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Team:Warsaw/SyntheticCloning/SyntheticCloning
From 2011.igem.org
(Difference between revisions)
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<li>After 12 hours of amplification DNA can be used in downstream processing</li> | <li>After 12 hours of amplification DNA can be used in downstream processing</li> | ||
</ul> | </ul> | ||
| - | + | <br> | |
| - | + | This is our protocol: | |
<ul> | <ul> | ||
<li>1. Digest insert and vector with Fermentas Fast enzymes</li> | <li>1. Digest insert and vector with Fermentas Fast enzymes</li> | ||
| + | <ul> | ||
<li>insert with XBAI and at the same time add CIAP(Digest 1: 3ul reaction buffer; 1restriction enzyme; 5 ul DNA; 20ul water and 1ul CIAP), deactivate enzymes at 65C for 20 min, then digest insert with PSTI(simply add 1ul of the enzyme).</li> | <li>insert with XBAI and at the same time add CIAP(Digest 1: 3ul reaction buffer; 1restriction enzyme; 5 ul DNA; 20ul water and 1ul CIAP), deactivate enzymes at 65C for 20 min, then digest insert with PSTI(simply add 1ul of the enzyme).</li> | ||
<li>vector with PSTI and at the same time add CIAP(Digest 1: 3ul reaction buffer; 1restriction enzyme; 5 ul DNA; 20ul water and 1ul CIAP), deactivate enzymes at 80C 20 min, then digest insert with SPEI(simply add 1ul of the enzyme)</li> | <li>vector with PSTI and at the same time add CIAP(Digest 1: 3ul reaction buffer; 1restriction enzyme; 5 ul DNA; 20ul water and 1ul CIAP), deactivate enzymes at 80C 20 min, then digest insert with SPEI(simply add 1ul of the enzyme)</li> | ||
| - | <li> Prepare Lithium-botare agarose gel | + | </ul> |
| - | we use 300-400V and gel is ready in 15 minutes. Theoretically maximum you can use is max. 100V/cm, but we never tried that much.</li> | + | <li> Prepare Lithium-botare agarose gel. Gels in LB buffer can be can run on much higher voltage |
| + | we use 300-400V and gel is ready in 15 minutes. Theoretically maximum you can use is max. 100V/cm, but we never tried that much. <ul><li>(1L 20 times concentrated LB gel buffer =>950 mL of dH2O, 8.392 g lithium hydroxide monohydrate; 36 g of boric acid; pH 8.2. Volume to 1 L)</li></ul></li> | ||
| + | |||
<li>Run the DNA on the gel and extract insert and vector</li> | <li>Run the DNA on the gel and extract insert and vector</li> | ||
<li>Ligate:7 ul H20; 5 ul insetr; 5 ul vector; 2 ul buffer; 0.5 ul Ligase incubate for 15 min at 25C</li> | <li>Ligate:7 ul H20; 5 ul insetr; 5 ul vector; 2 ul buffer; 0.5 ul Ligase incubate for 15 min at 25C</li> | ||
<li>Perform exonuclease digestion (2,5 recBCD exonuclease buffer; 2ul ATP; 1ul recBCD (Epicentre) ; 1 exonuclease I (Fermentas); 1 ul ligation mixture; 17,5 h20. Inactivate the reaction at 80C for 20 min</li> | <li>Perform exonuclease digestion (2,5 recBCD exonuclease buffer; 2ul ATP; 1ul recBCD (Epicentre) ; 1 exonuclease I (Fermentas); 1 ul ligation mixture; 17,5 h20. Inactivate the reaction at 80C for 20 min</li> | ||
| + | |||
</ul> | </ul> | ||
| + | An excelent protocol on how to perform cell-free cloning is available here: <a href="http://www.biotechniques.com/multimedia/archive/00051/BTN_A_000113155_O_51382a.pdf" target="_blank">Takahashi H, Yamamoto K, Ohtani T, Sugiyama S. <i>Cell-free cloning using multiply-primed rolling circle amplification with modified RNA primers.</i> Biotechniques. 2009 Jul.</a> | ||
</div> | </div> | ||
<br> | <br> | ||
Revision as of 21:50, 20 September 2011
Step by step guide to synthetic cloning
Rationale behind the protocol
- 1. Cut DNA with one of the enzyme you want to use in cloning
- 2. Dephosphorylate 5' phosphate - this prevents DNA pieces from self-ligation
- 3. Cut DNA with the other of the enzyme you want to use in cloning
- 4. Run DNA on the gel
- 5. Extract vector and insert from the gel.
- 6. Ligate
- 7. After ligation some linear DNA may still remain, you can get rid of it by using recBCD exonuclease and Exonuclease I
- Linear DNA is a perfect template for RCR amplification with phi 29 polymerase. It generates the long linear concatamers of the DNA from circular templates.
- After 12 hours of amplification DNA can be used in downstream processing
This is our protocol:
- 1. Digest insert and vector with Fermentas Fast enzymes
- insert with XBAI and at the same time add CIAP(Digest 1: 3ul reaction buffer; 1restriction enzyme; 5 ul DNA; 20ul water and 1ul CIAP), deactivate enzymes at 65C for 20 min, then digest insert with PSTI(simply add 1ul of the enzyme).
- vector with PSTI and at the same time add CIAP(Digest 1: 3ul reaction buffer; 1restriction enzyme; 5 ul DNA; 20ul water and 1ul CIAP), deactivate enzymes at 80C 20 min, then digest insert with SPEI(simply add 1ul of the enzyme)
- Prepare Lithium-botare agarose gel. Gels in LB buffer can be can run on much higher voltage
we use 300-400V and gel is ready in 15 minutes. Theoretically maximum you can use is max. 100V/cm, but we never tried that much.
- (1L 20 times concentrated LB gel buffer =>950 mL of dH2O, 8.392 g lithium hydroxide monohydrate; 36 g of boric acid; pH 8.2. Volume to 1 L)
- Run the DNA on the gel and extract insert and vector
- Ligate:7 ul H20; 5 ul insetr; 5 ul vector; 2 ul buffer; 0.5 ul Ligase incubate for 15 min at 25C
- Perform exonuclease digestion (2,5 recBCD exonuclease buffer; 2ul ATP; 1ul recBCD (Epicentre) ; 1 exonuclease I (Fermentas); 1 ul ligation mixture; 17,5 h20. Inactivate the reaction at 80C for 20 min
Results of the cell-free cloning
