Barrick Lab :: MEGAWHOP

---+ Megaprimer whole plasmid cloning
aka <nop>MEGAWHOP cloning %BR%
aka Overlap Extension PCR cloning

Adapted from Bryksin AV, Matsumura I. 2010. Overlap extension PCR Cloning: a simple and reliable way to create recombinant plasmids. _Biotechniques_.48(6):463-5.

---++ Purpose
To insert a DNA sequence into a plasmid without restriction enzymes.

---++ Experimental Steps

   * Create primers that amplify region of interest and hybridize with target plasmid
   * Perform a Phusion PCR with primers using the region of interest as template
   * Perform a second Phusion PCR using the products of the first PCR and the target plasmid as template
   * Digest Second PCR with Dpn1 to remove parental plasmid
   * Transform in _E coli_

     <img src="%ATTACHURLPATH%/genome_mod_figure.JPG" alt="genome_mod_figure.JPG" width='763' height='146' />


---++ Designing Primers
   <img src="%ATTACHURLPATH%/primers.png" alt="primers.png" width='374' height='204' />

Primers need to have two components
   * a region that amplifies the insert (A(or B), 20-25nt)
   * a region that targets the new plasmid (C(or D), 30-40nt)

The target plasmid regions should preferably be 50-200nt apart (C to D).

Order (A+C) primer and (B+D) primer.

---++ PCR Insert
Use stardard 25ul Phusion (or other high fidelity polymerase) protocol
   * PCR 1(25ul reaction)
   * 5 ul 5x Buffer
   * 1.5 ul  dntps
   * 1.25 ul primer (A+C)
   * 1.25 ul primer (B+D)
   * x ul template plasmid (<250ng)
   * ddH20 to 24.5 ul
   * then add 0.5 ul Phusion

Set elongation time according to size of insert.

Purify PCR products. This can either be done through a gel extraction or by adding Dpn1 directly to the Phusion reaction mixture after PCR, digesting at 37°C for 1 hour, and then doing a standard PCR clean up. Dpn1 works efficiently in a Phusion reaction mixture. 

---++ PCR Recombinant Plasmid
Use modified 10ul Phusion (or other high fidelity polymerase) protocol 
   * 2 ul 5x Buffer
   * 1 ul  dntps
   * 500 ng PCR insert product (Note, for optimal results, have a 250-fold molar excess of your megaprimer to your target plasmid).
   * ~10 ng  target plasmid
   * ddH20 to 9.5 ul
   * then add 0.5 ul Phusion

Adjust Elongation time for the length of the entire plasmid (90 seconds per kb). 

OR


Use modified 25ul Phusion protocol 
   * 5 ul 5x Buffer
   * 0.5 ul  dntps 
   * 1 ul  DMSO
   * 100 ng PCR insert product 
   * 25 ng  target plasmid
   * ddH20 to 25 ul
   * then add 0.25 ul Phusion

68°C 5min+98°C 3min+(98°C 30s+68°C 30s+72°C X min)*30 +72°C 10min
Adjust Elongation time for the length of the entire plasmid (30 seconds per kb). 

---++ Digest 
Once the reaction is complete, digest the Recombinant Plasmid PCR product with 0.5 ul Dpn1 at 37°C for one and a half hours to remove parental DNA. [[ProtocolsDpnIDigestion][DpnI Digest]]
---++ Transform
Heatshock 5ul of the Dpn1-digested MEGAWHOP reaction mixture into 25ul of chemically competent _E coli_.

  
---++ Example
Change the promoter for sgRNA using MegaWHOP.

Template sequence: https://benchling.com/s/g4S95i24

Primers: 
   * T5-sgRNA-F: 5' CCGATAATTGCAGACGAACG cgcccttcccaacagttgcc3'
   * T5-sgRNA-R:5' TATTCTGGTGGAACTGGATG tgaatctattataattgtt  3'

UPCASE LETTERS: a region that amplifies the insert (A(or B)

lower case letters:  a region that targets the new plasmid (C(or D)

   *PCR MEGA_primer: <br />
     <img src="%ATTACHURLPATH%/MEGA_primer.png" alt="MEGA_primer.png" width='277' height='241.5' />

   *PCR Recombinant Plasmid: <br />
     <img src="%ATTACHURLPATH%/Recombinant_Plasmid.png" alt="Recombinant_Plasmid.png" width='222' height='235.2' />
This topic: Lab > WebHome > ProtocolList > MEGAWHOP
Topic revision: r9 - 2016-12-15 - PengGeng