Team:University of Lethbridge/Notebook/Project2July

From 2008.igem.org

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[[Team:University_of_Lethbridge/Notebook|Back to The University of Lethbridge Main Notebook]]
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===July 28, 2008===
===July 28, 2008===
====Nathan Puhl, Roxanne====
====Nathan Puhl, Roxanne====
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     4. Hold at 4 C
     4. Hold at 4 C
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===July 29, 2008===
===July 29, 2008===
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Samples:  
Samples:  
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Gel #1:
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  Gel #1:
  - Lane 1: 100 bp ladder
  - Lane 1: 100 bp ladder
  - Lane 2: Neg cntl
  - Lane 2: Neg cntl
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  - Lane 6: 1:100 template dilution, anneling tenp (49.0 C)
  - Lane 6: 1:100 template dilution, anneling tenp (49.0 C)
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Gel #2:
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  Gel #2:
  - Lane 1: 100 bp ladder
  - Lane 1: 100 bp ladder
  - Lane 2: 1:10 template dilution, annealing temp (53.0 C)
  - Lane 2: 1:10 template dilution, annealing temp (53.0 C)
Line 52: Line 55:
Results? Bands present in all lanes! (all around 100 bp) However, unsure if the bands are primer bands or Riboswitch sequence DNA bands. Nathan to run a 3% Agarose gel tonight to try and get better resolution.
Results? Bands present in all lanes! (all around 100 bp) However, unsure if the bands are primer bands or Riboswitch sequence DNA bands. Nathan to run a 3% Agarose gel tonight to try and get better resolution.
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note: Double bands present in this gel as well. Two bands at ~1kb and 1.5 kb are present in lanes L10 and H10.
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note: Double bands present in this gel as well. Two bands at ~1kb and 1.5 kb are present in lanes L10 and H100.
[[Image:08Jul28_RSPCR.jpg|250 px]]
[[Image:08Jul28_RSPCR.jpg|250 px]]
[[Image:08Jul28_RSPCR2.jpg|125 px]]
[[Image:08Jul28_RSPCR2.jpg|125 px]]

Latest revision as of 02:34, 30 October 2008

Back to The University of Lethbridge Main Notebook

Contents

July 28, 2008

Nathan Puhl, Roxanne

Objective: Amplify Riboswitch sequence from pTopp plasmid using PCR Reaction

PCR reaction setup:

-Enzyme = Phusion -Template = pTopp plasmid, dilution series of 1:10, 1:100 and (-) control -Buffer = HF Phusion buffer -Primers = IDT, designed & shipped July 16/08 -Total # of reactions = 20

PCR cycle conditions (programmed into Brent's PCR machine under "iGEM":

   1. Initial denaturation @ 98 C for 30 sec (1 cycle)
   
   2a. Denaturation @ 98 C for 30 sec (35 cycles for step #2)
   
   2b. Annealing via gradient for 15 sec (45.0 C to 53.0 C)
          
   2c. Extension @ 72 C for 30 sec
   
   3. Final extension @ 72 C for 7 mins (1 cycle)
   
   4. Hold at 4 C


July 29, 2008

Roxanne, Selina

Objective: Visualize whether any Ribswitch PCR reactions (July 28) were successful. Expect to see a band around 75 bp.

Ran 1% TAE agarose gel at 100 V for 30 mins

Loaded 5 uL sample, 1 uL ladder

Samples:

 Gel #1:
- Lane 1: 100 bp ladder
- Lane 2: Neg cntl
- Lane 3: 1:10 template dilution, annealing temp  (45.0 C)
- Lane 4: 1:100 template dilution, annealing temp (45.0 C)
- Lane 5: 1:10 template dilution, annealing temp (49.0 C)
- Lane 6: 1:100 template dilution, anneling tenp (49.0 C)
 Gel #2:
- Lane 1: 100 bp ladder
- Lane 2: 1:10 template dilution, annealing temp (53.0 C)
- Lane 3: 1:100 template dilution, annealing temp (53.0 C)

Results? Bands present in all lanes! (all around 100 bp) However, unsure if the bands are primer bands or Riboswitch sequence DNA bands. Nathan to run a 3% Agarose gel tonight to try and get better resolution.

note: Double bands present in this gel as well. Two bands at ~1kb and 1.5 kb are present in lanes L10 and H100.


08Jul28 RSPCR.jpg 08Jul28 RSPCR2.jpg