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| - | {{:Team:EPF-Lausanne/Template/Header}} | + | <noinclude>{{:Team:EPF-Lausanne/Template/Header}}</noinclude> |
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| - | Quick and dirty digestion protocol for DNA that has concentrations on the order of 80ng - 30ng / microliter | + | <noinclude>{{:Team:EPF-Lausanne/Template/SetTitle|Quick and Dirty Digestion for DNA that has concentrations around 80-30 ng/µl}}</noinclude> |
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| - | Since nanodrop concentration results for pcr and samples extracted from gels have proved unreliable we have arrived at a sort of default protocol for DNA of an uncertain concentration.
| + | {{:Team:EPF-Lausanne/Template/ProtocolHeader|Quick and Dirty Digestion|{{{1|}}}}} |
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| - | For a ligation or when large quantities of DNA are needed.
| + | Since Nanodrop concentration results for PCR and samples extracted from gels have proved unreliable, we have arrived at a sort of a default protocol for DNA of an uncertain concentration. |
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| - | *DNA 15 microliters | + | For a ligation or when large quantities of DNA are needed: |
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| | + | *DNA 15 microliters |
| | *Restriction enzyme 1 @ 100x 1 microliters | | *Restriction enzyme 1 @ 100x 1 microliters |
| | *Restriction enzyme 2 @ 100x 1 microliters | | *Restriction enzyme 2 @ 100x 1 microliters |
| - | *BSA (if needed) @ 10x 5 microliter | + | *BSA (if needed) @ 10 x 5 microliters |
| | *Demineralized water 28 microliters | | *Demineralized water 28 microliters |
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| - | For checking restriction site presence on a gel. | + | For checking the presence of a restriction site on a gel: |
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| | *DNA 5 microliters | | *DNA 5 microliters |
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| | *Demineralized water 38 microliters | | *Demineralized water 38 microliters |
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| - | The total volume should be 50ⷧⷧ microliters | + | The total volume should be 50 microliters |
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| - | Incubation should ideally be at 37 C. When in doubt on the quantity of DNA used, favor a longer (20 to 30 minutes longer) incubation time than what is indicated on the NEB double digest guide. Avoid enzyme pairs with different incubation temperatures. This doubles the incubation time. | + | Incubation should ideally be at 37°C. When in doubt on the quantity of DNA used, favor a longer (20 to 30 minutes longer) incubation time than what is indicated on the NEB double digest guide. Avoid enzyme pairs with different incubation temperatures. This doubles the incubation time. |
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| - | After the incubation period the enzymes need to be heat inactivated. Heat inactivation temperatures are usually on the order of 80 C. 20 minutes usually does the job. | + | After the incubation period, the enzymes need to be heat-inactivated. Heat inactivation temperatures are usually on the order of 80 C. 20 minutes usually does the job. |
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| | The samples can then be frozen if needed. | | The samples can then be frozen if needed. |
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| - | {{:Team:EPF-Lausanne/Template/Footer}} | + | |
| | + | {{:Team:EPF-Lausanne/Template/ProtocolFooter}} |
| | + | <noinclude>{{:Team:EPF-Lausanne/Template/Footer}}</noinclude> |
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