Team:Alberta/Project/BeadBindingCapacity
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<li>Set up a set of microcentrifuge tubes with 10, 20, 30, 40, 50, 60, 70, 80 μL of 4 mg mL<sup>-1</sup> beads dispensed into the respectively labelled tubes. | <li>Set up a set of microcentrifuge tubes with 10, 20, 30, 40, 50, 60, 70, 80 μL of 4 mg mL<sup>-1</sup> beads dispensed into the respectively labelled tubes. | ||
<li>Wash the beads twice with 100 μL Wash/Binding buffer and once with 100 μL water, then aspirate water off the beads. | <li>Wash the beads twice with 100 μL Wash/Binding buffer and once with 100 μL water, then aspirate water off the beads. | ||
- | <li> | + | <li>Prepare 4 μL of the 20 μM Anchor solution to separate tubes (corresponding to which bead-containing tube they will be added to) along with enough water to bring the final solution volume up to half the dispensed bead volume. (i.e. to the 40 μL tube add 4 μL Anchor + 16 μL water). |
+ | <li>Add half of this solution to the tubes containing the washed beads. Retain the other half. | ||
+ | <li>Suspend the beads in the DNA solution. | ||
<li>Let bind at room temperature for 10 minutes. | <li>Let bind at room temperature for 10 minutes. | ||
- | <li>Take readings at A<sub>260</sub> with a UV-Vis Spectrophotometer of the | + | <li>Pellet the beads with a magnet and aspirate the solution. |
+ | <li>Take readings at A<sub>260</sub> with a UV-Vis Spectrophotometer of the DNA solutions prior to binding to bead (the half you retained) and after binding to bead (the aspirated solution). (ng of DNA can also be found by in-gel band intensity quantification methods) | ||
<li>Convert DNA measurements to pmol and plot pmol DNA versus mg of beads. The slope gives the binding capacity | <li>Convert DNA measurements to pmol and plot pmol DNA versus mg of beads. The slope gives the binding capacity | ||
</ul> | </ul> |
Revision as of 17:35, 21 October 2009
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Anchor Binding CapacityWhat you will need:
Binding Capacity
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