Team:NYMU-Taipei/ymiw1.html
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- | <div class="title"> | + | <div class="title">Week 1 ~ Week 4 (7/1~7/28)</div> |
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<li><a title="Reprogramming of Somatic Cells into Stem & Separation of iPS cells" | <li><a title="Reprogramming of Somatic Cells into Stem & Separation of iPS cells" | ||
- | href="https://2012.igem.org/Team:NYMU-Taipei/ymip3.html">Reprogramming of Somatic | + | href="https://2012.igem.org/Team:NYMU-Taipei/ymip3.html">Reprogramming of Somatic Cells into Stem & Separation of iPS cells</a></li> |
- | Cells into Stem | + | |
- | Separation of iPS cells</a></li> | + | |
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Latest revision as of 17:35, 26 October 2012
Week 1 (7/1~7/7)
Sunday
* Group meeting for topic decision-Venus project/endosynbiosis
* preparation and cultivation of vector pSB1C3 & Ptrc-PNSII-Strep
-25c.c LB medium +25ul Strep + Ptrc-PNSII-Strep
-25c.c LB medium +25ul Cm + pSB1C3
Monday
SRB
* Find for expertise and discuss with them to make a novel project:
NTU/Fujen U/Fu In U/Chung Shin U
- SQR
* extraction of plasmid DNA(pSB1C3 & Ptrc-PNSII-Strep)
* extract plasmid DNA of Synechococcus elongatus PCC 7002
(a kind of cyanobacteria)
* waiting for primer of SQR
Tuesday
SRB
* bacteria choosing: purple sulfur bacteria/ hot spring bacteria / sulfur reducing bacteria
* Figure out the biochemistry characteristic of Desufulvibrio Defulficans
- SQR(Cloning of SQR from PCC7002 begin)
* PCR of SQR
Template: plasmid DNA of sp.PCC7002
Forward primer: SQR-FP (EX_SQR_F)
Reverse primer: SQR-RP (S_SQR_R)
conclusion: positive
*PCR clean up
*enzyme cut
Rescrition enzyme: pSB1C3: EcoRI.SpeI
Ptrc-PNSII-Strep: EcoRI.XbaI
SQR: EcoRI.SpeI
Wednesday
SRB
* Figure out the biochemistry characteristic of Desufulvibrio Defulficans
- SQR
* Clean up
* Ligation: pSB1C3-SQR & Ptrc-PNSII-Strep-SQR
conclusion: positive
* Transformation of competent cell
-prepare Cm20 & Strep plate
- Plate the bacteria onto plates and place at 37oC overnight
Thursday
SQR
* acquire many colony on the plate
-pick 8 colony on each plate(Cm1~Cm8&Strep1~Strep8)
* Colony PCR
Forward primer: VF2
Reverse primer: SQR-RP
Conclusion: Cm1~Cm8 no band
Strep1~Strep8 : positive
Cm1~Cm8 colony PCR again
Conclusion: positive
Friday
SQR
* Enzyme check
-pSB1C3-SQR
Enzyme: NotI-HF (1307+2406)
Conclusion: positive
-Ptrc-PNSII-Strep-SQR
Enzyme: KpnI (3137+2679)
Conclusion: positive
Saturday
SQR
* Send for sequencing
Conclusion: positive
Week 2 (7/8~7/14)
Sunday
SRB
* Set up whole artificial "sulfur" metabolism pathway
- SQR
* Prepare for chemical compound (order DCMU, Na2S)
Monday
- SRB
* Set up whole artificial "sulfur" metabolism pathway
- SQR
* Transform Ptrc-PNSII-Strep-SQR into cyanbacteria (sp. PCC 7942)
* The transformation will take 2 weeks
Tuesday
SRB
* Order for bacteria from BCRC: SRB- Desufulvibrio Desuficans ATCC #27774
- SmtA (Cloning of SmtA from PCC7942 begin)
* PCR of SmtA
Template: plasmid DNA of sp.PCC7942
Forward primer: SmtA-FP (EX_ SmtA _F)
Reverse primer: SmtA -RP (S_ SmtA _R)
conclusion: positive
*PCR clean up
*enzyme cut
Rescrition enzyme: pSB1C3: EcoRI.SpeI
SmtA: EcoRI.SpeI
Wednesday
SRB
* Meeting with Prof. chu ( researcher in sinica academic,the top research institute in Taiwan) topic: 1.photosynthesis pathway I and II 2. Replace the H2O function with H2S inside the whole photosynthesis pathway
- smtA
* Clean up
* Ligation: pSB1C3-SmtA
conclusion: positive
* Transformation of competent cell
-prepare Cm20 plate
- Plate the bacteria onto plates and place at 37oC overnight
Thursday
SRB
* Meeting with Prof. chu ( researcher in sinica academic,the top research institute in Taiwan) topic: 1.photosynthesis pathway I and II 2. Replace the H2O function with H2S inside the whole photosynthesis pathway
- SmtA
* acquire many colony on the plate
-pick 8 colony on each plate(Cm1~Cm8)
* Colony PCR
Forward primer: CmR gene-R-SpeI
Reverse primer: SmtA-RP
Conclusion: Cm1.Cm2.Cm4.Cm5.Cm6.Cm8 positive
Friday
SRB
* SRB genome blast : Desufulvibrio Defulficans/ Desulculvibrio gigas/ Desufulvibrio Vulgas
- SmtA
* Enzyme check
-pSB1C3- SmtA
Enzyme: AgeI-HF + NcoI-HF (1350+893)
Conclusion: positive
Saturday
* Send for sequencing
Conclusion: positive
Week 3(7/15~7/21)
Sunday
SRB
* Prepare special anaerobic medium for Desufulvibrio ssp. ( several pro it'll ingredient kindly from NTU Prof. Lin, expertise in SRB)
Monday
SRB
* Culture for anaerobe bacteria- sulfur reducing bacteria: Desufulvibrio Desulficans
Tuesday
SRB
* Culture for anaerobe bacteria- sulfur reducing bacteria: Desufulvibrio Desulficans
- Invasin+LLO
* Ask for invasion+llo on Ptrc-PNSIII-Amp from Harvard prof. Pamela A. Silver
Wednesday
SRB
* Gene design for cloning: whole genome data from NCBI, specific enzyme chosen from KEGG- Adenylyl sulfate reductase, sulfate Adenylyl transferase, pyrophosphatase, sulfur reductase
Thursday
SRB
* cloning site decision for cloning: 5':MfeI,XbaI. 3':SbfI, SpeI. Middle: BamHI
Friday
* A big typhoon is coming!! (exp delayed for two days!!)
Saturday
* A big typhoon is coming!! (exp delayed for two days!!)
Week 4(7/22~7/28)
Sunday
SRB
* Subculture for Desufulvibrio Desuficans (fail 1st time)
Monday
SRB
* Subculture for Desufulvibrio Desuficans (fail 2nd time)
- Invasin+LLO
* The invasion +llo on Ptrc-PNSIII-AMP from professor in Harvard finally come!!!
* Enzyme check
- Ptrc-PNSIII-AMP-invasion +llo
Enzyme: EcoRI-HF (2006+7437)
Conclusion: positive
Tuesday
SRB
* Looking for technique support for anaerobe bacteria culture: NTU and BCRC
- Invasin+LLO
* Send for sequencing
Conclusion: positive
Wednesday
SRB
* Go sinica academic ( the top research constitute in Taiwan ) and make a discussion about synthetic biology with prof. Wu ( interested in ecology, Cyanobacteria and species diversity research)
Thursday
SRB
* Go sinica academic and make a discussion about synthetic biology with prof. Wu ( interested in ecology, Cyanobacteria and species diversity research)
Saturday
Human practice
* Human practice: thinking twice about that whether human beings have right to create a new organism? ( to become God and change the world)