Team:UIUC Illinois/Notebook

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Revision as of 02:02, 17 October 2014

PROJECT NOTES
- NOTES BY MONTH

Monday 9^th June

Made LB broth using 10 grams of bacto agar + 12 grams HiVeg LB broth + 600 mL ddH2O

Autoclaved 1.5 mL Eppendorf tubes as well as LB

Poured plates of LB and chloramphenicol (CAM)

Streaked 2 plates with E. coli DguaB (pDCAF3)

Incubated in 37 degrees celsius

Aliquoted kanamycin (KAN) in four 1mL tubes

Tuesday 10^th June

ASDF

Autoclaved at 1:30pm

0.8 grams of YNB + 156 mL H2O
28 grams of salts + 490 mL H2O

Used sterile filter for 1M MgSO4 and 1M CaCl2

Suspended 5 uL of CM34 (antibiotic) + 5 mL of LB + 1 colony of pDCAF3 E. coli

Added .5 grams of caffeine + 400 uL of 1M MgSO4 + 20 uL 1M CaCl2 + 40 mL M95x salts + H2O to YNB + H2O mixture

Labeled this "M9 media"

Inoculated frozen stock of E. coli guaB pDCAF3 in 5 mL of M9 media

Placed sample in 30 degree celsius shaker for culturing

Wednesday 11^th June

ASDF

Inoculated CBB1 frozen stock in 5 mL of M9 media

Placed sample in 30 degree celsius shaker

Purified pDCAF plasmid using DNA mini kit

Plasmid concentration was 132.9 ng/uL

Friday 13^th June

ASDF

Added 10 uL deionized H2O into the J23114 promoter plasmid (Ampᴿ)

Followed bacterial transformation protocol to prepare/grow culture overnight

Inoculated 5 mL of M9 with CBB1 and placed it in 30 degree celsius shaker for 3 days

Previous CBB1 culture did not grow, showed slight growth
pDCAF3 strain in M9 did grow in the 30 degree celsius shaker

Monday 16^th June

ASDF

No growth in M9 by CBB1

To grow the promoter plasmid:

5 mL of LB + 1 uL Amp
Label tubes
Grow in 30 degree celsius shaker overnight

New CBB1 trials:

2 tubes of 1 mL M9 + 2 tubes of 1 mL LB each with 10 uL of sample

Purify genomic DNA plasmid following the Wizard Protocol

Added lysis buffer before centrifuging. So we separated (translate) sample into 2 tubes and will (translate) accordingly
We put our 2 promoter plasmid plates in the 4 degree celsius shelf

Tuesday 17^th June

ASDF

Quantified gDNA with TECAN

Result: 5.4 ng/uL

Made 2 plates of M9 culture and 2 plates of CBB1 culture (100 uL used) then placed them in 37 degree celsius shaker

Wednesday 18^th June

ASDF

Autoclaved 50% glycerol

Made four 25% glycerol stock solutions (stored in the -80 degree celsius freezer):

CBB1 in M9 (x2 1.5 mL tubes)
Promoter 1
Promoter 2 (both promoter plasmids are J23114 Ampᴿ)

Purified both promoter plasmids using the purification protocol

Stored in the -20 degree celsius freezer in the DNA box

@@ Line 340: / Line 340: @@
 				<li>Label tubes</li>
 				<li>Grow in 30 degree celsius shaker overnight</li>
-			</ul><br><br>
+			</ul>
 			New CBB1 trials:<br><br>
 				<ul style="text-indent:30px;"><li>2 tubes of 1 mL M9 + 2 tubes of 1 mL LB each with 10 uL of sample</li></ul><br><br>
@@ Line 377: / Line 377: @@
 				<li>Promoter 1 </li>
 				<li>Promoter 2 (both promoter plasmids are J23114 Ampᴿ)</li>
-			</ul><br><br>
+			</ul>
-			Purified both promoter plasmids using the purification protocol<br><br>
+			Purified both promoter plasmids using the purification protocol<br>
 				<ul style="text-indent:30px;"><li>Stored in the -20 degree celsius freezer in the DNA box</li></ul><br><br>
 </div>
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 {{:Team:UIUC_Illinois/Footer}}

Team:UIUC Illinois/Notebook

From 2014.igem.org

Revision as of 02:02, 17 October 2014

Monday 9th June

Tuesday 10th June

Wednesday 11th June

Friday 13th June

Monday 16th June

Tuesday 17th June

Wednesday 18th June

Monday 9^th June

Tuesday 10^th June

Wednesday 11^th June

Friday 13^th June

Monday 16^th June

Tuesday 17^th June

Wednesday 18^th June