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Team:UFAM Brazil/Protocol7
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Make sure that:</p> | Make sure that:</p> | ||
| - | <p style="margin-left: | + | <p style="margin-left:50px">• The final concentration of BSA and buffer is 1x.</p> |
| - | <p style="margin-left: | + | <p style="margin-left:50px">• 5 to 10 enzyme’s unit are necessary for 1 µg plasmidial DNA digest.</p> |
| - | <p style="margin-left: | + | <p style="margin-left:50px">• Add to digest system the quantity of DNA enough for 0.5 – 1 µg. If the system will be purified from the agarose gel lately, add quantity of DNA for the digest system of 1 – 2 µg.</p> |
<p>2. Pipet aliquots to each sample tube and add DNA.</p> | <p>2. Pipet aliquots to each sample tube and add DNA.</p> | ||
Revision as of 14:09, 16 October 2014
BioBrick Restriction Digest | ||
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Reagents: - dsH2O; - 10x Buffer (1 – 2 – 3 – 4); - 10x BSA; - Restriction Enzymes (EcoRI, Xbal, SpeI, PstI); - DNA. Steps: 1. Make a master mix with everything except the DNA. Make sure that: • The final concentration of BSA and buffer is 1x. • 5 to 10 enzyme’s unit are necessary for 1 µg plasmidial DNA digest. • Add to digest system the quantity of DNA enough for 0.5 – 1 µg. If the system will be purified from the agarose gel lately, add quantity of DNA for the digest system of 1 – 2 µg. 2. Pipet aliquots to each sample tube and add DNA. 3. Incubate at 37°C for 2 – 3 hours. Check the eletrophorectic profile. | ||
| Methods | ||
