not expressed. However, from the picture we can be seen that there is a certain leakage.
  
===[[File:图片6.png|300px|center]]===
 
Figure 4: Apoptotic phenotype in Saccharomyces cerevisiae SEY6210 induced by Bax protein.We can see a significant decrease of yeast concentration.After centrifugation,fewer precipitated cells of induced medium were seen than that of uninduced medium.
 
  
===[[File:图片7.png|300px|center]]===
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Apoptotic phenotype in Saccharomyces cerevisiae SEY6210 induced by Bax protein:
Figure 5 : Observing yeast cells under a microscope.We have count the cell density of the yeast.
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[[File:图片6.png|400px|center]]
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Figure 4: We can see a significant decrease of yeast concentration.After centrifugation,fewer precipitated cells of induced medium were seen than that of uninduced medium.
  
===[[File:图片8.png|300px|center]]===
+
 
 +
We have count the cell density of the yeast:
 +
[[File:图片7.png|400px|center]]
 +
 
 +
Figure 5 :Observing yeast cells under a microscope.
 +
[[File:图片8.png|300px|center]]
 
Figure 6 : Typan Blue Staining Cell Viability Assay . The  stained cells in the view are dead cells.
 
Figure 6 : Typan Blue Staining Cell Viability Assay . The  stained cells in the view are dead cells.
  
===[[File:图片9.png|300px|center]]===
 
Figure7: CCK-8 testing
 
Method:Cells were added into 96-well microplates. Then CCK8 solution were added to the wells and the plates were incubated for additional 4 h at 30°C. Optical density was measured using a microplate reader at a wavelength of 450 nm.
 
  
===[[File:图片10.png|300px|center]]===
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CCK-8 testing
Figure8:CCK-8 testing
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Method:
 
Method:
Cells were added into 96-well microplates. Then CCK8 solution were added to the wells and the plates were incubated for additional 4 h at 30°C. Optical density was measured using a microplate reader at a wavelength of 450 nm.
+
Cells were added into 96-well microplates. Then CCK8 solution were added to the wells and the plates were incubated for additional 4 h at 30°C. Optical density was measured using a microplate reader at a wavelength of 450 nm.
 +
[[File:图片9.png|400px|center]]
 +
Figure7:Comparison between two groups was performed using Student's t-test. Results are expressed as mean ± SD of 3 independent experiments. Differences between means were considered significant when the two-tailed P-value was <0.05.
 +
 
 +
 
 +
Apoptotic features of Bax-expressing yeast:
 +
[[File:图片10.png|400px|center]]
 +
Figure 8: Bax-expressing yeast, the number is getting less and less over time.

Latest revision as of 18:14, 18 October 2021


Bax mutant form1

Coding sequence of Bax mutant form1 protein which releases cytochrome C and leads to apoptosis in the most broadly used eukaryotic chassis. This year we choose Saccharomyces cerevisiae as our chassis fungal, so we use this gene as the key gene in our biosafety device. It worked well when we detected it's function.We submitted as a improvement of already exist hbax biobrick. The link of original biobrick is here:https://parts.igem.org/Part:BBa_K364202

Characterization & Improvement by AFCM-Egypt 2021

Characterization Of Mutational Landscape

Team:AFCM-Egypt 2021has characterized & improved this part As shown in BBa_K3743013 by performing mutagenesis prediction of mutational landscape of Bax mutant and testing the effect of these mutations on the evolutionary fitness of the protein after generating multiple sequence alignment of the protein sequence and predict mutational landscapes. As shown in the chart, the (G36E) mutation showed the highest score compared to other mutations. On the contrary, we can see that the (G36K) contributed to the lowest evolutionary fitness to Bax mutant. As shown in Figure (1), That's why we changed the sequence according to the highest positive mutation.

Figure 1.shows the positive fit mutants upon saturation mutagenesis prediction of mutational landscape of BAX mutant

Improvement of RFC [21] Assembly compatibility

We improved BAX sequence by performing codon optimization on parts of the sequence that would be a target of restriction enzyme BamHI making it a better fit for assembly as shown in part BBa_K3743013












Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal BamHI site found at 452
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]


Introduction:

Coding sequence of Bax mutant form1 protein.

Bax.png

Figure1: Picture of gel electrophoresis (PCR validated products of Bax mutant form1 ; 579bp). Function:We use Bax protein to kill our engineered yeast when the fungal has finished its mission.


Improved design:

图片3.png

The 579bp fragment was cloned under the GAL1 promoter, followed by CYC1 terminator. The pYES2 vector is designed for native expression of protein of interest in S. cerevisiae. It contains the URA3 gene for selection in yeast and 2µ origin for high-copy maintenance. After verifying the right constructs by restriction enzyme digestions and sequencing, the plasmids were transformed into S. cerevisiae SEY6210.


Characterization:

图片4.png

Figure 2: Yeast growth curve induced by galactose. The expression of Bax protein was activated by inducer-2% galactose. The cells were washed and diluted 1:1000 into fresh medium to induce the GAL promoter. We use the microplate reader to test the value of OD600. By comparing pYES2-Bax’s growth-inhibiting effect with the control, we can see from the picture that the inhibition level of Bax mutant form1 induced by 2% galactose is significantly higher than the control. It is remarkable that expression of the proapoptotic protein Bax conferred a lethal phenotype in the yeast.

图片5.png

Figure 3: Yeast growth curve (with glucose as carbon source). In theory, when there is glucose, Bax protein is not expressed. However, from the picture we can be seen that there is a certain leakage.


Apoptotic phenotype in Saccharomyces cerevisiae SEY6210 induced by Bax protein:

图片6.png

Figure 4: We can see a significant decrease of yeast concentration.After centrifugation,fewer precipitated cells of induced medium were seen than that of uninduced medium.


We have count the cell density of the yeast:

图片7.png

Figure 5 :Observing yeast cells under a microscope.

图片8.png

Figure 6 : Typan Blue Staining Cell Viability Assay . The stained cells in the view are dead cells.


CCK-8 testing

Method: Cells were added into 96-well microplates. Then CCK8 solution were added to the wells and the plates were incubated for additional 4 h at 30°C. Optical density was measured using a microplate reader at a wavelength of 450 nm.

图片9.png

Figure7:Comparison between two groups was performed using Student's t-test. Results are expressed as mean ± SD of 3 independent experiments. Differences between means were considered significant when the two-tailed P-value was <0.05.


Apoptotic features of Bax-expressing yeast:

图片10.png

Figure 8: Bax-expressing yeast, the number is getting less and less over time.