IGEM:Harvard/2006/NES Notebook: Difference between revisions

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Reagants:
Reagants:
*Kaib PCR/Gel Insert: #10
*Kaib PCR/Gel Insert: #10
*KaiC PCR/Gel Insert: #2 PC/GP
*KaiC PCR/Gel Insert: #2 PC/GP
*PCR/Gel Backbone II: #5 II (8.22 Backbone) PC/GP
*PCR/Gel Backbone II: #5 II (8.22 Backbone) PC/GP


Line 113: Line 113:
*6:1 - 6ul:1ul DNA + 1ul H20 + 2ul 5x dilution buf + 10ul Ligation Buf + 1ul ligase  
*6:1 - 6ul:1ul DNA + 1ul H20 + 2ul 5x dilution buf + 10ul Ligation Buf + 1ul ligase  


The Result of transformations: No Dice.  Samples #1, #4, #7, #10, and #14 produced colonies, which I assume result from uncut backbone from the backbone PCR cleanup.


Vary ratio of insert to backbone
After corresponding with Perry:
''Two insert samples''
Ligation with: 2ul backbone, 8ul DNA + 10ul Ligation Buf + 1ul Roche ligase
Using
*KaiC PCR/Gel Insert #2
*Gel Backbone II #5 II (8.22 Backbone)
*Gel Backbone II #6 II (Top band)
*Gel Backbone II #6 II (Middle band)
Transform in 14ul cells


- Gel purification of most successful digest
# KaiC PCR + Gel Backbone #5 II at 21C
 
# KaiC PCR + Gel Backbone #6 II (top) at 21C
- Unpurified sample of most successful digest
# KaiC PCR + Gel Backbone #6 II (middle) at 21C
 
# KaiC Gel + Gel Backbone #5 II at 21C
''To backbone samples''
# KaiC Gel + Gel Backbone #6 II (top) at 21C
 
# KaiC Gel + Gel Backbone #6 II (middle) at 21C
- Gel purification of most successful digest
# KaiC Gel + Gel Backbone #5 II at 17C
 
# KaiC Gel + Gel Backbone #6 II (top) at 17C
- Unpurified sample of most successful digest
# KaiC Gel + Gel Backbone #6 II (middle) at 17C
 
# 1ul Uncut J04500
''For each combination creat samples''
 
- 3ul backbone + 9 ul insert + ligase
 
- 1.5ul backbone 15ul insert + Ligase
 
 
*Transform

Revision as of 13:38, 24 August 2006

To Order

  • DMSO
  • Sodium Thiosulfate
  • Small, Medium, Large, X-large Nitrile gloves

Introductory Materials

IGEM:Harvard/2006/Lab_Intro

New Reporters

Due to issues with T7 promoter, the following biobricks were rehydrated 6/14

Constitutive (IPTG-inducable?) GFP

Constitutive (IPTG?) RFP

Constitutive GFP using TetR promoter. No experience; might not work.

Constitutive (IPTG?) YFP. Apparently gives uneven YFP expression

Transformed with 2ul of DNA on 15ul bacteria; twice for each plasmid. Took 3 ul from each incubation of and added into two two mixed SOC cultures. Let's see what happens when LacI GFP, RFP, YFP are co-cultured.

One of each LacI plasmid type, GFP, RFP, YFP, LacI were cultured overnight on plates treated with 10mM IPTG.

Microscope Notes

Overlap between FITC and YGFP blocks prevents differentiation between YFP and GFP. RFP can be differentiated between YFP/GFP very well.

YFP/GFP fades ~3 hours after being taken out of the incubator after overnight incubation. RFP was still strong at +3h.

IPTG doesn't make an apparent difference in fluoresence.

Promoter Research

7/25/06 Made Glycerol cultures of

  • J04430 (lac GFP)
  • J04450 (lac RFP)
  • I13522 (tet GFP)

We need to transfer these constructs onto pSB4A3

Ligation Assay

  • Digestions - Vary enzyme concentration
  1. 8ul Midiprep KaiC DNA + .5 ul X+P enzyme + 2.5ul Buffer #3 + 2.5ul BSA + 11ul H2O -> 45C 6H
  2. 8ul Midiprep KaiC DNA + 1 ul X+P enzyme + 2.5ul Buffer #3 + 2.5ul BSA + 10ul H2O-> 45C 6H
  3. 8ul Midiprep KaiC DNA + 1 ul X+P enzyme + 2.5ul Buffer #3 + 2.5ul BSA + 10ul H2O-> 37C 6H
  4. 8ul Midiprep Backbone DNA + .5 ul S+P enzyme + 2.5ul Buffer #2 + 2.5ul BSA + 11ul H2O-> 45C 6H
  5. 8ul Midiprep Backbone DNA + 1 ul S+P enzyme + 2.5ul Buffer #2 + 2.5ul BSA + 10ul H2O-> 45C 6H
  6. 8ul Midiprep Backbone DNA + 1 ul S+P enzyme + 2.5ul Buffer #2 + 2.5ul BSA + 10ul H2O-> 37C 6H
  7. 8ul Midiprep Backbone DNA + 2.5ul Buffer #2 + 2.5ul BSA + 12ul H2O
  8. 25ul H20
  9. 8ul Midiprep KaiB DNA + .5 ul X+P enzyme to 25ul + 2.5ul Buffer #3 + 2.5ul BSA + 6ul H2O -> 45C 6H
  10. 8ul Midiprep KaiB DNA + 1 ul X+P enzyme to 25ul + 2.5ul Buffer #3 + 2.5ul BSA + 5ul H2O-> 45C 6H
  11. 8ul Midiprep KaiB DNA + 1 ul X+P enzyme to 25ul + 2.5ul Buffer #3 + 2.5ul BSA + 5ul H2O-> 37C 6H
  12. 20ul H20 + 1.75ul Buffer #2 + 1.75ul Buffer #3 + 2.5ul BSA


Due to the ambiguous backbone lanes above, four digetss were redone with new backbone midiprep.

4II. Same as 4 above with new (8.22) backbone midiprep.

5II. Same as 4 above with new (8.22) backbone midiprep.

6II. Same as 4 above with new (8.22) backbone midiprep.

7II. same as 4 above with new (8.22) backbone midiprep

12. 8ul Midiprep Backbone cut once with S.


  • Phosphatase

- 25ul Digest + 1ul Phosphatase 1H at 45


  • Run on Gel - Create purified and unpurified samples

Add 12 ul of each to the gel.

Chose the most successful digest and run a gel extraction.


  • Ligation -
  • "PCR Insert": DNA from GeneArt Plasmid cleaned up with PCR cleanup kit.
  • "Gel Insert": DNA from GeneArt Plasmid cleaned up with Gel Extraction Kit.
  • "XXX Backbone": DNA from BB_J0450 midiprep
  1. KaiB PCR Insert + PCR Backbone: I:B + NEB Enz= 3:1
  2. KaiB PCR Insert + Gel Backbone: I:B + NEB Enz= 3:1
  3. KaiB Gel Insert + Gel Backbone: I:B + NEB Enz= 3:1
  4. KaiB PCR Insert + PCR Backbone: I:B + NEB Enz= 6:1
  5. KaiB PCR Insert + Gel Backbone: I:B + NEB Enz= 6:1
  6. KaiB Gel Insert + Gel Backbone: I:B + NEB Enz= 6:1
  7. KaiB PCR Insert + PCR Backbone: I:B + Roche Enz= 3:1
  8. KaiB PCR Insert + Gel Backbone: I:B + Roche Enz= 3:1
  9. KaiB Gel Insert + Gel Backbone: I:B + Roche Enz= 3:1
  10. KaiC PCR Insert + PCR Backbone: I:B = 3:1
  11. KaiC PCR Insert + Gel Backbone: I:B = 3:1
  12. KaiC Gel Insert + PCR Backbone: I:B = 3:1
  13. Uncut J04500

Reagants:

  • Kaib PCR/Gel Insert: #10
  • KaiC PCR/Gel Insert: #2 PC/GP
  • PCR/Gel Backbone II: #5 II (8.22 Backbone) PC/GP

Mixtures: NEB

  • 3:1 - 3ul:1ul DNA + 1ul ligase + 2 ul 10x buf + 13ul H2O
  • 6:1 - 6ul:1ul DNA + 1ul ligase + 2 ul 10x buf + 10ul H2O

Roche

  • 3:1 - 3ul:1ul DNA + 4ul H2O + 2ul 5x dilution buf + 10ul Ligation Buf + 1ul ligase
  • 6:1 - 6ul:1ul DNA + 1ul H20 + 2ul 5x dilution buf + 10ul Ligation Buf + 1ul ligase

The Result of transformations: No Dice. Samples #1, #4, #7, #10, and #14 produced colonies, which I assume result from uncut backbone from the backbone PCR cleanup.

After corresponding with Perry: Ligation with: 2ul backbone, 8ul DNA + 10ul Ligation Buf + 1ul Roche ligase Using

  • KaiC PCR/Gel Insert #2
  • Gel Backbone II #5 II (8.22 Backbone)
  • Gel Backbone II #6 II (Top band)
  • Gel Backbone II #6 II (Middle band)

Transform in 14ul cells

  1. KaiC PCR + Gel Backbone #5 II at 21C
  2. KaiC PCR + Gel Backbone #6 II (top) at 21C
  3. KaiC PCR + Gel Backbone #6 II (middle) at 21C
  4. KaiC Gel + Gel Backbone #5 II at 21C
  5. KaiC Gel + Gel Backbone #6 II (top) at 21C
  6. KaiC Gel + Gel Backbone #6 II (middle) at 21C
  7. KaiC Gel + Gel Backbone #5 II at 17C
  8. KaiC Gel + Gel Backbone #6 II (top) at 17C
  9. KaiC Gel + Gel Backbone #6 II (middle) at 17C
  10. 1ul Uncut J04500
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