SummaryThis step is only part of Experiment A in the cDNA synthesis for serial analysis of gene expression. In Experiment B, the cDNA is already bound to the streptavidin-antibiotin-coated PCR tubes and therefore does not need to be bound with magnetic beads.
Modern Neuroscience Research Techniques
Author(s): U. Windhorst & H. Johansson Translator(s): Zhao Zhiqi Chen Jun
Operation method
Combined with magnetic bead experiments
Materials and Instruments
Magnetic Beads
Dynabead M-280 Streptavidin Antibiotics
Magnetic DevicesMove
Experimental program A - Shake for lmin to reconstitute the Dynabead M-280 Streptavidin anti-biotin into a suspension.
- Transfer 2X of 100 ul Dynabeads into U-unit 1.5 ml Eppendorf tubes.
- Fix the beads with a magnetic device and remove the supernatant.
- Resuspend the beads 3 times with 200 ul of IX Binding and Rinse Buffer, immobilize the beads, and remove the rinse solution.
- Divide the NlaIII digested cDNA into two 10ul portions, add 90ul of redistilled water and 100ul of 2X Binding and Flushing Buffer to each portion; add one portion of the rinsed beads to the mixture.
- After mixing, incubate at room temperature for 30 min (mixing every IOmin).
- The beads were immobilized with a magnetic device and the supernatant was discarded.
- Rinse the immobilized beads 3 times with 200ul of IX Binding and Rinse Buffer, then rinse once with 200ul of LoTE.
- After the last rinse, immobilize the beads and remove the LoTE.
- Proceed to step 5
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