Difference between revisions of "PCR Analysis of Tail DNA"

From Bridges Lab Protocols
Jump to: navigation, search
(Protocol)
 
(8 intermediate revisions by 2 users not shown)
Line 1: Line 1:
see [[Genotyping Details]] for strain specific details
+
see [[Genotyping Program]] for strain specific details
  
 
==Materials==
 
==Materials==
 +
# Dream Taq Green master mix
 +
# Specific gene Primers (0.4um Working stock)
 +
# Tail digest DNA
 +
# ddH2O
  
 
==Protocol==
 
==Protocol==
Use the following Volumes per 50ul Reaction:
+
First, make 250ul of 0.4um working stock primers from 100um Primary Stocks.
 +
#248 ul ddH20
 +
#1ul forward primer (100um)
 +
#1ul reverse primer (100um)
  
#10X GoTaq Buffer: 5uL ("Molecular Biology Stuff" box in freezer)
 
#Primer Mix: 5ul
 
#dNTPs: 0.5uL of 10 mM ("Molecular Biology Stuff" box in freezer)
 
#Sterile water: 29ul
 
#Polymerase Go-Taq: 0.125uL ("Molecular Biology Stuff"  box in freezer)
 
#Template: 1 uL
 
  
Master Mix (Per 5mL -- Make 1mL Aliquots)
+
Use the following Volumes per 25ul Reaction:
#10X GoTaq Buffer: 625uL ("Molecular Biology Stuff" box in freezer)
+
#Primer Mix: 625ul
+
#dNTPs: 62.5uL of 10 mM ("Molecular Biology Stuff" box in freezer)
+
#Sterile water: 3625ul
+
#Polymerase Go-Taq: 15.625ul ("Molecular Biology Stuff"  box in freezer)
+
*Add Template Individually
+
  
Run PCR Program (approx 2 hours).
+
Per sample (1X)
Use Cycler 1 on 6th Floor
+
#Dream Tag Master mix: 12.5uL ("Molecular Biology Stuff" box in freezer)
*Login: Sergey, Just press enter to Login
+
#0.4um Primer Mix: 5ul
*Under Genotype folder, pick Ingles program for Ingles genotyping
+
#Sterile ddH2O: 7.5ul
*Under Genotype folder, pick regpcr program for PLT genotyping
+
  
Make sure to press enter 2x once to confirm Tubes and second time to start PCR
+
*Template: 1 uL
 +
 
 +
 
 +
Run "specfic" PCR Program for gene of interest (approx 2 hours).
 +
 
 +
*[[Genotyping Program]]
 +
*[[PCR Amplification of DNA]]
  
 
see [[Preparing an Agarose Gel]] for details on preparing a DNA gel
 
see [[Preparing an Agarose Gel]] for details on preparing a DNA gel

Latest revision as of 17:00, 8 June 2020

see Genotyping Program for strain specific details

Materials

  1. Dream Taq Green master mix
  2. Specific gene Primers (0.4um Working stock)
  3. Tail digest DNA
  4. ddH2O

Protocol

First, make 250ul of 0.4um working stock primers from 100um Primary Stocks.

  1. 248 ul ddH20
  2. 1ul forward primer (100um)
  3. 1ul reverse primer (100um)


Use the following Volumes per 25ul Reaction:

Per sample (1X)

  1. Dream Tag Master mix: 12.5uL ("Molecular Biology Stuff" box in freezer)
  2. 0.4um Primer Mix: 5ul
  3. Sterile ddH2O: 7.5ul
  • Template: 1 uL


Run "specfic" PCR Program for gene of interest (approx 2 hours).

see Preparing an Agarose Gel for details on preparing a DNA gel

Retrieved from "http://bridgeslab.sph.umich.edu/protocols/index.php?title=PCR_Analysis_of_Tail_DNA&oldid=1629"