Team:TUDelft/19 August 2009

From 2009.igem.org

(Difference between revisions)

Revision as of 20:07, 19 October 2009

Lab Notebook

July
M	T	W	T	F	S	S
		1	2	3	4	5
6	7	8	9	10	11	12
13	14	15	16	17	18	19
20	21	22	23	24	25	26
27	28	29	30	31

August
M	T	W	T	F	S	S
					1	2
3	4	5	6	7	8	9
10	11	12	13	14	15	16
17	18	19	20	21	22	23
24	25	26	27	28	29	30
31

September
M	T	W	T	F	S	S
	1	2	3	4	5	6
7	8	9	10	11	12	13
14	15	16	17	18	19	20
21	22	23	24	25	26	27
28	29	30

October
M	T	W	T	F	S	S
			1	2	3	4
5	6	7	8	9	10	11
12	13	14	15	16	17	18
19	20	21	22	23	24	25
26	27	28	29	30	31

19 August 2009

Tim Weenink

After yesterdays horrible discovery that the I-SceI Homing Endonuclease we got from MIT was actually T4 DNA ligase we had to adjust our cloning strategy. The more primitive part without promoter was found to be the correct one, except that is was assembled with part !A instead of p(LacI). So we did that assembly again today. With p(LacI) from the delay team upstream, *T1 (downstream) and backbone pSB1C3 (also from the delay team). Both RbCl chemically comp and EC electrocomp cells were transformed.

Saeed

lane	Part	Expected Plasmid Size	Status
1	[http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder]
2	!Fr1n upstream	1900	ok, but not needed
3	!Fr1n downstream	1900	ok
4	destination plasmid	3000	ok

!Fr1n downstream will be purified from the gel by gel extraction and used for the new stategy as Tim mentioned before.

Daniel

Digestion of biobricks:

Well	Biobrick	Expected Plasmid Size	Status
1	[http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder]
2	C0051	750	✔
3	I13507	861	✔
4	P0440	840	✔
5	I13504	875	✔
6	J04630	857	✔
7	R0051	44	too small
8	B0015	129	✔
9	J13002	74	✔
10	pSB1C3	2072	✔
11	pSB1AK3	3426	✔
12	pSB1A3	2157	✔
13	CB
14	CC
15	[http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder]

Assemblies 1A, 2A, 3A, 4A, 5A and 6A

Transformation and culture in plates and tubes

Calin

Good results on the conjugation test. All plates were imaged on the safe imager with the 5 Megapixel camera. Colony counting was done with [http://www.pubmedcentral.nih.gov/articlerender.fcgi?artid=1770926 Clono-Counter].

For the trbK conjugation test:

Set 1
Plate ID	Antibiotics	Dilution	# Colonies
D1tr	TRI	10⁰	overgrown
D2tr	TRI	10^-1	overgrown
D3tr	TRI	10^-2	4450
D4tr	TRI	10^-3	714
D5tr	TRI	10^-4	86
T1tr	TRI + CAM	10⁰	2
T2tr	TRI + CAM	10^-1	0
T3tr	TRI + CAM	10^-2	0
T4tr	TRI + CAM	10^-3	0
T5tr	TRI + CAM	10^-4	0
R1tr	CAM	10⁰	overgrown
R2tr	CAM	10^-1	8636

Set 2
Plate ID	Antibiotics	Dilution	# Colonies
D6tr	TRI	10⁰	overgrown
D7tr	TRI	10^-1	overgrown
D8tr	TRI	10^-2	6930
D9tr	TRI	10^-3	720
D10tr	TRI	10^-4	81
T6tr	TRI + CAM	10⁰	2
T7tr	TRI + CAM	10^-1	0
T8tr	TRI + CAM	10^-2	0
T9tr	TRI + CAM	10^-3	0
T10tr	TRI + CAM	10^-4	0
R3tr	CAM	10⁰	overgrown
R4tr	CAM	10^-1	6333

also 3 positive control plates with no TrbK expression.

Results
Set #	Conjugation Efficinecy
1	4.49E-6
2	2.89E-6
control	0.031

This successfully shows a reduction in the conjugation efficiency by four orders of magnitude when the entry exclusion protein is expressed.

For the oriTR conjugation test:

Set 1
Plate ID	Antibiotics	Dilution	# Colonies
D1ori	TRI + CAM	10⁰	overgrown
D2ori	TRI + CAM	10^-1	overgrown
D3ori	TRI + CAM	10^-2	2939
D4ori	TRI + CAM	10^-3	470
D5ori	TRI + CAM	10^-4	48
Ts1ori	AMP + CAM	10⁰	520
Ts2ori	AMP + CAM	10^-1	1
Ts3ori	AMP + CAM	10^-2	0
Ts4ori	AMP + CAM	10^-3	0
Ts5ori	AMP + CAM	10^-4	0
TL1ori	TRI + AMP	10⁰	4092
TL2ori	TRI + AMP	10^-1	802
TL3ori	TRI + AMP	10^-2	94
TL4ori	TRI + AMP	10^-3	7
TL5ori	TRI + AMP	10^-4	0
R1ori	AMP	10⁰	overgrown
R2ori	AMP	10^-1	5187

Set 2
Plate ID	Antibiotics	Dilution	# Colonies
D6ori	TRI + CAM	10⁰	overgrown
D7ori	TRI + CAM	10^-1	overgrown
D8ori	TRI + CAM	10^-2	4950
D9ori	TRI + CAM	10^-3	1066
D10ori	TRI + CAM	10^-4	114
Ts6ori	AMP + CAM	10⁰	1105
Ts7ori	AMP + CAM	10^-1	12
Ts8ori	AMP + CAM	10^-2	0
Ts9ori	AMP + CAM	10^-3	0
Ts10ori	AMP + CAM	10^-4	0
TL6ori	TRI + AMP	10⁰	overgrown
TL7ori	TRI + AMP	10^-1	2251
TL8ori	TRI + AMP	10^-2	352
TL9ori	TRI + AMP	10^-3	39
TL10ori	TRI + AMP	10^-4	7
R3ori	AMP	10⁰	overgrown
R4ori	AMP	10^-1	3961

Set 3
Plate ID	Antibiotics	Dilution	# Colonies
D11ori	TRI + CAM	10⁰	overgrown
D12ori	TRI + CAM	10^-1	overgrown
D13ori	TRI + CAM	10^-2	4180
D14ori	TRI + CAM	10^-3	737
D15ori	TRI + CAM	10^-4	46
Ts11ori	AMP + CAM	10⁰	bad plate
Ts12ori	AMP + CAM	10^-1	3
Ts13ori	AMP + CAM	10^-2	0
Ts14ori	AMP + CAM	10^-3	0
Ts15ori	AMP + CAM	10^-4	0
TL11ori	TRI + AMP	10⁰	overgrown
TL12ori	TRI + AMP	10^-1	1436
TL13ori	TRI + AMP	10^-2	172
TL14ori	TRI + AMP	10^-3	18
TL15ori	TRI + AMP	10^-4	3
R5ori	AMP	10⁰	overgrown
R6ori	AMP	10^-1	3679

Results
Set #	Conjugation Efficiency for Plasmid 1	Conjugation Efficiency for wild R751
1	0.00177	0.0141
2	0.00224	0.0476
3	n/a	0.0356

This shows that Conjugation Plasmid 1 is successfully transmitted but with a lower efficiency in the presence of R751.

Attempted 2nd knockout

Made 4 0.5xKAN plates, 2 0.1xKAN plates, 2 1xTRI plates and 2 5mL tubes with 0.5xKAN.

Started centrifuging when R751 was at OD 0.507.

Used 7 μL oriTR_PCR_KO vector for oriTR electroporation and 12 μL trbK_KO_PCR vector for trbK electroporation. Both time constants 3.7. In incubator at 4:13 pm.

Modifications made to protocol:

Arabinose added the night before
used 4 mL from the 5 mL culture, higher density of cells in elctroporation
used 10% glycerol in the last spin down step

Retrieved from "http://2009.igem.org/Team:TUDelft/19_August_2009"

@@ Line 292: / Line 292: @@
 | <b>Results</b>
 |- align="center"
-| Set # || Conjugation Efficinecy for Plasmid 1 || Conjugation Efficinecy for wild R751
+| Set # || Conjugation Efficiency for Plasmid 1 || Conjugation Efficiency for wild R751
 |- align="center"
 | 1 || 0.00177 || 0.0141