Team:TUDelft/30 July 2009

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Revision as of 21:50, 30 July 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

30 July 2009

Tim Weenink

prepared assembly mixes for !B, !C and !D constructs. Standard Ginko assembly kit was used. DNA concentrations as below (these mixtures were added to 7.5 µl of digestion mixture):

Assembly name	position	Components	volume in µl
!B	Upstream	!A DNA	33.0
		H20	9.5
	Downstream	BBa_B0015 DNA	10.0
		H20	32.5
	Backbone	pSB1AC3 DNA	6.5
		H20	36
!C	Upstream	BBa_R0040 DNA	10.0
		H20	32.5
	Downstream	*I6 DNA	5.5
		H20	37.0
	Backbone	pSB1AC3 DNA	6.5
		H20	36
!D	Upstream	*I6 DNA	5.5
		H20	37.0
	Downstream	BBa_K145201 DNA	18.0
		H20	24.5
	Backbone	pSB1AC3 DNA	6.5
		H20	36

Ligated and transformed assemblies according to protocol.

15:20 Done plating the assemblies.

15:40 inoculated *S and *T cultures, four colonies each

16:55 Inoculated !A cultures from glycerole stock. Two tubes.

Calin

Plated three backbones left over from the transformation the other day. Did a digest on oriT-R with E and P. Made 3 x 5ml culture tubes for the pSB4C5 backbone which had a few colonies. Made electrocompetent cells with the [http://openwetware.org/wiki/Knight:Preparing_electrocompetent_cells Knight:Preparing electrocompetent cells] protocol. Flash froze tube in liquid nitrogen. Checked backbone concentrations:

Part	Concentration (ng/uL)
rbs-GFP-term I	102.6
rbs-GFP-term II	113.5
pSB1A3 I	89.1
pSB1A3 II	83.2
pSB1A3 III	91.9
pSB1A3 IV	84.7
pSB4A5 I	77.7
pSB4A5 II	83.9
pSB4A5 III	99.0
pSB4A5 IV	116.1
pSB1C3 I	102.3
pSB1C3 II	49.4
pSB1C3 III	81.5
pSB1C3 IV	66.0

Ran gel on backbones and oriT digest. Gel left for too long.

Well	Part	Plasmid Size
1	rbs-GFP-term I	2957
2	rbs-GFP-term II	2957
3	pSB1A3 I	2832
4	pSB1A3 II	2832
5	pSB1A3 III	2832
6	pSB1A3 IV	2832
7	pSB4A5 I	4070
8	pSB4A5 II	4070
9	pSB4A5 III	4070
10	pSB4A5 IV	4070
11	[http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder]
12	pSB1C3 I	2747
13	pSB1C3 II	2747
14	pSB1C3 III	2747
15	pSB1C3 IV	2747
16	oriT E + P digest	2079
17	oriT E + P digest	2079
18	[http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder]

Tim Vos

Minipreped 4 x pSB1C3, 4 x pSB4A5, 2 x rbs-GFP, and 4 x pSB1A3. One pSB4A5 tube is incorrect, it shows RFP expression. Also loaded the gel.

Orr

Made some chemically competent cells using the TSS buffer protocol. Started making a Java program that will allow lock sequence design based on the chosen RBS, and will design the equivalent key based on the lock sequence. The program will incorporate a database with all the working RBS segments in the iGEM registry, so that the user can choose which RBS he wants to use.

Retrieved from "http://2009.igem.org/Team:TUDelft/30_July_2009"

@@ Line 105: / Line 105: @@
 | Well || Part || Plasmid Size
 |- align="center"
-| 1 || rbs-GFP-term I ||
+| 1 || rbs-GFP-term I || 2957
 |- align="center"
-| 2 || rbs-GFP-term II ||
+| 2 || rbs-GFP-term II || 2957
 |- align="center"
 | 3 || pSB1A3 I || 2832
@@ Line 135: / Line 135: @@
 | 15 || pSB1C3 IV || 2747
 |- align="center"
-| 16 || oriT E + P digest ||
+| 16 || oriT E + P digest || 2079
 |- align="center"
-| 17 || oriT E + P digest ||
+| 17 || oriT E + P digest || 2079
 |- align="center"
 | 18 || [http://www.eurogentec.com/EGT/Images/RESALES/Electrophoresis/Regular%20DNA%20Ladder/7-SmartLadder.jpg DNA Ladder] ||