Single-objective high-resolution confocal light sheet fluorescence microscopy for standard biological sample geometries.
Stoyan YordanovKonstantin NeuhausRaimo HartmannFrancisco Díaz-PascualLucia VidakovicPraveen K SinghKnut DrescherPublished in: Biomedical optics express (2021)
Three-dimensional fluorescence-based imaging of living cells and organisms requires the sample to be exposed to substantial excitation illumination energy, typically causing phototoxicity and photobleaching. Light sheet fluorescence microscopy dramatically reduces phototoxicity, yet most implementations are limited to objective lenses with low numerical aperture and particular sample geometries that are built for specific biological systems. To overcome these limitations, we developed a single-objective light sheet fluorescence system for biological imaging based on axial plane optical microscopy and digital confocal slit detection, using either Bessel or Gaussian beam shapes. Compared to spinning disk confocal microscopy, this system displays similar optical resolution, but a significantly reduced photobleaching at the same signal level. This single-objective light sheet technique is built as an add-on module for standard research microscopes and the technique is compatible with high-numerical aperture oil immersion objectives and standard samples mounted on coverslips. We demonstrate the performance of this technique by imaging three-dimensional dynamic processes, including bacterial biofilm dispersal, the response of biofilms to osmotic shocks, and macrophage phagocytosis of bacterial cells.
Keyphrases
- high resolution
- single molecule
- living cells
- energy transfer
- high speed
- mass spectrometry
- tandem mass spectrometry
- optical coherence tomography
- fluorescent probe
- pseudomonas aeruginosa
- candida albicans
- adipose tissue
- staphylococcus aureus
- cystic fibrosis
- label free
- oxidative stress
- escherichia coli
- photodynamic therapy
- cell death
- biofilm formation