Team:Lethbridge/Notebook/Planning

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<BLOCKQUOTE>
Back To:
Back To:
Line 65: Line 109:
Work to be done:
Work to be done:
-
=Week of June 14/2010=
+
=<font color="white">Week of June 14/2010=
-
==Justin <i>et al</i>==
+
==<font color="white">Justin <i>et al</i>==
-
===Finish mms6-dT work===
+
===<font color="white">Finish mms6-dT work===
*<del>Heat kill ligase</del>
*<del>Heat kill ligase</del>
*<del>take small sample for gel</del>
*<del>take small sample for gel</del>
Line 74: Line 118:
*<del>Transform into DH5&alpha;</del>
*<del>Transform into DH5&alpha;</del>
-
===Test T4 DNA Ligase:===
+
===<font color="white">Test T4 DNA Ligase:===
*<del>Restrict rbs-xylE with EcoRI and SpeI (take sample for analysis on gel)</del>
*<del>Restrict rbs-xylE with EcoRI and SpeI (take sample for analysis on gel)</del>
*<del>Heat kill EcoRI and SpeI</del>
*<del>Heat kill EcoRI and SpeI</del>
Line 80: Line 124:
*<del>Run unrestricted, restricted and ligated samples on a gel.</del>
*<del>Run unrestricted, restricted and ligated samples on a gel.</del>
-
===Prepare plasmid DNA for sequencing===
+
===<font color="white">Prepare plasmid DNA for sequencing===
*<del>Adam to upload guidelines for preparation.</del>
*<del>Adam to upload guidelines for preparation.</del>
-
===Test PCR conditions for confirmation of ligation via PCR:===
+
===<font color="white">Test PCR conditions for confirmation of ligation via PCR:===
*Run a PCR of lumazine synthase gene that was sent for sequencing (and subsequently confirmed)
*Run a PCR of lumazine synthase gene that was sent for sequencing (and subsequently confirmed)
**using VF2 and VR primers
**using VF2 and VR primers
*Run this PCR on a 2% agarose gel
*Run this PCR on a 2% agarose gel
-
===PCR Confirm previous ligations===
+
===<font color="white">PCR Confirm previous ligations===
If (AND ONLY IF) PCR conditions amplified our known lumazine synthase gene, set up PCR of our previous ligation reactions to see if there is any ligated product.
If (AND ONLY IF) PCR conditions amplified our known lumazine synthase gene, set up PCR of our previous ligation reactions to see if there is any ligated product.
-
==Adam==
+
==<font color="white">Adam==
*<del>Finish VWR order (1000&micro;L tips); test tubes; test tube racks; 96 well plates for sequencing, petri dishes</del>
*<del>Finish VWR order (1000&micro;L tips); test tubes; test tube racks; 96 well plates for sequencing, petri dishes</del>
*<del>Get RMA for VWR order (ie wrong test tube and test tube racks)</del>
*<del>Get RMA for VWR order (ie wrong test tube and test tube racks)</del>
Line 103: Line 147:
**Send for sequencing
**Send for sequencing
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=Week of July 5th/2010=
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=<font color="white">Week of July 5th/2010=
-
==One==
+
==<font color="white">One==
<del>1) Maxiprep cells with the following BioBricks:</del><br>
<del>1) Maxiprep cells with the following BioBricks:</del><br>
<del>*pLacI</del><br>
<del>*pLacI</del><br>
Line 123: Line 167:
<del>5) Put flow chart on wall</del>
<del>5) Put flow chart on wall</del>
-
==Two==
+
==<font color="white">Two==
1) Add dT (from maxiprep above) to  
1) Add dT (from maxiprep above) to  
*<del>Mms6</del>
*<del>Mms6</del>
Line 131: Line 175:
<del>2)Overexpression test of "CFP Complete" and mms6</del><br>
<del>2)Overexpression test of "CFP Complete" and mms6</del><br>
-
==Three==
+
==<font color="white">Three==
*Restrict lumazine, mms6, and xylE from BioBrick plasmid with NotI, and ligate into pET28a plasmid (pre-cut with NotI).
*Restrict lumazine, mms6, and xylE from BioBrick plasmid with NotI, and ligate into pET28a plasmid (pre-cut with NotI).
**Check ligation and gel extract bands of proper size (Check for double insertion, plasmid self-ligation)
**Check ligation and gel extract bands of proper size (Check for double insertion, plasmid self-ligation)
Line 139: Line 183:
**Send for sequencing
**Send for sequencing
-
=Week of July 12th/2010=
+
=<font color="white">Week of July 12th/2010=
-
==One==
+
==<font color="white">One==
1) <del>Add dt to Mms6,Lumazine, and xylE</del>
1) <del>Add dt to Mms6,Lumazine, and xylE</del>
*<del>Restrict Individual Parts</del>
*<del>Restrict Individual Parts</del>
Line 175: Line 219:
12) Talk to Hayes lab about borrowing some Argon that they have on tap...<br>
12) Talk to Hayes lab about borrowing some Argon that they have on tap...<br>
-
==Two==
+
==<font color="white">Two==
1) maxiprep
1) maxiprep
*pET28(a)<br>
*pET28(a)<br>
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*pLacI-sRBS<br>
*pLacI-sRBS<br>
-
==Three==
+
==<font color="white">Three==
1) Assemble
1) Assemble
*pLacI-sRBS-lumazine-dt
*pLacI-sRBS-lumazine-dt
Line 190: Line 234:
2) Insert Mms6, xylE, and Lumazine Synthase into pET28(a) over-expression vector
2) Insert Mms6, xylE, and Lumazine Synthase into pET28(a) over-expression vector
-
=Week of August 3rd/2010=
+
=<font color="white">Week of August 3rd/2010=
-
==One==
+
==<font color="white">One==
1) Send samples for sequencing<br>
1) Send samples for sequencing<br>
Line 203: Line 247:
4) Assemble
4) Assemble
-
==Two==
+
==<font color="white">Two==
-
==Three==
+
==<font color="white">Three==
-
=Week of August 3rd/2010=
+
=<font color="white">Week of August 9th/2010=
1) PCR:  
1) PCR:  
*Mms6 Mr. Gene with prefix/suffix<br>
*Mms6 Mr. Gene with prefix/suffix<br>
Line 223: Line 267:
6) Assemble lumazine at dT<br>
6) Assemble lumazine at dT<br>
-
=Week of August 3rd/2010=
+
=<font color="white">Week of August 16th/2010=

Latest revision as of 22:04, 20 September 2010




Back To:


Work to be done:

Contents

Week of June 14/2010

Justin et al

Finish mms6-dT work

  • Heat kill ligase
  • take small sample for gel
  • take another sample for restriction (cut out entire biobrick)
  • Run gel of above
  • Transform into DH5α

Test T4 DNA Ligase:

  • Restrict rbs-xylE with EcoRI and SpeI (take sample for analysis on gel)
  • Heat kill EcoRI and SpeI
  • Ligate with T4 DNA Ligase
  • Run unrestricted, restricted and ligated samples on a gel.

Prepare plasmid DNA for sequencing

  • Adam to upload guidelines for preparation.

Test PCR conditions for confirmation of ligation via PCR:

  • Run a PCR of lumazine synthase gene that was sent for sequencing (and subsequently confirmed)
    • using VF2 and VR primers
  • Run this PCR on a 2% agarose gel

PCR Confirm previous ligations

If (AND ONLY IF) PCR conditions amplified our known lumazine synthase gene, set up PCR of our previous ligation reactions to see if there is any ligated product.

Adam

  • Finish VWR order (1000µL tips); test tubes; test tube racks; 96 well plates for sequencing, petri dishes
  • Get RMA for VWR order (ie wrong test tube and test tube racks)
  • Get guidelines for sequencing.
  • Make primers for inserting mms6, xylE, lumazine, (C and N terminal labelled CFP/YFP-maybe) into pET28a expression vectors.No longer required.
  • Order polymerase, SpeI, NotI, and (maybe, depending on results) T4 DNA ligase from Fermentas.
    • Check with HJ's lab to see which polymerase they use and from whom.
  • Restrict lumazine, mms6, and xylE from BioBrick plasmid with NotI, and ligate into pET28a plasmid (pre-cut with NotI).
    • Check ligation and gel extract bands of proper size (Check for double insertion, plasmid self-ligation)
    • Transform into DH5α and purify plasmid DNA
    • Perform restriction analysis (using EcoRI and EcoRV) to check orientation of insert
    • Perform overexpression tests
    • Send for sequencing

Week of July 5th/2010

One

1) Maxiprep cells with the following BioBricks:
*pLacI
*pBad
*dT
*CFP compete
*Mms6 Mr. Gene
*pBad-TetR
*Lumazine
*EYFP

2) Request parts from the Registry

3) Send in for sequencing the products of PCR from June X/2010

4) Come up with PET28a plan B

5) Put flow chart on wall

Two

1) Add dT (from maxiprep above) to

  • Mms6
  • xylE
  • Lumazine synthase

All above already maxiprepped
2)Overexpression test of "CFP Complete" and mms6

Three

  • Restrict lumazine, mms6, and xylE from BioBrick plasmid with NotI, and ligate into pET28a plasmid (pre-cut with NotI).
    • Check ligation and gel extract bands of proper size (Check for double insertion, plasmid self-ligation)
    • Transform into DH5α and purify plasmid DNA
    • Perform restriction analysis (using EcoRI and EcoRV) to check orientation of insert
    • Perform overexpression tests
    • Send for sequencing

Week of July 12th/2010

One

1) Add dt to Mms6,Lumazine, and xylE

  • Restrict Individual Parts
  • Set up ligation reaction
  • Confirm ligation using PCR
  • Transform confirmed parts into DH5α
  • Miniprep confirmed parts

2) Maxipreps

  • pLacI

3) Jeff to finalize signal sequences by Wednesday for Friday order

4) Friday order for four fluorescent proteins

  • CEYFP
  • NEYFP
  • CECFP
  • NECFP

5) Successful meeting with Bob

6) Adam to talk to Lisza about Mms6

7) Adam to compile list of confirmed parts for Lisza

8) Transform Mms6 into BL21(DE3)

9) Justin/Mackenzie to talk to David about working with Argon to make nanoparticles

10) Send away all maxipreps for sequencing

11) Quantify maxipreps using gel method

12) Talk to Hayes lab about borrowing some Argon that they have on tap...

Two

1) maxiprep

  • pET28(a)

2) Assemble

  • pLacI-sRBS

Three

1) Assemble

  • pLacI-sRBS-lumazine-dt
  • pLacI-sRBS-xylE-dt
  • pLacI-sRBS-Mms6-dt

2) Insert Mms6, xylE, and Lumazine Synthase into pET28(a) over-expression vector

Week of August 3rd/2010

One

1) Send samples for sequencing

  • Registry Samples
  • Miniprep samples

2) Talk to Nathan about PCR conditions for xylE

3) Justin to show other team members how to enter data into the wiki

4) Assemble

Two

Three

Week of August 9th/2010

1) PCR:

  • Mms6 Mr. Gene with prefix/suffix
  • xylE with xylE primers
  • colonies with Phusion
  • Fusion standards to fluorescent proteins

2) Prepare samples for sequencing

3) Prepare a list of parts for Lisza

4) Ligate Mms6 into pET-28(a)

5) Ligate lumazine into pET-28(a)

6) Assemble lumazine at dT

=Week of August 16th/2010=