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		+	<!--- The Mission, Experiments --->
		+	[[image:331.jpeg|center|]]
		+	{| style="color:#1b2c8a;background-color:#0c6;" cellpadding="3" cellspacing="1" border="1" bordercolor="#fff" width="100%" align="center"
		+	!align="center"|[[Team:Tsinghua|HOME]]
		+	!align="center"|[[Team:Tsinghua/Team|Team]]
		+	!align="center"|[[Team:Tsinghua/Project|Project 1]]
		+	!align="center"|[[Team:Tsinghua/Project2|Project 2]]
		+	!align="center"|[[Team:Tsinghua/Parts|Parts]]
		+	!align="center"|[[Team:Tsinghua/Modelling|Modelling]]
		+	!align="center"|[[Team:Tsinghua/Notebook|Notebook]]
		+	!align="center"|[[Team:Tsinghua/Doodle|Doodle Board]]
		+	|}
	== PHA Project ==		== PHA Project ==
		+	&nbsp;&nbsp;&nbsp;[[Project Description ]]
		+	&nbsp;&nbsp;&nbsp;[[Designed Charts]]
-	DNA Template Resources:	+	&nbsp;&nbsp;&nbsp;[[Molecular Cloning]]
-	PhbCAB: PBHR68 Plasmid	+
-	Lac I: PET28a	+
-	CRE:	+
-	PpPhaP: Ralstonia eutropha H16 genome	+
-	PrPhaR: Ralstonia eutropha H16 genome	+
-	SRRz:	+
-	EGFP:	+
		+	&nbsp;&nbsp;&nbsp;[[WetLab Results]]
-	Primers:	+	&nbsp;&nbsp;&nbsp;[[PHA Project Modeling]]
-	(1) SRRz Primers	+
-	IGEM-ZouYLP-SRRZ-NcoI-for	+
-	5- ATCCATGGATGAAGATGCCAGAAAAACATGACCTGTTG-3	+
-	IGEM-ZouYLP-SRRZ-rev-in	+	&nbsp;&nbsp;&nbsp;[[Reference]]
-	5 - ACCCCGCCGAAGCGGGGTTTTTTTTTCTACTATCTGCACTGCTCATTAATA-3	+
-	IGEM-ZouYLP-SRRZ-BamHI-rev-out
-	5 -TATGGATCCAAAAAAAAACCCCGCCGAAGCGGGGTT-3
-	(2)
-	IGEM-ZouYLP-PP-PhaP-NotI-for
-	5- TATGCGGCCGCTGTTTGTGCATTGCACAAAATCCA-3
-	IGEM-ZouYLP-PP-PhaP-HindIII-rev	+	{| style="color:#1b2c8a;background-color:#0c6;" cellpadding="3" cellspacing="1" border="1" bordercolor="#fff" width="100%" align="center"
-	5- CACCATGTCGACTTTCTCCTCTTTAAGCTTTCAGGCAGCCGTCGTCTTCTTTG-3	+	!align="center"|[[Team:Tsinghua|HOME]]
-		+	!align="center"|[[Team:Tsinghua/Team|Team]]
-	IGEM-ZouYLP-LacILVA-HindIII-for	+	!align="center"|[[Team:Tsinghua/Project|Project 1]]
-	5-TGCCTGAAAGCTTAAAGAGGAGAAAGTCGACATGGTGAATGTGAAACCAGTAAC-3	+	!align="center"|[[Team:Tsinghua/Project2|Project 2]]
-		+	!align="center"|[[Team:Tsinghua/Parts|Parts]]
-	IGEM-ZouYLP-LacILVA-rev-in	+	!align="center"|[[Team:Tsinghua/Modelling|Modelling]]
-	5- AGCTACTAAAGCGTAGTTTTCGTCGTTTGCAGCCTGCCCGCTTTCCAGTCGGGAAACCT-3	+	!align="center"|[[Team:Tsinghua/Notebook|Notebook]]
-		+	!align="center"|[[Team:Tsinghua/Doodle|Doodle Board]]
-	IGEM-ZouYLP-LacILVA-rev-PstI-out	+	|}
-	5- ATTGGACATGCGCGCTTTCTCCTCTTTCTGCAGTTATTAAGCTACTAAAGCGTAGTTTT-3	+	<!--- The Mission, Experiments --->
-		+	[[image:06.jpeg|center|]]
-	IGEM-ZouYLP-CreT7ter—PstI-for	+
-	5- TGCAGAAAGAGGAGAAAGCGCGCATGTCCAATTTACTGACCGTACACCAAAATT-3	+
-		+
-	IGEM-ZouYLP-CreT7ter-rev-in	+
-	5-AGCGGGGTTTTTTTTTCTACTAATCGCCATCTTCCAGCAG-3	+
-		+
-	IGEM-ZouYLP-CreT7ter-EcoRI-rev-out	+
-	5-ATGAATTCGAGCTCGAAAAAAAAACCCCGCCGAAGCGGGGTTTTTTTTTCTACTAAT-3	+
-		+
-	(3)	+
-	IGEM-ZouYLP-PR-PhaR-NotI-for	+
-	5-ATGCGGCCGCAGTGCCTTGTTGGGCATAGAATCAGGGCAGCGGCGCAGC-3	+
-		+
-	IGEM-ZouYLP-PR-PhaR-NdeI-rev	+
-	5-ACGAAGTTATCATATGTTATTACTTCTTGTCCGGCTGGTTGAACGGGAACGTCCCGAAC-3	+
-		+
-	IGEM-ZouYLP-LRLacILP-for-in	+
-	5-TGCTATACGAAGTTATAAAGAGGAGAAACTCGAGATGGTGAATGTGAAACCAGTAACGT-3	+
-		+
-	IGEM-ZouYLP-LRLacILP-NdeI-for-out	+
-	5-ACAAGAAGTAATAACATATGATAACTTCGTATAATGTATGCTATACGAAGTTATAAAGA-3	+
-		+
-	IGEM-ZouYLP-LRLacILP-rev-in	+
-	5-TACGAAGTTATCTACTGCCCGCTTTCCAGTCGGGAAACCT-3	+
-		+
-	IGEM-ZouYLP-LRLacILP-KpnI-rev-out	+
-	5-ATGGTACCATAACTTCGTATAGCATACATTATACGAAGTTATCTACTGCCCGCTT-3	+
-		+
-	(4) EGFP	+
-	IGEMZouYLP-EGFP-for-KoZg-for	+
-	5-ccatgggcagcaagggcgaggagctgttc-3	+
-		+
-	IGEMZouYLP-EGFP-rev-in	+
-	5-AAAAAAAAACCCCGCCGAAGCGGGGTTTTTTTTTCTATCACTTGTACAGCTCGTC-3	+
-		+
-	IGEMZouYLP-EGFP-rev-out	+
-	5-TTTTC GAGCTC GAATTC GGATCCAAAAAAAAACCCCGCCGAA-3	+
-		+
-	IGEMZouYLP-EGFP-KoZg-rev	+
-	5-TTTTCGAGCTCGAATTCGG-3	+
-		+
-		+
-	Designed Molecule	+
-		+
-	[[Image:SRRz-Duet.jpg]]	+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-		+
-	[[Image:EGFP-Duet.jpg]]	+
-		+
-		+
-		+
-	Plasmid constructs:	+
-	1 pUCPhbCAB	+
-		+
-	2 pACYC(lacI+) DuetSRRz	+
-		+
-	3  pACYC(lacI+) DuetEGFP	+
-		+
-	4  pACYC(lacI-) DuetSRRz	+
-		+
-	5  pACYC(lacI-) DuetEGFP	+
-		+
-	6  pACYC(LacI-)DuetSRRzPpPhaPLacILVACret7terPrPhaRLoxPLacILoxP	+
-		+
-	7  pACYC(LacI-)DuetEGFPPpPhaPLacILVACret7terPrPhaRLoxPLacILoxP	+
-		+
-		+
-		+
-	Cloning Strategy:	+
-	(1) Fragment Preparation:	+
-	SRRz: PCR with primer SRRZ-NcoI-for and SRRZ-rev-in;	+
-	Purify the product and run PCR with primer SRRZ-NcoI-for and primer SRRZ-BamHI-rev-out;	+
-		+
-	EGFP: PCR with primer EGFP-for-KoZg-for and EGFP-rev-in;	+
-	Purify the product and run PCR with primer EGFP-for-KoZg-for and primer EGFP-rev-out;	+
-		+
-	PpPhaP: PCR with primer PP-PhaP-NotI-for and PP-PhaP-HindIII-rev;	+
-		+
-	LacI(LVA): PCR with primer LacILVA-HindIII-for and LacILVA-rev-in;	+
-	Purify the product and run PCR with primer LacILVA-HindIII-for and primer LacILVA-rev-PstI-out;	+
-		+
-	CRE(T7ter): PCR with primer CreT7ter—PstI-for and CreT7ter-rev-in	+
-	Purify the product and run PCR with primer CreT7ter—PstI-for and  CreT7ter-EcoRI-rev-out;	+
-		+
-	PrPhaR: PCR with primer PR-PhaR-NotI-for and PR-PhaR-NdeI-rev;	+
-		+
-	LoxPLacILoxP: PCR with primer LRLacILP-for-in and LRLacILP-rev-in	+
-	Purify the product and run PCR with primer LRLacILP-NdeI-for-out and primer LRLacILP-KpnI-rev-out.	+
-		+
-	(2) Fragment Fusion	+
-	Fuse LacI(LVA) and CRE(T7ter) together and amplify with the primer LacILVA-HindIII-for and CreT7ter-EcoRI-rev-out;	+
-	Fuse PrPhaR and LoxPLacILoxP together and amplify with the Primer PR-PhaR-NotI-for and LRLacILP-KpnI-rev-out.	+
-	We’ve tried to fuse more by PCR, but failed.	+
-	(3) Vector preparation	+
-	We choose pACYCDuet-1 as our second vector while PhbCAB operon is cloned into PUC18.	+
-	Since lacI is one of the elements we also used in our own system, we knocked out the lacI coding region in pACYCDuet-1 successfully.	+
-	(4) Cut and Insert	+
-	The restriction enzymes are chosen as following:	+
-	Fragment Enzyme A Enzyme B	+
-	SRRz/EGFP NcoI BamHI	+
-	PpPhaP NotI HindIII	+
-	LacI(LVA)Cre(T7ter) HindIII SacI	+
-	PrPhaRLoxPLacILoxP NotI KpnI	+
-		+
-		+
-	== Reference ==	+
-	1	+
-	A sensitive, viable-colony staining method using Nile red	+
-	for direct screening of bacteria that accumulate polyhydroxyalkanoic	+
-	acids and other lipid storage compounds. Patricia Spiekermann · Bernd H. A. Rehm ·	+
-	Rainer Kalscheuer · Dirk Baumeister ·	+
-	Alexander Steinbüchel. Arch Microbiol (1999) 171:73–80	+
-		+
-	'''This literature explains how pBHR68 works and how PHA granules are detected.'''	+
-		+
-	2  Construction and Selection of  the  Novel  Recombinant Escherichia cob Strain  for Poly(Hydroxybutyrate)  Production.HUIMIN YU,JIN  YIN,HONGQI LI,SHENGLI  YANG,AND  ZHONGYAO. JOURNALOF BIOSCIENCEAND BIOENGWEERING	+
-	Vol. 89,  No. 4, 307-311.  2000	+
-		+
-	'''This literature indicates how PHA sysnthesis is realized in Escherichia coli.'''	+

---

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