Team:University College London/LabBook/Week14

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(Difference between revisions)

Revision as of 00:31, 27 September 2012

Monday 10.09.12

Aim: Day 2 of Generating competent cells. The aim is to incubate cells in the presence of CaCl2 to prepare the cell wall, such that it becomes permeable to DNA

Method: https://2012.igem.org/Team:University_College_London/Protocols/Competency2

Tuesday 11.09.12

Aim: Day 3 of Generating competent cells

Method: https://2012.igem.org/Team:University_College_London/Protocols/Competency3

14-2

14-3

14-4

Friday 14.09.13

Aim: To characterise nuclease activity BL21 cells

Method: To add protocol

Results:

The following table shows readings of the diameters and OD at different time points:

Date	Time	Colony diameter/mm	Halo diameter/mm	Absorbance at 600 OD
Friday	12.30	0	0	0
Friday	16.30	0	0	0
Friday	19.30	0	0	0
Friday	22.30	0	0	0
Saturday	01.30	0.5	1.5	0.068
Saturday	04.30	1	2	0.098
Saturday	07.30	1.5	3	0.159
Saturday	10.30	1.5	3.5	0.192
Saturday	12.30pm	2	4	0.203
Saturday	14.30	2	4	0.209
Saturday	16.30	2.5	5	0.215

The average depth of the colonies was noted to be 0.5 - 1mm

Conclusion:

It can be seen that nuclease works as expected in BL21 cells. However, nuclease activity is less efficient when compared to nuclease activity in WnU cells. This is in line with expectations, since nuclease is found naturally in WnU cells but not in BL21 cells.

@@ Line 38: / Line 38: @@
-'''Aim:''' To characterise nuclease activity
+'''Aim:''' To characterise nuclease activity BL21 cells
@@ Line 82: / Line 82: @@
-'''Conclusion:''' works bust in comparision to one found naturally in wnu it produces less nucles, as expected.
+'''Conclusion:'''
+It can be seen that nuclease works as expected in BL21 cells. However, nuclease activity is less efficient when compared to nuclease activity in WnU cells. This is in line with expectations, since nuclease is found naturally in WnU cells but not in BL21 cells.