Correlative two-color two-photon (2C2P) excitation STED microscopy

Christoph Polzer; Stefan Ness; Mojtaba Mohseni; Thomas Kellerer; Markus Hilleringmann; Joachim Rädler; Thomas Hellerer

doi:10.1364/BOE.10.004516

Correlative two-color two-photon (2C2P) excitation STED microscopy

Biomed Opt Express. 2019 Aug 7;10(9):4516-4530. doi: 10.1364/BOE.10.004516. eCollection 2019 Sep 1.

Authors

Christoph Polzer^{1

2}, Stefan Ness³, Mojtaba Mohseni¹, Thomas Kellerer¹, Markus Hilleringmann³, Joachim Rädler², Thomas Hellerer¹

Affiliations

¹ Multiphoton Imaging Lab, Munich University of Applied Sciences, 80335 Munich, Germany.
² Faculty of Physics, Soft Condensed Matter, Ludwig-Maximilians-University, 80539 Munich, Germany.
³ FG Protein Biochemistry & Cellular Microbiology, University of Applied Sciences Munich, 80335 Munich, Germany.

Abstract

We present a two-color two-photon stimulated emission depletion microscopy technique (2C2P-STED) that correlates a confocal image with a super-resolved image employing the inherent self-referencing mechanism of nonlinear excitation. The novel approach overcomes the substantial challenge posed by two different imaging modalities in laser-scanning fluorescence microscopy for colocalization on the nanometer scale. Demonstrating the principle of 2C2P-STED, we show for the first time super-resolved images of the gram-positive bacteria Streptococcus pneumoniae TIGR4 pilus type-1. A signal-to-noise ratio (SNR) greater than 10 was achieved in 2C2P excitation mode and approximately 70 nm details were resolved in 2P-STED.