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University of Aberdeen iGEM 2009

University of Aberdeen - Pico Plumber

iGEM 2009

Quorum Sensing Notebook

Week 1 - Research and Biobrick Rescues (08/06/09 - 12/06/09)

Day 1 Monday (08/06/09)

Researching the Registry for Biobricks
- Identified K081008, J23100, C0062, K091156, B0034,B0030, B0015, R0061 and R0062 for possible use in our project.
- Other biobricks identified for other sub-projects include R0011.

Day 2 Tuesday (09/06/09)

Researching the literature for information on Quorum Sensing.
Researching for information on LVA tags

Day 3 Wednesday (10/06/09)

Preparing for biobrick rescue and transformation
- Prepare LB and Agar
- Prepare Cacl2 solution,
- Prepare 1M MgCl2, 1MMgSO4 and 2M glucose solutions (for SOC medium)
- Inoculate e.coli and grow overnight

Day 4 Thursday (11/06/09)

Rescue Biobricks (K081008, J37033, B0015, J23100, R0011, R0062, K112808, C0051, C0040, I732100, R0051, K145001 and B0034)
Prepare competent e.coli, using calcium chloride method
Transform e.coli with biobricks listed above
- grow overnight on agar/amp plates.

Day 5 Friday (12/06/09)

Results from yesterday indicate that only I732100 was successfully transformed into e.coli
Identify possible recipient plasmids for QS module (psB4C5).
Propose a cloning strategy
Team meeting

Week 2 - Biobrick rescue and purification (15/06/09 - 19/06/09)

Day 1 Monday (15/06/09)

Inoculation of transformants - B0015, I732100, R0011 and K081008.

Day 2 Tuesday (16/06/09)

Inspection of inoculations, after overnight growth, revealed, as suspected, that only I732100 had grown

Perform plasmid prep on I732100
Digest I732100
- 1 Double digest E+ S
- 4 single digests - E, S, X and P
Prepare TSS buffer, for TSS method of competency (to be performed tomorrow)
Inoculate e.coli and grow overnight for tomorrow's TSS method.

Day 3 Wednesday (17/06/09)

Rescue additional biobricks - K112022, R0040, I732094, K093005, E0840
Prepare competent e.coli using TSS method.
Transform with biobricks rescued today + B0015, R0011, R0051, K112808 and K081008, grow overnight

Day 4 Thursday (18/06/09)

Prepare for miniprep
- inoculate transformed e.coli and grow overnight in liquid medium
Create master plates to keep record of colonies used

Day 5 Friday (19/06/09)

Perform miniprep to purify R0011, R0051, B0015, K112808, K081008
Team meeting

Week 3 - Digestions (22/06/09 - 26/06/09)

Day 1 Monday (22/06/09)

Day 2 Tuesday (23/06/09)

Transformation of ccdB resistant e.coli with plasmids psB3C5, psB3K5, psB3T5, psB4C5, psB4T5 and psB4K5.
Digestion of purified biobricks - (R0011, C0051, I732094, B0015, E0840, R0040, K112022, K112808, K093005, R0051, K081008, J37033, R0062 and I732100)
Perform gel electrophoresis of today's digests
- unsuccessful - C0051+ R0062 + B0015 + R0040 + E0840 (double digest problem), J37033(empty lane), I732100 (unusual bands),
- Successful - C0040, K145001

Day 3 Wednesday (24/06/09)

Digestion of lysis cassettes- K112022 + K112808
- Using BamHI and BglI
Repeat digestion of I732100
- Double digests - E + S and X + P
- Single digests - E, S, X and P
Run gels for above digestions
- Results indicate digestion needs to be repeated
Inoculate trasnformed e.coli and grow overnight

Day 4 Thursday (25/06/09)

Plasmid prep to purify biobricks - B0030, I0462, J23105, J23107, J23115, S03518, psB4K5 and psB3T5.
Digestion of above plasmid preps, plus additional C0051, psB1AC3 + psB1AT3
Perform gel electrophoresis of above digestions
- successful digestions - psB3T5 and psB1AT3
- unsuccessful digestions - psB1AC3, psB4K5, B0030 and C0051.
- Results also indicated that double digests using X + P were unsuccessful and should be repeated- S03518 and I0462

Note: Difficult to see difference between single and double digests for J series promoters (J23105, J23107 + J23115). This should be expected since all ~30bp in length.

Day 5 Friday (26/06/09)

Digestion of K081008
- double digest using E + S
- Single digests using E
Perform gel electrophoresis for K081008 digest
- Results indicate incomplete digestion.
Team meeting

Week 4 - Solving digestion problem (29/06/09 - 03/07/09)

Day 1 Monday (29/06/09)

Digestion of lambda DNA
- using HindIII
Repeat digestion of E0840 -
- using alternative digestion protocol (see wet lab)
Run gels for above digests
- gel indicates that alternative digestion method eliminates double digest problems seen previously
Inoculate I0462, psB4C5 and psB3K3 from master plates

Day 2 Tuesday (30/06/09)

Perform plasmid prep to purify psB3K3, psB4C5 + I0462.
Digestion of above plasmid preps
- using alternative method
Run gels using above digests
- Gels indicate that I0462 and psB4C5 were successfully digested, psB3K3 yielded empty lanes

Day 3 Wednesday (01/07/09)

Perform transformation using psB3C5
Inoculate K081008, psB1AT3 and psB1AC3
- No overnight growth was detected for K081008 - repeat transformation

Day 4 Thursday (02/07/09)

Research primer ordering
Transformation of K081008

Day 5 Friday (03/07/09)

Perform plasmid prep to purify K081008, psB1AT3 and psB1AC3

Digestion of above plasmid preps
- using E + P double digests for plasmids and E + S for K081008.
Team meeting

Week 5 (06/07/09 - 10/07/09)

Day 1 Monday (06/07/09)

Digestion of psB4C5
- in a total volume of 40µl (more concentrated than previous digestion)
Run gels from today's and Friday's digests (psB4C5, K081008, psB1AT3 + psB1AC3)
- successful digestions - K081008, I0462
- incomplete digestions - psB1AT3, psB1AC3

Concentration of psB4C5 was too low to proceed with cloning

Solution: Perform multiple plasmid preps and combine, check conc. using uv spectrophotometer.

Day 2 Tuesday (07/07/09)

Multiple plasmid preps of psB4C5.
Digestion of psB4C5
- Using E + P for double digest
Purification of I0462 digest (to concentrate)
Run gels for psB4C5 and I0462
- gel indicates conc. of psB4C5 = 7ng/µl
- gel indicates conc of I0462 = 15ng/µl

Day 3 Wednesday (08/07/09)

Alkaline phosphatase treat psB4C5
Calculations for ligation
Perform ligation
Transform ligation mixes
- grow overnight on agar plates containing chloramphenicol (50%).

Day 4 Thursday (09/07/09)

Result: Cloning from yesterday yielded unusual results

many more colonies on controls (vector only and vector + ligase) than on Vector + ligase + inserts.

Conclude: Repeat transformation repeated using 100% chloramphenicol plates and repeat digestion of psB4C5, ensuring complete digestion

Day 5 Friday (10/07/09)

Perform colony screening
- patch out colonies to identify red colonies (indicate intact vector)
Repeat digestion of psB4C5
Run above digestion on gel
- digest appears incomplete (linearised plasmid is still evident in double digest lane)
Team meeting

Week 6 (13/07/09 - 16/07/09)

Day 1 Monday (13/07/09)

Repeat digestion of psB4C5
- using alternative PstI
Run gel
- Results indicate incomplete digestion
Perform colony screening PCR
Run PCR gel.
- primer dimers are evident in most lanes, indicating PCR amplification was unsuccessful.
Repeat digestion of psB4C5
- incubate overnight

Day 2 Tuesday (14/07/09)

Alkaline phophatase psB4C5
Repeat ligations (psB4C5 + I0462 + K081008)
Transformation of ligations

Day 3 Wednesday (15/07/09)

PCR colony screening
Run PCR products on gel
- None of the PCR products show presence of expected insert length (~1.6kb)
- Primr dimers are evident in most lanes

Conclude: Create fresh screening plates and perform new PCR

Day 4 Thursday (16/07/09)

Perform PCR using fresh screening plates
Run gel of above PCR
- Non of our PCR products yielded expected insert length.

Day 5 Friday (17/07/09)

Team meeting

Week 7 (20/07/09 - 24/07/09)

===Day 1 Monday (20/07/09)

Perform diagnostic ligation
- using alternative plasmid (psB1AC3) and inserts (I732820 + S03518) known to work.
Transformation of above ligations

Results: Transformants indicate problem with K081008 (insert 1)

- Many colonies when I0462 (insert 2) cloned with I732820 (insert 1)
- few colonies when K081008 (insert1 )cloned with S03518 (insert 2)

Day 2 Tuesday (21/07/09)

Repeat transformation of K081008
Prepare colony screening plates for diagnostic ligations

Day 3 Wednesday (22/07/09)

Perform colony screening PCR
Run above PCR products on gel
- results indicate problem with PCR - no amplification, even in positive control lane

Day 4 Thursday (23/07/09)

Plasmid prep to purify K081008
Digestion of K081008
- using Roche enzymes
Run above digest on gel
- gel indicates complete digestion and good concentration

Day 5 Friday (24/07/09)

Team meeting

Week 8 27/07/09 - 31/07/09

Week 9 03/08/09 - 07/08/09

Week 10 10/08/09 - 14/08/09

Week 11 17/08/09 - 21/08/09

Back to Notebook, LacI-Latch Section

Continue to Notebook, Modeling Section

Back to Top of Page

@@ Line 266: / Line 266: @@
 <br><br>
-==Week 7 20/07/09 - 24/07/09==
+==Week 7 (20/07/09 - 24/07/09)==
+<br><br>
+===Day 1 Monday (20/07/09)
+* Perform diagnostic ligation
+**using alternative plasmid (psB1AC3) and inserts (I732820 + S03518) known to work.
+*Transformation of above ligations
+'''Results:''' Transformants indicate problem with K081008 (insert 1)
+** Many colonies when I0462 (insert 2) cloned with I732820 (insert 1)
+**few colonies when K081008 (insert1 )cloned with S03518 (insert 2)
+<br><br>
+===Day 2 Tuesday (21/07/09)===
+*Repeat transformation of K081008
+*Prepare colony screening plates for diagnostic ligations
+<br><br>
+===Day 3 Wednesday (22/07/09)===
+*Perform colony screening PCR
+*Run above PCR products on gel
+**results indicate problem with PCR - no amplification, even in positive control lane
+<br><br>
+===Day 4 Thursday (23/07/09)===
+*Plasmid prep to purify K081008
+*Digestion of K081008
+**using Roche enzymes
+*Run above digest on gel
+**gel indicates complete digestion and good concentration
+<br><br>
+===Day 5 Friday (24/07/09)===
+*Team meeting
+<br><br>
 ==Week 8 27/07/09 - 31/07/09==

Team:Aberdeen Scotland/notebook/quorumsensing