Team:University of Chicago/Notebook/Norayucel

From 2008.igem.org

(Difference between revisions)
(Welcome to Nora's Notebook!)
(July 18, 2008)
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==July 18, 2008==
==July 18, 2008==
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1. Diluted 1ng/microliter pGreen plasmid to 10pg/microliter with 100X dilution
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1. Diluted 1ng/microliter pGreen plasmid to 10pg/microliter with 100X dilution<br>
-
2. 1microliter of plasmid to 50 microliters competent cells
+
2. 1microliter of plasmid to 50 microliters competent cells<br>
-
3. Will grow up 50microliters of TOP10 untransformed as a control
+
3. Will grow up 50microliters of TOP10 untransformed as a control<br>
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4. Put on ice at 2:03
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4. Put on ice at 2:03<br>
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5. Took off ice at 2:34
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5. Took off ice at 2:34<br>
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6. Incubated for 1minute at 42C
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6. Incubated for 1minute at 42C<br>
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7. Added 250microliters SOC media (prepared at 1:30)
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7. Added 250microliters SOC media (prepared at 1:30)<br>
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8. Start incubated at 37C at 2:36
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8. Start incubated at 37C at 2:36<br>
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9. Take out at 3:40pm
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9. Take out at 3:40pm<br>
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10. Streaked 20microliters onto Amp. Plates
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10. Streaked 20microliters onto Amp. Plates<br>
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11. Dan will come in Saturday morning to pick up the plates and count colonies.
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11. Dan will come in Saturday morning to pick up the plates and count colonies.<br>

Revision as of 21:24, 18 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
11. Dan will come in Saturday morning to pick up the plates and count colonies.