From 2013hs.igem.org

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Latest revision as of 03:49, 22 June 2013

Notebook Links

Restriction - Ligation

Names: Yoyo Y, Wesley M
Date: April 2, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
J06702 - mCherry
J61002 - RFP Reporter
Promoters: J23113, J23108, J23114, J23100
Cut Promoters at sites E & S
Cut mCherry at sites X & P
Cut Destination Plasmid E1010_pSB1C3 sites E&P
Promoter Master Mix
- MilliQ: 66.25µL
- BSA: 1.25µL
- Buffer #2: 12.5µL
- DNA: 8µL
- Add 0.5µL EcoR1 and 0.5µL Spel to 16µL MM
J06702 Master Mix
- MilliQ: 66.25µL
- BSA: 1.25µL
- Buffer #2: 12.5µL
- J06702: 40µL
- Add 0.5µL Xbal and 0.5µL Pst1 to 24MM
pSB1C3 Master Mix
- MilliQ: 66.25µL
- BSA: 1.25µL
- Buffer #2: 12.5µL
- E1010 pSB1C3: 40µL
- Add 0.5µL EcR1 and 0.5µL Pst1 to 24MM
Incubated at 37°C for 1 hour
Heat killed enzyme for 20 mins at 65°C

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Ligations

Name: Yoyo Y
Date: April 2, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Tube 1 - J23100_J06702_pSB1C3
Tube 2 - J23108_J06702_pSB1C3
Tube 3 - J23113_J06702_pSB1C3
Tube 4 - J23114_J06702_pSB1C3
Left overnight at 16°C
Agarose Gel of Digested Parts 1%

Lane #	Contents	Volume
1	1 kb DNA Ladder	6µL
2	E1010 pSB1c3 #4	15µL
3	E1010 pSB1c3 #3	15µL
4	E1010 pSB1c3 #2	15µL
5	E1010 pSB1c3 #1	15µL
6	J06702 #4	15µL
7	J06702 #3	15µL
8	J06702 #2	15µL
9	J06702 #1	15µL
10	J23100	15µL
11	J23108	15µL
12	J23113	15µL
13	J23114	15µL

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Transformation

Name: Fiona S, Chris I, Yoyo Y
Date: April 3, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Antibiotic: CAM
Part Number and Plasmid: J23100_J06702_pSB1C3, J23108_J06702_pSB1C3, J23113_J06702_pSB1C3, J23114_J06702_pSB1C3
Results: TBA

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Re-Plating Transformation

Names: Chris I, Fiona S
Date: April 4, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Part Number and Plasmid: J23100_J06702_pSB1C3, J23108_J06702_pSB1C3, J23113_J06702_pSB1C3, J23114_J06702_pSB1C3
Antibiotic CAM

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Miniprep of ON Cultures

Names: Chris I, Yoyo Y
Date: April 5, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Miniprepped J23108_pSB1A2, J23113_pSB1A2, J23114_pSB1A2, J06702_pSB1AK2, used 50µL of Elution Buffer

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UV Spectroscopy DNA Concentrations

Names: Chris I, Yoyo Y, Elaine B
Date: April 5, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe

	A260	A280	A260/A280	DNA Concentration at 50-fold dilution ug/mL
J23108	0.1017	0.0092	11.05435	254.25
J23113	0.1289	0.0338	3.813609	322.25
J23114	0.135	0.0397	3.400504	337.5
J06702-1	0.13	0.0373	3.485255	325

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Miniprep From Ligation

Names: Shikhar M, Krista F, Austin K
Date: April 6, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Miniprepped J23108_J06702_pSB1C3, J23113_J06702_pSB1C3, J23100_J06702_pSB1C3 used 50µL of Elution Buffer
Note: left plates to grow longer, need DNA sequenced.

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PCR

Name: Erin K
Date: April 7, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2
Separately added 2µL of appropriate DNA and 0.2µL of Pfu Polymerase to 17.8µL MM
Agarose Gel confirmation of PCR: Success

MM 5x Reagent	Volume(µL)
MilliQ H2O	67
10X Pfu Buffer with MgSO4	20
10mM dNTPs	2
VF2	5
V4	5

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Restriction Digestion of PCR Parts

Name: Erin K
April 8, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
2 samples of J06702_pSB1AK2: Added 0.5µL XbaI and 0.5µL PstI to 24µL MM

J06702 MM 2x	Volume (µL)
MIlliQ	29.5
BSA	0.5
NEB 10x Buffer 2	5
J06702_pSB1AK2	10

2 samples of TAT-E1010_pSB1C3: Added 0.5µL EcoRIand 0.5µL PstI to 24µL MM

TAT-E1010_pSB1C3 MM 2x	Volume (µL)
MIlliQ	12.5
BSA	0.5
NEB 10x Buffer 2	5
TAT-E1010_pSB1C3	30

2 samples of each of the 3 promoters: Added 5µL appropriate DNA and 0.5µL EcoRI and 0.5µL SpeI to 16µL MM

Promoter MM 7x	Volume (µL)
MIlliQ	95.75
BSA	1.75
NEB 10x Buffer 2	17.5

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3% Agarose Gel of Digested PCR Parts

Names: Wesley M, Riley M, Krista F
Date: April 8, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Parts: J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2
Results: Unsuccessful

Lane #	Contents	Volume(µL)
1	Ladder 100bp	5
2	J23108	29
3	J23108	29
4	Blank	N/A
5	J23113	29
6	Blank	N/A
7	Blank	N/A
8	Blank	N/A
9	J23113	29
10	Blank	N/A
11	J23114	29
12	Blank	N/A
13	J23114	29

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Gel Extraction

Names: Wesley M, Riley M, Krista F
Date: April 8, 2013
Species: E. coli
Strain: DH5α
Protocol: Biobasic Kit: Eluted with 30µL elution buffer

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Repeat PCR

Name: Elaine B, Chris I, Fiona S, Wesley M, Riley M
Date: April 9, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2
Separately added 2µL of appropriate DNA and 0.2µL of Pfu Polymerase to 17.8µL MM

MM 5x Reagent	Volume (μL)
MIlliQ	67
10X Pfu Buffer with MgSO4	2
10mM dNTPs	2
VF2	5
V4	5

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Picking Cells

Names: Chris I, Elaine B, Fiona S, Wesley M, Riley M,
Date: April 9, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Picked: J23113_J61002, J23108_J61002, J23114_J61002, J23100_J61002, J06702_pSB_1AK2
5mL cultures, 5µL Amp. grown overnight at 37°C

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Mini Prep

Names: Yoyo Y
Date: April 10, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Mini Prep of (x2 of 35µL): J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002
Mini-prepped with EZ-10 columns
Eluted 35µL
Purified DNA in HS iGEM Kit #1

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Restriction

Names: Dylan S
Date: April 10, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Add 33µL DNA to 17µL MM
17µL MM to promoter tubes
33µL DNA to promoter tubes
Same procedure for J06702_pSB1AK3
Incubated at 37°C for 2 hours
Heat killed at 65°C for 20 minutes

Promoter MM 50μL rxn x4	Volume (μL)
MIlliQ	44
BSA	20
NEB 10 x Buffer 2	20

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Agarose Gel of PCR 1%

Result: Successful

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Miniprep

Names: Dylan S, Patrick O
Date: April 11, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Mini prep of (35µL EB): J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002
Mini-prepped with EZ-10 columns
Eluted 35µL
Purified DNA in HS iGEM Kit #1

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Restriction Digestion

Names: Wesley M, Yoyo Y
Date: April 12, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Restriction of E1010_pSB1C3 at sites E & P
50µL rxn
Add 30µL DNA to 20µL MM
Added 0.5µL EcoR1 & Pst1
Incubated 2 hours at 37°C
Heat killed 20 minutes at 65°C

MM x 2.5	Volume (μL)
MIlliQ	22.5
10x Buffer 2 (NEB)	12.5
BSA	12.5

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PCR and Cell Reculturization

Names: Patrick O, Shikhar M
Date: April 12, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Reculturization of: J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002
PCR: Master mix created with: Annealing temperature: 55.6°C

MM for Promoters (x5)		Conditions for tube "a"
MIlliQ	67 μL	MIlliQ	13.4 μL
10X Pfu Buffer + MgSO4	20 μL	10X Pfu Buffer + MgSO4	4 μL
10mM dNTPs	2 μL	10mM dNTPs	0.4 μL
VF2	5 μL	VF2	1 μL
VR	5 μL	VR	1 μL
Pfu polymerase	0.2 μL	Pfu polymerase	0.2 μL
DNA part		2 μL

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Miniprep

Names: Amrinder G, Steven T
Date: April 12, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Mini prep of (35µL EB): J06702_pSB1AK3, J23100_J61002, J23108_J61002 ,J23113_J61002, J23114_J61002
Mini-prepped with EZ-10 columns
Eluted 35µL
Purified DNA in HS iGEM Kit #1

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Miniprep

Names: Fiona S, Katie T
Date: April 14, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Mini prep of (35µL EB): J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2
Mini-prepped with EZ-10 columns
Eluted 35µL

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1% Agarose Gel

Names: Fiona S, Katie T
April 14, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe
Parts: J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002
Gel Extraction
Parts: J23108_J61002, J23113_J61002
Eluted 50 µL

Lane #	Contents	Volume(µL)
1	1 µL Dye, 5µL DNA kB ladder	6
2	J23100_J61002	25
3	J23100_J61002	25
4	J23100_J61002	~10
5	J23108_J61002	25
6	J23108_J61002	25
7	J23108_J61002	~10
8	J23113_J61002	25
9	J23113_J61002	25
10	J23113_J61002	~10
11	J23114_J61002	25
12	J23114_J61002	25
13	J23114_J61002	~10

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Restriction/Digestion

Master Mix: Yoyo Yao promoters x9
35uL DNA, 14µL MM, 0.5µL Spe1, 0.5µL Pst1
Date: April 15, 2013

Master Mix	Volume (μL)
MIlliQ	36
BSA	45
10x buffer 2 NEB	45

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Restriction/Digestion

Master Mix: FS, KT ½ promoter ½ insulin/glucose x17
(Promoters) 25µL DNA, 24µL MM, 0.5µL Spe1, 0.5µL Pst1
(Insulin/Glucose) 25µL DNA, 24µL MM, 0.5µL EcoR1, 0.5µL Pst1
Date: April 15, 2013

Master Mix	Volume (μL)
MIlliQ	238
BSA	85
10x buffer 2 NEB	85

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1% Agarose Gel of Promoters

Names: Yoyo Y, Erin K
April 15, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe

Lane #	Contents	Volume (μL)
1	1 KB Ladder	6
2	J23100-1 YYSP	25
3	J23100-1 YYSP	25
4	J23100-1 YYSP	<10
5	J23100-2 YYSP	25
6	J23100-2 YYSP	25
7	J23100-2 YYSP	<10
8	J23108-1 YYSP	25
9	J23108-1 YYSP	25
10	J23108-1 YYSP	<10
11	J23108-2 YYSP	25
12	J23108-2 YYSP	~25

Lane #	Contents	Volume (μL)
1	1 KB Ladder	6
2	J23113-1 YYSP	25
3	J23113-1 YYSP	25
4	J23113-2 YYSP	25
5	J23113-2 YYSP	25
6	J23113-2 YYSP	<10
7	J23114-1 YYSP	25
8	J23114-1 YYSP	25
9	J23114-2 YYSP	25
10	J23114-2 YYSP	25

Lane #	Contents	Volume (μL)
1	1 KB Ladder	6
2	J23100-1 YYSP	25
3	J23100-1 YYSP	25
4	J23100-1 YYSP	25
5	J23100-2 YYSP	25
6	J23100-2 YYSP	<25
7	J23108-1 YYSP	25
8	J23108-1 YYSP	25
9	J23108-1 YYSP	10
10	J23108-2 YYSP	25
11	J23108-2 YYSP	25

Lane #	Contents	Volume (μL)
1	1 KB Ladder	6
2	J23113-1 YYSP	25
3	J23113-1 YYSP	25
4	J23113-2 YYSP	25
5	J23113-2 YYSP	25
6	J23114-1 YYSP	<10
7	J23114-1 YYSP	25
8	J23224-1 YYSP	25
9	J23114-2 YYSP	10
10	J23114-2 YYSP	25

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Transformation

Name: Dylan S
Date: April 17, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe

Tube #	Part #	Plasmid	Volume of Competent Cells(µL)
1	J23100+J06702	J61002	100
2	J23108+J06702	J61002	100
3	J23113+J06702	J61002	50
4	J23114+J06702	J61002	50
5	J23100 mlc J06702	pSB3C5	50
6	J23100 mlc J06702	pSB3C5	50
+/- Controls		PUC19 Amp resistance	50 each

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1% Agarose Gel of Promoter Constructs

Name: Chris I
Date: April 30, 2013
Species: E. coli
Strain: DH5α
Protocol: Ute Kothe

Lane #	Contents	Volume(µL)
1	1 KB Ladder	6
2	J23100_J61002	25
3	J23100_J61002	25
4	J23100_J61002	25
5	J23100_J61002	25
6	J23108_J61002	25
7	J23108_J61002	25
8	J23108_J61002	25
9	J23108_J61002	25
10	J23108_J61002	<20
11	J23108_J61002	25
13	1 KB Ladder	25
12	J23100_J61002	<20
1	1 KB Ladder	6
2	J23113_J61002	25
3	J23113_J61002	25
4	J23113_J61002	<20
5	J6702_pSB1AK2	20
6	J6702_pSB1AK2	20
7	J6702_pSB1AK2	20
8	J6702_pSB1AK2	25
9	J6702_pSB1AK2	25
10	J6702_pSB1AK2	20
11	J6702_pSB1AK2	20
12	J6702_pSB1AK2	20
13	None	N/A

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@@ Line 29: / Line 29: @@
 			<div class="cleafix>">
 			<div id="navigation">
-				<li class="navigation_project decrease_opacity"><a href="#" class="strict">Project</a>
+				<li class="navigation_project"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/project" class="strict">Project</a>
 					<ul>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/project">Description</a></li>
+                                                <li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/project#video_oxy">Visual Modeling</a></li>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/math">Math Model</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/results">Results</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/wikifreeze">Wikifreeze</a></li>
 					</ul>
 				</li>
 				<li class="navigation_parts decrease_opacity"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/parts" class="strict">Parts</a></li>
-				<li class="navigation_notebook decrease_opacity"><a href="#" class="strict">Notebook</a>
+				<li class="navigation_notebook decrease_opacity"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/protocols" class="strict">Notebook</a>
 					<ul>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/protocols#protocol_header">Protocols</a></li>
@@ Line 42: / Line 45: @@
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_april">Notebook: April</a></li>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may">Notebook: May</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june">Notebook: June</a></li>
 					</ul>
 				</li>
 				<li class="navigation_safety decrease_opacity"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/safety" class="strict">Safety</a></li>
-				<li class="navigation_outreach decrease_opacity"><a href="#" class="strict">Outreach</a>
+				<li class="navigation_outreach decrease_opacity"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/outreach" class="strict">Outreach</a>
 					<ul>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/outreach">Overview</a></li>
@@ Line 51: / Line 55: @@
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/interviews">Interviews</a></li>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/videos">Videos</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/surveys">Parent Surveys</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/novel_study">Novel Study</a></li>
 					</ul>
 				</li>
-				<li class="navigation_team decrease_opacity"><a href="#" class="strict">Team</a>
+				<li class="navigation_team decrease_opacity"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/team" class="strict">Team</a>
 					<ul>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/team#the_team">The Team</a></li>
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 				<div id="notebook_header">
 				<div id="notebook_links">
-				<h1 id="notebook_links_header">Notebook Links</h1>
+<h1 id="notebook_links_header"> Notebook Links</h1>
 					<ul id="notebook_march_links">
 						<li class="notebook_link_title"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_march">March</a></li>
@@ Line 138: / Line 146: @@
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_eighteen">May 17, 2013: Miniprep</a></li>
 						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_nineteen">May 17, 2013: Glycerol Stock</a></li>
+					        <li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_one">May 22, 2013: Ligation</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_two">May 22, 2013: Transformations</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_three">May 23, 2013: Transformations</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_four">May 23, 2013: Picked Oxytocin and Transformations</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_five">May 24, 2013: Glycerol Stock</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_six">May 24, 2013: Miniprep</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_seven">May 26, 2013: Miniprep</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_eight">May 26, 2013: Restriction Digestion</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_twenty_nine">May 26, 2013: Agarose gel of Digestion</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_thirty">May 26, 2013: Digestion Protocol</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_thirty_one">May 31, 2013: Agarose Gel</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_thirty_two">May 31, 2013: Everything</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_may#entry_thirty_three">May 31, 2013: Everything</a></li>
+					</ul>
+					<ul id="notebook_june_links">
+						<li class="notebook_link_title"><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june">June</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_one">June 1, 2013: Restrictions</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_two">June 2, 2013: Transformation</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_three">June 4, 2013: Picked Colonies</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_four">June 10, 2013: Sent constructs for sequencing</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_five">June 13, 2013: Transformation of OXY into BL21</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_six">June 13, 2013: Restricted and Ligated and Transformed</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_seven">June 13, 2013: Picked Cells</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_eight">June 15, 2013: Ni-Sepharose Purification</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_nine">June 18, 2013: Tris-Tricine PAGE</a></li>
+						<li><a href="https://2013hs.igem.org/Team:Lethbridge_Canada/notebook_june#entry_ten">June 21, 2013: Anti-His Slot Blot</a></li>
 					</ul>
 				</div>
 				</div>
+<div class="pull_banner_left">
+<img src="https://static.igem.org/mediawiki/2013hs/e/ea/Lethbridge_hs_igem_2013_banner_notbookapril.png">
+</div>
 				<div id="notebook_body">
@@ Line 150: / Line 187: @@
 					<li>Names: Yoyo Y, Wesley M</li>
 					<li>Date: April 2, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>J06702 - mCherry</li>
@@ Line 161: / Line 198: @@
 					<li class="notebook_nested_start">Promoter Master Mix</li>
 						<li><ul class="notebook_nested_list">
-							<li>MilliQ: 66.25uL</li>
+							<li>MilliQ: 66.25µL</li>
-							<li>BSA: 1.25 uL</li>
+							<li>BSA: 1.25µL</li>
-							<li>Buffer #2: 12.5 uL</li>
+							<li>Buffer #2: 12.5µL</li>
-							<li>DNA: 8 uL</li>
+							<li>DNA: 8µL</li>
-							<li>Add 0.5 uL EcoR1 and 0.5 uL Spel to 16 uL MM</li>
+							<li>Add 0.5µL EcoR1 and 0.5µL Spel to 16µL MM</li>
 						</ul>
 						</li>
@@ Line 171: / Line 208: @@
 					<li class="notebook_nested_start">J06702 Master Mix</li>
 						<li><ul class="notebook_nested_list">
-							<li>MilliQ: 66.25 uL</li>
+							<li>MilliQ: 66.25µL</li>
-							<li>BSA: 1.25 uL</li>
+							<li>BSA: 1.25µL</li>
-							<li>Buffer #2: 12.5 uL</li>
+							<li>Buffer #2: 12.5µL</li>
-							<li>J06702: 40 uL</li>
+							<li>J06702: 40µL</li>
-							<li>Add 0.5 uL Xbal and 0.5 uL Pst1 to 24MM</li>
+							<li>Add 0.5µL Xbal and 0.5µL Pst1 to 24MM</li>
 						</ul>
 						</li>
@@ Line 181: / Line 218: @@
 					<li class="notebook_nested_start">pSB1C3 Master Mix</li>
 						<li><ul class="notebook_nested_list">
-							<li>MilliQ: 66.25uL</li>
+							<li>MilliQ: 66.25µL</li>
-							<li>BSA: 1.25 uL</li>
+							<li>BSA: 1.25µL</li>
-							<li>Buffer #2: 12.5 uL</li>
+							<li>Buffer #2: 12.5µL</li>
-							<li>E1010 pSB1C3: 40 uL</li>
+							<li>E1010 pSB1C3: 40µL</li>
-							<li>Add 0.5 uL EcR1 and 0.5 uL Pst1 to 24MM</li>
+							<li>Add 0.5µL EcR1 and 0.5µL Pst1 to 24MM</li>
 						</ul>
 						</li>
 					</li>
-					<li>Incubated at 37 degrees Celsuis for 1 hour</li>
+					<li>Incubated at 37°C for 1 hour</li>
-					<li>Heat killed enzyme for 20mins at 65 degrees Celsius</li>
+					<li>Heat killed enzyme for 20 mins at 65°C</li>
 					</ul>
 					<p class="top_notebook"><a href="#wrapper">Back to Top</a></p>
@@ Line 203: / Line 240: @@
 					<li>Name: Yoyo Y</li>
 					<li>Date: April 2, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Tube 1 - J23100_J06702_pSB1C3</li>
@@ Line 210: / Line 247: @@
 					<li>Tube 3 - J23113_J06702_pSB1C3</li>
 					<li>Tube 4 - J23114_J06702_pSB1C3</li>
-					<li>Left overnight at 16 degrees Celsuis</li>
+					<li>Left overnight at 16°C</li>
 					<li>Agarose Gel of Digested Parts 1%</li>
-					<li><img src="images/lethbridgehs2013-4-2-agarose-picture.gif" alt=" " width="400px" /></li>
+					<li><img src="https://static.igem.org/mediawiki/2013hs/0/05/Lethbridge_hs_igem_2013-4-2-agarose-picture.gif" alt=" " width="400px" /></li>
 					</ul>
 					</div>
@@ Line 305: / Line 342: @@
 					<li>Name: Fiona S, Chris I, Yoyo Y</li>
 					<li>Date: April 3, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Antibiotic: CAM</li>
@@ Line 322: / Line 359: @@
 					<li>Names: Chris I, Fiona S</li>
 					<li>Date: April 4, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Part Number and Plasmid: J23100_J06702_pSB1C3, J23108_J06702_pSB1C3, J23113_J06702_pSB1C3, J23114_J06702_pSB1C3</li>
@@ Line 338: / Line 375: @@
 					<li>Names: Chris I, Yoyo Y</li>
 					<li>Date: April 5, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Miniprepped J23108_pSB1A2, J23113_pSB1A2, J23114_pSB1A2, J06702_pSB1AK2, used 50uL of Elution Buffer</li>
+					<li>Miniprepped J23108_pSB1A2, J23113_pSB1A2, J23114_pSB1A2, J06702_pSB1AK2, used 50µL of Elution Buffer</li>
 					</ul>
 					<p class="top_notebook"><a href="#wrapper">Back to Top</a></p>
@@ Line 354: / Line 391: @@
 					<li>Names: Chris I, Yoyo Y, Elaine B</li>
 					<li>Date: April 5, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					</ul>
@@ Line 418: / Line 455: @@
 					<li>Names: Shikhar M, Krista F, Austin K</li>
 					<li>Date: April 6, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Miniprepped J23108_J06702_pSB1C3, J23113_J06702_pSB1C3, J23100_J06702_pSB1C3 used 50uL of Elution Buffer</li>
+					<li>Miniprepped J23108_J06702_pSB1C3, J23113_J06702_pSB1C3, J23100_J06702_pSB1C3 used 50µL of Elution Buffer</li>
 					<li>Note: left plates to grow longer, need DNA sequenced.</li>
 					</ul>
@@ Line 435: / Line 472: @@
 					<li>Name: Erin K</li>
 					<li>Date: April 7, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSb1Ak2</li>
+					<li>J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2</li>
-					<li>Separately added 2uL of appropriate DNA  and 0.2uL of Pfu Polymerase to 17.8 uL MM</li>
+					<li>Separately added 2µL of appropriate DNA  and 0.2µL of Pfu Polymerase to 17.8µL MM</li>
 					<li>Agarose Gel confirmation of PCR: Success</li>
 					</ul>
@@ Line 450: / Line 487: @@
 									<tr>
 										<th>MM 5x Reagent</th>
-										<th>Volume(uL)</th>
+										<th>Volume(µL)</th>
 									</tr>
 								</thead>
@@ Line 488: / Line 525: @@
 					<li>Name: Erin K</li>
 					<li>April 8, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>2 samples of J06702_pSB1AK2: Added 0.5uL XbaI and 0.5uL PstI to 24uL MM</li>
+					<li>2 samples of J06702_pSB1AK2: Added 0.5µL XbaI and 0.5µL PstI to 24µL MM</li>
 					<li>
 						<table class="table_two_left">
@@ Line 497: / Line 534: @@
 								<tr>
 									<th>J06702 MM 2x</th>
-									<th>Volume (uL)</th>
+									<th>Volume (µL)</th>
 								</tr>
 							</thead>
@@ Line 520: / Line 557: @@
 						</table>
 					</li>
-					<li>2 samples of TAT-E1010_pSB1C3: Added 0.5uL EcoRIand 0.5uL PstI to 24uL MM</li>
+					<li>2 samples of TAT-E1010_pSB1C3: Added 0.5µL EcoRIand 0.5µL PstI to 24µL MM</li>
 					<li>
 						<li>
@@ Line 527: / Line 564: @@
 								<tr>
 									<th>TAT-E1010_pSB1C3 MM 2x</th>
-									<th>Volume (uL)</th>
+									<th>Volume (µL)</th>
 								</tr>
 							</thead>
@@ Line 551: / Line 588: @@
 					</li>
 					</li>
-					<li>2 samples of each of the 3 promoters: Added 5uL appropriate DNA and 0.5uL EcoRI and 0.5uL SpeI to 16uL MM</li>
+					<li>2 samples of each of the 3 promoters: Added 5µL appropriate DNA and 0.5µL EcoRI and 0.5µL SpeI to 16µL MM</li>
 					<li>
 						<table class="table_two_left">
@@ Line 557: / Line 594: @@
 								<tr>
 									<th>Promoter MM 7x</th>
-									<th>Volume (uL)</th>
+									<th>Volume (µL)</th>
 								</tr>
 							</thead>
@@ Line 588: / Line 625: @@
 					<li>Names: Wesley M, Riley M, Krista F</li>
 					<li>Date: April 8, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Parts: J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1ak2</li>
+					<li>Parts: J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2</li>
 					<li>Results: Unsuccessful</li>
 					</ul>
@@ Line 685: / Line 722: @@
 					<li>Names: Wesley M, Riley M, Krista F</li>
 					<li>Date: April 8, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
-					<li>Protocol: Biobasic Kit: Eluted with 30uL elution buffer</li>
+					<li>Protocol: Biobasic Kit: Eluted with 30µL elution buffer</li>
 					</ul>
 					<p class="top_notebook"><a href="#wrapper">Back to Top</a></p>
@@ Line 700: / Line 737: @@
 					<li>Name: Elaine B, Chris I, Fiona S, Wesley M, Riley M</li>
 					<li>Date: April 9, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSb1Ak2</li>
+					<li>J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2</li>
-					<li>Separately added 2uL of appropriate DNA  and 0.2uL of Pfu Polymerase to 17.8 uL MM</li>\
+					<li>Separately added 2µL of appropriate DNA  and 0.2µL of Pfu Polymerase to 17.8µL MM</li>\
 					</ul>
 					</div>
@@ Line 753: / Line 790: @@
 					<li>Names: Chris I, Elaine B, Fiona S, Wesley M, Riley M,</li>
 					<li>Date: April 9, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Picked: J23113_J61002, J23108_J61002, J23114_J61002, J23100_J61002, J06702_pSB_1AK2</li>
-					<li>5 mL cultures, 5uL Amp. grown overnight at 37 degrees Celsius</li>
+					<li>5mL cultures, 5µL Amp. grown overnight at 37°C</li>
 					</ul>
 					<p class="top_notebook"><a href="#wrapper">Back to Top</a></p>
@@ Line 769: / Line 806: @@
 					<li>Names: Yoyo Y</li>
 					<li>Date: April 10, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Mini Prep of (x2 of 35uL): J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002</li>
+					<li>Mini Prep of (x2 of 35µL): J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002</li>
 					<li>Mini-prepped with EZ-10 columns</li>
-					<li>Eluted 35uL</li>
+					<li>Eluted 35µL</li>
 					<li>Purified DNA in HS iGEM Kit #1</li>
 					</ul>
@@ Line 788: / Line 825: @@
 					<li>Names: Dylan S</li>
 					<li>Date: April 10, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Add 33uL DNA to 17uL MM</li>
+					<li>Add 33µL DNA to 17µL MM</li>
-					<li>17uL MM to promoter tubes</li>
+					<li>17µL MM to promoter tubes</li>
-					<li>33uL DNA to promoter tubes</li>
+					<li>33µL DNA to promoter tubes</li>
 					<li>Same procedure for J06702_pSB1AK3</li>
-					<li>Incubated at 37 degrees Celsius for 2hours</li>
+					<li>Incubated at 37°C for 2 hours</li>
-					<li>Heat killed at 65 degrees Celsius for 20minutes</li>
+					<li>Heat killed at 65°C for 20 minutes</li>
 					</ul>
 					</div>
@@ Line 845: / Line 882: @@
 					<li>Names: Dylan S, Patrick O</li>
 					<li>Date: April 11, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Mini prep of (35uL EB): J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002</li>
+					<li>Mini prep of (35µL EB): J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002</li>
 					<li>Mini-prepped with EZ-10 columns</li>
-					<li>Eluted 35uL</li>
+					<li>Eluted 35µL</li>
 					<li>Purified DNA in HS iGEM Kit #1</li>
 					</ul>
@@ Line 864: / Line 901: @@
 					<li>Names: Wesley M, Yoyo Y</li>
 					<li>Date: April 12, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Restriction of E1010_pSB1C3 at sites E & P</li>
-					<li>50uL rxn</li>
+					<li>50µL rxn</li>
-					<li>Add 30uL DNA to 20uL MM</li>
+					<li>Add 30µL DNA to 20µL MM</li>
-					<li>Added 0.5uL EcroR1 & Pst1</li>
+					<li>Added 0.5µL EcoR1 & Pst1</li>
-					<li>Incubated 2hours at 37 degrees Celsius</li>
+					<li>Incubated 2 hours at 37°C</li>
-					<li>Heat killed 20minutes at 65 degrees Celsius</li>
+					<li>Heat killed 20 minutes at 65°C</li>
 					</ul>
 					</div>
@@ Line 912: / Line 949: @@
 					<li>Names: Patrick O, Shikhar M</li>
 					<li>Date: April 12, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Reculturization of: J06702_pSB1AK3, J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002</li>
-					<li>PCR: Master mix created with: Annealing temperature: 55.6 degrees Celsius</li>
+					<li>PCR: Master mix created with: Annealing temperature: 55.6°C</li>
 					</ul>
 					</div>
@@ Line 985: / Line 1,022: @@
 					<li>Names: Amrinder G, Steven T</li>
 					<li>Date: April 12, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Mini prep of (35uL EB): J06702_pSB1AK3, J23100_J61002, J23108_J61002 ,J23113_J61002, J23114_J61002</li>
+					<li>Mini prep of (35µL EB): J06702_pSB1AK3, J23100_J61002, J23108_J61002 ,J23113_J61002, J23114_J61002</li>
 					<li>Mini-prepped with EZ-10 columns</li>
-					<li>Eluted 35uL</li>
+					<li>Eluted 35µL</li>
 					<li>Purified DNA in HS iGEM Kit #1</li>
 					</ul>
@@ Line 1,003: / Line 1,040: @@
 					<li>Names: Fiona S, Katie T</li>
 					<li>Date: April 14, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
-					<li>Mini prep of (35uL EB): J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002, J06702_PSB1AK2</li>
+					<li>Mini prep of (35µL EB): J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002, J06702_pSB1AK2</li>
 					<li>Mini-prepped with EZ-10 columns</li>
-					<li>Eluted 35uL</li>
+					<li>Eluted 35µL</li>
 					</ul>
 					<p class="top_notebook"><a href="#wrapper">Back to Top</a></p>
@@ Line 1,021: / Line 1,058: @@
 					<li>Names: Fiona S, Katie T</li>
 					<li>April 14, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					<li>Parts: J23100_J61002, J23108_J61002, J23113_J61002, J23114_J61002</li>
 					<li>Gel Extraction</li>
-					<li>Parts: J23108_J61002, J23113 J61002</li>
+					<li>Parts: J23108_J61002, J23113_J61002</li>
-					<li>Eluted 50 uL</li>
+					<li>Eluted 50 µL</li>
 					</ul>
 					</div>
@@ Line 1,119: / Line 1,156: @@
 					<ul class="notebook_entry_list">
 					<li>Master Mix: Yoyo Yao promoters x9</li>
-					<li>35uL DNA, 14uL MM, 0.5uL Spe1, 0.5uL Pst1</li>
+					<li>35uL DNA, 14µL MM, 0.5µL Spe1, 0.5µL Pst1</li>
 					<li>Date: April 15, 2013</li>
 					</ul>
@@ Line 1,159: / Line 1,196: @@
 					<ul class="notebook_entry_list">
 					<li>Master Mix: FS, KT ½ promoter ½ insulin/glucose x17</li>
-					<li>(Promoters) 25uL DNA, 24uL MM, 0.5uL Spe1, 0.5uL Pst1</li>
+					<li>(Promoters) 25µL DNA, 24µL MM, 0.5µL Spe1, 0.5µL Pst1</li>
-					<li>(Insulin/Glucose) 25uL DNA, 24uL MM, 0.5uL EcoR1, 0.5uL Pst1</li>
+					<li>(Insulin/Glucose) 25µL DNA, 24µL MM, 0.5µL EcoR1, 0.5µL Pst1</li>
 					<li>Date: April 15, 2013</li>
 					</ul>
@@ Line 1,201: / Line 1,238: @@
 					<li>Names: Yoyo Y, Erin K</li>
 					<li>April 15, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					</ul>
@@ Line 1,486: / Line 1,523: @@
 					<li>Name: Dylan S</li>
 					<li>Date: April 17, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					</ul>
@@ Line 1,530: / Line 1,567: @@
 									<td>5</td>
 									<td>J23100 mlc J06702</td>
-									<td>PSB3C5</td>
+									<td>pSB3C5</td>
 									<td>50</td>
 								</tr>
@@ Line 1,536: / Line 1,573: @@
 									<td>6</td>
 									<td>J23100 mlc J06702</td>
-									<td>PSB3C5</td>
+									<td>pSB3C5</td>
 									<td>50</td>
 								</tr>
@@ Line 1,560: / Line 1,597: @@
 					<li>Name: Chris I</li>
 					<li>Date: April 30, 2013</li>
-					<li>Species: E. Coli</li>
+					<li>Species: E. coli</li>
-					<li>Strain: DH5A</li>
+					<li>Strain: DH5α</li>
 					<li>Protocol: Ute Kothe</li>
 					</ul>

Team:Lethbridge Canada/notebook april

From 2013hs.igem.org

Latest revision as of 03:49, 22 June 2013

Notebook Links

Restriction - Ligation

Ligations

Transformation

Re-Plating Transformation

Miniprep of ON Cultures

UV Spectroscopy DNA Concentrations

Miniprep From Ligation

PCR

Restriction Digestion of PCR Parts

3% Agarose Gel of Digested PCR Parts

Gel Extraction

Repeat PCR

Picking Cells

Mini Prep

Restriction

Agarose Gel of PCR 1%

Miniprep

Restriction Digestion

PCR and Cell Reculturization

Miniprep

Miniprep

1% Agarose Gel

Restriction/Digestion

Restriction/Digestion

1% Agarose Gel of Promoters

Transformation

1% Agarose Gel of Promoter Constructs