Team:IIT Madras/Protocols

From 2010.igem.org

(Difference between revisions)
(New page: {{iitm/main_new}} This is where the protocols go. {{iitm/footbar}})
Line 1: Line 1:
{{iitm/main_new}}
{{iitm/main_new}}
-
This is where the protocols go.
+
<b>PCR Protocol</b>
 +
 
 +
Composition of PCR reaction:
 +
*PHusion Phusion® High-Fidelity DNA Polymerase(from Finnzymes) - 0.2 mul
 +
*5x Phusion HF Buffer (from Finnzymes)  - 4 mul
 +
*dNTP – 1 mul
 +
*DNA Template – 1 mul
 +
*Primers(from Bioserve) – 1 mul each.
 +
*Water – 12.8 mul
 +
 
 +
Total volume for the reaction is 20 mul.
 +
 
 +
 
 +
 
 +
<b>Digestion Protocol</b>
 +
 
 +
Composition of the digestion mixture:
 +
*DNA - 4 mul
 +
*Enzyme 1 - 1.2 mul
 +
*Enzyme 2 - 1.2 mul
 +
*Buffer - 2 mul
 +
*Water - 11.6 mul
 +
Total volume for the reaction is 20 mul.
 +
 
 +
Steps:
 +
#For EcorRI, PstI – The reaction mixture is kept at 37 degrees for 1.5 hours. For other Enzymes – The reaction mixture is kept at 37 degrees for 5 hours.
 +
#Inactivate enzyme by heating at 80 degrees for 20 mins.
 +
 
 +
 
 +
<b>T4 Ligation Protocol</b>
 +
 
 +
Composition of Ligation mixture:
 +
*T4 Ligase Buffer - 1mul
 +
*6:1 molar insert:vector (vector~10ng)
 +
*miliQ water - (8.5 - DNA volume) mul
 +
*T4 ligase – 0.5 mul
 +
 
 +
Steps:
 +
#Leave reaction at 22.5degC for 30min
 +
#Denaturate ligase at 65degC for 10min
 +
#Store at -20degC
 +
 
 +
 
{{iitm/footbar}}
{{iitm/footbar}}

Revision as of 18:28, 27 October 2010

PCR Protocol

Composition of PCR reaction:

  • PHusion Phusion® High-Fidelity DNA Polymerase(from Finnzymes) - 0.2 mul
  • 5x Phusion HF Buffer (from Finnzymes) - 4 mul
  • dNTP – 1 mul
  • DNA Template – 1 mul
  • Primers(from Bioserve) – 1 mul each.
  • Water – 12.8 mul

Total volume for the reaction is 20 mul.


Digestion Protocol

Composition of the digestion mixture:

  • DNA - 4 mul
  • Enzyme 1 - 1.2 mul
  • Enzyme 2 - 1.2 mul
  • Buffer - 2 mul
  • Water - 11.6 mul

Total volume for the reaction is 20 mul.

Steps:

  1. For EcorRI, PstI – The reaction mixture is kept at 37 degrees for 1.5 hours. For other Enzymes – The reaction mixture is kept at 37 degrees for 5 hours.
  2. Inactivate enzyme by heating at 80 degrees for 20 mins.


T4 Ligation Protocol

Composition of Ligation mixture:

  • T4 Ligase Buffer - 1mul
  • 6:1 molar insert:vector (vector~10ng)
  • miliQ water - (8.5 - DNA volume) mul
  • T4 ligase – 0.5 mul

Steps:

  1. Leave reaction at 22.5degC for 30min
  2. Denaturate ligase at 65degC for 10min
  3. Store at -20degC


 

Retrieved from "http://2010.igem.org/Team:IIT_Madras/Protocols"