Difference between revisions of "Team:HZAU-China/Results"
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<a class="HZAU_title">Results</a> | <a class="HZAU_title">Results</a> | ||
<a class="fubiaoti">The function of dCas9 and gRNA</a> | <a class="fubiaoti">The function of dCas9 and gRNA</a> | ||
| − | <a class="zhengwen">We first construct the gRNA targeting at OriC and test if it could work as we expected. | + | <a class="zhengwen">We first construct the gRNA targeting at OriC and test if it could work as we expected. Through OD measurement we |
| − | + | observed an inhibition of growth when dCas9 and gRNA are all expressed.</a> | |
| − | <img src="https://static.igem.org/mediawiki/2017/ | + | <img src="https://static.igem.org/mediawiki/2017/9/97/T--HZAU-China--Results_Figure1.png" width="60%"> |
| − | <a class="zhengwen">For further description of this synchronization method, we quantifying the number of oriC versus terC by using qPCR. | + | <a class="tuzhu_wenzi"> Figure 1. In this figure, several controls are conducted to demonstrate that it is the function of CRISPR that affect |
| − | + | the growth of culture not the function of gOriC nor the toxicity of dCas9. The purple line represents the experimental | |
| − | <img src="https://static.igem.org/mediawiki/2017/ | + | group while the others represent different controls.</a> |
| − | <a class="zhengwen"> | + | <a class="zhengwen">For further description of this synchronization method, we quantifying the number of |
| − | <img src=" " width=" | + | <i>oriC</i>, the origin of chromosome replication, versus |
| − | <a class="zhengwen">According to our results, we can conclude that the dCas9 and gRNA(oriC) can be used to synchronize the cell | + | <i>terC</i>, the terimination of chromosome replication, by using qPCR. The results confirm that the initiation |
| + | of chromosome replication is inhibited.</a> | ||
| + | <img src="https://static.igem.org/mediawiki/2017/3/31/T--HZAU-China--Results_Figure2.png" style="width: 700px;"> | ||
| + | <a class="tuzhu_wenzi"> Figure 2. In this figure, the blue column represents the ratio of | ||
| + | <i>oriC</i> to | ||
| + | <i>terC</i> of cells growing in common condition. The red column represents that of cells suppressed by dCas9-oriC | ||
| + | for 1 hour and the green column for 2 hours. The purple column shows the ratio of oriC to terC of cells treated | ||
| + | with Rifampicin, a widly used chemical agent to block chromosome replication initiation. The results shows that | ||
| + | the efficiency of dCas9-oriC system is relatively comparable to this widly used agent. </a> | ||
| + | <a class="zhengwen">Flow cytometry is also used to conduct the run-out experiment to verify the synchronization.</a> | ||
| + | <img src="https://static.igem.org/mediawiki/2017/a/a0/T--HZAU-China--Results_Figure3.png" style="width: 700px;"> | ||
| + | <a class="tuzhu_wenzi"> Figure 3. In this figure, different peaks represent different oriC numbers. The untreated sample have 4 peaks while | ||
| + | after treated with dCas9-oriC system the copy number of the same sample has reduced to 2 peaks, which shows that | ||
| + | the oriC number of each cell is reduced.</a> | ||
| + | <a class="zhengwen">According to our results, we can conclude that the dCas9 and gRNA(oriC) can be used to synchronize the cell cycles | ||
| + | of | ||
| + | <i>E. coli</i>.</a> | ||
<a class="fubiaoti">The light induced CRISPR/dCas9 system at transcription level</a> | <a class="fubiaoti">The light induced CRISPR/dCas9 system at transcription level</a> | ||
<a class="zhengwen">An optimized CcaS-CcaR system is constructed under the design of our advisor, the performance of optimized system | <a class="zhengwen">An optimized CcaS-CcaR system is constructed under the design of our advisor, the performance of optimized system | ||
| Line 243: | Line 262: | ||
<a class="zhengwen">We next insert the sequence of gRNA(OirC) after the Pcpcg2, and measure the OD performance under the green light | <a class="zhengwen">We next insert the sequence of gRNA(OirC) after the Pcpcg2, and measure the OD performance under the green light | ||
or red light separately.</a> | or red light separately.</a> | ||
| − | <img src="https://static.igem.org/mediawiki/2017/ | + | <img src="https://static.igem.org/mediawiki/2017/6/68/T--HZAU-China--Results_Figure5.png" width="60%"> |
| − | <a class=" | + | <a class="zhengwen_disblock">The result shows a difference in growth rate under green light and red light. But simply repression cannot achieve |
| − | + | a computer-controlled system. We further tested if this regulation is reversible. For more information please | |
| − | + | click </a> | |
| − | + | <a class="zhengwen_disblock" href="https://2017.igem.org/Team:HZAU-China/Demonstrate">DEMONSTRATION.</a> | |
| − | + | ||
| − | <a class="zhengwen_disblock" href="https://2017.igem.org/Team:HZAU-China/Demonstrate">DEMONSTRATION | + | |
| − | + | ||
<a class="fubiaoti">The light induced CRISPR/dCas9 system at protein level</a> | <a class="fubiaoti">The light induced CRISPR/dCas9 system at protein level</a> | ||
| − | <a class="zhengwen">After getting DNA from IDT, we first constructed and tested the function of pMag and nMag through Luciferase assay.<img src="https://static.igem.org/mediawiki/2017/2/25/T--HZAU-China--magluciferase.png" width="60%" | + | <a class="zhengwen">After getting DNA from IDT, we first constructed and tested the function of pMag and nMag through Luciferase assay.</a> |
| − | <a class="zhengwen">The result verifies the function of pMag and nMag. We next | + | <img src="https://static.igem.org/mediawiki/2017/2/25/T--HZAU-China--magluciferase.png" width="60%"> |
| − | + | <a class="zhengwen">The result verifies the function of pMag and nMag. We next tested the expression of split dCas9 to check if it is hydrolysis by SDS-PAGE.</a> | |
| − | + | <img src="https://static.igem.org/mediawiki/2017/4/4a/T--HZAU-China--sdspage1.png" width="50%"> | |
| − | + | <img src="https://static.igem.org/mediawiki/2017/3/3b/T--HZAU-China--F1.png" width="50%"> | |
| − | + | <img src="https://static.igem.org/mediawiki/2017/f/fe/T--HZAU-China--sdspage3.png" width="50%"> | |
| − | + | <img src="https://static.igem.org/mediawiki/2017/6/64/T--HZAU-China--F3.png" width="50%"> | |
| − | + | ||
| − | + | <a class="zhengwen">After inserting it into pET plasmid, the results turnout that the protein is not hydrolysis.</a> | |
| − | + | <a class="zhengwen">The last reason we doubt is that if it is because the split method that makes the split dCas9 can’t complement.</a> | |
| + | <a class="zhengwen">We replaced the pMag and nMag with a more reliable chemical induced dimerization protein, FKBP & FRB. The result | ||
shows that no inhibition of growth is observed after adding rapamycin, which induces the dimerization of FKBP | shows that no inhibition of growth is observed after adding rapamycin, which induces the dimerization of FKBP | ||
| − | and FRB | + | and FRB (data not shown).</a> |
| − | + | <a class="zhengwen_disblock">In summary, in this project we achieved controlling cell in the level of DNA replication, proved the feasibility | |
| − | of using CRISPR to regulate cell cycle | + | of using CRISPR to regulate cell cycle and further regulate it with light. A reverse regulation of our system |
| − | is demonstrated by OD measurement and qPCR. At the same time, | + | is demonstrated by OD measurement and qPCR. At the same time, corresponding software and hardware are developed |
to achieve the computer-controlled cell cycle. The software is used to predict the internal replication procession | to achieve the computer-controlled cell cycle. The software is used to predict the internal replication procession | ||
and control the hardware to regulate cell by light. For more information, please view</a> | and control the hardware to regulate cell by light. For more information, please view</a> | ||
| − | + | <a class="zhengwen_disblock" href="https://2017.igem.org/Team:HZAU-China/Demonstrate">Demonstrate.</a> | |
</a> | </a> | ||
<a class="biaoti"> Notes</a> | <a class="biaoti"> Notes</a> | ||
| Line 277: | Line 294: | ||
sensitive to aTc. A final concentration of 200ng/ml will be toxic to the bacteria, and a working concentration | sensitive to aTc. A final concentration of 200ng/ml will be toxic to the bacteria, and a working concentration | ||
as 0.1~1ng/ml is recommended.</li> | as 0.1~1ng/ml is recommended.</li> | ||
| − | <li>In a light-control system, the | + | <li>In a light-control system, the existence of light sensing molecule is very important, but it is also very easy to be neglected.</li> |
| − | <li> The aTc may lose its inducing function if added into a relatively high concentration culture (OD~0.6) when you | + | <li>The aTc may lose its inducing function if added into a relatively high concentration culture (OD~0.6) when you |
use CcaS-CcaR system.</li> | use CcaS-CcaR system.</li> | ||
</a> | </a> | ||
<a class="biaoti"> Future plan</a> | <a class="biaoti"> Future plan</a> | ||
| − | <a class="zhengwen">The future plan | + | <a class="zhengwen">The future plan includes two aspects. One is further developing the system. First we plan to replace the inducible |
promoter with a constitutive promoter J23115. We plan to developing CcaS-CcaR CRISPRi system by knocking it into | promoter with a constitutive promoter J23115. We plan to developing CcaS-CcaR CRISPRi system by knocking it into | ||
genome to make it more significant. At the same time, we hope that we can make the pMag-nMag system work because | genome to make it more significant. At the same time, we hope that we can make the pMag-nMag system work because | ||
| − | this system is smaller and less | + | this system is smaller and less-affecting on bacterial metabolism. The other aspect is using this system for several |
| − | certain applications, like | + | certain applications, like characterizing the stability of genome gene expression after synchronization, and so on. |
We plan to knock the sfGFP into the genome and measure the fluorescence per cell to determine the noise between | We plan to knock the sfGFP into the genome and measure the fluorescence per cell to determine the noise between | ||
each cell and characterize whether synchronization can make the gene on genome more stable. | each cell and characterize whether synchronization can make the gene on genome more stable. | ||
Latest revision as of 03:59, 16 December 2017
Results
The function of dCas9 and gRNA
We first construct the gRNA targeting at OriC and test if it could work as we expected. Through OD measurement we
observed an inhibition of growth when dCas9 and gRNA are all expressed.
Figure 1. In this figure, several controls are conducted to demonstrate that it is the function of CRISPR that affect
the growth of culture not the function of gOriC nor the toxicity of dCas9. The purple line represents the experimental
group while the others represent different controls.
For further description of this synchronization method, we quantifying the number of
oriC, the origin of chromosome replication, versus
terC, the terimination of chromosome replication, by using qPCR. The results confirm that the initiation
of chromosome replication is inhibited.
Figure 2. In this figure, the blue column represents the ratio of
oriC to
terC of cells growing in common condition. The red column represents that of cells suppressed by dCas9-oriC
for 1 hour and the green column for 2 hours. The purple column shows the ratio of oriC to terC of cells treated
with Rifampicin, a widly used chemical agent to block chromosome replication initiation. The results shows that
the efficiency of dCas9-oriC system is relatively comparable to this widly used agent.
Flow cytometry is also used to conduct the run-out experiment to verify the synchronization.
Figure 3. In this figure, different peaks represent different oriC numbers. The untreated sample have 4 peaks while
after treated with dCas9-oriC system the copy number of the same sample has reduced to 2 peaks, which shows that
the oriC number of each cell is reduced.
According to our results, we can conclude that the dCas9 and gRNA(oriC) can be used to synchronize the cell cycles
of
E. coli.
The light induced CRISPR/dCas9 system at transcription level
An optimized CcaS-CcaR system is constructed under the design of our advisor, the performance of optimized system
is as following.
We next insert the sequence of gRNA(OirC) after the Pcpcg2, and measure the OD performance under the green light
or red light separately.
The result shows a difference in growth rate under green light and red light. But simply repression cannot achieve
a computer-controlled system. We further tested if this regulation is reversible. For more information please
click
DEMONSTRATION.
The light induced CRISPR/dCas9 system at protein level
After getting DNA from IDT, we first constructed and tested the function of pMag and nMag through Luciferase assay.
The result verifies the function of pMag and nMag. We next tested the expression of split dCas9 to check if it is hydrolysis by SDS-PAGE.
After inserting it into pET plasmid, the results turnout that the protein is not hydrolysis.
The last reason we doubt is that if it is because the split method that makes the split dCas9 can’t complement.
We replaced the pMag and nMag with a more reliable chemical induced dimerization protein, FKBP & FRB. The result
shows that no inhibition of growth is observed after adding rapamycin, which induces the dimerization of FKBP
and FRB (data not shown).
In summary, in this project we achieved controlling cell in the level of DNA replication, proved the feasibility
of using CRISPR to regulate cell cycle and further regulate it with light. A reverse regulation of our system
is demonstrated by OD measurement and qPCR. At the same time, corresponding software and hardware are developed
to achieve the computer-controlled cell cycle. The software is used to predict the internal replication procession
and control the hardware to regulate cell by light. For more information, please view
Demonstrate.
Notes
When using the CcaS-CcaR system please note that the atc concentration is different from the former concentration
200ng/ml. After transformation of two plasmids related to CcaS-CcaR system into bacteria, it becomes more
sensitive to aTc. A final concentration of 200ng/ml will be toxic to the bacteria, and a working concentration
as 0.1~1ng/ml is recommended.
In a light-control system, the existence of light sensing molecule is very important, but it is also very easy to be neglected.
The aTc may lose its inducing function if added into a relatively high concentration culture (OD~0.6) when you
use CcaS-CcaR system.
Future plan
The future plan includes two aspects. One is further developing the system. First we plan to replace the inducible
promoter with a constitutive promoter J23115. We plan to developing CcaS-CcaR CRISPRi system by knocking it into
genome to make it more significant. At the same time, we hope that we can make the pMag-nMag system work because
this system is smaller and less-affecting on bacterial metabolism. The other aspect is using this system for several
certain applications, like characterizing the stability of genome gene expression after synchronization, and so on.
We plan to knock the sfGFP into the genome and measure the fluorescence per cell to determine the noise between
each cell and characterize whether synchronization can make the gene on genome more stable.
Figure 1. In this figure, several controls are conducted to demonstrate that it is the function of CRISPR that affect
the growth of culture not the function of gOriC nor the toxicity of dCas9. The purple line represents the experimental
group while the others represent different controls.
For further description of this synchronization method, we quantifying the number of
oriC, the origin of chromosome replication, versus
terC, the terimination of chromosome replication, by using qPCR. The results confirm that the initiation
of chromosome replication is inhibited.
Figure 2. In this figure, the blue column represents the ratio of
oriC to
terC of cells growing in common condition. The red column represents that of cells suppressed by dCas9-oriC
for 1 hour and the green column for 2 hours. The purple column shows the ratio of oriC to terC of cells treated
with Rifampicin, a widly used chemical agent to block chromosome replication initiation. The results shows that
the efficiency of dCas9-oriC system is relatively comparable to this widly used agent.
Flow cytometry is also used to conduct the run-out experiment to verify the synchronization.
Figure 3. In this figure, different peaks represent different oriC numbers. The untreated sample have 4 peaks while
after treated with dCas9-oriC system the copy number of the same sample has reduced to 2 peaks, which shows that
the oriC number of each cell is reduced.
According to our results, we can conclude that the dCas9 and gRNA(oriC) can be used to synchronize the cell cycles
of
E. coli.
The light induced CRISPR/dCas9 system at transcription level
An optimized CcaS-CcaR system is constructed under the design of our advisor, the performance of optimized system
is as following.
We next insert the sequence of gRNA(OirC) after the Pcpcg2, and measure the OD performance under the green light
or red light separately.
The result shows a difference in growth rate under green light and red light. But simply repression cannot achieve
a computer-controlled system. We further tested if this regulation is reversible. For more information please
click
DEMONSTRATION.
The light induced CRISPR/dCas9 system at protein level
After getting DNA from IDT, we first constructed and tested the function of pMag and nMag through Luciferase assay.
The result verifies the function of pMag and nMag. We next tested the expression of split dCas9 to check if it is hydrolysis by SDS-PAGE.
After inserting it into pET plasmid, the results turnout that the protein is not hydrolysis.
The last reason we doubt is that if it is because the split method that makes the split dCas9 can’t complement.
We replaced the pMag and nMag with a more reliable chemical induced dimerization protein, FKBP & FRB. The result
shows that no inhibition of growth is observed after adding rapamycin, which induces the dimerization of FKBP
and FRB (data not shown).
In summary, in this project we achieved controlling cell in the level of DNA replication, proved the feasibility
of using CRISPR to regulate cell cycle and further regulate it with light. A reverse regulation of our system
is demonstrated by OD measurement and qPCR. At the same time, corresponding software and hardware are developed
to achieve the computer-controlled cell cycle. The software is used to predict the internal replication procession
and control the hardware to regulate cell by light. For more information, please view
Demonstrate.
Notes
