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A window with a view: spying brain function at the two-photon microscope

What is two photon microscopy ? Sensing of brain structure and function in vivo Two photon spectroscopy in vivo: towards the quantitative measure of pH and [Cl]. A window with a view: spying brain function at the two-photon microscope.

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A window with a view: spying brain function at the two-photon microscope

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  1. Whatistwophotonmicroscopy? Sensingofbrainstructure and function in vivo Twophotonspectroscopy in vivo: towards the quantitative measureof pH and [Cl]. A window with a view: spying brain function at the two-photon microscope

  2. Neuroscience fordummies: whatis and whereis the brain

  3. Imaging in deeptissue: confocalmicroscopy Z

  4. Twophotons are more thanone t = 0.1 fs (1 10-16 s) ≈ 3 108 m → 3 1014µm/s 0.03 µm

  5. 2 photon vs. 1-photon excitation

  6. Dependency of total fluorescence as a function of z Fluorescent spheres 0.2 mm (m)

  7. A windowwith a view

  8. A trip into the brain

  9. Spine motility in the juvenilecortex (SSctx, p25) 0 min 30 min 60 min

  10. Watching the brain in operation Functional imaging of the brainwith single cellresolution

  11. Watching a mouse brain that is watching TV

  12. Watching the brain in operation pH and Clhoride imaging in vivo

  13. Excitation and inhibition in the brain + - + - + + +

  14. The space and timeresolvedmeasureof Cl gradientsis the key tounderstandinhibition in the brain -85 mV +60 mV

  15. NerstpotentialforChloride

  16. NerstpotentialforChloride

  17. NerstpotentialforChloride

  18. ClopHensor λecc=543 nm λecc=543 nm λecc=458 nm λecc=488 nm +H+ O- Ka +Cl- Kd OH Static quenching OH Cl- Arosio et al. Nature Meth. 2010.

  19. Gradients of intracellular Chloride 042 043 048 049 050 054 053 058

  20. A newhope: E2-mKate A newsensorformedby the fusionof E2GFP with the Red proteinmKate

  21. ExcitingpropertiesofmKateexcitation

  22. How to evaluate the integrity of the bi-molecular sensor? The correct measure of Cl concentration requires that the ratio between red and green fuorescent proteins is equal to 1. If we can demonstrate that the protein remains in the correct conformation, with the green and red proteins attached, the stechiometry is ensured.

  23. G/R @458nm exc FCS 0 2

  24. G/R @458nm exc FCS 0 2

  25. 5 s 60 s 240 s Measuring the shuttlingbetweennucleus and cytoplasm pre-bleach

  26. 5 s 60 s 240 s Measuring the shuttlingbetweennucleus and cytoplasm pre-bleach Fun facts about N/C shuttling: proteins with MW<30kD freely diffuse between these two compartments. Larger MW are associated to a very slow turnover

  27. 5 s 60 s 240 s We can use the nuclear membrane as a molecularsievetomeasure the sizeof the fluorescentproteins! pre-bleach

  28. In vivo FRAP measure in cortical neurons Pre bleach

  29. Recovery of fluorescence of YFP

  30. Diffusion of CloPhensor is strongly limited

  31. Linear spectralcompositionformeasuringcells pH pH 8.0 pH 6.0

  32. Houston, wehave a problem…

  33. IMG_0823

  34. Effects of excitation scattering on the spectra 770 800 830 860 890 920 950 980

  35. Unmixing the E2-mKate spectra R(l) = Rrfp(l) + aGsensor(l) G(l) = Gsensor + b Rrfp(l)

  36. In vivo mouse cortex P4 P18

  37. Road mapto pH and Cl computation Spectralunmixingof R and G channels Useof the pH/Cl invariant R channeltocomputeexcitationscattering Correctionof G channelforexcitationscattering Projectionof the corrected G spectra on the referencespectra: pH computation

  38. Looking at the redraw data

  39. Comparing the effectsofspectracorrections

  40. Comparing the effectsofspectracorrections

  41. Computing pH in vivo (p18)

  42. Sum ofresiduesallows a statistical test of the data treatment

  43. Computing pH in vivo (p18)

  44. What about extinction of the emitted light? Cl measure depends on an equally efficient collection of the fluorescence emitted at the green and red channels. Sadly, in a few seconds, I will provide evidences, that that is not the case We can build a model for differential extinction to correct the data. Or…

  45. Modeling extinction of emitted fluorescence

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