Griffitts:PCR: Difference between revisions

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<font size="5">PCR with ''Taq'' Polymerase</font>
<font size="5">PCR with ''Taq'' Polymerase</font>
__NOTOC__


==Procedure==
==Procedure==
* Prepare your template sample
* Prepare your template sample
** For amplifying rhizobium sequences, boil a dense suspension of cells in 35 μL [[Griffitts:Common buffers#colony lysis solution (for PCR) (100 mL)|PCR lysis buffer]] for ~2 min and vortex
** For amplifying ''Sinorhizobium'' sequences, boil a dense suspension of cells in 35 μL [[Griffitts:Common buffers#colony lysis solution (for PCR) (100 mL)|PCR lysis buffer]] for ~2 min and vortex
** For amplifying ''E. coli'', adding cells directly to the reaction is sufficient
** For amplifying ''E. coli'' with ''Taq'' polymerase (but not ''Pfx50'' polymerase), adding cells directly to the reaction is sufficient
* Thaw the ''Taq'' buffer, dNTPs, and primers
* Thaw the ''Taq'' buffer, dNTPs, and primers
** Keep ''Taq'' polymerase on ice throughout the procedure
** Keep ''Taq'' polymerase on ice throughout the procedure
* In standard PCR tube(s) combine components according to one of [[Griffitts:TaqPCR#Reaction recipes|the recipes below]]
* Combine components according to one of [[Griffitts:TaqPCR#Reaction recipes|the recipes below]]
** Set the reaction up on ice
** Set the reaction up on ice
* Select the appropriate cycling program and verify that all of the parameters are correct
* Select the appropriate cycling program and verify that all of the parameters are correct
** Allow 1 minute of extension time per 1 KB DNA being amplified
** Allow 1 minute of extension time per 1 KB DNA being amplified (15-30 seconds is sufficient for Q5)
* Select "Run program" and select "YES" when asked about heated lid
* Select "Run program" and select "YES" when asked about heated lid
* Wait until block has reached the beginning temperature. Place PCR tube into the machine
* Wait until block has reached at least 70°C (this takes a little over 2 min)
* Place PCR tube into the machine
* Lower the lid until it latches and slightly tighten the heated lid onto the tubes
* Lower the lid until it latches and slightly tighten the heated lid onto the tubes
NOTE: When the PCR machine has finished cycling, your samples may be stored at -20°C. You may now proceed to [[Griffitts:Gel_electrophoresis|gel electrophoresis]] and/or [[Griffitts:PCR_clean-up|PCR clean-up]].


==Reaction recipes==
==Reaction recipes==
===Standard recipe===
===20 μL ''Taq'' reactions===
Use this for 2 reactions
Use this for diagnostic purposes.
* 37 μL dH<sub>2</sub>O
{| border="1" cellpadding="5" cellspacing="0"
* 5 μL [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Taq'' buffer]]
|-
* 1 μL [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
! width="120" style="background:#efefef;" | Ingredient
* 0.4 μL ''Taq'' polymerase<br>
! width="120" style="background:#efefef;" | Per reaction
* 1 μL template
|-
* 3 μL forward primer
| dH<sub>2</sub>O
* 3 μL reverse primer
| 14.35 μL
Note: [[Griffitts:TaqPCR#Standard Primers|dilute the primers]] to 10X from the 100X stock in the freezer
|-
| [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Taq'' buffer]]
| 2.0 μL
|-
| [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
| 0.5 μL
|-
| ''Taq'' polymerase
| 0.15 μL
|-
| forward primer
| 1.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| reverse primer
| 1.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| DNA template
| 1.0 μL
|}
<br>


===Master Mix (without primers)===
===40 μL ''Taq'' reactions===
Use this for 3 to 4 reactions or reactions with multiple primer pairs<br>
This is the standard recipe. Use it in most cases for fragment amplification and sequencing.
Multiply by the number of reactions:
{| border="1" cellpadding="5" cellspacing="0"
* 40 μL dH<sub>2</sub>O
|-
* 5 μL [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Taq'' buffer]]
! width="120" style="background:#efefef;" | Ingredient
* 1 μL [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
! width="120" style="background:#efefef;" | Per reaction
* 0.4 μL ''Taq'' polymerase
|-
Add 46.4 μL to each PCR tube and use a [[Griffitts:TaqPCR#Primer Master Mix|Primer Master Mix]]<br>
| dH<sub>2</sub>O
| 28.7 μL
|-
| [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Taq'' buffer]]
| 4.0 μL
|-
| [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
| 1.0 μL
|-
| ''Taq'' polymerase
| 0.3 μL
|-
| forward primer
| 2.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| reverse primer
| 2.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| DNA template
| 2.0 μL
|}
<br>


===Master Mix (with primers)===
===40 μL reaction with ''Pfx'' polymerase===
Use this for 5 or more reactions with the same primer pairs<br>
Use this for high-fidelity cloning.
Multiply by the number of reactions:
{| border="1" cellpadding="5" cellspacing="0"
* 42.4 μL dH<sub>2</sub>O
|-
* 5 μL [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Taq'' buffer]]
! width="120" style="background:#efefef;" | Ingredient
* 1 μL [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
! width="120" style="background:#efefef;" | Per reaction
* 0.4 μL ''Taq'' polymerase
|-
* 0.3 μL forward primer
| dH<sub>2</sub>O
* 0.3 μL reverse primer
| 27 μL
Note: Use the 100X stock in the freezer (''don't'' dilute)<br>
|-
Add 49.4 μL to each PCR tube
| [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Pfx'' buffer]]
| 4.0 μL
|-
| [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
| 1.2 μL
|-
| ''Pfx'' polymerase
| 1.0 μL
|-
| forward primer
| 2.4 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| reverse primer
| 2.4 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| DNA template
| 2.0 μL
|}
<br>
 
===20 μL reaction with ''Q5'' polymerase===
Use this for high-fidelity cloning, especially for products >3kb.
{| border="1" cellpadding="5" cellspacing="0"
|-
! width="120" style="background:#efefef;" | Ingredient
! width="120" style="background:#efefef;" | Per reaction
|-
| dH<sub>2</sub>O
| 12.4 μL
|-
| [[Griffitss:Stock_solutions#5X_Q5_buffer|5X ''Q5'' buffer]]
| 4.0 μL
|-
| [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
| 0.4 μL
|-
| ''Q5'' polymerase
| 0.2 μL
|-
| forward primer
| 1.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| reverse primer
| 1.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| DNA template
| 1.0 μL
|}
<br>
 
===40 μL reaction with ''Q5'' polymerase===
Use this for high-fidelity cloning, especially for products >3kb.
{| border="1" cellpadding="5" cellspacing="0"
|-
! width="120" style="background:#efefef;" | Ingredient
! width="120" style="background:#efefef;" | Per reaction
|-
| dH<sub>2</sub>O
| 24.8 μL
|-
| [[Griffitss:Stock_solutions#5X_Q5_buffer|5X ''Q5'' buffer]]
| 8.0 μL
|-
| [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
| 0.8 μL
|-
| ''Q5'' polymerase
| 0.4 μL
|-
| forward primer
| 2.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| reverse primer
| 2.0 μL [[Griffitts:TaqPCR#Primer Dilution|diluted 1:10]]
|-
| DNA template
| 2.0 μL
|}
<br>
 
===Master Mix Calculations===
{| border="1" cellpadding="5" cellspacing="0"
|-
! width="200" style="background:#efefef;" | Ingredient
! width="150" style="background:#efefef;" | 20 μL reaction
with ''Taq'' polymerase
! width="150" style="background:#efefef;" | 40 μL reaction
with ''Taq'' polymerase
! width="150" style="background:#efefef;" | 40 μL reaction
with ''Pfx'' polymerase
! width="150" style="background:#efefef;" | 40 μL reaction
with ''Q5'' polymerase
|-
| dH<sub>2</sub>O
| 16.15 μL
| 32.3 μL
| 31.3 μL
| 24.8 μL
|-
| [[Griffitss:Stock_solutions#10X_Taq_buffer|10X ''Taq'' buffer]]
| 2.0 μL
| 4.0 μL
| 4.0 μL
| 8.0 μL
|-
| [[Griffitss:Stock_solutions#10_mM_DNTPs|dNTPs]]
| 0.5 μL
| 1.0 μL
| 1.2 μL
| 0.8 μL
|-
| polymerase
| 0.15 μL
| 0.3 μL
| 1.0 μL
| 0.4 μL
|-
| forward primer
| 0.1 μL ''undiluted''
| 0.2 μL ''undiluted''
| 0.25 μL ''undiluted''
| 0.2 μL ''undiluted''
|-
| reverse primer
| 0.1 μL ''undiluted''
| 0.2 μL ''undiluted''
| 0.25 μL ''undiluted''
| 0.2 μL ''undiluted''
|-
| '''Total volume (without template)'''
| '''19 μL'''
| '''38 μL'''
| '''38 μL'''
| '''38 μL'''
|}
<br>
<br>


==Primer Dilution==
==Primer Dilution==
===Standard Primers===
* 27 μL dH<sub>2</sub>O
* 27 μL dH<sub>2</sub>O
* 3 μL primer
* 3 μL primer
Repeat for both primers
Repeat for both primers
===Primer Master Mix===
* 24 μL dH<sub>2</sub>O
* 3 μL forward primer
* 3 μL reverse primer

Latest revision as of 16:02, 30 September 2013


PCR with Taq Polymerase

Procedure

  • Prepare your template sample
    • For amplifying Sinorhizobium sequences, boil a dense suspension of cells in 35 μL PCR lysis buffer for ~2 min and vortex
    • For amplifying E. coli with Taq polymerase (but not Pfx50 polymerase), adding cells directly to the reaction is sufficient
  • Thaw the Taq buffer, dNTPs, and primers
    • Keep Taq polymerase on ice throughout the procedure
  • Combine components according to one of the recipes below
    • Set the reaction up on ice
  • Select the appropriate cycling program and verify that all of the parameters are correct
    • Allow 1 minute of extension time per 1 KB DNA being amplified (15-30 seconds is sufficient for Q5)
  • Select "Run program" and select "YES" when asked about heated lid
  • Wait until block has reached at least 70°C (this takes a little over 2 min)
  • Place PCR tube into the machine
  • Lower the lid until it latches and slightly tighten the heated lid onto the tubes

NOTE: When the PCR machine has finished cycling, your samples may be stored at -20°C. You may now proceed to gel electrophoresis and/or PCR clean-up.

Reaction recipes

20 μL Taq reactions

Use this for diagnostic purposes.

Ingredient Per reaction
dH2O 14.35 μL
10X Taq buffer 2.0 μL
dNTPs 0.5 μL
Taq polymerase 0.15 μL
forward primer 1.0 μL diluted 1:10
reverse primer 1.0 μL diluted 1:10
DNA template 1.0 μL


40 μL Taq reactions

This is the standard recipe. Use it in most cases for fragment amplification and sequencing.

Ingredient Per reaction
dH2O 28.7 μL
10X Taq buffer 4.0 μL
dNTPs 1.0 μL
Taq polymerase 0.3 μL
forward primer 2.0 μL diluted 1:10
reverse primer 2.0 μL diluted 1:10
DNA template 2.0 μL


40 μL reaction with Pfx polymerase

Use this for high-fidelity cloning.

Ingredient Per reaction
dH2O 27 μL
10X Pfx buffer 4.0 μL
dNTPs 1.2 μL
Pfx polymerase 1.0 μL
forward primer 2.4 μL diluted 1:10
reverse primer 2.4 μL diluted 1:10
DNA template 2.0 μL


20 μL reaction with Q5 polymerase

Use this for high-fidelity cloning, especially for products >3kb.

Ingredient Per reaction
dH2O 12.4 μL
5X Q5 buffer 4.0 μL
dNTPs 0.4 μL
Q5 polymerase 0.2 μL
forward primer 1.0 μL diluted 1:10
reverse primer 1.0 μL diluted 1:10
DNA template 1.0 μL


40 μL reaction with Q5 polymerase

Use this for high-fidelity cloning, especially for products >3kb.

Ingredient Per reaction
dH2O 24.8 μL
5X Q5 buffer 8.0 μL
dNTPs 0.8 μL
Q5 polymerase 0.4 μL
forward primer 2.0 μL diluted 1:10
reverse primer 2.0 μL diluted 1:10
DNA template 2.0 μL


Master Mix Calculations

Ingredient 20 μL reaction

with Taq polymerase

40 μL reaction

with Taq polymerase

40 μL reaction

with Pfx polymerase

40 μL reaction

with Q5 polymerase

dH2O 16.15 μL 32.3 μL 31.3 μL 24.8 μL
10X Taq buffer 2.0 μL 4.0 μL 4.0 μL 8.0 μL
dNTPs 0.5 μL 1.0 μL 1.2 μL 0.8 μL
polymerase 0.15 μL 0.3 μL 1.0 μL 0.4 μL
forward primer 0.1 μL undiluted 0.2 μL undiluted 0.25 μL undiluted 0.2 μL undiluted
reverse primer 0.1 μL undiluted 0.2 μL undiluted 0.25 μL undiluted 0.2 μL undiluted
Total volume (without template) 19 μL 38 μL 38 μL 38 μL



Primer Dilution

  • 27 μL dH2O
  • 3 μL primer

Repeat for both primers

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