Team:KU Seoul/Details

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Latest revision as of 07:59, 20 October 2009

The Experiments

Materials

Backbone Plasmids
- Plasmid pSB3C5 with [http://partsregistry.org/Part:BBa_J04450 BBa_J04450] : 2009 Kit Plate 1 [5C]
- Plasmid pSB3T5 with [http://partsregistry.org/Part:BBa_J04450 BBa_J04450] : 2009 Kit Plate 1 [9C]
Promoters
- Promoter arsR [ParsR], zntA [Pznt] and yodA [PyodA](ref) originated from genomic DNA of Escherichia coli XL-1 Blue
Protein Coding Sequences
- [http://partsregistry.org/Part:BBa_E0044 Green fluorescent protein(BBa_E0044)] : 2009 Kit Plate 1 [14G]
- [http://partsregistry.org/Part:BBa_E1010 Red fluorescent protein(BBa_E1010)] : 2009 Kit Plate 1 [18F]
- Aryl acylamidase protein(ref) : [http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=Nucleotide&list_uids=227462445&dopt=GenBank new biological part]
Primers

Template	Primer	Sequence	Length(bp)
Plasmid pSB3C5	pSB3C5_F	gctgctgttTAATAAtactagtagcggccgctgc	34
Plasmid pSB3C5	pSB3C5(+Pars)_R	taataggtgtgaattttgagttggCtctagaagcggccgcga	42
Plasmid pSB3T5	pSB3T5_F	gacgaaaactacgctgctgctgttTAATAAtactagtagcggccgctgc	49
Plasmid pSB3T5	pSB3T5_R	GTCGGCAATATGAAGctctagaagcggccgcga	33
Promoter yodA	PyodA_F	cggccgcttctagagCTTCATATTGCCGACAAAGTACG	38
Promoter yodA	PyodA_R	ATGTGACTTACCCATaacAGTTTCCTCCAGAGTCATTG	38
Green fluorescent protein	GR(+Pars)_F	aattcacacctattaccttcctctgcacttacacattcgttaagtcatatATGc	78
	GR(+Pars)_F	gtaaaggagaagaacttttcactg	78
	GR(+Pznt)_R	ctggagtcgactccagagtcaagttttatcagagatacagcgagcggacg	84
	GR(+Pznt)_R	TCTAGTttattaaacagcagcagcgtagttttcg	84
Red fluorescent protein	RF(+Pznt)_F	tgataaaacttgactctggagtcgactccagagtgtatccttcggttaatATG	75
	RF(+Pznt)_F	gcttcctccgaagacgttatca	75
	RF(+AAV tag)_R	TTATTAaacagcagcagcgtagttttcgtcgtttgctgcAgcaccggtgg	59
	RF(+AAV tag)_R	agtgacgac	59
Aryl acylamidase	AMD_F	CTGGAGGAAACTGTTatgGGTAAGTCACATTCGCCAG	37
	AMD(+AAV tag)_R	TTATTAaacagcagcagcgtagttttcgtcgtttgctgcCAGGGGC	55
	AMD(+AAV tag)_R	CGTCCGGCG	55

Chemicals
- Acetaminophen (Sigma)
- CdCl2∙H2O (Junsei)
- ZnCl2 (Sigma)
- KH2AsO3 (Sigma)
- Luria-Bertani broth & Bacto agar (Difco)
- o-Cresol (Sigma)
- CuSO4∙5H2O (Sigma)

Experiment Dairy

090914

Streaking of E. coli XL-1 Blue
Preparation of LB plate (containing 100μg/ml ampicillin, 12.5μg/ml tetracycline, 50μg/ml kanamycin and 25μg/ml chloramphenicol of final concentration, respectively) & dry in 37℃ incubator for 12 hours
Inoculation of E. coli DH5a to 5ml LB broth for preparation of competent cell
Design of cloning primers & ordering the primers

090915

Inoculation of E. coli XL-1 Blue to 2ml LB broth for genomic DNA extraction
Preparation of E. coli DH5a competent cell (based on BSGC protocol)

090917

Transformation for amplification of BioBrick parts (BBa_E0044, BBa_E1010, pSB3C5 and pSB3T5) (based on BSGC protocol)
Genomic DNA extraction of E. coli XL-1 Blue by AccuPrep® Genomic DNA Extraction Kit

090918

Inoculation of colonies to 2ml LBAmp(BBa_E0044), LBKan(BBa_E1010), LBCm(pSB3C5) and LBTet(pSB3T5) broth

090919

Plasmid extraction of each part by LaboPass™ Mini Plasmid DNA Purification Kit
0.8% agarose gel electrophoresis (Figure 1)

090921

PCR of BioBrick Parts

General PCR condition : 94℃(3’)-[94℃(1’)-53℃(1’)-72℃(3’)]30-72℃(5’)-4℃

PCR mixture	volume (μl)
Template (mini prep. samples of plasmid : aryl acylamidase, rfp, gfp and PyodA)	1
2.5mM dNTP	4
forward-primer (10pmol/μl)	2
reverse-primer (10pmol/μl)	2
10x Synergy™ buffer	5
Synergy™ DNA polymerase [Gene Ctraft Germany] (10U/μl)	0.5
D.W.	35.5

Hot start PCR condition : 95℃(15’)-[95℃(1’)-53℃(1’)-72℃(3’)]30-72℃(10’)-4℃

PCR mixture	volume (μl)
Template [mini prep. samples of plasmid : pSB3C5 and pSB3T5]	1
2.5mM dNTP	4
forward-primer (10pmol/μl)	2
reverse-primer (10pmol/μl)	2
10x Synergy™ buffer	5
5x Q-solution	10
Hot start taq™ (Qiagen) (5U/μl)	0.05
D.W.	25.5

2. Result (Figure 2)

090922

Part linkage PCR

Linkage PCR condition : 94℃(3’)-[94℃(1’)-53℃(1’)-72℃(3’)]30-72℃(5’)-4℃

PCR mixture	volume (μl)
Template [PCR products of each part diluted 10-fold]]	1
2.5mM dNTP	4
forward-primer (10pmol/μl)	2
reverse-primer (10pmol/μl)	2
10x Synergy™ buffer	5
Synergy™ DNA polymerase [Gene Ctraft Germany] (10U/μl)	0.05
D.W.	35.5

2. Result (Figure 3)

090923

1.Cloning of gfp-rfp to pSB3C5 by Infusion Assembly

1) Clean-up of each PCR products by LaboPass™ Gel and PCR Clean-up Kit – elution : 43ul

2) DpnI (10U/μl) reaction of pSB3C5 and pSB3T5 PCR product at 37℃ for 3-h and clean-up – elution : 43ul

3) T4 DNA polymerase reaction of purified PCR products : Incubation at room temperature for 30min

Reaction mixture	volume (μl)
Purified PCR product	43
BSA (NEB) (10mg/ml)	1
10x NEB buffer 2	5
T4 DNA polymerase (0.6U/μl)	1

4) Clean-up – eleution : 40ul

5) 0.8% agarose gel electrophoresis

090923~090924

Cloning of Pars-gfp-Pznt-rfp to pSB3C5 & PyodA-AMD to pSB3T5
1. Annealing & Transformation : 2ul insert + 2ul pSB3 vector at room temperature for 30min
2. Transformation to E. coli DH5a
3. Results >> vector only : 2, vector + INS : 4

090925-27, 090929~091001

1. Cloning results

Plate	Number of colonies	Plasmid prep.
pSB3C5 vector	2	1
pSB3C5 + Pars-gfp-Pznt-rfp	5	1/3
pSB3T5 vector	3	1
pSB3T5 + PyodA-AMD	14	5/6

2. Plasmid mini prep. & 0.8% agarose gel electrophoresis (Figure 4)

091005~091006

Sequencing by Macrogen
Transformation to E. coli DH5a

091010~091020

Procedure for detecting Zn2+ and AsO3- & Construction of calibration curve for red fluorescence
1. E. coli DH5a harboring pSB3C5/Pars-gfp-Pznt-rfp >> inoculation to 5ml LBC broth and incubation at 37℃ for 12h
2. Inoculation 50ml LBC and incubation to OD600 ~0.5 at 37℃
3. Addition of various concentration of Zn2+ (0, 0.25, 0.5, 1, 1.5, 2mM) & AsO3- (0, 0.0625, 0.125, 0.25, 0.5, 0.75, 1mM) to 1ml incubated broth
4. Incubation for 60min at 37℃
5. Detection by Multilabel Plate Reader (FL/LU) (Perkin Elmer) and Microplate Spectrophotometer (Bio-Tek)
Procedure for detecting Cd2+ & Construction of calibration curve
1. E. coli DH5a harboring pSB3T5/PyodA-AMD >> inoculation to 5ml LBT broth and incubation at 37℃ for 12h
2. Inoculation 50ml LBC and incubation to OD600 ~0.5 at 37℃
3. Addition of various concentration of Cd2+ (0, 0.05, 0.1, 0.2, 0.4 and 0.8mM) to 1ml incubated broth and storage at 4℃
4. Incubation for 60min at 37℃ and centrifugation at 8,000rpm for 1min
5. Resuspension to 1ml reaction mixture ( 100mM AAP in 0.1M Tris buffer pH 9.0) and incubation for 10min at 37℃
6. Stopped with the addition of 2 mL of 1 % (vol/vol) o-cresol and 0.2 mL of 0.2 % (wt/vol) CuSO4 in 1.6 % (vol/vol) NH4OH. After 10 min of incubation at room temperature
7. The amount of p-aminophenol was determined by a spectrophotometer (615 nm)

@@ Line 100: / Line 100: @@
 *090921
 #PCR of BioBrick Parts
-##General PCR condition : 94℃(3’)-[94℃(1’)-53℃(1’)-72℃(3’)]30-72℃(5’)-4℃
+::General PCR condition : 94℃(3’)-[94℃(1’)-53℃(1’)-72℃(3’)]30-72℃(5’)-4℃
-##Hot start PCR condition : 95℃(15’)-[95℃(1’)-53℃(1’)-72℃(3’)]30-72℃(10’)-4℃
+{| style="color:green; background-color:#ffffcc;" cellpadding="3" cellspacing="0" border="1"
-##Result (Figure 2)
+! PCR mixture
+! volume (μl)
+|-
+|Template (mini prep. samples of plasmid : aryl acylamidase, rfp, gfp and PyodA) ||align="center"| 1
+|-
+|2.5mM dNTP ||align="center"| 4
+|-
+|forward-primer (10pmol/μl) ||align="center"| 2
+|-
+|reverse-primer (10pmol/μl) || align="center"| 2
+|-
+|10x Synergy™ buffer || align="center"| 5
+|-
+|Synergy™ DNA polymerase [Gene Ctraft Germany] (10U/μl) || align="center"| 0.5
+|-
+|D.W. || align="center"| 35.5
+|}
+::Hot start PCR condition : 95℃(15’)-[95℃(1’)-53℃(1’)-72℃(3’)]30-72℃(10’)-4℃
+{| style="color:green; background-color:#ffffcc;" cellpadding="3" cellspacing="0" border="1"
+! PCR mixture
+! volume (μl)
+|-
+|Template [mini prep. samples of plasmid : pSB3C5 and pSB3T5] ||align="center"| 1
+|-
+|2.5mM dNTP ||align="center"| 4
+|-
+|forward-primer (10pmol/μl) ||align="center"| 2
+|-
+|reverse-primer (10pmol/μl) || align="center"| 2
+|-
+|10x Synergy™ buffer || align="center"| 5
+|-
+|5x Q-solution || align="center"| 10
+|-
+|Hot start taq™ (Qiagen) (5U/μl) || align="center"| 0.05
+|-
+|D.W. || align="center"| 25.5
+|}
+:2. Result (Figure 2)
 [[Image:KU_Seoul_2.jpg]]
+*090922
+#Part linkage PCR
+::Linkage PCR condition : 94℃(3’)-[94℃(1’)-53℃(1’)-72℃(3’)]30-72℃(5’)-4℃
+{| style="color:green; background-color:#ffffcc;" cellpadding="3" cellspacing="0" border="1"
+! PCR mixture
+! volume (μl)
+|-
+|Template [PCR products of each part diluted 10-fold]] ||align="center"| 1
+|-
+|2.5mM dNTP ||align="center"| 4
+|-
+|forward-primer (10pmol/μl) ||align="center"| 2
+|-
+|reverse-primer (10pmol/μl) || align="center"| 2
+|-
+|10x Synergy™ buffer || align="center"| 5
+|-
+|Synergy™ DNA polymerase [Gene Ctraft Germany] (10U/μl) || align="center"| 0.05
+|-
+|D.W. || align="center"| 35.5
+|}
+:2. Result (Figure 3)
+[[Image:KU_Seoul_3.jpg]]
+*090923
+:1.Cloning of gfp-rfp to pSB3C5 by Infusion Assembly
+::1) Clean-up of each PCR products by LaboPass™ Gel and PCR Clean-up Kit – elution : 43ul
+::2) DpnI (10U/μl) reaction of pSB3C5 and pSB3T5 PCR product at 37℃ for 3-h and clean-up – elution : 43ul
+::3) T4 DNA polymerase reaction of purified PCR products : Incubation at room temperature for 30min
+{| style="color:green; background-color:#ffffcc;" cellpadding="3" cellspacing="0" border="1"
+! Reaction mixture
+! volume (μl)
+|-
+|Purified PCR product ||align="center"| 43
+|-
+|BSA (NEB) (10mg/ml) ||align="center"| 1
+|-
+|10x NEB buffer 2 ||align="center"| 5
+|-
+|T4 DNA polymerase (0.6U/μl) || align="center"| 1
+|}
+::4) Clean-up – eleution : 40ul
+::5) 0.8% agarose gel electrophoresis
+*090923~090924
+#Cloning of Pars-gfp-Pznt-rfp to pSB3C5 & PyodA-AMD to pSB3T5
+##Annealing & Transformation : 2ul insert + 2ul pSB3 vector at room temperature for 30min
+##Transformation to E. coli DH5a
+##Results >> vector only : 2, vector + INS : 4
+*090925-27, 090929~091001
+:1. Cloning results
+{| style="color:green; background-color:#ffffcc;" cellpadding="3" cellspacing="0" border="1"
+! Plate
+! Number of colonies
+! Plasmid prep.
+|-
+|pSB3C5 vector || align="center"|2 ||align="center"| 1
+|-
+|pSB3C5 + Pars-gfp-Pznt-rfp || align="center"|5 ||align="center"| 1/3
+|-
+|pSB3T5 vector || align="center"|3 ||align="center"| 1
+|-
+|pSB3T5 + PyodA-AMD || align="center"|14 ||align="center"| 5/6
+|}
+:2. Plasmid mini prep. & 0.8% agarose gel electrophoresis (Figure 4)
+[[Image:KU_Seoul_4.jpg]]
+*091005~091006
+#Sequencing by Macrogen
+#Transformation to E. coli DH5a
+*091010~091020
+#Procedure for detecting Zn2+ and AsO3- & Construction of calibration curve for red fluorescence
+##E. coli DH5a harboring pSB3C5/Pars-gfp-Pznt-rfp >> inoculation to 5ml LBC broth and incubation  at 37℃ for 12h
+##Inoculation 50ml LBC and incubation to OD600 ~0.5 at 37℃
+##Addition of various concentration of Zn2+ (0, 0.25, 0.5, 1, 1.5, 2mM) & AsO3- (0, 0.0625, 0.125, 0.25, 0.5, 0.75, 1mM) to 1ml incubated broth
+##Incubation for 60min at 37℃
+##Detection by Multilabel Plate Reader (FL/LU) (Perkin Elmer) and Microplate Spectrophotometer (Bio-Tek)
+#Procedure for detecting Cd2+ & Construction of calibration curve
+##E. coli DH5a harboring pSB3T5/PyodA-AMD >> inoculation to 5ml LBT broth and incubation  at 37℃ for 12h
+##Inoculation 50ml LBC and incubation to OD600 ~0.5 at 37℃
+##Addition of various concentration of Cd2+ (0, 0.05, 0.1, 0.2, 0.4 and 0.8mM) to 1ml incubated broth and storage at 4℃
+##Incubation for 60min at 37℃ and centrifugation at 8,000rpm for 1min
+##Resuspension to 1ml reaction mixture ( 100mM AAP in 0.1M Tris buffer pH 9.0) and incubation for 10min at 37℃
+##Stopped with the addition of 2 mL of 1 % (vol/vol) o-cresol and 0.2 mL of 0.2 % (wt/vol) CuSO4 in 1.6 % (vol/vol) NH4OH. After 10 min of incubation at room temperature
+##The amount of p-aminophenol was determined by a spectrophotometer (615 nm)
 |}