Team:DTU-Denmark/Notebook/13 August 2013

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(lab 208)
(SLP screening PCR)
 
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{{:Team:DTU-Denmark/Templates/StartPage|13 August 2013}}
{{:Team:DTU-Denmark/Templates/StartPage|13 August 2013}}
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Navigate to the [[Team:DTU-Denmark/Notebook/12_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/14_August_2013|Next]] Entry
Navigate to the [[Team:DTU-Denmark/Notebook/12_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/14_August_2013|Next]] Entry
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=Lab 208=
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=lab 208=
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<hr/>
<hr/>
==Main purpose==
==Main purpose==
<hr/>
<hr/>
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*PCR to amplify USER fragments of the constitutive SPL;
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*PCR of Nir2 with USER primers;
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*Gel purification of araBAD SPL.
==Who was in the lab==
==Who was in the lab==
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===PCR Nir2===
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===PCR of Nir2 with USER primers===
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PCR to gain a bigger amount of the extraction fragment of Nir2
 
{| class="wikitable" style="text-align: right"
{| class="wikitable" style="text-align: right"
! sample nr. !! buffer !! %DMSO !! program
! sample nr. !! buffer !! %DMSO !! program
|-
|-
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|  1 || || ||  
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|  1 || GC || 2 || 55C
|-
|-
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|  2 || || ||
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|  2 ||GC || 3 || 55C
|-
|-
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|  3 || || ||
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|  3 || GC || 5 || 55C
|-
|-
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|  4 ||  || ||
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|  4 ||  HF|| 2 || 55C
|-
|-
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|  5 || || ||
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|  5 || HF || 3 || 55C
|-
|-
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|  6 || || ||
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|  6 || HF || 5 || 55C
|-
|-
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|  7 || || || ramp
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|  7 || GC || 2 || ramp
|-
|-
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|  8 || || || ramp
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|  8 || GC || 3 || ramp
|-
|-
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|  9 || || || ramp
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|  9 || GC || 5 || ramp
|-
|-
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|  10 || || || ramp
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|  10 || HF || 2 || ramp
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|-
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|  11 || || || ramp
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|  11 || HF || 3 || ramp
|-
|-
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|  12 || || || ramp
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|  12 || HF || 5 || ramp
|-
|-
|}
|}
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===PCR for Nir2 with USER primers===
 
* PCR mix according to standard protocol with changes: addition of DMSO in 3 different final concentrations (2%, 3%, 5%); two different buffers (HF 5x and GC 5x), amount of added water was dependent on volume of added DMSO.
* PCR mix according to standard protocol with changes: addition of DMSO in 3 different final concentrations (2%, 3%, 5%); two different buffers (HF 5x and GC 5x), amount of added water was dependent on volume of added DMSO.
* Primers for Nir2 - 40a, 40b
* Primers for Nir2 - 40a, 40b
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* Templates - fragment Nir2 amplified with non-uracil primers, 3uL were used
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* Template - fragment Nir2 amplified with non-uracil primers, 3uL were used
* Polymerase x7
* Polymerase x7
* Program A99, samles 1-6, was based on standard PCR program with 55 C and 1 min of annealing parameters and 5 min of extension time.
* Program A99, samles 1-6, was based on standard PCR program with 55 C and 1 min of annealing parameters and 5 min of extension time.
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* Program A1, samples 7-12, touch-down PCR with initial temperature of 59C falling down to 53C (rate 0.1 C/min).
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* Program A1, samples 7-12, PCR with initial annealing temperature of 59C falling down to 53C (rate 0.1 C/min). 5 min of extension time.
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* Samples names:
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# Nir2, GC buffer, 2% DMSO
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# Nir2, GC buffer, 3% DMSO
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# Nir2, GC buffer, 5% DMSO
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# Nir2, HF buffer, 2% DMSO
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# Nir2, HF buffer, 3% DMSO
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# Nir2, HF buffer, 5% DMSO
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===Gel purification===
===Gel purification===
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<hr/>
<hr/>
===SLP screening PCR===
===SLP screening PCR===
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The PCR run with condition E (5% DMSO, 2mM MgCl2 with GC buffer) had the highest flexibility; it yields the expected product at different annealing temperatures: 58.4 C, 59.6, C 60.6 C, 61.9 C, 63.2 C, 64.6 C, 65 C.
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The PCR run with condition E (5% DMSO, 2mM MgCl<sub>2</sub> with GC buffer) had the highest flexibility; it yields the expected product at different annealing temperatures: 58.4 C, 59.6, C 60.6 C, 61.9 C, 63.2 C, 64.6 C, 65 C.
Navigate to the [[Team:DTU-Denmark/Notebook/12_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/14_August_2013|Next]] Entry
Navigate to the [[Team:DTU-Denmark/Notebook/12_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/14_August_2013|Next]] Entry
{{:Team:DTU-Denmark/Templates/EndPage}}
{{:Team:DTU-Denmark/Templates/EndPage}}

Latest revision as of 11:57, 4 October 2013

13 August 2013

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Contents

Lab 208


Main purpose


  • PCR to amplify USER fragments of the constitutive SPL;
  • PCR of Nir2 with USER primers;
  • Gel purification of araBAD SPL.

Who was in the lab


Kristian, Henrike, Gosia

Procedure


PCR (promoter library)

PCR to amplify USER fragments of the constitutive SPL, the constitutive reference promoter and the arabinose reference promoter.

Used 5% DMSO, 2 uL of mM MgCl2 and GC-buffer.

constitutive SPL

  • template: pZA21::RFP
  • primers: 52a, 52b1
  • annealing temp: 58.1C
  • elongation time: 3:00

constitutive reference

  • template: pZA21::RFP
  • primers: 52a, 52b2
  • annealing temp: 58.1C
  • elongation time: 3:00

Wanted to make negative for the two above reactions but accidentally put the template in the master mix.

arabinose reference

  • template: pZA21:araBAD:RFP (labeled Ara)
  • primers: 51a,51b1
  • annealing temp: 60.3C
  • elongation time: 4:00

program (used for all 3 reactions):

temperature time cycles
98C 2:00 -
98C 0:20 36
annealing temp 1:00 36
72C extension time 36
72C 5:00 -
10C hold -

PCR of Nir2 with USER primers

sample nr. buffer  %DMSO program
1 GC 2 55C
2 GC 3 55C
3 GC 5 55C
4 HF 2 55C
5 HF 3 55C
6 HF 5 55C
7 GC 2 ramp
8 GC 3 ramp
9 GC 5 ramp
10 HF 2 ramp
11 HF 3 ramp
12 HF 5 ramp
  • PCR mix according to standard protocol with changes: addition of DMSO in 3 different final concentrations (2%, 3%, 5%); two different buffers (HF 5x and GC 5x), amount of added water was dependent on volume of added DMSO.
  • Primers for Nir2 - 40a, 40b
  • Template - fragment Nir2 amplified with non-uracil primers, 3uL were used
  • Polymerase x7
  • Program A99, samles 1-6, was based on standard PCR program with 55 C and 1 min of annealing parameters and 5 min of extension time.
  • Program A1, samples 7-12, PCR with initial annealing temperature of 59C falling down to 53C (rate 0.1 C/min). 5 min of extension time.

Gel purification

Gel purified araBAD SPL from yesterdays screening PCR

Results


Gel of SLP screening PCR products (yesterday)

Each gel is representing one row; from left to right and up to down is row A to H:

Gel of todays PCR reactions

  • 1kb ladder
  • Nir2 PCR - sample 1
  • Nir2 PCR - sample 2
  • Nir2 PCR - sample 3
  • Nir2 PCR - sample 4
  • Nir2 PCR - sample 5
  • Nir2 PCR - sample 6
  • Nir2 PCR - sample 7
  • Nir2 PCR - sample 8
  • Nir2 PCR - sample 9
  • Nir2 PCR - sample 10
  • Nir2 PCR - sample 11
  • Nir2 PCR - sample 12
  • constitutive SPL 1
  • constitutive SPL 2 (duplicate)
  • constitutive promoter reference 1
  • constitutive promoter reference 2 (duplicate)
  • constitutive promoter reference 3 (very small sample, there was almost nothing left in the master mix)
  • 1kb ladder

2013-08-13 nir2 const spl ref.jpg

Conclusion


SLP screening PCR

The PCR run with condition E (5% DMSO, 2mM MgCl2 with GC buffer) had the highest flexibility; it yields the expected product at different annealing temperatures: 58.4 C, 59.6, C 60.6 C, 61.9 C, 63.2 C, 64.6 C, 65 C.

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