Team:BYU Provo/Notebook/SmallPhage/Winterexp/Period1/Dailylog
From 2013.igem.org
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- | | colspan="3" | <font color="#333399" size="5" font face="Calibri"> '''Small Phage March - April Notebook: March 15 - March 31 Daily Log'''</font> | + | | colspan="3" | <font color="#333399" size="5" font face="Calibri"> |
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+ | : '''Small Phage March - April Notebook: March 15 - March 31 Daily Log'''</font> | ||
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<font color="#333399" size="3" font face="Calibri"> | <font color="#333399" size="3" font face="Calibri"> | ||
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+ | : <u> '''Small Phage''' </u> </font> | ||
: [[Team:BYU Provo/Notebook/SmallPhage/Winterexp|March-April]] | : [[Team:BYU Provo/Notebook/SmallPhage/Winterexp|March-April]] | ||
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<font size="4"> '''3/15/13''' </font> | <font size="4"> '''3/15/13''' </font> | ||
- | - Today | + | -Today we began research on phage purification |
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+ | -Focused on T4 and T7 as this is what the other groups will be focusing on | ||
+ | :-T7 can self assemble with the help of scaffolding proteins without forming procapsids | ||
+ | :-T4 assembles using procapsids | ||
+ | -Some phage can have their DNA polymerase genes knocked out to make a hollow phage | ||
+ | :-Possibility for making ghost capsids | ||
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<font size="4"> '''3/16/13''' </font> | <font size="4"> '''3/16/13''' </font> | ||
- | - | + | - Created a priority list of things we need to complete: |
- | + | :-Find out how drugs are put into capsids | |
- | : | + | :-Possibly contact F. W. Studier for his amber T7 phage strain |
+ | ::-This strain had the knocked out DNA polymerase gene | ||
+ | :-Perform a phage titer on the phage we have to see if we have enough to work with | ||
+ | :-Find a procedure that we can use to test if our purified phage are viable by filling the capsid with liquid | ||
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<font size="4"> '''3/25/13''' </font> | <font size="4"> '''3/25/13''' </font> | ||
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- Reported on past week and plans for this week | - Reported on past week and plans for this week | ||
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: T7 major vs minor | : T7 major vs minor | ||
:: Minor is longer, but not necessary – the tail overhang is due to ribosome moving two codons downstream instead of three | :: Minor is longer, but not necessary – the tail overhang is due to ribosome moving two codons downstream instead of three | ||
- | : Suggest we can direct mutation to the poly-U site and prevent ribosome slippage | + | :: Suggest we can direct mutation to the poly-U site and prevent ribosome slippage |
: Qbeta major vs minor | : Qbeta major vs minor | ||
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- Outlined protocol for producing stock top agar | - Outlined protocol for producing stock top agar | ||
- | : [[Team:BYU_Provo/Notebook/SmallPhage/Winterexp/ | + | : [[Team:BYU_Provo/Notebook/SmallPhage/Winterexp/Period3/Exp/4.3 Top Agar Stock Preparation|4.3 Top Agar Stock Preparation]] |
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Latest revision as of 13:23, 9 September 2013
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3/15/13 -Today we began research on phage purification -Focused on T4 and T7 as this is what the other groups will be focusing on
-Some phage can have their DNA polymerase genes knocked out to make a hollow phage
3/16/13 - Created a priority list of things we need to complete:
3/18/13 - Presented current understanding and plans for the future
- More background research
3/20/13 - Background research on phiX174: the only phage we have in stock - Performed 3.20 Phage Viability Test
3/21/13 - Checked up on results for 3.20 Phage Viability Test
3/22/13 - Discussed results from tittering experiment (preliminary experiment 1)
- Discussed step of attack with Dr. Grose
- Sequencing will be for individual genes to cut down cost
- Learnt about Mega5 to compare genome and protein sequence
3/25/13 - Reported on past week and plans for this week
- Start working on designing our site directed mutagenesis
- Research into in-vitro assembly vs direct mutation of phage genome
3/27/13 - More research on genome of enterobacteria phage
- Outlined protocol for producing stock top agar
3/29/13 - Worked on our first team presentation.
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