Team:BYU Provo/Notebook/SmallPhage/Springexp/Period3/Dailylog

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(Difference between revisions)

Latest revision as of 15:30, 9 September 2013

Small Phage May - June Notebook: May 27 - June 16 Daily Log

Small Phage

5/28/13

- Started three 8mL E coli BL21 liquid culture at around 4pm.

5/29/13

- Continued 5.20 Mutagen Concentration Experiment

- Prepared sample for sequencing. This is done as part of 5.20 T7 Minor Capsid Protein PCR

- Dr. Studier responded to our email today! We also received the E coli stains containing plasmids with clone T7 genes.

5/30/13

- Plates from yesterday are taken out of incubation at around 4:00pm

5/31/13

- Discussed results for 5.20 Mutagen Concentration Experiment -> will need to try this one more time with minor adjustment to experimental design: plate -4 dilution using x6 and x8 top agar.

- Discussed plans for next week.

- Made new LB and x6 top agar.

6/2/13

- Made about 20ml of BL21 overnight

6/3/13

- Made new LB plates

- Plated -4 titer on x6 and x8 plates for 5.20 Mutagen Concentration Experiment

6/5/13

- Discussed plans for the selection process of 5.20 Mutagen Concentration Experiment and calculated the needed volume of agar, overnight, and phage

- Made 500mL x8 agar

- Performed dilution series to generate enough 200ug -4 phage stock for selection.

6/6/13

- Started approximately 50mL of BL21 liquid culture overnight.

6/7/13

- Performed the selection process of 5.20 Mutagen Concentration Experiment. Specifically, we plated 45 plates of 200ug mutagen, -4 phage dilution using x8 agar. 5 plates of 0ug, -3 phage dilution were also done a control.

6/9/13

- Started 21mL of BL21 overnight.

6/10/13

- Made 1250mL of x8 top agar

- Attempted to amplify phage from larger plaques in 5.20 Mutagen Concentration Experiment

6/11/13

- Started approximately 70mL of BL21 liquid culture overnight

6/12/13

- Perfected protocol for applying mutagen to phage

- Started 6.12 Mutagen Concentration Test - Second Protocol

6/13/13

- Started approximately 30mL of BL21 liquid culture overnight.

6/14/13

- Titered the mutagenesis product from Wednesday as part of 6.12 Mutagen Concentration Test - Second Protocol

6/16/13

- Started approximately 100mL of BL21 liquid culture overnight.

@@ Line 4: / Line 4: @@
 {| width="100%"
-| colspan="3" | <font color="#333399" size="5" font face="Calibri"> '''Small Phage May - June Notebook: May 27 - June 9 Daily Log'''</font>
+| colspan="3" | <font color="#333399" size="5" font face="Calibri"> '''Small Phage May - June Notebook: May 27 - June 16 Daily Log'''</font>
 <br>
@@ Line 14: / Line 14: @@
 <font color="#333399" size="3" font face="Calibri">
-: [[Team:BYU_Provo/Small_Phage|Overview]]
+<font size = "4">
+: <u> '''Small Phage''' </u> </font>
 : [[Team:BYU Provo/Notebook/SmallPhage/Winterexp|March-April]]
@@ Line 42: / Line 44: @@
 - Prepared sample for sequencing. This is done as part of [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 T7 Minor Capsid Protein PCR|5.20 T7 Minor Capsid Protein PCR]]
-- Dr. Studier responded to our email today! We also received the E coli stains containing plasmids with clone T7 genes. WE CAN START SITE DIRECTED MUTAGENESIS SOON!
+- Dr. Studier responded to our email today! We also received the E coli stains containing plasmids with clone T7 genes.
 <br>
@@ Line 62: / Line 64: @@
 <br>
-<font size="4"> '''5/17/13''' </font>
+<font size="4"> '''6/2/13''' </font>
-- Determined that all LB plates from 5.8 had contamination
+- Made about 20ml of BL21 overnight
-- Poured new LB plates
+<br>
-- Made x8 top agar
+<font size="4"> '''6/3/13''' </font>
+- Made new LB plates
+- Plated -4 titer on x6 and x8 plates for [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]]
 <br>
-<font size="4"> '''5/18/13''' </font>
+<font size="4"> '''6/5/13''' </font>
+- Discussed plans for the selection process of [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]] and calculated the needed volume of agar, overnight, and phage
-- Stacked up the LB plates made yesterday. No obvious sign of contamination seen.
+- Made 500mL x8 agar
-- Threw away the 5.8 LB plates (the ones with contamination).
+- Performed dilution series to generate enough 200ug -4 phage stock for selection.
 <br>
-<font size="4"> '''5/19/13''' </font>
+<font size="4"> '''6/6/13''' </font>
-- Started two 5mL of E coli BL21 overnight
+- Started approximately 50mL of BL21 liquid culture overnight.
-- Designed procedure for applying mutagen and selecting for T7
 <br>
-<font size="4"> '''5/20/13''' </font>
+<font size="4"> '''6/7/13''' </font>
-- Performed T7 Mutagen Concentration Test
+- Performed the selection process of  [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]]. Specifically, we plated 45 plates of 200ug mutagen, -4 phage dilution using x8 agar. 5 plates of 0ug, -3 phage dilution were also done a control.
-: [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]]
+<br>
-- Performed T7 Minor Capsid Protein PCR
+<font size="4"> '''6/9/13''' </font>
-: [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 T7 Minor Capsid Protein PCR|5.20 T7 Minor Capsid Protein PCR]]
+- Started 21mL of BL21 overnight.
 <br>
-<font size="4"> '''5/21/13''' </font>
+<font size="4"> '''6/10/13''' </font>
-- Started two 5mL E coli BL21 overnight at around 7:00pm
+- Made 1250mL of x8 top agar
+- Attempted to amplify phage from larger plaques in [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]]
 <br>
-<font size="4"> '''5/22/13''' </font>
+<font size="4"> '''6/11/13''' </font>
+- Started approximately 70mL of BL21 liquid culture overnight
+<br>
-- Performed spot test for [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]]
+<font size="4"> '''6/12/13''' </font>
-- Ran agarose gel to confirm PCR product
+- Perfected protocol for applying mutagen to phage
-: [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 T7 Minor Capsid Protein PCR|5.20 T7 Minor Capsid Protein PCR]]
+- Started [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period3/Exp/6.12 Mutagen Concentration Test - Perfected Protocol|6.12 Mutagen Concentration Test - Second Protocol]]
 <br>
-<font size="4"> '''5/23/13''' </font>
+<font size="4"> '''6/13/13''' </font>
-- Started two 25mL E coli BL21 liquid culture over night at around 6:00pm
+- Started approximately 30mL of BL21 liquid culture overnight.
 <br>
-<font size="4"> '''5/24/13''' </font>
+<font size="4"> '''6/14/13''' </font>
-- Proceeded with [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/Exp/5.20 Mutagen Concentration Experiment|5.20 Mutagen Concentration Experiment]] by performing preliminary selection using x8 top agar
+- Titered the mutagenesis product from Wednesday as part of [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period3/Exp/6.12 Mutagen Concentration Test - Perfected Protocol|6.12 Mutagen Concentration Test - Second Protocol]]
 <br>
-<font size="4"> '''5/25/13''' </font>
+<font size="4"> '''6/16/13''' </font>
-- Took pictures in preparation for [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period2/PR|Progress Report]]
+- Started approximately 100mL of BL21 liquid culture overnight.
 <br>
 </font>