Q5® Hot Start High-Fidelity 2X Master Mix
PCR Hot start PCR - Mammalian DNA
Protocol tips
| Upstream tips |
|---|
| Amplicon size should be consistent for each target sequence and limited to approximately 65 - 100 bp. |
| Protocol tips |
| Always thaw on ice |
Publication protocol
General methodsDNA amplification was conducted by PCR using Phusion U Green Multiplex PCR Master Mix (ThermoFisher Scientific) or Q5 Hot Start High-Fidelity 2× Master Mix (New England BioLabs) unless otherwise noted. All mammalian cell and bacterial plasmids generated in this work were assembled using the USER cloning method as previously described39 and starting material gene templates were synthetically accessed as either bacterial or mammalian codon-optimized gBlock Gene Fragments (Integrated DNA Technologies). All sgRNA expression plasmids were constructed by a 1-piece blunt-end ligation of a PCR product containing a variable 20-nt sequence corresponding to the desired sgRNA targeted site. Primers and templates used in the synthesis of all sgRNA plasmids used in this work are listed in Supplementary Table 5. All mammalian ABE constructs, sgRNA plasmids and bacterial constructs were transformed and stored as glycerol stocks at −80°C in Mach1 T1R Competent Cells (Thermo Fisher Scientific), which are recA−. Molecular Biology grade, Hyclone water (GE Healthcare Life Sciences) was used in all assays and PCR reactions. All vectors used in evolution experiments and mammalian cell assays were purified using ZympPURE Plasmid Midiprep (Zymo Research Corportion), which includes endotoxin removal. Antibiotics used for either plasmid maintenance or selection during evolution were purchased from Gold Biotechnology.
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Discussion
Discussion
4 years ago
Author:
When should I add the polymerase for hot start PCR?
I keep getting a non-specific band in PCR so I would like to try a hot start PCR manually. How should I prepare the mix and at which step should I be adding the polymerase?
Discussion
4 years ago
Author:
Janina Reinhardt
Hot start PCR using phusion green DNA polymerase
I am currently performing hot start PCR using phusion green hot start DNA polymerase in order to amplify a 8.8kb insert. However, I cannot get any amplified product at all. I have tried changing some parameters but I am not sure what to do. Any help?
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Manufacturer protocol
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