Team:BYU Provo/Notebook/SmallPhage/Winterexp/Period1/Dailylog

From 2013.igem.org

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(Created page with "{{TeamBYUProvo}} <br> {| width="100%" | colspan="3" | <font color="#333399" size="5" font face="Calibri"> '''Small Phage March - April Notebook: March 15 - March 31 Daily Log''...")
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- Did more background research and brainstormed ideas for a plan of attack
- Did more background research and brainstormed ideas for a plan of attack
: Decided to focus on T7 first, since it’s easily acquired and more info is available
: Decided to focus on T7 first, since it’s easily acquired and more info is available
-
 
<br>
<br>
-
<font size="4"> '''5/2/13''' </font>
+
<font size="4"> '''3/16/13''' </font>
-
- Designed primers for amplifying and sequencing phage capsid protein
+
- Did more background reading for T7; literature search for possible plan of attack
-
- Wrote emails inquiring mutagen (NG) and plasmid for in vitro assembly
+
: [[Team:BYU_Provo/Notebook/SmallPhage/Winterexp/Period1/Exp/PlanOfAttack|3.16 Plan of Attack]]
<br>
<br>
-
<font size="4"> '''5/3/13''' </font>
+
<font size="4"> '''3/18/13''' </font>
-
- Performed agar test, focusing primarily on ×8
+
- Presented current understanding and plans for the future
 +
: Decided on a two-focus attack
 +
:: Evolution – selecting naturally occurring smaller phages
 +
:: Site directed mutagenesis – using genome info and comparative studies to identify sites to target
 +
- More background research
 +
: Possible ways of making phage smaller
-
: [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU_Provo/5.3 T7 phage selection method test|5.3 T7 phage selection method test]]
+
<br>
-
- Processed phage amplification
+
<font size="4"> '''3/20/13''' </font>
-
: [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU_Provo/5.3 Phage Amplification/Purification|5.3 T7 phage amplification/purification]]
+
- Background research on phiX174: the only phage we have in stock
 +
 
 +
- Performed [[Team:BYU_Provo/Notebook/SmallPhage/Winterexp/Period1/Exp/3.20 Phage Viability Test|3.20 Phage Viability Test]]
<br>
<br>
-
<font size="4"> '''5/4/13''' </font>
+
<font size="4"> '''3/21/13''' </font>
-
- Performed dilution series using stock 5.3 (-1 through -11)
+
- Checked up on results for [[Team:BYU_Provo/Notebook/SmallPhage/Winterexp/Period1/Exp/3.20 Phage Viability Test|3.20 Phage Viability Test]]
-
 
+
-
- Started two 5mL overnights of BL21
+
<br>
<br>
-
<font size="4"> '''5/5/13''' </font>
+
<font size="4"> '''3/22/13''' </font>
-
- Spot test using stock 5.3 and its dilution series (from 5.4)
+
- Discussed results from tittering experiment (preliminary experiment 1)
-
: [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU_Provo/5.3 Phage Amplification/Purification|5.3 T7 phage amplification/purification]]
+
: Contamination mostly likely resulted from the step involving suspending phage in LB – obvious contamination in the LB bottle
-
- Started liquid culture for purification team (at around noon)
+
: One of the stock phage solution had contamination as well
-
: 1mL of BL21 overnight + 4mL of LB + 100μL -2 phage (received stock)
+
- Discussed step of attack with Dr. Grose
-
- Started 5.5 amplification from a plaque test
+
: Decided to go with T7, if necessary Qbeta
-
: [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU_Provo/5.5_Amplification_from_a_plaque_test|5.5 Amplification from a plaque test]]
+
: Need to learn to make top agar at various concentrations
-
<br>
+
: Need to do more background research and decide whether to assemble phage capsid in vitro (plasmid + E coli) or do direct mutagenesis of phage genome
-
<font size="4"> '''5/6/13''' </font>
+
:: Need to correspond with the isolation team
-
- Continued [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU_Provo/5.3 T7 phage selection method test|5.3 T7 phage amplification/purification]]
+
- Sequencing will be for individual genes to cut down cost
-
- Performed liquid culture phage concentration test
+
: Need to design primers and get to know the genome of the phage
-
: [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU Provo/5.6 T7+ Liquid Culture Phage Concentration Test|5.6 T7+ Liquid Culture Phage Concentration Test]]
+
- Learnt about Mega5 to compare genome and protein sequence
<br>
<br>
-
<font size="4"> '''5/7/13''' </font>
+
<font size="4"> '''3/25/13''' </font>
-
- Started two 5mL of E coli BL21 overnight
+
March 25, 2013
-
- Designed procedure for applying mutagen and selecting for T7
+
- Reported on past week and plans for this week
 +
: From last week: titering experiment
 +
: This week
 +
:: Learn to make top agar at various concentrations
 +
:: Background research to determine in vitro assembly vs altering genome – look into specific techniques
 +
:: Comparing genome of phage and decide on possible site-directed mutagenesis options
-
<br>
+
- Start working on designing our site directed mutagenesis
 +
: Qbeta vs MS2
 +
:: Look for places where sequences are significantly different
 +
:: Might be worthwhile to look at capsid structure to identify the regions where interactions between subunits take place
-
<font size="4"> '''5/8/13''' </font>
+
: Qbeta vs T7 major
 +
:: No real consensus – more worthwhile to compare capsid protein sequence of T7 with those that have similar size to it
-
- Went over procedure for applying mutagen and PCR with Dr. Grose
+
: T7 major vs minor
 +
:: 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
-
- Performed spot tests under [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period1/Exp/Team:BYU Provo/5.6 T7+ Liquid Culture Phage Concentration Test|5.6 T7+ Liquid Culture Phage Concentration Test]]
+
: Qbeta major vs minor
 +
:: Just continue transcribing after it reaches the stop codon. What does the stop codon code for?
-
- Started two 5mL BL21 overnights
+
- Research into in-vitro assembly vs direct mutation of phage genome
-
 
+
: It seems that we’ll need to clone the genome of the phage into a plasmid and let it assemble in an E coli
-
- Learned how to create LB plates
+
: Using chemicals we can induce random mutations in phage – might be worthwhile if selection in agar is not working as well.
<br>
<br>
-
<font size="4"> '''5/9/13''' </font>
+
<font size="4"> '''3/27/13''' </font>
-
- Practiced with ×6 and ×8 top agar
+
- More research on genome of enterobacteria phage
-
 
+
-
: [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/Exp/5.9_T7_selection_method_test|5.9 T7 Selection Method Test #2]]
+
-
 
+
-
- Started [[Team:BYU Provo/Notebook/SmallPhage/Springexp/Period1/Exp/5.9 T7+ Liquid Culture Phage Concentration Test|5.9 T7+ Liquid Culture Phage Concentration Test #2]]
+
-
 
+
-
- Discussed plans and schedule for next week.
+
-
 
+
-
<br>
+
-
<font size="4"> '''5/10/13''' </font>
+
: Generation of the major and minor capsid in Q beta
 +
: Capsid protein information research
 +
: Capsid protein sequence comparison
-
- Worked on [[Team:BYU_Provo/Notebook/SmallPhage/Springexp/Period1/PR|Progress Report]]
+
- Outlined protocol for producing stock top agar
 +
: [[Team:BYU_Provo/Notebook/SmallPhage/Winterexp/Period1/Exp/4.3 Top Agar Stock Preparation|4.3 Top Agar Stock Preparation]]
<br>
<br>
-
<font size="4"> '''5/12/13''' </font>
+
<font size="4"> '''3/29/13''' </font>
-
- Started two 5mL overnight at around 6pm
+
- Worked on our first team presentation.
<br>
<br>

Revision as of 00:03, 30 May 2013


Small Phage March - April Notebook: March 15 - March 31 Daily Log



Overview
March-April
May-June
July-August
September-October

3/15/13

- Today marks the start of our Small Phage Team!

- Went over iGem parts database, PCR database.

- Shared results from individual background research.

Our small phage group will focus on T7 and Q beta
T7 – very well studied, research done on its use for drug delivery
Q beta – relatively well characterized, much smaller than T7 28nm vs 60nm

- Did more background research and brainstormed ideas for a plan of attack

Decided to focus on T7 first, since it’s easily acquired and more info is available


3/16/13

- Did more background reading for T7; literature search for possible plan of attack

3.16 Plan of Attack


3/18/13

- Presented current understanding and plans for the future

Decided on a two-focus attack
Evolution – selecting naturally occurring smaller phages
Site directed mutagenesis – using genome info and comparative studies to identify sites to target

- More background research

Possible ways of making phage smaller


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)

Contamination mostly likely resulted from the step involving suspending phage in LB – obvious contamination in the LB bottle
One of the stock phage solution had contamination as well

- Discussed step of attack with Dr. Grose

Decided to go with T7, if necessary Qbeta
Need to learn to make top agar at various concentrations
Need to do more background research and decide whether to assemble phage capsid in vitro (plasmid + E coli) or do direct mutagenesis of phage genome
Need to correspond with the isolation team

- Sequencing will be for individual genes to cut down cost

Need to design primers and get to know the genome of the phage

- Learnt about Mega5 to compare genome and protein sequence


3/25/13

March 25, 2013

- Reported on past week and plans for this week

From last week: titering experiment
This week
Learn to make top agar at various concentrations
Background research to determine in vitro assembly vs altering genome – look into specific techniques
Comparing genome of phage and decide on possible site-directed mutagenesis options

- Start working on designing our site directed mutagenesis

Qbeta vs MS2
Look for places where sequences are significantly different
Might be worthwhile to look at capsid structure to identify the regions where interactions between subunits take place
Qbeta vs T7 major
No real consensus – more worthwhile to compare capsid protein sequence of T7 with those that have similar size to it
T7 major vs minor
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
Qbeta major vs minor
Just continue transcribing after it reaches the stop codon. What does the stop codon code for?

- Research into in-vitro assembly vs direct mutation of phage genome

It seems that we’ll need to clone the genome of the phage into a plasmid and let it assemble in an E coli
Using chemicals we can induce random mutations in phage – might be worthwhile if selection in agar is not working as well.


3/27/13

- More research on genome of enterobacteria phage

Generation of the major and minor capsid in Q beta
Capsid protein information research
Capsid protein sequence comparison

- Outlined protocol for producing stock top agar

4.3 Top Agar Stock Preparation


3/29/13

- Worked on our first team presentation.


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