Difference between revisions of "PCR Amplification of DNA"

From Bridges Lab Protocols
Jump to: navigation, search
(updated)
 
(One intermediate revision by the same user not shown)
Line 9: Line 9:
 
==Protocol==
 
==Protocol==
 
*Use the following volumes per reaction
 
*Use the following volumes per reaction
::*Buffer, 5 uL of 10X buffer (Dave's fridge)
+
::*12.5 uL DreamTaq
::*Primers, 10uL of 1uM stock solution in water (both primers combined)
+
::*7.5 uL RNAse-Free water
::*dNTPs, 5uL of 2 mM ("molecular biology stuff" box in freezer)
+
::*5.0 uL Working stock Primer (of 0.4-1uM stock solution in water (both primers combined))
::*Sterile water, 28 uL
+
 
::*Template 1 uL
+
==PCR Program==
::*Polymerase 1 uL (turbo pfu found in "enzymes" box in freezer)
+
*For animals: use programs denoted in [[Genotyping Program]]
  
 
*Run PCR Program (approx 3.5 to 4 hours).  Normally use touchdown PCR ('''DAVETD''') as follows:
 
*Run PCR Program (approx 3.5 to 4 hours).  Normally use touchdown PCR ('''DAVETD''') as follows:

Latest revision as of 16:57, 8 June 2020

SOP

Materials

Protocol

  • Use the following volumes per reaction
  • 12.5 uL DreamTaq
  • 7.5 uL RNAse-Free water
  • 5.0 uL Working stock Primer (of 0.4-1uM stock solution in water (both primers combined))

PCR Program

  • Run PCR Program (approx 3.5 to 4 hours). Normally use touchdown PCR (DAVETD) as follows:
  1. 1 min at 94
  2. 30s at 65
  3. 2 min/kb at 72
  4. 30s at 94
  5. 30s at 63 then -0.5/cycle
  6. 2 min/kb at 72
  7. Repeat steps 4-6 28 times
  8. 30s at 94
  9. 30s at 45
  10. 11 min at 72
  11. Hold at 4 until ready
  • Purify PCR product if necessary using Qiagen kit (Add 5x PB)