Jennifer-M. Masch scite author profile

SignificanceIn vivo fluorescence microscopy with resolution well beyond the diffraction limit entails complexities that challenge the attainment of sufficient image brightness and contrast. These challenges have so far hampered investigations of the nanoscale distributions of synaptic proteins in the living mouse. Here, we describe a combination of stimulated emission depletion microscopy and endogenous protein labeling, providing high-quality in vivo data of the key scaffolding protein PSD95 at the postsynaptic membrane, which frequently appeared in extended distributions rather than as isolated nanoclusters. Operating in the far-red to near-IR wavelength range, this combination promises reduced photostress compared with prior in vivo nanoscopy at much shorter wavelengths.

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Resection of Calcified Aortic Heart Leaflets In Vitro by Q-Switched 2 µm Microsecond Laser Radiation

Rohde

Masch

Theisen-Kunde³

et al. 2014

J Card Surg

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Cardiovascular damage after cw and Q-switched 2μm laser irradiation

Rohde

Masch

Theisen-Kunde

et al. 2013

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Jennifer-M. Masch

Robust nanoscopy of a synaptic protein in living mice by organic-fluorophore labeling

Resection of Calcified Aortic Heart Leaflets In Vitro by Q-Switched 2 µm Microsecond Laser Radiation

Cardiovascular damage after cw and Q-switched 2μm laser irradiation

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