Minnesota/17 July 2008

From 2008.igem.org

(Difference between revisions)
 
(One intermediate revision not shown)
Line 20: Line 20:
|6. '''Double digest of all ligations:''' from previous days. Do a double digest to cut the components linearly, which will then be able to run through a gel to check if correct DNA  
|6. '''Double digest of all ligations:''' from previous days. Do a double digest to cut the components linearly, which will then be able to run through a gel to check if correct DNA  
is present. Follow the table below:  
is present. Follow the table below:  
-
 
{|border="1" align="left"
{|border="1" align="left"
Line 50: Line 49:
|L4j, LAMBDAcI:Term ||5.0uL ||0.5uL ||32.5uL ||10.0uL || EcoRI || Xba1
|L4j, LAMBDAcI:Term ||5.0uL ||0.5uL ||32.5uL ||10.0uL || EcoRI || Xba1
|-
|-
-
|L5c, GFP:Term ||5.0uL ||0.5uL ||40.5uL ||2.0uL || EcorI || Xba1
+
|L5c, GFP:Term ||5.0uL ||0.5uL ||40.5uL ||2.0uL || EcoRI || Xba1
|-
|-
|L6a, Pro:LAMBDAcI:Term ||5.0uL ||0.5uL ||39.5uL ||3.0uL || EcoRI || Xba1
|L6a, Pro:LAMBDAcI:Term ||5.0uL ||0.5uL ||39.5uL ||3.0uL || EcoRI || Xba1

Latest revision as of 20:55, 5 August 2008

Back to Notebook Home
Go to Previous Day (July 16)Go to Next Day (July 18)
1. Plasmid prep dual promoters: (1) Tet & P22mnt, (2) LacI & LAMBDAcI.
2. Model: Figure out why have such a low GFP output when run model.
3. Sequence L5, L6-L9
4. Re-transform RFP, TetR promoter, terminator, and MCherry because no cell growth on plates. Place in 2mL LB cultures, allow growth in incubator @37C for 2 hours. Plate samples on Ampicillin resistant plates. Allow growth O/N.
5. Discuss problems with sequences
6. Double digest of all ligations: from previous days. Do a double digest to cut the components linearly, which will then be able to run through a gel to check if correct DNA

is present. Follow the table below:

Parts 10x Buffer BSA H20 DNA RE 1 RE 2
L2a, LAMBDAcI:Term 5.0uL 0.5uL 32.5uL 10.0uL EcoRI Xba1
L2b, LAMBDAcI:Term 5.0uL 0.5uL 32.5uL 10.0uL EcoRI Xba1
L3i, Pro:LAMBDAcI 5.0uL 0.5uL 32.5uL 10.0uL Pst1 Spe1
L3j, Pro:LAMBDAcI 5.0uL 0.5uL 32.5uL 10.0uL Pst1 Spe1
L4b, LAMBDAcI:Term 5.0uL 0.5uL 40.5uL 2.0uL EcoRI Xba1
L4c, LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L4d, LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L4e, LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L4g, LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L4h, LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L4i, LAMBDAcI:Term 5.0uL 0.5uL 37.5uL 5.0uL EcoRI Xba1
L4j, LAMBDAcI:Term 5.0uL 0.5uL 32.5uL 10.0uL EcoRI Xba1
L5c, GFP:Term 5.0uL 0.5uL 40.5uL 2.0uL EcoRI Xba1
L6a, Pro:LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L6b, Pro:LAMBDAcI:Term 5.0uL 0.5uL 41.5uL 1.0uL EcoRI Xba1
L6e, Pro:LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L6d, Pro:LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L7a, Pro:LAMBDAcI:Term 5.0uL 0.5uL 38.5uL 4.0uL EcoRI Xba1
L7b, Pro:LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L7d, Pro:LAMBDAcI:Term 5.0uL 0.5uL 37.5uL 5.0uL EcoRI Xba1
L8a, Pro:LAMBDAcI:Term 5.0uL 0.5uL 39.5uL 3.0uL EcoRI Xba1
L9a, Pro:LAMBDAcI:Term 5.0uL 0.5uL 41.5uL 1.0uL EcoRI Xba1
L9c, Pro:LAMBDAcI:Term 5.0uL 0.5uL 40.5uL 2.0uL EcoRI Xba1
L9d, Pro:LAMBDAcI:Term 5.0uL 0.5uL 41.5uL 1.0uL EcoRI Xba1


7. Gel Electrophoresis: Performed on double digest reaction from above. Refer to picture below for results.
Gel from 07-17-2008
Left to Right: Ladder, --, L9E, L9C, L9A, L8A, L7D, L7B, L7A, L6E, L6D, L6B, L6A, L5C, --, Ladder, L4j, L4i, L4h, L4g, L4d, L4e, L4c, L4b, L3j, L3i, L2b, L2a, --, Ladder