{1473} revision 1 modified: 09-10-2019 01:42 gmt

PMID-17179937 Major signal increase in fluorescence microscopy through dark-state relaxation (2007)

  • 5-25x increase in fluorescence yields.
  • Idea: allow the (dark) triplet states to decay naturally by keeping inter-pulse intervals of illumination greater than 1us.
  • Works for both 1p and 2p.
  • For volume imaging via 2p, I don’t think that 1um decay time is much of an issue; revisit given fluorophores after >1ms!
  • Suggests again that transition from triplet dark state to excited higher state is a prominent or significant cause of photobleaching; also suggests that triple quenching will have limited utility in scanned or pulsed 2p systems (will have more utility in 1p systems, perhaps..)
  • Atto532 dye has low intersystem crossing to the triplet state (1%) [3,5,14] .. humm.
  • 2p total photon emission seems to flatten above 100GW/cm^2 intensity.
  • 2p absorption is easily saturated independent of pulse width: for short pulses, high intensity leads to absorption to T1 state, which has high cross-section to the Tn>1 state; longer pulses give more time for single-photon absorption.
  • τp by m = 200 and hence the pulse energy by 14-fold does not have a considerable effect on G2p. This obviously indicates that the saturation of the S0 → S1 or of the T1 → Tn > 1 excitation eliminates any dependence on pulse peak intensity or energy.