Team:Tokyo Metropolitan/Project/Pattern/Result

From 2010.igem.org

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{{:Team:Tokyo_Metropolitan/Header}}
{{:Team:Tokyo_Metropolitan/Header}}
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=Result=
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<br><font size="5"><b>Result</b></font></html>
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==DNA amplifying==
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=DNA amplifying=
Amplified all genes which are necessary for our projects.
Amplified all genes which are necessary for our projects.
These are result of electrophoresis.
These are result of electrophoresis.
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Each tube number is the same as [https://2010.igem.org/wiki/index.php?title=Team:Tokyo_Metropolitan/Project/Pattern/Protocol#AboutSample this gene number].
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<gallery widths=95px heights=120px perrow=5 caption="Result of electrophoresis">
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<gallery widths=110px heights=120px perrow=4 caption="Result of electrophoresis">
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Image:Tube1.JPG|Tube 1
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Image:Tube2.JPG|Tube 2
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Image:Tube3.JPG|Tube 3
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Image:Tube4.JPG|Tube 4
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Image:Tube5.JPG|Tube 5
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Image:Tube6.JPG|Tube 6
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Image:Tube7.JPG|Tube 7
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Image:Tube8.JPG|Tube 8
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Image:Tube9.JPG|Tube 9
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Image:Tube10.JPG|Tube 10
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Image:Tube210.jpg|Ligated 2 and 10
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Image:Tube7810.JPG|Ligated 7, 8 and 10
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==activator==
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=Activator=
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We succeed to do PCR 3 DNA fragments which consist Activator. and we could ligate lac promoter to cyaA. but we couldn’t connect mRFP to terminators. 
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We succeed to do PCR 3 DNA fragments which consist Activator. and we could ligate lac promoter to cyaA. but we couldn’t connect mRFP to terminators.
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==Inhibitor==
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=Inhibitor=
We succeed to do PCR 5 DNA fragments which consist Inhibitor. but we couldn’t  ligate and amplify them.
We succeed to do PCR 5 DNA fragments which consist Inhibitor. but we couldn’t  ligate and amplify them.
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==Device==
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=Device=
We succeed to do PCR 3 DNA fragments which consist device to express CRP consecutively. and we could ligate them. but we couldn’t connect them to ruled vector and transform into compitent-cell to cloning. we could detect inserted parts by colony PCR(Insert check) but couldn’t read sequence.
We succeed to do PCR 3 DNA fragments which consist device to express CRP consecutively. and we could ligate them. but we couldn’t connect them to ruled vector and transform into compitent-cell to cloning. we could detect inserted parts by colony PCR(Insert check) but couldn’t read sequence.
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==Discussion==
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=Discussion=
So, why we couldn’t complete our project?
So, why we couldn’t complete our project?

Latest revision as of 18:33, 27 October 2010



Result


Contents

DNA amplifying

Amplified all genes which are necessary for our projects. These are result of electrophoresis. Each tube number is the same as this gene number.


Activator

We succeed to do PCR 3 DNA fragments which consist Activator. and we could ligate lac promoter to cyaA. but we couldn’t connect mRFP to terminators.

Inhibitor

We succeed to do PCR 5 DNA fragments which consist Inhibitor. but we couldn’t ligate and amplify them.


Device

We succeed to do PCR 3 DNA fragments which consist device to express CRP consecutively. and we could ligate them. but we couldn’t connect them to ruled vector and transform into compitent-cell to cloning. we could detect inserted parts by colony PCR(Insert check) but couldn’t read sequence.


So, unfortunately, we couldn’t reach to reproduct our expected RD model based pattern.


Discussion

So, why we couldn’t complete our project?

- We didn’t have enough skills to do genetic experiments. this is first time that we participate iGEM. and almost all members are ungraduated students. we studied very much about protocols and methods about genetic experiments. but it was very difficult work more than we could imagine.And, because of our low reliance of experimental skill, we can’t examine accuracy of our model. but, its not meaningless experience. we learn and got skills through this project. In next year, we ensure that we can do more good experiments and results.




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