IGEM:MIT/2005/Input reception Experiments

Questions

 * 1) Is our fluorescein dimer entering into the cell?
 * 2) Distance in space between flurs. -- might depend on 3D conformation/wobblyness
 * 3) Separate out single from double stranded

Experiments

 * 1) Lets throw the oligos in, wash the media, look for flur. and we can hope that means its diffused
 * 2) * control: normal fluor. -- don't touch the oligos just yet
 * 3) * READOUT: can we see it under a microscope? get antibody -- into cytoplasm? selectivly trash outer membrane? will's oligo thingy?