Difference between revisions of "PCR for Bio113"

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(PCR Verification of Successful GGA)
 
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==PCR Verification of Successful GGA==
 
==PCR Verification of Successful GGA==
 
If you want to use PCR to verify that GGA has happened, you can amplify the plasmid DNA inside the cells you grew overnight. After PCR, you will need to analyze the PCR product (often called an amplicon) by gel electrophoresis (2.0% agarose gel).  
 
If you want to use PCR to verify that GGA has happened, you can amplify the plasmid DNA inside the cells you grew overnight. After PCR, you will need to analyze the PCR product (often called an amplicon) by gel electrophoresis (2.0% agarose gel).  
# For each PCR you want to perform on your eXperimental cells (e.g. X1, X2, X3), remove 10 µL of cells from the overnight culture. This will serve as your template.  
+
# For each PCR you want to perform on your eXperimental cells (e.g. X1, X2, X3), remove 2 µL of cells from the overnight culture. This will serve as your template.  
# Use 10 µL of negative control (N) cells as template to see the MW of the PCR product when no GGA has occurred.  
+
# Use 2 µL of negative control (N) cells as template to see the MW of the PCR product when no GGA has occurred.  
# Add the 10 µL of cell cultures to the labeled tubes for your particular receiving plasmid.  
+
# Add the 2 µL of cell cultures to the labeled tubes for your particular receiving plasmid.  
# The tubes already contain two primers (see list below) and the green GoTaq master mix that contains buffer, dNTPs and Taq DNA polymerase. The volume of this tube is currently 15 µL and will be 25 µL after you add the template cells.  
+
# The tubes already contain the paired PCR primers (see list below) and the green GoTaq master mix that includes buffer, dNTPs and Taq DNA polymerase. The volume of this tube is currently 23 µL and will be 25 µL after you add the template cells.  
 +
# Put your labeled tubes (treatment and group name) into the thermocycler. Your tubes will be incubated as follows:
  
 +
----
  
== PCR Primers to Confirm Successful GGA (Using Green GoTac DNA polymerase from Promega) ==
+
# 95° C for 5 minutes, 1 time
 +
# 95° C for 30 seconds
 +
# 54° C for 30 seconds
 +
#72° C for 30 seconds
 +
# return to step #2 29 more times
 +
# store at 22° C indefinitely
  
'''J119137; pClone Red  (remove 70 bp, insert <60 bp)'''<br>
+
* When the PCR is completed, they will be stored until next week when you will load 20 µL of each into the wells of a 2% agarose gel.
113_pClone_confirm_For; CTCCTCTTTAATTACTAGACGAC Tm = 60 C<br>
+
 
 +
== PCR Primers to Confirm Successful GGA (Using Green GoTac DNA polymerase from Promega) ==
 +
'''J119137; pClone Red  (remove 70 bp, insert <61 bp)'''<br>
 +
113_pClone_confirm_For (Same as 113_pClone_SeqFor); CTAATTCAACAAGAATTGGGAC Tm = 60 C<br>
 +
113_pClone_confirm_Rev; AAGTGAACTTGGGCCC Tm = 62 C<br>
 +
177 bp amplicon for J119137<br>
 +
167 bp amplicon for 60 bp insertion<br>
 +
<br>
 +
<br>
 +
'''J100384; pClone mScarlet  (remove 70 bp, insert <61 bp)'''<br>
 +
113_pClone_confirm_For (Same as 113_pClone_SeqFor); CTAATTCAACAAGAATTGGGAC Tm = 60 C<br>
 
113_pClone_confirm_Rev; AAGTGAACTTGGGCCC Tm = 62 C<br>
 
113_pClone_confirm_Rev; AAGTGAACTTGGGCCC Tm = 62 C<br>
113 bp amplicon for J119137<br>
+
228 bp amplicon for J100384<br>
 +
220 bp amplicon for 60 bp insertion<br>
 
<br>
 
<br>
 
<br>
 
<br>
'''J119384; rClone Red  (remove 815 bp, insert <60 bp)'''<br>
+
'''J119384; rClone Red  (remove 819 bp, insert <61 bp)'''<br>
113_rClone_confirm_For; CTCGTAATTTATGTGGACGAC TM = 61 C<br>
+
113_rClone_confirm_For; CTCGTAATTTATGTGGACGAC Tm = 61 C<br>
 
113_rClone_confirm_Rev; TCGGAGGAAGCCATCTC Tm = 63 C<br>
 
113_rClone_confirm_Rev; TCGGAGGAAGCCATCTC Tm = 63 C<br>
 
856 bp amplicon for J119384<br>
 
856 bp amplicon for J119384<br>
 +
58 bp amplicon for 15 bp insertion <br>
 
<br>
 
<br>
 
<br>
 
<br>
'''J100204; actClone Red (remove 119 bp, insert <60 bp)'''<br>
+
'''J100419; rClone mScarlet  (remove 819 bp, insert <61 bp)'''<br>
 +
113_rClone_confirm_For; CTCGTAATTTATGTGGACGAC Tm = 61 C<br>
 +
113_mScarlet_Rev; CACTTTGAAGCGCATGAATTC Tm = 55 C<br>
 +
914 bp amplicon for J100419<br>
 +
95 bp amplicon for 15 bp insertion <br>
 +
<br>
 +
<br>
 +
<br>
 +
<br>
 +
<br>
 +
<br>
 +
 
 +
'''Previous plasmids used in 113'''<br>
 +
'''J100204; actClone Red (remove 119 bp, insert <61 bp)'''<br>
 
113_actClone_confirm_For; ACAGCTCTTCGCCTTTAC Tm = 62 C<br>
 
113_actClone_confirm_For; ACAGCTCTTCGCCTTTAC Tm = 62 C<br>
 
113_actClone_confirm_Rev; ATGCAGAATAATCCAACACG  Tm = 61 C<br>
 
113_actClone_confirm_Rev; ATGCAGAATAATCCAACACG  Tm = 61 C<br>
Line 27: Line 59:
 
<br>
 
<br>
 
<br>
 
<br>
'''J100205; repClone Red (remove 129 bp, insert <60 bp)'''<br>
+
'''J100205; repClone Red (remove 129 bp, insert <61 bp)'''<br>
113_repClone_confirm_For; ACAGCTCTTCGCCTTTAC Tm = 62 C<br>
+
113_repClone_confirm_For; CTCCTCTTTAATTACTAGACGAC Tm = 60 C<br>
113_repClone_confirm_Rev; GGTTTCTAATGGCTTCCTC Tm = 60 C<br>
+
113_repClone_confirm_Rev; CCTTCGTACGGACGACCTTC Tm = 58 C<br>
340 bp amplicon for J100205<br>
+
424 bp amplicon for J100205<br>
 
<br>
 
<br>
 
<br>
 
<br>

Latest revision as of 12:02, 15 September 2022

PCR Verification of Successful GGA

If you want to use PCR to verify that GGA has happened, you can amplify the plasmid DNA inside the cells you grew overnight. After PCR, you will need to analyze the PCR product (often called an amplicon) by gel electrophoresis (2.0% agarose gel).

  1. For each PCR you want to perform on your eXperimental cells (e.g. X1, X2, X3), remove 2 µL of cells from the overnight culture. This will serve as your template.
  2. Use 2 µL of negative control (N) cells as template to see the MW of the PCR product when no GGA has occurred.
  3. Add the 2 µL of cell cultures to the labeled tubes for your particular receiving plasmid.
  4. The tubes already contain the paired PCR primers (see list below) and the green GoTaq master mix that includes buffer, dNTPs and Taq DNA polymerase. The volume of this tube is currently 23 µL and will be 25 µL after you add the template cells.
  5. Put your labeled tubes (treatment and group name) into the thermocycler. Your tubes will be incubated as follows:

  1. 95° C for 5 minutes, 1 time
  2. 95° C for 30 seconds
  3. 54° C for 30 seconds
  4. 72° C for 30 seconds
  5. return to step #2 29 more times
  6. store at 22° C indefinitely
  • When the PCR is completed, they will be stored until next week when you will load 20 µL of each into the wells of a 2% agarose gel.

PCR Primers to Confirm Successful GGA (Using Green GoTac DNA polymerase from Promega)

J119137; pClone Red (remove 70 bp, insert <61 bp)
113_pClone_confirm_For (Same as 113_pClone_SeqFor); CTAATTCAACAAGAATTGGGAC Tm = 60 C
113_pClone_confirm_Rev; AAGTGAACTTGGGCCC Tm = 62 C
177 bp amplicon for J119137
167 bp amplicon for 60 bp insertion


J100384; pClone mScarlet (remove 70 bp, insert <61 bp)
113_pClone_confirm_For (Same as 113_pClone_SeqFor); CTAATTCAACAAGAATTGGGAC Tm = 60 C
113_pClone_confirm_Rev; AAGTGAACTTGGGCCC Tm = 62 C
228 bp amplicon for J100384
220 bp amplicon for 60 bp insertion


J119384; rClone Red (remove 819 bp, insert <61 bp)
113_rClone_confirm_For; CTCGTAATTTATGTGGACGAC Tm = 61 C
113_rClone_confirm_Rev; TCGGAGGAAGCCATCTC Tm = 63 C
856 bp amplicon for J119384
58 bp amplicon for 15 bp insertion


J100419; rClone mScarlet (remove 819 bp, insert <61 bp)
113_rClone_confirm_For; CTCGTAATTTATGTGGACGAC Tm = 61 C
113_mScarlet_Rev; CACTTTGAAGCGCATGAATTC Tm = 55 C
914 bp amplicon for J100419
95 bp amplicon for 15 bp insertion






Previous plasmids used in 113
J100204; actClone Red (remove 119 bp, insert <61 bp)
113_actClone_confirm_For; ACAGCTCTTCGCCTTTAC Tm = 62 C
113_actClone_confirm_Rev; ATGCAGAATAATCCAACACG Tm = 61 C
250 bp amplicon for J100204


J100205; repClone Red (remove 129 bp, insert <61 bp)
113_repClone_confirm_For; CTCCTCTTTAATTACTAGACGAC Tm = 60 C
113_repClone_confirm_Rev; CCTTCGTACGGACGACCTTC Tm = 58 C
424 bp amplicon for J100205