Team:University of Chicago/Notebook/Norayucel

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Revision as of 17:32, 29 July 2008

July 18, 2008

1. Diluted 1ng/microliter pGreen plasmid to 10pg/microliter with 100X dilution
2. 1microliter of plasmid to 50 microliters competent cells
3. Will grow up 50microliters of TOP10 untransformed as a control
4. Put on ice at 2:03
5. Took off ice at 2:34
6. Incubated for 1minute at 42C
7. Added 250microliters SOC media (prepared at 1:30)
8. Start incubated at 37C at 2:36
9. Take out at 3:40pm
10. Streaked 20microliters onto Amp. Plates

+pGreen
NO plasmid

11. Dan will come in Saturday morning to pick up the plates and count colonies.

July 21, 2008

No colonies grew on 10pg/microliter.
Try transformation again before trying to grow up new TOP10
- DNA could be bad
- Wrong antibiotic (double checked: ampicillin is correct)
- Something went wrong with transformation--perhaps too long at 42C?
Bad cells (nooooo....)

Retry

10pg/microliter
100pg/microliter
1ng/microliter
no plasmid on LB (test if cells are completely dead)

Also try Dr. Schonbaum's stocks to compare

10pg/microliter
1ng/microliter

transformed at 4pm and put in 37C incubator. Check tomorrow morning.

July 22, 2008

We have cells!!

10pg: 3 colonies.
100pg: 25 colonies
1ng: 200 colonies

Efficiency of cells is ~3x10^6. Need to redo.

NO plasmid on LB: big streaky mess. Cell mos' def' alive.
STOCKS, 10pg: 22
Stocks, 1ng: 300-400

Weird. Should be 100X more than 10pg. Perhaps bad dilution.
Efficiency going off 10pg is 3-4x10^7. Sadly Dr. Schonbaum's stocks aren't efficient enough. What to do....

July 25, 2008

Remade TOP10 competent cells--will try to make more competent
Inoculated 500mL of SOB at ~10am with 1mL each of TOP10 starter culture
- Two 2L flasks with 250mL each
At 5:30 OD was .28 and .29 for each flask respectively
Final OD after following competent cell protocol was 1.04 (between 1-1.5 as required)
Put into -80C at 7:30pm.

July 28, 2008

Transformation with pGreen

10pg/microliter on LB Amp
1 ng/microliter on LB Amp
NO plasmid on LB Amp
NO plasmid on plain LB
Put into 37C incubator ~1:30pm

Plates

Running out of plates
500mL of LB and LB Amp agar
- 100mg/mL stock of Ampicillan
- After cooling for ~45 minutes at room temp, added .5mL
Poured around 4:30 pm. Turned over at 5:30

Checked plates before I left at ~6pm. No growth (as expected). Will look again in the morning

July 29, 2008

Checked plates
10 pg/microliter plate had ~20 colonies. Competency still off by factor of 10 :(
1ng/microliter plate was a big streaky mess (too many to count)
NO plasmid on LB+Amp also big streaky mess. Possibly mislabeled plate??
NO plasmid +LB big streaky mess (as expected)

@@ Line 11: / Line 11: @@
 .	Take out at 3:40pm<br>
 .	Streaked 20microliters onto Amp. Plates<br>
+*+pGreen
+*NO plasmid
 .	Dan will come in Saturday morning to pick up the plates and count colonies.<br>
+==July 21, 2008==
+#No colonies grew on 10pg/microliter.
+#Try transformation again before trying to grow up new TOP10
+#*DNA could be bad
+#*Wrong antibiotic (double checked: ampicillin is correct)
+#*Something went wrong with transformation--perhaps too long at 42C?
+#Bad cells (nooooo....)<br>
+'''Retry'''
+*10pg/microliter
+*100pg/microliter
+*1ng/microliter
+*no plasmid on LB (test if cells are completely dead)
+'''Also try Dr. Schonbaum's stocks to compare'''
+*10pg/microliter
+*1ng/microliter<br>
+transformed at 4pm and put in 37C incubator. Check tomorrow morning.
+==July 22, 2008==
+'''We have cells!!'''
+#10pg: 3 colonies.
+#100pg: 25 colonies
+#1ng: 200 colonies
+*Efficiency of cells is ~3x10^6. Need to redo.
+#NO plasmid on LB: big streaky mess. Cell mos' def' alive.
+#STOCKS, 10pg: 22
+#Stocks, 1ng: 300-400
+*Weird. Should be 100X more than 10pg. Perhaps bad dilution.
+*Efficiency going off 10pg is 3-4x10^7. Sadly Dr. Schonbaum's stocks aren't efficient enough. What to do....
 ==July 25, 2008==