Team:BYU Provo/Notebook/SmallPhage/Fallexp/Period1/Dailylog
From 2013.igem.org
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<font size="4"> '''9/4/13''' </font> | <font size="4"> '''9/4/13''' </font> | ||
- | JL, | + | JL, LP |
* Discussed results from recent spot test for [[Team:BYU Provo/Notebook/SmallPhage/Summerexp/8.26 Mutagen Concentration Test|8.26 Mutagen Concentration Test - Eighth Protocol]]. Phage too spread out to effectively select for mutant phage. Decided to stop until the Phage Purification Team can get the wildtype T7 phage to band. | * Discussed results from recent spot test for [[Team:BYU Provo/Notebook/SmallPhage/Summerexp/8.26 Mutagen Concentration Test|8.26 Mutagen Concentration Test - Eighth Protocol]]. Phage too spread out to effectively select for mutant phage. Decided to stop until the Phage Purification Team can get the wildtype T7 phage to band. | ||
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<font size="4"> '''9/5/13''' </font> | <font size="4"> '''9/5/13''' </font> | ||
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* Started approximately 10mL of E coli B liquid culture overnight. | * Started approximately 10mL of E coli B liquid culture overnight. | ||
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<font size="4"> '''9/6/13''' </font> | <font size="4"> '''9/6/13''' </font> | ||
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* Purified phage propagation sample from 9.4 via centrifugation (5 minutes at 3000 rpm) and cholorform. Spot tests were then performed to estimate phage titer. | * Purified phage propagation sample from 9.4 via centrifugation (5 minutes at 3000 rpm) and cholorform. Spot tests were then performed to estimate phage titer. | ||
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- | <font size="4"> ''' | + | <font size="4"> '''9/8/13''' </font> |
- | + | JL | |
- | + | * Continued data analysis / picture processing for [[Team:BYU Provo/Notebook/SmallPhage/Summerexp/8.16 Modeling phage plaque size|8.16 Modeling phage plaque size - Experiment One]]. | |
- | - Started approximately | + | * Performed preliminary titer in preparation for repeating the modeling experiment with T1 and T2. For specifics, please see [[Team:BYU Provo/Notebook/SmallPhage/Summerexp/8.16 Modeling phage plaque size|8.16 Modeling phage plaque size - Experiment One]]. |
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+ | * Started approximately 25mL of E coli B liquid culture overnight | ||
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- | <font size="4"> ''' | + | <font size="4"> '''9/9/13''' </font> |
- | + | JL, LP | |
- | - Started | + | * Discussed analysis of modeling result using ImageJ. |
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+ | * Repeated the modeling procedure in [[Team:BYU Provo/Notebook/SmallPhage/Summerexp/8.16 Modeling phage plaque size|8.16 Modeling phage plaque size - Experiment One]] for T1 and T2. Incubation started at 4:30pm. | ||
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+ | * Started a fresh round for phage propagation for the Phage Purification Team. Specifically, to a 15mL centrifuge tube we added 8mL of LB, 2mL of E coli B liquid culture overnight, and 20uL of 8.24 T7 phage stock. | ||
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+ | * Divided up assignments for updating the wiki. | ||
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- | <font size="4"> ''' | + | <font size="4"> '''9/10/13''' </font> |
- | + | JL, LP | |
- | + | * Took the T1 and T2 modeling plates our the incubation at 4:30pm. | |
- | + | * Started approximately 25mL of E coli B liquid culture overnight. | |
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+ | * Measured plaque sizes using ImageJ. | ||
<br> | <br> | ||
- | <font size="4"> ''' | + | <font size="4"> '''9/11/13''' </font> |
- | + | JL, LP | |
+ | * Isolated the phage (from 9.9) by centrifuging down the bacteria, transferring the supernatant to a new 15mL centrifuge tube, and adding 900ul of chloroform to the supernatant. | ||
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+ | * Took pictures of T1 and T2 plates for [[Team:BYU Provo/Notebook/SmallPhage/Summerexp/8.16 Modeling phage plaque size|8.16 Modeling phage plaque size - Experiment One]]. | ||
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- | <font size="4"> ''' | + | <font size="4"> '''9/12/13''' </font> |
- | + | JL | |
- | - | + | * Spot test showed plaques up to -7. This indicate that the phage suspension solution we gave the Phage Purification Team for CsCl was at least 10E9 pfu/mL. |
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+ | * Started approximately 30mL of E coli B liquid culture overnight. | ||
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- | <font size="4"> '''8/ | + | <font size="4"> '''9/13/13''' </font> |
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+ | JL, LP | ||
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+ | * The Phage Purification Team has good news for us. They were able to observe banding in their latest CsCl gradient for T7. We thus decided to perform a new round of mutagenesis this weekend and hopefully selection next week. | ||
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+ | * In preparation for mutagenesis tomorrow, we performed titers for 8.24 T7 stock. | ||
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+ | * Started approximately 5mL of E coli B liquid culture overnight. | ||
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+ | * Streaked out E coli B. | ||
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+ | <font size="4"> '''9/14/13''' </font> | ||
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+ | JL | ||
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+ | * Autoclaved ddH<sub>2</sub>O, LB, x2 top agar. | ||
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+ | * Used the autoclaved ddH<sub>2</sub>O to make adenine and uracil solution. Specifically, | ||
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+ | : - 254mg of uracil was dissolved in 10mL of ddH<sub>2</sub>O to produce a uracil solution with a concentration of approximately 2.5mg/mL | ||
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+ | : - 753mg of adenine hemisulfate dihydrate was dissolved in 10mL of ddH<sub>2</sub>O to produce a adenine solution with a concentration of approximately 5mg/mL | ||
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+ | * Started approximately 5mL of E coli B liquid culture overnight. | ||
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+ | <font size="4"> '''9/15/13''' </font> | ||
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+ | JL, LP | ||
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+ | * Performed the mutagenesis procedure in [[Team:BYU_Provo/Notebook/SmallPhage/Summerexp/9.13_Mutagen_Concentration_Test|9.13 Mutagen Concentration Test - Ninth Protocol]] | ||
- | + | * Started approximately 20mL of E coli B liquid culture overnight | |
- | + | * Started phage propagation | |
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Latest revision as of 21:37, 9 October 2013
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9/1/13
9/2/13
9/3/13
9/4/13 JL, LP
9/5/13 LP
9/6/13 JL, LP
9/7/13 JL
9/8/13 JL
9/9/13 JL, LP
9/10/13 JL, LP
9/11/13 JL, LP
9/12/13 JL
9/13/13 JL, LP
9/14/13 JL
9/15/13 JL, LP
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