Latest revision as of 23:20, 18 September 2015

Research Notebook

Week 12 (13/9 - 18/9)

▪ Sep 13

Invasin + Listerolysin Anaerobic Promoter
☀ Chi Yan ☀

Ran gel for placgfp-psB1C3 colonies from Chi Yan 12/9 11pm. 1% 110V 30min
▶ no bands
▶ no positive colonies

Ran gel for PCRs to make Prefix-pNirB-inv-Suffix from Chi Yan 12/9 11pm
▶ E: successful, cut bands.
▶ F, G, H,I no bands

PCR for YT, Template used is gel extract ‘1.5.2’ (26ng/ul)
Primers used are FP2’ and RP2

8 cycles 50-60degrees 2 min for annealing step
30 cycles 55-65 degrees 40s for annealing step

50ul, 3 tubes, put in columns 4, 8 12. Negative control added.

Buffer	15
dNTPs	6
MgCl2	6
Primers	1.5/1.5
Template	15
H2O	104.25
Taq	0.75

Invasin + Listerolysin Anaerobic Promoter
☀ Yi Han ☀

Ran gel for YT PCR

PCR using F2 to produce F2/invendsuffix
Primer pairs are invlloF3new/invendsuffix and invlloF6/invendsuffix

PCR for YT, Template used is gel extract ‘1.5.2’ (26ng/ul)
Primers used are FP2’ and RP2

invlloF3new/invendsuffix
Template (1000ng)	18
Primer	2/2
Buffer	20
sNTP	8
Taq	1
H2O	149
Total	200

invlloF6/invendsuffix
Template 500ng	9
Primer	1/1
Buffer	10
dNTP	4
Taq	0.5
H2O	74.5
Total	100

Attempt to make more of inv fragment from Yun Ting’s gel extract
Primers are FP2’/RP

Template	8.2
Primer	1/1
Buffer	10
dNTP	4
Taw	0.5
H2O	75.3
Total	100

Invasin + Listerolysin Anaerobic Promoter
☀ Chi Yan & Yi Han ☀

PCR of invlloF1/lloendBBSuffix R with invasin D plasmid as template
▶ 5 cycles gradient 40-50degrees
▶ 20 cycles 62 degrees

Buffer	40
MgCl2	16
dNTPs	16
Primers	4/4
Template	9.2
H2O	308.8
Taq	2
Total	400

▶ 12 tubes at each temp, 33ul each

For YT: PCR of RP2/FP2’ using gel extract 1.6

Buffer	20
dNTP	8
MgCl2	8
Primers	2/2
Taq	1
H2O	135
Total	200
(3 tubes + 5ul template, 1 tube control)

Gel extract F1 invlloendsuffix
PCR of invlloend/BBsuffixR with invD
PCR of invlloF2/lloendBBsuffixR with F1/invlloendsuffix

F1invlloendsuffix
BUffer	80
MgCl2	32
dNTPs	32
Primers	8/8
Template	18.4
H2O	617.6
Taq	4
Total	800

Buffer	20
MgCl2	8
dNTPs	8
Primers	2/2
Template	84
H2O	75
Taq	1
Total	200

▶ 5 cycles 44-48 degrees
25 cycles 60degrees

Colony PCR new placgfp-pSB1C3 following CY 12/9 11pm
Primers FP_KpnI_GFP/GFP_BBSuffix_new
60 degrees 25 cycles

▪ Sep 14

Anaerobic Promoter ☀ Yi Han ☀

Ran gel for Chi Yan 13/9 9pm and 11pm
▶ Colony PCR no bands
▶ B1-12 no bands
▶ A1-16 bright band , correct size, extract

Anaerobic Promoter ☀ Chi Yan ☀

PCR of invlloF1/lloendBBsuffixR with invD

Buffer	160
MgCl2	32
dNTPs	32
Primers	32/32
Template	18.3
H2O	517.7
Taq	8
Total	800

PCR of invloF2/lloendBBsuffix R with invlloF1endsuffixR

Buffer	80
MgCl2	16
dNTPs	16
Primers	16/16
Template	100
H2O	152
Taq	4
Total	400

Cycle conditions as of Chi Yan 13/9
Positions of tubes, A-C B-D
PCR done with GoTaq kit

Anaerobic Promoter ☀ Yi Han ☀

Screen placgfp colonies for gfp using microscope
▶ Colonies 1, 4, 8 look promising

Miniprepped placgfp colonies

RE of colony 1, 4, 8
Template	1
EcoRI/PstI	0.1/0.1
Buffer	1
H2O	8
Total	10.2

Anaerobic Promoter ☀ Chi Yan ☀

Sent colonies 1, 4, 8 of placgfppSB1C3 for sequencing with FP_BB_Prefix, RP_BB_Suffix, VF2.
Ran gel for YH placgfp pSB1C3 colonies RE 1, 4, 8
Incomplete digestion as only digested for 1.5hours
PCR of placgfp pSB1C3 colonies 1, 4, 8 from plasmids and with placfp pAC with FP_BB_Prefix and RP_BB_Suffix
Annealing temp 55degrees for 30s, extension for 60 seconds, for 25 cycles

GOTaq Master Mix 1
Buffer	20
MgCl2	10
dNTPs	4
Primers	4/4
Taq	1

Anaerobic Promoter ☀ Yi Han ☀

PCR with GoTaq kit to make Fragment 8 from Fragment 1

Template (500ng)	40
dNTPs	4
MgCl2	16
Primers	2/2
GoTaq	0.5
PCR Buffer	20
H2O	19.5
Total	104.5

Continued from previous
Ran gradient at annealing temperature for 55-65, in wells 1, 4, 7, 12

Ran gel, no bands in all
1. Made more F1 invsuffixendloger from invD
2. Use BB PrefixpBirBinvstart/invendBBSuffixend to generate whole fragment
3. Make fragment 8 using F8/invendsuffixlonger

Set PCR machine to 10 cycles at Ta gradient 40-55 degrees
30 cycles Ta 60 degrees
Ramp of 10%

PCR mix for 1 and 2
InvD Template	9.2
dNTPs	20
MgCl2	16
Primers	4/4
GoTaq	0.5
H2O	105.8

PCR mix for 3
Template	45
dNTP	8
MgCl2	8
Primers	1/1
GoTaq	1
PCR Buffer	20
H2O	16
Total	100

▶ Result: 1, 2 had clear bands, 3 had no bands

Anaerobic Promoter ☀ Chi Yan ☀

PCR of placgfp colonies 1, 4, and 8 plasmids and placgfp pAC colony plasmid using VF2/VR
Annealing temperature is 52degrees for 30seconds, extension of 60s 30 cycles using GoTaq kit

Buffer	20
MgCl2	16
dNTPs	4
Primers	4/4
Taq	1

▶ Colony 1: Template 0.4/12.35 H2O
▶ Colony 4: Template 0.8/11.85 H2O
▶ Colony 8: Template 0.7/12.05 H2O
▶ pAC: Template 2.5/10.25

▪ Sep 15

esa Quorum Sensing ☀ Adrian ☀

BBa_B0015 RE D
Buffer	4
H2O	6
EcoRI-HF	1
PstI-HF	1
Template	10
Total	20

Colony pcr for two samples
H2O	13.5
Buffer	5
MgCl2	2
dNTP	2
FP_BBPrefix_Junk	1
RP_BBPrefix_Junk	1
Taq	0.5
Total	25

Rapid DNA Ligation: 200ng insert: 21.4 ng vector

Anaerobic Promoter ☀ Yi Han ☀

PCR with prefix-pNirB ultramer was successful.

PCR with Junk primers to add sequence
dNTPS	20
MgCl2	16
Primers	4/4
GoTaq	2
Buffer	40
Template (1500ng)	88
H2O	26
Total	200

PCR 12 tubes, gradient (58-62degrees) for 30cycles
Ran gel first three tubes had PCR product (Junk-pNirB-inv-suffix-Junk) with large bands-gel extract

RE of above PCR product with EcoRI/PstI
DNA	50
Buffer	5
EcoRI	0.5
PstI	0.5
Total	55

esa Quorum Sensing ☀ Kenneth ☀

GFP Thingy
Buffer 4	2
H2O	6
EcoRI-HF	1
PstI-HF	1
Template	10
Total	20

Anaerobic Promoter ☀ Chi Yan ☀

Colony PCR (and inoculation in 3mL LB+chl) of psB1C3-placgfp colonies 1, 4, 8, 11-31, placgfppAC, water. 15ul reaction *26 = 650

Mastermix
Buffer	130
MgCl2	104
dNTPs	26
Primers	26/26
Taq	6.5
(H2O 11.75 each)
(12.25ul mastermix each tube)

Run gel for YH 15/9 RE of pSB1C3 (gel purified) and Junk-pref-pNirB-inv-suffix-junk with EcoRI/PstI

Anaerobic Promoter ☀ Yi Han ☀

Extract of the RE digested BB-Prefix-pirB-inv-suffix

Ligation Reaction

Template (insert)	60
Ligase	3
10X buffer	3
Cut pSB13	1.35

PCR to get more Junk-prefix-pNirB-Suffix-junk

Template (2550ng)	150
dNTPs	33
MgCl2	25.6
Primer	6.4/6.4
GoTaq	3.2
Buffer	64
Total	250

Anaerobic Promoter ☀ Chi Yan ☀

Run gel for CY 15/9 4pm colony pcr
▶ 1kb, 100bp, 1, 4, 8, 11-23, 100bp, 1kb
▶ 1kb, 100bp, 24-31, PCR Junk-Prefix-placgfp-suffix-Junk, pSC, H2O, 100bp, 1kb

Positive result with colony PCR for colonies 12, 13, 15, 17 (does not glow), 19, 20
▶ Duy used confocal microscopy to check for GFP expression
▶ Sequencing results showed that colonies 12, 13 and 19 has correct sequence.

Anaerobic Promoter ☀ Chi Yan ☀

gel extract Junk-prefix-pNirB-inv-suffix-junk from YH 15/9 7pm

RE with EcoRI/PstI 2hours at 37 degrees
DNA	30
Buffer	3
EcoRI	0.5
PstI	0.5

The ligated plasmid was then transformed into 10ul BL21.

7:1 ligation reaction
Insert	10.4
Vector	1.5
Ligase	1
Buffer	2
Water	5.1

5:1 ligation reaction
Insert	7.56
Vector	1.5
Ligase	1
Buffer	2
Water	8.04

▪ Sep 16

Anaerobic Promoter ☀ Yi Han ☀

Inoculated colonies 12, 13, 19 of pSB1C3 placgfp and pAC placgfp, BL21 in 3mL LB at 7 am and 8am

Colony PCR for pNirBinv in pSB1C3 using Biobricks suffix/prefix primers

H2O	22.75
PCR Buffer	35
dNTP	7
Primer	7/7
MgCl2	17.5
Taq	1.75

▶ PCR was run for 24 cycles at Annealing temperature of 54, using the ‘COLONY protocol’
▶ Faint band of correct size was produced for colony 4

▪ Sep 17

Anaerobic Promoter ☀ Yi Han ☀

Colony PCR for colony 4 of pSB1C3 was conducted using:
1. VF/VR primers for Ta of 55
2. BiobricksPrefix/Suffix primers for Ta of 57
3. invlloF1/invendBBsuffixlonger for Ta of 65
with separate negative controls for each
▶ A band of the correct size, 2.8kb was produced for 2. and 3.

Anaerobic Promoter ☀ Chi Yan ☀

PCR of placgfppSB1C3 colony 12, JUnk prefix-placgfp-suffix-junk, placgfppAC, negative control of water

Mastermix
Buffer	20
MgCl2	16
dNTPs	4
Primers	4/4
Taq	1

PCR of same templates as above
▶ Primers: F2’_Prefixplac/RP_VR
▶ Same master mix as above
Ran gel for above PCRs

Anaerobic Promoter ☀ Yi Han ☀

Mammalian cell invasion assay with BL21 and BL21+pSB1C3-pNirB-invasin under aerobic and anaerobic conditions

Anaerobic Promoter ☀ Duy ☀

Confocal microscopy to determine relative levels of GFP fluorescence

@@ Line 61: / Line 61: @@
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 </div>
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 <ul>
-   <li><a href='https://2015.igem.org/Team:SPSingapore/'><span>Home</span></a></li>
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-   <li><a href='https://2015.igem.org/Team:SPSingapore/Team'><span>Team</span></a></li>
+	<li><a href='https://2015.igem.org/Team:SPSingapore/Team'><span>Team</span></a>
-   <li><a href='https://2015.igem.org/Team:SPSingapore/Project'><span>Project</span></a></li>
+	<ul>
-   <li><a href='https://2015.igem.org/Team:SPSingapore/Protocol'><span>Protocol</span></a></li>
+		<li><a href="https://2015.igem.org/Team:SPSingapore/Team">Overview</a></li>
-   <li><a href='https://2015.igem.org/Team:SPSingapore/Parts'><span>Parts</span></a></li>
+		<li><a href="https://igem.org/Team.cgi?id=1804">Official Profile</a></li>
-   <li class = 'active'><a href='https://2015.igem.org/Team:SPSingapore/Notebook'><span>Notebook</span></a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Team Bios">Team Bios</a></li>
-   <li><a href='https://2015.igem.org/Team:SPSingapore/Practices'><span>Human Practices</span></a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Mentors">Mentors</a></li>
-   <li class='last'><a href='https://2015.igem.org/Team:SPSingapore/Safety'><span>Safety</span></a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Attributions">Attributions</a></li>
+	</ul>
+	</li>
+	<li><a href='https://2015.igem.org/Team:SPSingapore/Project'><span>Project</span></a>
+	<ul>
+		<li><a href='https://2015.igem.org/Team:SPSingapore/Project'>Overview</a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Invasin">Invasin + Listerolysin</a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/ESAQS">esa Quorum Sensing</a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Anaerobic Promoter">Anaerobic Promoter</a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Parts">Parts</a></li>
+	</ul>
+	</li>
+	<li><a href='https://2015.igem.org/Team:SPSingapore/Notebook'><span>Notebook</span></a>
+	<ul>
+		<li><a href="https://2015.igem.org/Team:SPSingapore/Protocol">Protocols</a></li>
+        <li><a href="https://2015.igem.org/Team:SPSingapore/Notebook">Entries</a></li>
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+	</ul>
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+	<li class='last'><a href='https://2015.igem.org/Team:SPSingapore/Medals'><span>Medals</span></a></li>
 </ul>
 </div>
@@ Line 77: / Line 105: @@
 <div id='sidemenu' style = "float:left">
 <ul>
+   <li><a href = "https://2015.igem.org/Team:SPSingapore/Notebook"><span>NOTEBOOK</span></a>
-<li><a href = "https://2015.igem.org/Team:SPSingapore/Notebook"><span>NOTEBOOK</span></a>
     <ul><li class = 'last'>&nbsp;</li></ul></li>
@@ Line 601: / Line 628: @@
+<tr class = "tablenotebook"><td><div class = "paper">
+&#9642; Sep 15
+<br><br>
+<span class = "black"> esa Quorum Sensing</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Adrian &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	BBa_B0015	RE	D							</b>	</td></tr>
+<tr><td>	Buffer						</td><td>	4			</td></tr>
+<tr><td>	H2O						</td><td>	6			</td></tr>
+<tr><td>	EcoRI-HF						</td><td>	1			</td></tr>
+<tr><td>	PstI-HF						</td><td>	1			</td></tr>
+<tr><td>	Template						</td><td>	10			</td></tr>
+<tr><td>	Total						</td><td>	20			</td></tr>
+</table>
+<br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	Colony	pcr	for	two	samples					</b>	</td></tr>
+<tr><td>	H2O						</td><td>	13.5			</td></tr>
+<tr><td>	Buffer						</td><td>	5			</td></tr>
+<tr><td>	MgCl2						</td><td>	2			</td></tr>
+<tr><td>	dNTP						</td><td>	2			</td></tr>
+<tr><td>	FP_BBPrefix_Junk						</td><td>	1			</td></tr>
+<tr><td>	RP_BBPrefix_Junk						</td><td>	1			</td></tr>
+<tr><td>	Taq						</td><td>	0.5			</td></tr>
+<tr><td>	Total						</td><td>	25			</td></tr>
+</table>
+<br>
+<span class = "nbcontent">
+Rapid DNA Ligation: 200ng insert: 21.4 ng vector
+</span>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Yi Han &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+PCR with prefix-pNirB ultramer was successful.
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	PCR	with	Junk	primers	to	add	sequence			</b>	</td></tr>
+<tr><td>	dNTPS				</td><td>			20			</td></tr>
+<tr><td>	MgCl2		</td><td>					16			</td></tr>
+<tr><td>	Primers		</td><td>					4/4			</td></tr>
+<tr><td>	GoTaq		</td><td>					2			</td></tr>
+<tr><td>	Buffer		</td><td>					40			</td></tr>
+<tr><td>	Template	(1500ng)	</td><td>					88			</td></tr>
+<tr><td>	H2O			</td><td>				26			</td></tr>
+<tr><td>	Total			</td><td>				200			</td></tr>
+</table>
+<br><br>
+<span class = "nbcontent">
+PCR 12 tubes, gradient (58-62degrees) for 30cycles
+<br> Ran gel first three tubes had PCR product (Junk-pNirB-inv-suffix-Junk) with large bands-gel extract
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	RE	of	above	PCR	product		with	EcoRI/PstI		</b>	</td></tr>
+<tr><td>	DNA				</td><td>			50			</td></tr>
+<tr><td>	Buffer				</td><td>			5			</td></tr>
+<tr><td>	EcoRI				</td><td>			0.5			</td></tr>
+<tr><td>	PstI				</td><td>			0.5			</td></tr>
+<tr><td>	Total				</td><td>			55			</td></tr>
+</table>
+</div>
+<br><br>
+<span class = "black"> esa Quorum Sensing</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Kenneth &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	GFP	Thingy								</b>	</td></tr>
+<tr><td>	Buffer	4			</td><td>			2			</td></tr>
+<tr><td>	H2O				</td><td>			6			</td></tr>
+<tr><td>	EcoRI-HF				</td><td>			1			</td></tr>
+<tr><td>	PstI-HF				</td><td>			1			</td></tr>
+<tr><td>	Template				</td><td>			10			</td></tr>
+<tr><td>	Total				</td><td>			20			</td></tr>
+</table>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Chi Yan &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Colony PCR (and inoculation in 3mL LB+chl) of psB1C3-placgfp colonies 1, 4, 8, 11-31, placgfppAC, water. 15ul reaction *26 = 650
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	Mastermix									</b>	</td></tr>
+<tr><td>	Buffer				</td><td>			130			</td></tr>
+<tr><td>	MgCl2				</td><td>			104			</td></tr>
+<tr><td>	dNTPs				</td><td>			26			</td></tr>
+<tr><td>	Primers				</td><td>			26/26			</td></tr>
+<tr><td>	Taq				</td><td>			6.5			</td></tr>
+<tr><td style = "text-align:center" colspan = 2> (H2O 11.75 each)</td></tr>
+<tr><td style = "text-align:center" colspan = 2> (12.25ul mastermix each tube)</td></tr>
+</table>
+<br>
+<span class = "nbcontent">
+Run gel for YH 15/9 RE of pSB1C3 (gel purified) and Junk-pref-pNirB-inv-suffix-junk with EcoRI/PstI
+</span>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Yi Han &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Extract of the RE digested BB-Prefix-pirB-inv-suffix
+</span><br><br>
+<span class = "nbcontent">
+Ligation Reaction
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td>	Template	(insert)			</td><td>			60			</td></tr>
+<tr><td>	Ligase				</td><td>			3			</td></tr>
+<tr><td>	10X	buffer			</td><td>			3			</td></tr>
+<tr><td>	Cut	pSB13			</td><td>			1.35			</td></tr>
+</table>
+<br><br>
+<span class = "nbcontent">
+PCR to get more Junk-prefix-pNirB-Suffix-junk
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td>	Template	(2550ng)			</td><td>			150			</td></tr>
+<tr><td>	dNTPs				</td><td>			33			</td></tr>
+<tr><td>	MgCl2				</td><td>			25.6			</td></tr>
+<tr><td>	Primer				</td><td>			6.4/6.4			</td></tr>
+<tr><td>	GoTaq				</td><td>			3.2			</td></tr>
+<tr><td>	Buffer				</td><td>			64			</td></tr>
+<tr><td>	Total				</td><td>			250			</td></tr>
+</table>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Chi Yan &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Run gel for CY 15/9 4pm colony pcr
+<br> &#9654; 1kb, 100bp, 1, 4, 8, 11-23, 100bp, 1kb
+<br> &#9654; 1kb, 100bp, 24-31, PCR Junk-Prefix-placgfp-suffix-Junk, pSC, H2O, 100bp, 1kb
+</span>
+<br><br>
+<span class = "nbcontent">
+Positive result with colony PCR for colonies 12, 13, 15, 17 (does not glow), 19, 20
+<br> &#9654; Duy used confocal microscopy to check for GFP expression
+<br> &#9654; Sequencing results showed that colonies 12, 13 and 19 has correct sequence.
+</span>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Chi Yan &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+gel extract Junk-prefix-pNirB-inv-suffix-junk from YH 15/9 7pm
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	RE	with	EcoRI/PstI	2hours	at	37	degrees			</b>	</td></tr>
+<tr><td>	DNA				</td><td>			30			</td></tr>
+<tr><td>	Buffer				</td><td>			3			</td></tr>
+<tr><td>	EcoRI				</td><td>			0.5			</td></tr>
+<tr><td>	PstI				</td><td>			0.5			</td></tr>
+</table>
+<br><br>
+<span class = "nbcontent">
+The ligated plasmid was then transformed into 10ul BL21.
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	7:1	ligation	reaction							</b>	</td></tr>
+<tr><td>	Insert				</td><td>			10.4			</td></tr>
+<tr><td>	Vector				</td><td>			1.5			</td></tr>
+<tr><td>	Ligase				</td><td>			1			</td></tr>
+<tr><td>	Buffer				</td><td>			2			</td></tr>
+<tr><td>	Water				</td><td>			5.1			</td></tr>
+</table>
+<br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	5:1	ligation	reaction							</b>	</td></tr>
+<tr><td>	Insert				</td><td>			7.56			</td></tr>
+<tr><td>	Vector				</td><td>			1.5			</td></tr>
+<tr><td>	Ligase				</td><td>			1			</td></tr>
+<tr><td>	Buffer				</td><td>			2			</td></tr>
+<tr><td>	Water				</td><td>			8.04			</td></tr>
+</table>
+</div>
+<br><br>
+</div>
+<div style = "border-top: 2px solid turquoise;"></div>
+</td>
+</tr>
 <!----------------------new day------------------------------>
+<tr class = "tablenotebook"><td><div class = "paper">
+&#9642; Sep 16
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Yi Han &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Inoculated colonies 12, 13, 19 of pSB1C3 placgfp and pAC placgfp, BL21 in 3mL LB at 7 am and 8am
+</span><br><br>
+<span class = "nbcontent">
+Colony PCR for pNirBinv in pSB1C3 using Biobricks suffix/prefix primers
+</span>
+<br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td>	H2O				</td><td>		22.75				</td></tr>
+<tr><td>	PCR	Buffer			</td><td>			35			</td></tr>
+<tr><td>	dNTP				</td><td>		7				</td></tr>
+<tr><td>	Primer				</td><td>		7/7				</td></tr>
+<tr><td>	MgCl2				</td><td>		17.5				</td></tr>
+<tr><td>	Taq				</td><td>		1.75				</td></tr>
+</table>
+<br>
+<span>
+&#9654; PCR was run for 24 cycles at Annealing temperature of 54, using the ‘COLONY protocol’
+<br> &#9654; Faint band of correct size was produced for colony 4
+</span>
+</div>
+<br><br>
+</div>
+<div style = "border-top: 2px solid turquoise;"></div>
+</td>
+</tr>
 <!----------------------new day------------------------------>
+<tr class = "tablenotebook"><td><div class = "paper">
+&#9642; Sep 17
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Yi Han &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Colony PCR for colony 4 of pSB1C3 was conducted using:
+<br> &emsp;&emsp;&emsp;&emsp; 1.	 VF/VR primers for Ta of 55
+<br> &emsp;&emsp;&emsp;&emsp; 2.	BiobricksPrefix/Suffix primers for Ta of 57
+<br> &emsp;&emsp;&emsp;&emsp; 3.	invlloF1/invendBBsuffixlonger for Ta of 65
+<br> with separate negative controls for each
+<br> &#9654; A band of the correct size, 2.8kb was produced for 2. and 3.
+</span>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Chi Yan &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+PCR of placgfppSB1C3 colony 12, JUnk prefix-placgfp-suffix-junk, placgfppAC, negative control of water
+</span><br>
+<table class = "nbtable" style = "margin-left:50px;">
+<tr><td colspan = 2><b>	Mastermix									</b>	</td></tr>
+<tr><td>	Buffer				</td><td>		20				</td></tr>
+<tr><td>	MgCl2				</td><td>		16				</td></tr>
+<tr><td>	dNTPs				</td><td>		4				</td></tr>
+<tr><td>	Primers				</td><td>		4/4			</td></tr>
+<tr><td>	Taq				</td><td>		1				</td></tr>
+</table>
+<br><br>
+<span class = "nbcontent">
+PCR of same templates as above
+<br> &#9654; Primers: F2’_Prefixplac/RP_VR
+<br> &#9654; Same master mix as above
+</span><br>
+<span class = "nbcontent">
+Ran gel for above PCRs
+</span>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Yi Han &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Mammalian cell invasion assay with BL21 and BL21+pSB1C3-pNirB-invasin under aerobic and anaerobic conditions
+</span>
+</div>
+<br><br>
+<span class = "brown"> Anaerobic Promoter</span>&emsp;&emsp;
+<font style = "color:blue;font-weight:bold;font-size:11pt;">&#9728; Duy &#9728;</font>
+<br><br>
+<div class = "divnbcontent">
+<span class = "nbcontent">
+Confocal microscopy to determine relative levels of GFP fluorescence
+</span>
+</div>
+<br><br>
+</div>
+<div style = "border-top: 2px solid turquoise;"></div>
+</td>
+</tr>

Difference between revisions of "Team:SPSingapore/Notebook-Week-17"

Latest revision as of 23:20, 18 September 2015

Research Notebook

Week 12 (13/9 - 18/9)