Your search keyword '"selective plane illumination microscopy"' showing total 46 results

1. Mirror-assisted light-sheet microscopy: a simple upgrade to enable bi-directional sample excitation.

Author

Zylbertal, Asaph and Bianco, Isaac H.

Abstract

Significance: Light-sheet microscopy is a powerful imaging technique that achieves optical sectioning via selective illumination of individual sample planes. However, when the sample contains opaque or scattering tissues, the incident light sheet may not be able to uniformly excite the entire sample. For example, in the context of larval zebrafish whole-brain imaging, occlusion by the eyes prevents access to a significant portion of the brain during common implementations using unidirectional illumination. Aim: We introduce mirror-assisted light-sheet microscopy (mLSM), a simple inexpensive method that can be implemented on existing digitally scanned light-sheet setups by adding a single optical element--a mirrored micro-prism. The prism is placed near the sample to generate a second excitation path for accessing previously obstructed regions. Approach: Scanning the laser beam onto the mirror generates a second, reflected illumination path that circumvents the occlusion. Online tuning of the scanning and laser power waveforms enables near uniform sample excitation with dual illumination. Results: mLSM produces cellular-resolution images of zebrafish brain regions inaccessible to unidirectional illumination. The imaging quality in regions illuminated by the direct or reflected sheet is adjustable by translating the excitation objective. The prism does not interfere with visually guided behavior. Conclusions: mLSM presents an easy-to-implement, cost-effective way to upgrade an existing light-sheet system to obtain more imaging data from a biological sample. [ABSTRACT FROM AUTHOR]

Published

2024

2. Beyond Early Development: Observing Zebrafish over 6 Weeks with Hybrid Optical and Optoacoustic Imaging.

Author

Vetschera, Paul, Koberstein‐Schwarz, Benno, Schmitt‐Manderbach, Tobias, Dietrich, Christian, Hellmich, Wibke, Chekkoury, Andrei, Symvoulidis, Panagiotis, Reber, Josefine, Westmeyer, Gil, López‐Schier, Hernán, Omar, Murad, and Ntziachristos, Vasilis

Subjects

*BRACHYDANIO, *OPTICAL images, *HYBRID systems, *DRUG discovery, *FUNCTIONAL genomics, *MICROSCOPY, *DEVELOPMENTAL biology

Abstract

Zebrafish are common model organisms in developmental biology, but have recently emerged as imaging targets of research in cancer, tissue regeneration, metabolic disorders, functional genomics, and phenotype‐based drug discovery. Conventionally, zebrafish are studied during the first few days of development using optical microscopy methods. However, optical methods are not suited for imaging at later stages, since the fish become opaque. To address needs to visualize beyond the first days of development, a novel multimodality system for observing zebrafish from larval stage to adulthood is developed. Using a hybrid platform for concurrent selective plane illumination microscopy (SPIM) and optoacoustic mesoscopy, fish (ex vivo) at stages of development up to 47 days at a similar object size‐to‐resolution ratio are imaged. Using multiple wavelength illumination over the visible and short‐wavelength infrared regions, it is demonstrated that the optoacoustic method can follow GFP‐based contrast used in SPIM, enabling molecular imaging interrogation in adult fish. Moreover, the optoacoustic modality reveals zebrafish features based on optical contrast absent in SPIM, including contrast from endogenous blood, water, and lipids. It is discussed how the hybrid system method can enable the study of zebrafish in a wider range of applications and over time‐scales not possible currently when using optical microscopy. [ABSTRACT FROM AUTHOR]

Published

2023

3. Imaging the developing human external and internal urogenital organs with light sheet fluorescence microscopy.

Author

Isaacson, Dylan, McCreedy, Dylan, Calvert, Meredith, Shen, Joel, Sinclair, Adriane, Cao, Mei, Li, Yi, McDevitt, Todd, Cunha, Gerald, and Baskin, Laurence

Subjects

Urogenital System, Humans, Imaging, Three-Dimensional, Microscopy, Fluorescence, Specimen Handling, Image Processing, Computer-Assisted, CLARITY, Genital development, Light sheet fluorescence microscopy, Microscopy, Selective plane illumination microscopy, Urogenital development, Urologic Diseases, Pediatric, Biochemistry and Cell Biology, Paediatrics and Reproductive Medicine, Developmental Biology

Abstract

Technological advances in three-dimensional (3D) reconstruction techniques have previously enabled paradigm shifts in our understanding of human embryonic and fetal development. Light sheet fluorescence microscopy (LSFM) is a recently-developed technique that uses thin planes of light to optically section whole-mount cleared and immunolabeled biologic specimens. The advent of commercially-available light sheet microscopes has facilitated a new generation of research into protein localization and tissue dynamics at extremely high resolution. Our group has applied LSFM to study developing human fetal external genitalia, internal genitalia and kidneys. This review describes LSFM and presents our group's technique for preparing, clearing, immunostaining and imaging human fetal urogenital specimens. We then present light sheet images and videos of each element of the developing human urogenital system. To the extent of our knowledge, the work conducted by our laboratory represents the first description of a method for performing LSFM on the full human urogenital system during the embryonic and fetal periods.

Published

2020

4. Tracing uptake, biodistribution and efficacy of NanoDrugs in aquatic organisms using advanced imaging

Author

Windell, D., Tyler, C., Owen, S., and Moger, J.

Subjects

Gold Nanoparticles, Light sheet, Nanodrugs, Selective Plane Illumination Microscopy, Zebrafish, Nanotoxicology, Ecotoxicology, Microscopy

Abstract

Gold nanoparticles (AuNPs) are increasingly being used in biomedicine for enhancing drug delivery and facilitating imaging, as well as directly in applications such as cancer photothermal therapy. Despite this, very little is known about their potential impacts on the environment. Importantly, the effectiveness of AuNPs in such applications depends on a range of particle specifications that have been optimised during development to serve their specific purpose. The manipulations include their size and the addition of coatings, usually to enhance biocompatibility. How these different particle characteristics affect their bioavailability and biological effects on wildlife once released into the environment, has received very little research attention. Consequently, the main aims of this thesis were to investigate, principally via imaging methods, how the characteristics of size and surface coatings of gold nanoparticle (AuNP) affected bioavailability, tissue distribution and potential for toxicity using zebrafish (Danio rerio) as an experimental model. To undertake this work, a second major objective of the thesis work was to construct an imaging platform to trace the uptake and biodistribution of the gold nanoparticles. For this, I constructed an open source selective-plane illumination microscopy system (OpenSPIM) which allowed me to quantitatively trace fluorescently tagged AuNPs in exposed zebrafish embryos with relatively high-throughput. Applying SPIM through multiple angles, the fluorescence tag on the AuNPs was detectable throughout the zebrafish embryo body enabling concentration-response uptake analyses. Having built the OpenSPIM system from the ground up, careful method developments were undertaken to optimise the SPIM which included the imaging of multiple transgenic models of zebrafish such as the MPO:GFP model with fluorescent neutrophils, the elavl3:GCaMP6s utilised in chapter 6 to measure neural activity, and the casper model which was utilised in all uptake studies. Studies into the toxicity of the AuNPs were carried out with models for detecting assess oxidative stress responses in the 3EpRE:hsp70:mCherry model (using the Zeiss inverted microscope) and the pod::NTR-mCherry/l-fabp::VDBP-GFP model to assess for damage to the pronephric glomerular filtration barrier (using the EVOS fluorescent microscope). The OpenSPIM system was applied to image uptake and distribution of quantum dots (CdTe) in the casper model which indicated minimal uptake in the entire zebrafish embryo. Extensive oxidative stress was detected for exposures to aqueous levels of CdTe QDs down to 10 µg/L in the lateral line neuromasts, fionocytes and pronephros (undeveloped kidney) but there were no effects to the glomerular filtration barrier. Aqueous exposure to AuNPs illustrated a size selective uptake with the highest uptake for 40-80 nm AuNPs across a size range between 10 to 100 nm. This was principally found accumulating in the pronephros and gut with some fluorescence visualised in the heart. The effect of AuNP functionalisation on uptake in the casper model demonstrated varied levels of uptake depending on surface modification. Modifications of the AuNPs resulted in enhanced uptake levels for coatings with PEG and TNFα but not for NHS/PAMAM where there was decreased uptake. Depuration studies with all AuNP studies indicated that the AuNPs were cleared (but not completely) from the zebrafish embryos over a period of 4 days. No toxic effects were seen in any study with AuNP exposure in concentrations that exceed environmentally relevant doses (2 mg/L). This body of work illustrates the utility of SPIM for detecting the uptake and fate of selected NPs in exposed fish embryos. When combined with transgenic models that allow for functional analyses across specific tissue targets and effect mechanisms, thus providing a powerful tool for nanoparticle screening. Finer level details relating to the biological effects of NPs, however, require imaging methods that allow for sub-cellular resolution to analyse cell mechanics and how NPs influence cellular functions.

Published

2019

5. High-speed light-sheet fluorescent microscopy with an adaptive three-dimensional region-of-signal identification method.

Author

Wang, Dongyue, Hu, Huijie, Lu, Jing, and Gao, Liang

Subjects

*MICROSCOPY, *THREE-dimensional imaging, *DATA warehousing, *SPINAL cord, *SPATIAL resolution

Abstract

• Take a rough scan before imaging at each ROI for analyzing signal region. • The longitudinal distribution is analyzed to acquire the signal region result. • The overall imaging time is drastically decreased without losing signal. • Only software modifications on the original microscopy are needed. • Easy to be applied to other microscopy techniques. Light-sheet fluorescent microscopy (LSFM) is a crucial 3D imaging technique for tissues with advantages in high 3D spatial resolution, effective optical sectioning, and quick imaging. Prior to imaging, the sample's imaging depth, imaging region, and region of interest (ROI) division should all be established in accordance with the sample's outermost dimensions. However, because biological samples are inherently irregular a traditional imaging flow that images ROI by ROI, slice by slice, would waste a great deal of time and data storage space by additionally recording non-signal regions. In order to solve this problem, we create a high-speed LSFM with an adaptive three-dimensional region-of-signal identification method (RSI). We immediately perform crude imaging for each ROI before the software analyzes the longitudinal distribution and, ultimately, uses dimensionality reduction, binarization, filtering, and redundancy expansion to acquire the signal region result. By imaging two mouse spinal cord segments with a total of 170 ROIs and 180 ROIs on two channels, respectively, the high-speed imaging capability is validated. Our method reduced the overall imaging time and raw data size by more than treble and 14 times, respectively, without losing signal. With a programmable imaging range based on the real signal region, this method offers an efficient tool for flexible light-sheet microscopy. It can also be applied to other microscopy techniques to speed up imaging. [ABSTRACT FROM AUTHOR]

Published

2024

6. Single Molecule Imaging in Live Embryos Using Lattice Light-Sheet Microscopy

Author

Mir, Mustafa, Reimer, Armando, Stadler, Michael, Tangara, Astou, Hansen, Anders S, Hockemeyer, Dirk, Eisen, Michael B, Garcia, Hernan, and Darzacq, Xavier

Subjects

Genetics, Biotechnology, Underpinning research, 1.1 Normal biological development and functioning, Generic health relevance, Animals, Data Analysis, Drosophila melanogaster, Embryo, Mammalian, Embryo, Nonmammalian, Mice, Microscopy, Fluorescence, Reproducibility of Results, Single Molecule Imaging, Single molecule imaging, Single molecule kinetics, Lattice light-sheet microscopy, Live embryo imaging, Single molecule fluorescence, Transcription factor dynamics, Single particle tracking, Selective plane illumination microscopy, Other Chemical Sciences, Biochemistry and Cell Biology, Developmental Biology

Abstract

In the past decade, live-cell single molecule imaging studies have provided unique insights on how DNA-binding molecules such as transcription factors explore the nuclear environment to search for and bind to their targets. However, due to technological limitations, single molecule experiments in living specimens have largely been limited to monolayer cell cultures. Lattice light-sheet microscopy overcomes these limitations and has now enabled single molecule imaging within thicker specimens such as embryos. Here we describe a general procedure to perform single molecule imaging in living Drosophila melanogaster embryos using lattice light-sheet microscopy. This protocol allows direct observation of both transcription factor diffusion and binding dynamics. Finally, we illustrate how this Drosophila protocol can be extended to other thick samples using single molecule imaging in live mouse embryos as an example.

Published

2018

7. Multispectral imaging for characterizing autofluorescent tissues

Author

Universidad de Alicante. Departamento de Física, Ingeniería de Sistemas y Teoría de la Señal, Universidad Carlos III de Madrid. Departamento de Bioingeniería, Instituto de Investigación Sanitaria Gregorio Marañón, Centro de Investigación Biomédica en Red de Salud Mental (CIBERSAM), Centro Nacional de Investigaciones Cardiovasculares Carlos III (CNIC), Bentahar, Sara, Gómez-Gaviro, María Victoria, Desco, Manuel, Ripoll, Jorge, Fernandez, Roberto, Universidad de Alicante. Departamento de Física, Ingeniería de Sistemas y Teoría de la Señal, Universidad Carlos III de Madrid. Departamento de Bioingeniería, Instituto de Investigación Sanitaria Gregorio Marañón, Centro de Investigación Biomédica en Red de Salud Mental (CIBERSAM), Centro Nacional de Investigaciones Cardiovasculares Carlos III (CNIC), Bentahar, Sara, Gómez-Gaviro, María Victoria, Desco, Manuel, Ripoll, Jorge, and Fernandez, Roberto

Abstract

Selective Plane Illumination Microscopy (SPIM) has become an emerging technology since its first application for 3D in-vivo imaging of the development of a living organism. An extensive number of works have been published, improving both the speed of acquisition and the resolution of the systems. Furthermore, multispectral imaging allows the effective separation of overlapping signals associated with different fluorophores from the spectrum over the whole field-of-view of the analyzed sample. To eliminate the need of using fluorescent dyes, this technique can also be applied to autofluorescence imaging. However, the effective separation of the overlapped spectra in autofluorescence imaging necessitates the use of mathematical tools. In this work, we explore the application of a method based on Principal Component Analysis (PCA) that enables tissue characterization upon spectral autofluorescence data without the use of fluorophores. Thus, enabling the separation of different tissue types in fixed and living samples with no need of staining techniques. Two procedures are described for acquiring spectral data, including a single excitation based method and a multi-excitation scanning approach. In both cases, we demonstrate the effective separation of various tissue types based on their unique autofluorescence spectra.

Published

2024

8. Multiview tiling light sheet microscopy for 3D high-resolution live imaging.

Author

Aakhte, Mostafa and Müller, Hans-Arno J.

Subjects

*MICROSCOPY, *SPATIAL resolution, *NUCLEAR shapes, *MYOSIN, *DROSOPHILA

Abstract

Light-sheet or selective plane illumination microscopy (SPIM) is ideally suited for in toto imaging of living specimens at high temporal--spatial resolution. In SPIM, the light scattering that occurs during imaging of opaque specimens brings about limitations in terms of resolution and the imaging field of view. To ameliorate this shortcoming, the illumination beam can be engineered into a highly confined light sheet over a large field of view and multi-view imaging can be performed by applying multiple lenses combined with mechanical rotation of the sample. Here, we present a Multiview tiling SPIM (MT-SPIM) that combines the Multi-view SPIM (M-SPIM) with a confined, multi-tiled light sheet. The MT-SPIM provides high-resolution, robust and rotation-free imaging of living specimens. We applied the MT-SPIM to image nuclei and Myosin II from the cellular to subcellular spatial scale in early Drosophila embryogenesis. We show that the MT-SPIM improves the axial-resolution relative to the conventional M-SPIM by a factor of two. We further demonstrate that this axial resolution enhancement improves the automated segmentation of Myosin II distribution and of nuclear volumes and shapes. [ABSTRACT FROM AUTHOR]

Published

2021

9. Large-scale characterization of the microvascular geometry in development and disease by tissue clearing and quantitative ultramicroscopy.

Author

Hahn, Artur, Bode, Julia, Alexander, Allen, Karimian-Jazi, Kianush, Schregel, Katharina, Schwarz, Daniel, Sommerkamp, Alexander C, Krüwel, Thomas, Abdollahi, Amir, Wick, Wolfgang, Platten, Michael, Bendszus, Martin, Tews, Björn, Kurz, Felix T, and Breckwoldt, Michael O

Abstract

Three-dimensional assessment of optically cleared, entire organs and organisms has recently become possible by tissue clearing and selective plane illumination microscopy ("ultramicroscopy"). Resulting datasets can be highly complex, encompass over a thousand images with millions of objects and data of several gigabytes per acquisition. This constitutes a major challenge for quantitative analysis. We have developed post-processing tools to quantify millions of microvessels and their distribution in three-dimensional datasets from ultramicroscopy and demonstrate the capabilities of our pipeline within entire mouse brains and embryos. Using our developed acquisition, segmentation, and analysis platform, we quantify physiological vascular networks in development and the healthy brain. We compare various geometric vessel parameters (e.g. vessel density, radius, tortuosity) in the embryonic spinal cord and brain as well as in different brain regions (basal ganglia, corpus callosum, cortex). White matter tract structures (corpus callosum, spinal cord) showed lower microvascular branch densities and longer vessel branch length compared to grey matter (cortex, basal ganglia). Furthermore, we assess tumor neoangiogenesis in a mouse glioma model to compare tumor core and tumor border. The developed methodology allows rapid quantification of three-dimensional datasets by semi-automated segmentation of fluorescently labeled objects with conventional computer hardware. Our approach can aid preclinical investigations and paves the way towards "quantitative ultramicroscopy". [ABSTRACT FROM AUTHOR]

Published

2021

10. Wnt3 Is Lipidated at Conserved Cysteine and Serine Residues in Zebrafish Neural Tissue

Author

Divya Dhasmana, Sapthaswaran Veerapathiran, Yagmur Azbazdar, Ashwin Venkata Subba Nelanuthala, Cathleen Teh, Gunes Ozhan, and Thorsten Wohland

Subjects

Wnt3, zebrafish, fluorescence correlation spectroscopy, fluorescence cross-correlation spectroscopy, selective plane illumination microscopy, FCS diffusion law, Biology (General), QH301-705.5

Abstract

Wnt proteins are a family of hydrophobic cysteine-rich secreted glycoproteins that regulate a gamut of physiological processes involved in embryonic development and tissue homeostasis. Wnt ligands are post-translationally lipidated in the endoplasmic reticulum (ER), a step essential for its membrane targeting, association with lipid domains, secretion and interaction with receptors. However, at which residue(s) Wnts are lipidated remains an open question. Initially it was proposed that Wnts are lipid-modified at their conserved cysteine and serine residues (C77 and S209 in mWnt3a), and mutations in either residue impedes its secretion and activity. Conversely, some studies suggested that serine is the only lipidated residue in Wnts, and substitution of serine with alanine leads to retention of Wnts in the ER. In this work, we investigate whether in zebrafish neural tissues Wnt3 is lipidated at one or both conserved residues. To this end, we substitute the homologous cysteine and serine residues of zebrafish Wnt3 with alanine (C80A and S212A) and investigate their influence on Wnt3 membrane organization, secretion, interaction and signaling activity. Collectively, our results indicate that Wnt3 is lipid modified at its C80 and S212 residues. Further, we find that lipid addition at either C80 or S212 is sufficient for its secretion and membrane organization, while the lipid modification at S212 is indispensable for receptor interaction and signaling.

Published

2021

11. Development of digital fluorescence light sheet microscopy for high-resolution optical imaging

Author

Aakhte, Mostafa

Subjects

light sheet microscopy, Fluoreszenzmikroskopie, 3D-Technologie, drosophila embryo, Mikroskopie, selective plane illumination microscopy, developmental biology, SPIM, Lichtscheibenmikroskopie, Entwicklungsbiologie, Drosophila, structured illumination, tiling light sheet microscopy

Published

2022

12. Detection of Single Quantum Dots in Model Systems with Sheet Illumination Microscopy.

Author

Friedrich, Mike, Nozadze, Revaz, de Keijzer, Sandra, Steinmeyer, Ralf, Ermolayev, Vladimir, and Harms, Gregory S.

Subjects

*MICROSCOPY, *CONFOCAL microscopy, *BIOMOLECULES, *NANOCRYSTALS, *FLUORESCENCE

Abstract

Single molecule detection and tracking provides at times the only possible method to observe the interactions of low numbers of biomolecules, inlcuding DNA, receptors and signal mediating proteins in living systems. However, most existing imaging methods do not enable both high sensitivity and non-invasive imaging of large specimens. In this study we report a new setup for selective plane illumination microscopy (SPIM), which enables fast imaging and single molecule tracking with the resolution of confocal microscopy and the optical penetration beyond 300 μm. We detect and report our instrumental figures of merit, control values of fluorescence properties of single nano crystals in comparison to both standard widefield configurations, and also values of nanocrystals in multicellular “fruiting bodies” of Dictyostelium, an excellent control as a model developmental system. In the Dictyostelium, we also report some of our first tracking of single nanocrystals with SPIM. The new SPIM setup represents a new technique, which enables fast single molecule imaging and tracking in living systems. [ABSTRACT FROM AUTHOR]

Published

2018

13. Low-cost optofluidic add-on enables rapid selective plane illumination microscopy of C. elegans with a conventional wide-field microscope

Author

Mehran Behrouzi, Khaled Youssef, Pouya Rezai, and Nima Tabatabaei

Subjects

Paper, Microscopy, Biomedical Engineering, microfluidics, 01 natural sciences, Atomic and Molecular Physics, and Optics, Electronic, Optical and Magnetic Materials, 010309 optics, Biomaterials, optofluidic, selective plane illumination microscopy, light-sheet fluorescence microscopy, Cross-Sectional Studies, 0103 physical sciences, C. elegans, Animals, Caenorhabditis elegans, organism-on-a-chip, Lighting

Abstract

Significance: Selective plane illumination microscopy (SPIM) is an emerging fluorescent imaging technique suitable for noninvasive volumetric imaging of C. elegans. These promising microscopy systems, however, are scarce in academic and research institutions due to their high cost and technical complexities. Simple and low-cost solutions that enable conversion of commonplace wide-field microscopes to rapid SPIM platforms promote widespread adoption of SPIM by biologist for studying neuronal expressions of C. elegans. Aim: We sought to develop a simple and low-cost optofluidic add-on device that enables rapid and immobilization-free volumetric SPIM imaging of C. elegans with conventional fluorescent microscopes. Approach: A polydimethylsiloxane (PDMS)-based device with integrated optical and fluidic elements was developed as a low-cost and miniaturized SPIM add-on for the conventional wide-field microscope. The developed optofluidic chip contained an integrated PDMS cylindrical lens for on-chip generation of the light-sheet across a microchannel. Cross-sectional SPIM images of C. elegans were continuously acquired by the native objective of microscope as worms flowed in an L-shape microchannel and through the light sheet. Results: On-chip SPIM imaging of C. elegans strains demonstrated possibility of visualizing the entire neuronal system in few seconds at single-neuron resolution, with high contrast and without worm immobilization. Volumetric visualization of neuronal system from the acquired cross-sectional two-dimensional images is also demonstrated, enabling the standard microscope to acquire three-dimensional fluorescent images of C. elegans. The full-width at half-maximum width of the point spread function was measured as 1.1 and 2.4 μm in the lateral and axial directions, respectively. Conclusion: The developed low-cost optofluidic device is capable of continuous SPIM imaging of C. elegans model organism with a conventional fluorescent microscope, at high speed, and with single neuron resolution.

Published

2021

14. miniSPIM-A Miniaturized Light-Sheet Microscope

Author

Per Niklas Hedde

Subjects

three-dimensional imaging, Microscope, Materials science, Optical sectioning, particle detection, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Bioengineering, Article, law.invention, fluorescence fluctuation spectroscopy, Software portability, chemistry.chemical_compound, Imaging, Three-Dimensional, law, Animals, bacteria detection, Instrumentation, Zebrafish, Fluid Flow and Transfer Processes, image correlation spectroscopy, business.industry, Process Chemistry and Technology, Nile red, Characterization (materials science), Autofluorescence, selective plane illumination microscopy, chemistry, Microscopy, Fluorescence, Light sheet fluorescence microscopy, optical sectioning, Optoelectronics, Smartphone, business, Biosensor, light-sheet microscopy

Abstract

The miniSPIM is a miniaturized light-sheet microscope that enables imaging with optical sectioning on mobile camera devices such as smartphones and single-board computers. Applications of the miniSPIM include biosensing, field research, and education where maximum portability and robustness, low power consumption, and low cost are key. Here, it is shown how all of the components of a simple light-sheet microscope can be integrated within a footprint smaller than the average smartphone. Example applications include the quantification of the motion of microparticles and bacteria in fluids, the characterization of solvent polarity based on spectral shifts of the lipid probe Nile Red, and three-dimensional (3D) and time-lapse autofluorescence imaging of a live zebrafish embryo.

Published

2021

15. A combined light sheet fluorescence and differential interference contrast microscope for live imaging of multicellular specimens.

Author

BAKER, R.P., TAORMINA, M.J., JEMIELITA, M., and PARTHASARATHY, R.

Subjects

*FLUORESCENCE, *OPTICAL interference, *MICROSCOPY, *ZEBRA danio, *LIGHTING

Abstract

We describe a microscope capable of both light sheet fluorescence microscopy and differential interference contrast microscopy (DICM). The two imaging modes, which to the best of our knowledge have not previously been combined, are complementary: light sheet fluorescence microscopy provides three-dimensional imaging of fluorescently labelled components of multicellular systems with high speed, large fields of view, and low phototoxicity, whereas differential interference contrast microscopy reveals the unlabelled neighbourhood of tissues, organs, and other structures with high contrast and inherent optical sectioning. Use of a single Nomarski prism for differential interference contrast microscopy and a shared detection path for both imaging modes enables simple integration of the two techniques in one custom microscope. We provide several examples of the utility of the resulting instrument, focusing especially on the digestive tract of the larval zebrafish, revealing in this complex and heterogeneous environment anatomical features, the behaviour of commensal microbes, immune cell motions, and more. [ABSTRACT FROM AUTHOR]

Published

2015

16. Vertically scanned laser sheet microscopy.

Author

Di Dong, Arranz, Alicia, Shouping Zhu, Yujie Yang, Liangliang Shi, Jun Wang, Chen Shen, Jie Tian, and Ripoll, Jorge

Subjects

*LASER microscopy, *FLUORESCENCE, *SCATTERING (Physics), *LIGHTING, *LASERS

Abstract

Laser sheet microscopy is a widely used imaging technique for imaging the three-dimensional distribution of a fluorescence signal in fixed tissue or small organisms. In laser sheet microscopy, the stripe artifacts caused by high absorption or high scattering structures are very common, greatly affecting image quality. To solve this problem, we report here a two-step procedure which consists of continuously acquiring laser sheet images while vertically displacing the sample, and then using the variational stationary noise remover (VSNR) method to further reduce the remaining stripes. Images from a cleared murine colon acquired with a vertical scan are compared with common stitching procedures demonstrating that vertically scanned light sheet microscopy greatly improves the performance of current light sheet microscopy approaches without the need for complex changes to the imaging setup and allows imaging of elongated samples, extending the field of view in the vertical direction. [ABSTRACT FROM AUTHOR]

Published

2014

17. A Versatile Oblique Plane Microscope for Large-Scale and High-Resolution Imaging of Subcellular Dynamics - Public Data

Author

Sapoznik, Etai, Chang, Bo-Jui, Huh, Jaewon, Ju, Robert, Azarova, Evgenia V., Pohlkamp, Theresa, Welf, Erik S., Broadbent, David, Carisey, Alexandre F., Stehbens, Samantha J., Lee, Kyung-Min, Marin, Arnoldo, Hanker, Ariella B., Schmidt, Jens C., Arteaga, Carlos L., Yang, Bin, Koboyashi, Yoshihiko, Tata, Purushothama R., Kruithoff, Rory, Doubrovinski, Konstantin, Shepherd, Doug P., York, Andrew G., Millet-Sikking, Alfred, Dean, Kevin M., and Fiolka, Reto P.

Subjects

Selective plane illumination microscopy, Light-sheet microscopy, Oblique plane microscopy

Abstract

We present an Oblique Plane Microscope that uses a bespoke glass-tipped tertiary objective to improve the resolution, field of view, and usability over previous variants. Owing to its high numerical aperture optics, this microscope achieves lateral and axial resolutions that are comparable to the square illumination mode of Lattice Light-Sheet Microscopy, but in a user friendly and versatile format. Given this performance, we demonstrate high-resolution imaging of clathrin-mediated endocytosis, vimentin, the endoplasmic reticulum, membrane dynamics, and Natural Killer-mediated cytotoxicity. Furthermore, we image biological phenomena that would be otherwise challenging or impossible to perform in a traditional light-sheet microscope geometry, including cell migration through confined spaces within a microfluidic device, subcellular photoactivation of Rac1, diffusion of cytoplasmic rheological tracers at a volumetric rate of 14 Hz, and large field of view imaging of neurons, developing embryos, and centimeter-scale tissue sections.

Published

2020

18. Large-scale characterization of the microvascular geometry in development and disease by tissue clearing and quantitative ultramicroscopy

Author

Daniel Schwarz, Michael O. Breckwoldt, Michael Platten, Allen Alexander, Felix T. Kurz, Björn Tews, Katharina Schregel, Thomas Krüwel, Artur Hahn, Julia Bode, Martin Bendszus, Kianush Karimian-Jazi, Alexander C Sommerkamp, Amir Abdollahi, and Wolfgang Wick

Subjects

Male, Mice, SCID, Biology, Grey matter, Corpus callosum, White matter, 03 medical and health sciences, Mice, angiogenesis, 0302 clinical medicine, Imaging, Three-Dimensional, Mice, Inbred NOD, Cortex (anatomy), Basal ganglia, medicine, Animals, Segmentation, Ultramicroscopy, 030304 developmental biology, 0303 health sciences, Microscopy, Tissue clearing, Neovascularization, Pathologic, Brain, Glioma, Original Articles, Spinal cord, microvascular networks, selective plane illumination microscopy, medicine.anatomical_structure, clearing, Neurology, Microvessels, Neurology (clinical), Cardiology and Cardiovascular Medicine, 030217 neurology & neurosurgery, Biomedical engineering

Abstract

Three-dimensional assessment of optically cleared, entire organs and organisms has recently become possible by tissue clearing and selective plane illumination microscopy (“ultramicroscopy”). Resulting datasets can be highly complex, encompass over a thousand images with millions of objects and data of several gigabytes per acquisition. This constitutes a major challenge for quantitative analysis. We have developed post-processing tools to quantify millions of microvessels and their distribution in three-dimensional datasets from ultramicroscopy and demonstrate the capabilities of our pipeline within entire mouse brains and embryos. Using our developed acquisition, segmentation, and analysis platform, we quantify physiological vascular networks in development and the healthy brain. We compare various geometric vessel parameters (e.g. vessel density, radius, tortuosity) in the embryonic spinal cord and brain as well as in different brain regions (basal ganglia, corpus callosum, cortex). White matter tract structures (corpus callosum, spinal cord) showed lower microvascular branch densities and longer vessel branch length compared to grey matter (cortex, basal ganglia). Furthermore, we assess tumor neoangiogenesis in a mouse glioma model to compare tumor core and tumor border. The developed methodology allows rapid quantification of three-dimensional datasets by semi-automated segmentation of fluorescently labeled objects with conventional computer hardware. Our approach can aid preclinical investigations and paves the way towards “quantitative ultramicroscopy”.

Published

2020

19. Imaging the developing human external and internal urogenital organs with light sheet fluorescence microscopy

Author

Mei Cao, Todd C. McDevitt, Meredith E. K. Calvert, Gerald R. Cunha, Laurence S. Baskin, Dylan Isaacson, Adriane Sinclair, Yi Li, Joel Shen, and Dylan A. McCreedy

Subjects

0301 basic medicine, Internal genitalia, Urologic Diseases, Cancer Research, Microscope, Image Processing, Urogenital development, High resolution, Urogenital System, Biology, Fluorescence, law.invention, Imaging, Specimen Handling, Paediatrics and Reproductive Medicine, 03 medical and health sciences, Imaging, Three-Dimensional, 0302 clinical medicine, Computer-Assisted, law, Microscopy, Image Processing, Computer-Assisted, Humans, Molecular Biology, Pediatric, Light sheet fluorescence microscopy, Cell Biology, 030104 developmental biology, Selective plane illumination microscopy, Microscopy, Fluorescence, Genital development, External genitalia, CLARITY, Human fetal, Three-Dimensional, Biochemistry and Cell Biology, 030217 neurology & neurosurgery, Clearance, Biomedical engineering, Developmental Biology

Abstract

Technological advances in three-dimensional (3D) reconstruction techniques have previously enabled paradigm shifts in our understanding of human embryonic and fetal development. Light sheet fluorescence microscopy (LSFM) is a recently-developed technique that uses thin planes of light to optically section whole-mount cleared and immunolabeled biologic specimens. The advent of commercially-available light sheet microscopes has facilitated a new generation of research into protein localization and tissue dynamics at extremely high resolution. Our group has applied LSFM to study developing human fetal external genitalia, internal genitalia and kidneys. This review describes LSFM and presents our group's technique for preparing, clearing, immunostaining and imaging human fetal urogenital specimens. We then present light sheet images and videos of each element of the developing human urogenital system. To the extent of our knowledge, the work conducted by our laboratory represents the first description of a method for performing LSFM on the full human urogenital system during the embryonic and fetal periods.

Published

2020

20. Phase Retrieval for Hidden Tomography Reconstruction

Author

Asier Marcos Vidal, Stella Avtzi, Diego Di Battista, Giannis Zacharakis, Daniele Ancora, and Andrea Bassi

Subjects

Computer science, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Computed tomography, 02 engineering and technology, 01 natural sciences, 010309 optics, Speckle patterns, 0103 physical sciences, medicine, Computer vision, Three dimensional reconstruction, Tomography, Phase retrieval, Tomographic reconstruction, medicine.diagnostic_test, business.industry, Autocorrelation, 3D reconstruction, Random media, Computed tomography,Phase retrieval,Selective plane illumination microscopy,Speckle patterns,Three dimensional reconstruction,Tomography, 021001 nanoscience & nanotechnology, Selective plane illumination microscopy, Artificial intelligence, 0210 nano-technology, Focus (optics), business

Abstract

We discuss the problem of tomographic reconstruction of fluorescent objects hidden behind random media. To accomplish this, we focus on the properties of the autocorrelation, relying on phase retrieval algorithms to perform 3D reconstruction.

Published

2020

21. Fluorescent tags to explore cell wall structure and dynamics.

Author

Martine eGonneau, Herman eHöfte, and Samantha eVernhettes

Subjects

fluorescence microscopy, plant cell-wall, spinning disk microscopy, variable-angle epifluorescence microscopy, selective plane illumination microscopy, Plant culture, SB1-1110

Abstract

Plant cell walls are highly dynamic and heterogeneic structures, which vary between celltypes, growth stages but also between microdomains within a single cell wall. In this review, we summarize the imaging techniques using fluorescent tags that are currently being used and which should in the coming years revolutionize our understanding of the dynamics of cell wall architecture and the cellular processes involved in synthesis of cell wall components.

Published

2012

22. Lightsheet Microscopy.

Author

Dyer L, Parker A, Paphiti K, and Sanderson J

Subjects

Animals, Mice, Microscopy, Fluorescence methods, Imaging, Three-Dimensional methods, Lighting methods

Abstract

In this paper, we review lightsheet (selective plane illumination) microscopy for mouse developmental biologists. There are different means of forming the illumination sheet, and we discuss these. We explain how we introduced the lightsheet microscope economically into our core facility and present our results on fixed and living samples. We also describe methods of clearing fixed samples for three-dimensional imaging and discuss the various means of preparing samples with particular reference to mouse cilia, adipose spheroids, and cochleae. © 2022 The Authors. Current Protocols published by Wiley Periodicals LLC., (© 2022 The Authors. Current Protocols published by Wiley Periodicals LLC.)

Published

2022

23. A global 'imaging'' view on systems approaches in immunology.

Author

Ludewig, Burkhard, Stein, Jens V., Sharpe, James, Cervantes-Barragan, Luisa, Thiel, Volker, and Bocharov, Gennady

Abstract

The immune system exhibits an enormous complexity. High throughput methods such as the '-omic'' technologies generate vast amounts of data that facilitate dissection of immunological processes at ever finer resolution. Using high-resolution data-driven systems analysis, causal relationships between complex molecular processes and particular immunological phenotypes can be constructed. However, processes in tissues, organs, and the organism itself (so-called higher level processes) also control and regulate the molecular (lower level) processes. Reverse systems engineering approaches, which focus on the examination of the structure, dynamics and control of the immune system, can help to understand the construction principles of the immune system. Such integrative mechanistic models can properly describe, explain, and predict the behavior of the immune system in health and disease by combining both higher and lower level processes. Moving from molecular and cellular levels to a multiscale systems understanding requires the development of methodologies that integrate data from different biological levels into multiscale mechanistic models. In particular, 3D imaging techniques and 4D modeling of the spatiotemporal dynamics of immune processes within lymphoid tissues are central for such integrative approaches. Both dynamic and global organ imaging technologies will be instrumental in facilitating comprehensive multiscale systems immunology analyses as discussed in this review. [ABSTRACT FROM AUTHOR]

Published

2012

24. Analysis of properties of single molecules in vivo or ... why small fish is better than empty dish.

Author

Korzh, Vladimir and Wohland, Thorsten

Subjects

*BIOMOLECULES, *SPECTRUM analysis, *MOLECULES, *PROTEINS, *ORGANIC compounds

Abstract

The article analyzes single molecules properties in vivo using single molecule techniques (SMT). It mentions that the SMT based research faces challenges due to maturation of fluorescent proteins, and bleaching of fluorescent proteins. Further it focuses on the application of SMT for analysis of developmental processes that include Fluorescent Correlation Spectroscopy (FCS), Total Internal Reflection Fluorescence (TIRF), and Single Plane Illumination Microscopy (SPIM).

Published

2012

25. Detection of single quantum dots in model organisms with sheet illumination microscopy

Author

Friedrich, Mike, Nozadze, Revaz, Gan, Qiang, Zelman-Femiak, Monika, Ermolayev, Vladimir, Wagner, Toni U., and Harms, Gregory S.

Subjects

*QUANTUM dots, *FISH development, *FISH embryos, *LABORATORY zebrafish, *ANIMAL models in research, *NANOCRYSTALS, *DROSOPHILA, *INSECT larvae

Abstract

Abstract: Single-molecule detection and tracking is important for observing biomolecule interactions in the microenvironment. Here we report selective plane illumination microscopy (SPIM) with single-molecule detection in living organisms, which enables fast imaging and single-molecule tracking and optical penetration beyond 300μm. We detected single nanocrystals in Drosophila larvae and zebrafish embryo. We also report our first tracking of single quantum dots during zebrafish development, which displays a transition from flow to confined motion prior to the blastula stage. The new SPIM setup represents a new technique, which enables fast single-molecule imaging and tracking in living systems. [Copyright &y& Elsevier]

Published

2009

26. Low-cost optofluidic add-on enables rapid selective plane illumination microscopy of C. elegans with a conventional wide-field microscope.

Author

Behrouzi, Mehran, Youssef, Khaled, Rezai, Pouya, and Tabatabaei, Nima

Subjects

*CAENORHABDITIS elegans, *OPTICAL elements, *MICROSCOPY, *CROSS-sectional imaging, *THREE-dimensional imaging, *MICROSCOPES, *NEAR-field microscopy

Abstract

Significance: Selective plane illumination microscopy (SPIM) is an emerging fluorescent imaging technique suitable for noninvasive volumetric imaging of C. elegans. These promising microscopy systems, however, are scarce in academic and research institutions due to their high cost and technical complexities. Simple and low-cost solutions that enable conversion of commonplace wide-field microscopes to rapid SPIM platforms promote widespread adoption of SPIM by biologist for studying neuronal expressions of C. elegans. Aim: We sought to develop a simple and low-cost optofluidic add-on device that enables rapid and immobilization-free volumetric SPIM imaging of C. elegans with conventional fluorescent microscopes. Approach: A polydimethylsiloxane (PDMS)-based device with integrated optical and fluidic elements was developed as a low-cost and miniaturized SPIM add-on for the conventional wide-field microscope. The developed optofluidic chip contained an integrated PDMS cylindrical lens for on-chip generation of the light-sheet across a microchannel. Cross-sectional SPIM images of C. elegans were continuously acquired by the native objective of microscope as worms flowed in an L-shape microchannel and through the light sheet. Results: On-chip SPIM imaging of C. elegans strains demonstrated possibility of visualizing the entire neuronal system in few seconds at single-neuron resolution, with high contrast and without worm immobilization. Volumetric visualization of neuronal system from the acquired cross-sectional two-dimensional images is also demonstrated, enabling the standard microscope to acquire three-dimensional fluorescent images of C. elegans. The full-width at half-maximum width of the point spread function was measured as 1.1 and 2.4 μm in the lateral and axial directions, respectively. Conclusion: The developed low-cost optofluidic device is capable of continuous SPIM imaging of C. elegans model organism with a conventional fluorescent microscope, at high speed, and with single neuron resolution. [ABSTRACT FROM AUTHOR]

Published

2021

27. Quantification of in vitro mesenchymal stem cell invasion into tumor spheroids using selective plane illumination microscopy.

Author

Rühland, Svenja, Wechselberger, Alexandra, Spitzweg, Christine, Huss, Ralf, Nelson, Peter J., and Harz, Hartmann

Subjects

*MESENCHYMAL stem cells, *MULTIPOTENT stem cells, *STEM cell research, *TUMORS, *SPATIAL analysis (Statistics)

Abstract

Mesenchymal stem cell (MSC) homing and integration into tumors are under evaluation for clinical application. This approach requires the identification of conditions for optimal tumor invasion. We describe a tool for the in vitro comparison of parameters influencing invasion. Human MSC added to experimental tumor spheroids variably migrates toward the center of the structure. To determine MSC distribution inside the three-dimensional specimen, spatial analysis was performed using selective plane illumination microscopy. A standardized method to quantify and compare the invasion potential of variably treated MSC into experimental tumor environments allows efficient screening for optimizing conditions. [ABSTRACT FROM AUTHOR]

Published

2015

28. miniSPIM-A Miniaturized Light-Sheet Microscope.

Author

Hedde PN

Subjects

Animals, Microscopy, Fluorescence, Smartphone, Imaging, Three-Dimensional, Zebrafish

Abstract

The miniSPIM is a miniaturized light-sheet microscope that enables imaging with optical sectioning on mobile camera devices such as smartphones and single-board computers. Applications of the miniSPIM include biosensing, field research, and education where maximum portability and robustness, low power consumption, and low cost are key. Here, it is shown how all of the components of a simple light-sheet microscope can be integrated within a footprint smaller than the average smartphone. Example applications include the quantification of the motion of microparticles and bacteria in fluids, the characterization of solvent polarity based on spectral shifts of the lipid probe Nile Red, and three-dimensional (3D) and time-lapse autofluorescence imaging of a live zebrafish embryo.

Published

2021

29. Light Sheet Fluorescence Microscopy of Plant Roots Growing on the Surface of a Gel

Author

Daniel, von Wangenheim, Robert, Hauschild, and Jiří, Friml

Subjects

Light-sheet, Light, organogenesis, General Chemical Engineering, Arabidopsis, Plant Biology, Plant Roots, fluorescence microscopy, General Biochemistry, Genetics and Molecular Biology, Issue 119, Photosynthesis, development, LSFM, General Immunology and Microbiology, plants, General Neuroscience, Water, food and beverages, Lightsheet Microscopy, Darkness, Light Sheet Fluorescence Microscopy, 580 Plants, Plant Leaves, SPIM, Microscopy, Fluorescence, Gels, Selective Plane Illumination Microscopy

Abstract

One of the key questions in understanding plant development is how single cells behave in a larger context of the tissue. Therefore, it requires the observation of the whole organ with a high spatial- as well as temporal resolution over prolonged periods of time, which may cause photo-toxic effects. This protocol shows a plant sample preparation method for light-sheet microscopy, which is characterized by mounting the plant vertically on the surface of a gel. The plant is mounted in such a way that the roots are submerged in a liquid medium while the leaves remain in the air. In order to ensure photosynthetic activity of the plant, a custom-made lighting system illuminates the leaves. To keep the roots in darkness the water surface is covered with sheets of black plastic foil. This method allows long-term imaging of plant organ development in standardized conditions.

Published

2017

30. Fluorescence Microscopy Gets Faster and Clearer: Roles of Photochemistry and Selective Illumination

Author

Wolenski, Joseph S. and Julich, Doerthe

Subjects

light sheet microscopy, Embryo, Nonmammalian, Microscopy, Confocal, Light, Photochemistry, Reproducibility of Results, photoactivatable GFP, Focus: Microscopy and Imaging, confocal microscopy, superresolution microscopy, selective plane illumination microscopy, Luminescent Proteins, Microscopy, Fluorescence, Multiphoton, Luminescent Measurements, Animals, Zebrafish, 2-photon microscopy, Fluorescent Dyes

Abstract

Significant advances in fluorescence microscopy tend be a balance between two competing qualities wherein improvements in resolution and low light detection are typically accompanied by losses in acquisition rate and signal-to-noise, respectively. These trade-offs are becoming less of a barrier to biomedical research as recent advances in optoelectronic microscopy and developments in fluorophore chemistry have enabled scientists to see beyond the diffraction barrier, image deeper into live specimens, and acquire images at unprecedented speed. Selective plane illumination microscopy has provided significant gains in the spatial and temporal acquisition of fluorescence specimens several mm in thickness. With commercial systems now available, this method promises to expand on recent advances in 2-photon deep-tissue imaging with improved speed and reduced photobleaching compared to laser scanning confocal microscopy. Superresolution microscopes are also available in several modalities and can be coupled with selective plane illumination techniques. The combination of methods to increase resolution, acquisition speed, and depth of collection are now being married to common microscope systems, enabling scientists to make significant advances in live cell and in situ imaging in real time. We show that light sheet microscopy provides significant advantages for imaging live zebrafish embryos compared to laser scanning confocal microscopy.

Published

2014

31. Wnt3 Is Lipidated at Conserved Cysteine and Serine Residues in Zebrafish Neural Tissue.

Author

Dhasmana D, Veerapathiran S, Azbazdar Y, Nelanuthala AVS, Teh C, Ozhan G, and Wohland T

Abstract

Wnt proteins are a family of hydrophobic cysteine-rich secreted glycoproteins that regulate a gamut of physiological processes involved in embryonic development and tissue homeostasis. Wnt ligands are post-translationally lipidated in the endoplasmic reticulum (ER), a step essential for its membrane targeting, association with lipid domains, secretion and interaction with receptors. However, at which residue(s) Wnts are lipidated remains an open question. Initially it was proposed that Wnts are lipid-modified at their conserved cysteine and serine residues (C77 and S209 in mWnt3a), and mutations in either residue impedes its secretion and activity. Conversely, some studies suggested that serine is the only lipidated residue in Wnts, and substitution of serine with alanine leads to retention of Wnts in the ER. In this work, we investigate whether in zebrafish neural tissues Wnt3 is lipidated at one or both conserved residues. To this end, we substitute the homologous cysteine and serine residues of zebrafish Wnt3 with alanine (C80A and S212A) and investigate their influence on Wnt3 membrane organization, secretion, interaction and signaling activity. Collectively, our results indicate that Wnt3 is lipid modified at its C80 and S212 residues. Further, we find that lipid addition at either C80 or S212 is sufficient for its secretion and membrane organization, while the lipid modification at S212 is indispensable for receptor interaction and signaling., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Dhasmana, Veerapathiran, Azbazdar, Nelanuthala, Teh, Ozhan and Wohland.)

Published

2021

32. 4D (x-y-z-t) imaging of thick biological samples by means of Two-Photon inverted Selective Plane Illumination Microscopy (2PE-iSPIM)

Author

Philipp Follert, Marta d’Amora, Giuseppe Sancataldo, Zeno Lavagnino, Davide De Pietri Tonelli, Francesca Cella Zanacchi, Alberto Diaspro, LAVAGNINO, ZENO, SANCATALDO, GIUSEPPE, D'Amora, M, Follert, P, De Pietri Tonelli, D, DIASPRO, ALBERTO GIOVANNI, and CELLA ZANACCHI, FRANCESCA

Subjects

0301 basic medicine, Multidisciplinary, Materials science, Photon, Image quality, business.industry, Scattering, Bright-field microscopy, 01 natural sciences, Article, 010309 optics, 03 medical and health sciences, 030104 developmental biology, Optics, Two-photon excitation microscopy, Light sheet fluorescence microscopy, 0103 physical sciences, Microscopy, business, Selective Plane Illumination Microscopy, Excitation

Abstract

In the last decade light sheet fluorescence microscopy techniques, such as selective plane illumination microscopy (SPIM), has become a well established method for developmental biology. However, conventional SPIM architectures hardly permit imaging of certain tissues since the common sample mounting procedure, based on gel embedding, could interfere with the sample morphology. In this work we propose an inverted selective plane microscopy system (iSPIM), based on non-linear excitation, suitable for 3D tissue imaging. First, the iSPIM architecture provides flexibility on the sample mounting, getting rid of the gel-based mounting typical of conventional SPIM, permitting 3D imaging of hippocampal slices from mouse brain. Moreover, all the advantages brought by two photon excitation (2PE) in terms of reduction of scattering effects and contrast improvement are exploited, demonstrating an improved image quality and contrast compared to single photon excitation. The system proposed represents an optimal platform for tissue imaging and it smooths the way to the applicability of light sheet microscopy to a wider range of samples including those that have to be mounted on non-transparent surfaces.

Published

2016

33. Selective Plane Illumination Microscopy Using Non-spreading Airy Beams

Author

Leitis, Aleksandrs and Leitis, Aleksandrs

Abstract

Recently a new field of microscopy has emerged, known as selective plane illumination microscopy (SPIM). Using a SPIM setup the sample is illuminated with a thin light sheet from the side. The selective plane illumination overcomes many problems that conventional microscopes have. Conventional microscopes illuminate the sample axially and collects the light only from the focal plane of the microscope objective. Therefore parts of the sample which are out of focus are illuminated unnecessarily, leading to rapid fluorophore photobleaching and decrease of signal to noise ratio due to out of focus light. The $SPIM$ method overcomes these problems, because only the fluorophores in the focal plane of the objective are excited. Another problem with conventional microscopes is that they are capable of only two-dimensional imaging. The exception are confocal microscopes, but these microscopes are slow and the field of view is restricted to few hundred micrometers. The SPIM method significantly improves the three-dimensional imaging speed and can reach up to few hundred frames per second. This imaging speed enhancement is achieved, because the whole plane is captured with a single snapshot, instead of point by point scanning as in confocal microscopes. To take all the advantages of the SPIM method it is crucial to form a thin light sheet that extends for the whole field of view. Commercially available lasers have Gaussian beam. It is well known that tightly focused Gaussian beams spread out quickly, therefore there will be good axial resolution only in the central part of the image. Because of that the field of view will be restricted to the Rayleigh range of the Gaussian beam. In this work we present how to create non-spreading Airy beams using only two additional lens elements and how they can be implemented in the SPIM setup to significantly extend the field of view keeping high axial resolution. This is an important advancement since Airy beams would allow larger sized ob, The field of optical microscopy emerged in late 17th century, when famous Dutch draper and scientist Anton van Leeuwenhoek pioneered the techniques of microscopy. Since then the field has expanded and has greatly influenced the development of biology, chemistry, physics and medical research areas. Recently optical microscopy reached the realms of super resolution and nano scale, therefore allowing to see even single molecules. For this invention in 2014 three scientists were awarded with Nobel prize in chemistry. Overall, four Nobel prizes have been awarded for discoveries and inventions in microscopy. Most of the research in optical microscopy is done to increase the spatial resolution, neglecting the resolution in time. But obviously there are fast biological processes and understanding them would give significant contribution to medicine and biology. In the last decade a new field of microscopy emerged, called selective plane illumination microscopy (SPIM). What distinguishes SPIM from conventional microscopes is that the sample is illuminated with a thin laser sheet. Therefore fluorescent light will be emitted only from the plane where the light sheet lies. And the light sheet can be made as thin as one hundredth of a human hair width. Therefore the SPIM method allows to image large samples with high temporal resolution and high spatial resolution in all 3 dimensions. With this new technique it is possible to reach up to few thousand frames per second, and it is possible to follow neuron signal propagation in real time. It is a great step forwards for research in neurology. Not only for studying cellular interactions, but also neuronal network interactions throughout the body of small animals. Furthermore bigger and older sample imaging could give better understanding of the neurological diseases that come with age, for instance Alzheimer's disease. Besides significant increase in temporal resolution, with the SPIM technique it is possible to follow biological p

Published

2016

34. Imaging the developing human external and internal urogenital organs with light sheet fluorescence microscopy.

Author

Isaacson D, McCreedy D, Calvert M, Shen J, Sinclair A, Cao M, Li Y, McDevitt T, Cunha G, and Baskin L

Subjects

Humans, Image Processing, Computer-Assisted methods, Imaging, Three-Dimensional methods, Microscopy, Fluorescence methods, Specimen Handling methods, Urogenital System cytology

Abstract

Technological advances in three-dimensional (3D) reconstruction techniques have previously enabled paradigm shifts in our understanding of human embryonic and fetal development. Light sheet fluorescence microscopy (LSFM) is a recently-developed technique that uses thin planes of light to optically section whole-mount cleared and immunolabeled biologic specimens. The advent of commercially-available light sheet microscopes has facilitated a new generation of research into protein localization and tissue dynamics at extremely high resolution. Our group has applied LSFM to study developing human fetal external genitalia, internal genitalia and kidneys. This review describes LSFM and presents our group's technique for preparing, clearing, immunostaining and imaging human fetal urogenital specimens. We then present light sheet images and videos of each element of the developing human urogenital system. To the extent of our knowledge, the work conducted by our laboratory represents the first description of a method for performing LSFM on the full human urogenital system during the embryonic and fetal periods., (Copyright © 2019. Published by Elsevier B.V.)

Published

2020

35. Setting Up a Simple Light Sheet Microscope for In Toto Imaging of C. elegans Development

Author

Chardes, C., Melenec, P., Bertrand, Vincent, Lenne, P.F., Institut de Biologie du Développement de Marseille (IBDM), Aix Marseille Université (AMU)-Centre National de la Recherche Scientifique (CNRS), Aix Marseille Université (AMU)-Collège de France (CdF (institution))-Centre National de la Recherche Scientifique (CNRS), ATIP grants from CNRS, the Labex INFORM grant and a grant from Sanofi-Aventis, and ANR-10-INBS-0004,France-BioImaging,Développment d'une infrastructure française distribuée coordonnée(2010)

Subjects

Light Sheet, Caenorhabditis elegans Embryo Development, [SDV.BA]Life Sciences [q-bio]/Animal biology, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, in vivo imaging, Selective Plane Illumination Microscopy, Developmental Biology, Issue 87

Abstract

International audience; Fast and low phototoxic imaging techniques are pre-requisite to study the development of organisms in toto. Light sheet based microscopy reduces photo-bleaching and phototoxic effects compared to confocal microscopy, while providing 3D images with subcellular resolution. Here we present the setup of a light sheet based microscope, which is composed of an upright microscope and a small set of opto-mechanical elements for the generation of the light sheet. The protocol describes how to build, align the microscope and characterize the light sheet. In addition, it details how to implement the method for in toto imaging of C. elegans embryos using a simple observation chamber. The method allows the capture of 3D two-colors time-lapse movies over few hours of development. This should ease the tracking of cell shape, cell divisions and tagged proteins over long periods of time.

Published

2014

36. Wavefront shaping of a Bessel light field enhances light sheet microscopy with scattered light

Author

Tom Vettenburg, Claire A. Mitchell, Frank J. Gunn-Moore, Kishan Dholakia, Jonathan Nylk, Brown, TG, Cogswell, CJ, Wilson, T, University of St Andrews. School of Physics and Astronomy, University of St Andrews. School of Biology, University of St Andrews. Institute of Behavioural and Neural Sciences, and University of St Andrews. Biomedical Sciences Research Complex

Subjects

Fluorescence-lifetime imaging microscopy, Specimins, Microscope, Deconvolution, law.invention, Optics, Multifocal plane microscopy, law, Microscopy, LSM, High resolution, QC, Physics, Bessel beam, Fluorescence microscopy, Polarized light microscopy, business.industry, Beams, Plane illumination, Ultramicroscope, Beam shaping, Selective plane illumination microscopy, SPIM, QC Physics, Light sheet fluorescence microscopy, Light sheet microscopy, business, Light field

Abstract

The project was supported by the UK Engineering and Physical Sciences Research Council, RS MacDonald Charitable Trust, SULSA, and the St. Andrews 600th anniversary BRAINS appeal. K. D. is a Royal Society Wolfson Merit Award holder. Light sheet microscopy has seen a resurgence as it facilitates rapid, high contrast, volumetric imaging with minimal sample exposure. Initially developed for imaging scattered light, this application of light sheet microscopy has largely been overlooked but provides an endogenous contrast mechanism which can complement fluorescence imaging and requires very little or no modification to an existing light sheet fluorescence microscope. Fluorescence imaging and scattered light imaging differ in terms of image formation. In the former the detected light is incoherent and weak whereas in the latter the coherence properties of the illumination source, typically a laser, dictate the coherence of detected light, but both are dependent on the quality of the illuminating light sheet. Image formation in both schemes can be understood as the convolution of the light sheet with the specimen distribution. In this paper we explore wavefront shaping for the enhancement of light sheet microscopy with scattered light. We show experimental verification of this result, demonstrating the use of the propagation invariant Bessel beam to extend the field of view of a high resolution scattered light, light sheet microscope and its application to imaging of biological super-cellular structures with sub-cellular resolution. Additionally, complementary scattering and fluorescence imaging is used to characterize the enhancement, and to develop a deeper understanding of the differences of image formation between contrast mechanisms in light sheet microscopy. Publisher PDF

Published

2014

37. Multilayer Mounting for Long-term Light Sheet Microscopy of Zebrafish

Author

Michaela Mickoleit, Jan Huisken, and Michael Weber

Subjects

Male, General Chemical Engineering, time lapse microscopy, Time-Lapse Imaging, General Biochemistry, Genetics and Molecular Biology, Time-lapse microscopy, sample mounting, Animals, Zebrafish, light sheet microscopy, Microscopy, Danio rerio, General Immunology and Microbiology, biology, business.industry, General Neuroscience, Sepharose, Anatomy, biology.organism_classification, zebrafish, Light sheet fluorescence microscopy, Optoelectronics, Female, Imaging technique, business, Issue 84, long-term imaging, Selective Plane Illumination Microscopy, Developmental Biology

Abstract

Light sheet microscopy is the ideal imaging technique to study zebrafish embryonic development. Due to minimal photo-toxicity and bleaching, it is particularly suited for long-term time-lapse imaging over many hours up to several days. However, an appropriate sample mounting strategy is needed that offers both confinement and normal development of the sample. Multilayer mounting, a new embedding technique using low-concentration agarose in optically clear tubes, now overcomes this limitation and unleashes the full potential of light sheet microscopy for real-time developmental biology.

Published

2014

38. Luminance Changes Drive Directional Startle through a Thalamic Pathway.

Author

Heap, Lucy A.L., Vanwalleghem, Gilles, Thompson, Andrew W., Favre-Bulle, Itia A., and Scott, Ethan K.

Subjects

*THALAMUS, *VISUAL perception, *STIMULUS & response (Biology), *ZEBRA danio, *VERTEBRATES

Abstract

Summary Looming visual stimuli result in escape responses that are conserved from insects to humans. Despite their importance for survival, the circuits mediating visual startle have only recently been explored in vertebrates. Here we show that the zebrafish thalamus is a luminance detector critical to visual escape. Thalamic projection neurons deliver dim-specific information to the optic tectum, and ablations of these projections disrupt normal tectal responses to looms. Without this information, larvae are less likely to escape from dark looming stimuli and lose the ability to escape away from the source of the loom. Remarkably, when paired with an isoluminant loom stimulus to the opposite eye, dimming is sufficient to increase startle probability and to reverse the direction of the escape so that it is toward the loom. We suggest that bilateral comparisons of luminance, relayed from the thalamus to the tectum, facilitate escape responses and are essential for their directionality. [ABSTRACT FROM AUTHOR]

Published

2018

39. Fluorescent tags to explore cell wall structure and dynamics

Author

Herman Höfte, Martine Gonneau, Samantha Vernhettes, Institut Jean-Pierre Bourgin (IJPB), Institut National de la Recherche Agronomique (INRA)-AgroParisTech, and Vernhettes, Samantha

Subjects

variable-angle epifluorescence microscopy, 0106 biological sciences, plant cell-wall, [SDV]Life Sciences [q-bio], Plant Science, lcsh:Plant culture, Biology, Bioinformatics, fluorescence microscopy, spinning disk microscopy, 01 natural sciences, Cell wall, Mini Review Article, 03 medical and health sciences, [SDV.IDA]Life Sciences [q-bio]/Food engineering, Fluorescence microscope, [SDV.BV]Life Sciences [q-bio]/Vegetal Biology, [SPI.GPROC]Engineering Sciences [physics]/Chemical and Process Engineering, lcsh:SB1-1110, 030304 developmental biology, 0303 health sciences, plantcell-wall, fluorescencemicroscopy, Dynamics (mechanics), Fluorescence, selective plane illumination microscopy, Biophysics, 010606 plant biology & botany

Abstract

International audience; Plant cell walls are highly dynamic and heterogeneous structures, which vary between cell types, growth stages but also between microdomains within a single cell wall. In this review, we summarize the imaging techniques using fluorescent tags that are currently being used and which should in the coming years revolutionize our understanding of the dynamics of cell wall architecture and the cellular processes involved in the synthesis of cell wall components.

Published

2012

40. Comprehensive optical and data management infrastructure for high-throughput light-sheet microscopy of whole mouse brains

Author

Leonardo Sacconi, Francesco S. Pavone, Giulio Iannello, Ludovico Silvestri, Leonardo Onofri, Irene Costantini, M. Caroline Müllenbroich, and Marcel van ’t Hoff

Subjects

Microscope, Computer science, Data management, software management, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Neuroscience (miscellaneous), law.invention, Image stitching, Software, Data acquisition, law, Confocal microscopy, Microscopy, high-throughput imaging, Radiology, Nuclear Medicine and imaging, Computer vision, Radiological and Ultrasound Technology, business.industry, Special Section Papers, selective plane illumination microscopy, Light sheet fluorescence microscopy, data management, Artificial intelligence, whole brain imaging, business, light-sheet microscopy

Abstract

Comprehensive mapping and quantification of neuronal projections in the central nervous system requires high-throughput imaging of large volumes with microscopic resolution. To this end, we have developed a confocal light-sheet microscope that has been optimized for three-dimensional (3-D) imaging of structurally intact clarified whole-mount mouse brains. We describe the optical and electromechanical arrangement of the microscope and give details on the organization of the microscope management software. The software orchestrates all components of the microscope, coordinates critical timing and synchronization, and has been written in a versatile and modular structure using the LabVIEW language. It can easily be adapted and integrated to other microscope systems and has been made freely available to the light-sheet community. The tremendous amount of data routinely generated by light-sheet microscopy further requires novel strategies for data handling and storage. To complete the full imaging pipeline of our high-throughput microscope, we further elaborate on big data management from streaming of raw images up to stitching of 3-D datasets. The mesoscale neuroanatomy imaged at micron-scale resolution in those datasets allows characterization and quantification of neuronal projections in unsectioned mouse brains. (C) The Authors.

Published

2015

41. Single Molecule Imaging in Live Embryos Using Lattice Light-Sheet Microscopy.

Author

Mir M, Reimer A, Stadler M, Tangara A, Hansen AS, Hockemeyer D, Eisen MB, Garcia H, and Darzacq X

Subjects

Animals, Data Analysis, Embryo, Mammalian cytology, Embryo, Mammalian diagnostic imaging, Embryo, Nonmammalian cytology, Mice, Reproducibility of Results, Drosophila melanogaster embryology, Embryo, Nonmammalian diagnostic imaging, Microscopy, Fluorescence methods, Single Molecule Imaging methods

Abstract

In the past decade, live-cell single molecule imaging studies have provided unique insights on how DNA-binding molecules such as transcription factors explore the nuclear environment to search for and bind to their targets. However, due to technological limitations, single molecule experiments in living specimens have largely been limited to monolayer cell cultures. Lattice light-sheet microscopy overcomes these limitations and has now enabled single molecule imaging within thicker specimens such as embryos. Here we describe a general procedure to perform single molecule imaging in living Drosophila melanogaster embryos using lattice light-sheet microscopy. This protocol allows direct observation of both transcription factor diffusion and binding dynamics. Finally, we illustrate how this Drosophila protocol can be extended to other thick samples using single molecule imaging in live mouse embryos as an example.

Published

2018

42. Calcium Dynamics in Root Cells of Arabidopsis thaliana Visualized with Selective Plane Illumination Microscopy

Author

Andrea Bassi, Gianluca Valentini, Alessia Candeo, Alex Costa, and Luca Fieramonti

Subjects

Fluorescence-lifetime imaging microscopy, Science, Gene Expression, Plant Roots, selective plane illumination microscopy, arabidopsis, calcium imaging, Cytosol, Calcium imaging, Genes, Reporter, Plant Cells, Arabidopsis, Calcium-binding protein, Microscopy, Fluorescence Resonance Energy Transfer, Image Processing, Computer-Assisted, medicine, Calcium Signaling, Cell Nucleus, Ion Transport, Microscopy, Confocal, Multidisciplinary, biology, Calcium-Binding Proteins, Cameleon (protein), Plants, Genetically Modified, biology.organism_classification, Cell biology, Luminescent Proteins, Förster resonance energy transfer, medicine.anatomical_structure, biology.protein, Medicine, Calcium, Nucleus, Research Article

Abstract

Selective Plane Illumination Microscopy (SPIM) is an imaging technique particularly suited for long term in-vivo analysis of transparent specimens, able to visualize small organs or entire organisms, at cellular and eventually even subcellular resolution. Here we report the application of SPIM in Calcium imaging based on Förster Resonance Energy Transfer (FRET). Transgenic Arabidopsis plants expressing the genetically encoded-FRET-based Ca(2+) probe Cameleon, in the cytosol or nucleus, were used to demonstrate that SPIM enables ratiometric fluorescence imaging at high spatial and temporal resolution, both at tissue and single cell level. The SPIM-FRET technique enabled us to follow nuclear and cytosolic Ca(2+) dynamics in Arabidopsis root tip cells, deep inside the organ, in response to different stimuli. A relevant physiological phenomenon, namely Ca(2+) signal percolation, predicted in previous studies, has been directly visualized.

Published

2013

43. Comprehensive optical and data management infrastructure for high-throughput light-sheet microscopy of whole mouse brains.

Author

Müllenbroich MC, Silvestri L, Onofri L, Costantini I, Hoff MV, Sacconi L, Iannello G, and Pavone FS

Abstract

Comprehensive mapping and quantification of neuronal projections in the central nervous system requires high-throughput imaging of large volumes with microscopic resolution. To this end, we have developed a confocal light-sheet microscope that has been optimized for three-dimensional (3-D) imaging of structurally intact clarified whole-mount mouse brains. We describe the optical and electromechanical arrangement of the microscope and give details on the organization of the microscope management software. The software orchestrates all components of the microscope, coordinates critical timing and synchronization, and has been written in a versatile and modular structure using the LabVIEW language. It can easily be adapted and integrated to other microscope systems and has been made freely available to the light-sheet community. The tremendous amount of data routinely generated by light-sheet microscopy further requires novel strategies for data handling and storage. To complete the full imaging pipeline of our high-throughput microscope, we further elaborate on big data management from streaming of raw images up to stitching of 3-D datasets. The mesoscale neuroanatomy imaged at micron-scale resolution in those datasets allows characterization and quantification of neuronal projections in unsectioned mouse brains.

Published

2015

44. Light sheet microscopy.

Author

Weber M, Mickoleit M, and Huisken J

Subjects

Animals, Humans, Image Enhancement, Microscopy, Confocal methods, Microscopy, Fluorescence methods, Time-Lapse Imaging methods, Imaging, Three-Dimensional methods

Abstract

This chapter introduces the concept of light sheet microscopy along with practical advice on how to design and build such an instrument. Selective plane illumination microscopy is presented as an alternative to confocal microscopy due to several superior features such as high-speed full-frame acquisition, minimal phototoxicity, and multiview sample rotation. Based on our experience over the last 10 years, we summarize the key concepts in light sheet microscopy, typical implementations, and successful applications. In particular, sample mounting for long time-lapse imaging and the resulting challenges in data processing are discussed in detail., (© 2014 Elsevier Inc. All rights reserved.)

Published

2014

45. Large Volume Imaging of Rodent Brain Anatomy with Emphasis on Selective Plane Illumination Microscopy

Author

Ghobril, Jean Pierre, Markram, Henry, and Pavone, Francesco Saverio

Subjects

Tracing, Mesoscale Anatomy, Acute Brain Slices, Tissue Clearing, CLARITY, Whole Mount, Thiodiethanol, Somatosensory Cortex, Immunohistochemistry, Selective Plane Illumination Microscopy

Abstract

Inside the human brain there are 86 Billion neurons exchanging electrical impulses to allow reaction, homoeostasis and intelligence. Their coarse organization has been described, leaving us with a fair understanding of macrocircuitry. The microcircuitry of the brain is also being explored with patch clamp recordings. But a more integrative view on mesoscale organization of the central nervous system is still lacking. Recent developments in microscopy methods have opened new windows to address this point. It is the goal of this thesis to analyze and compare anatomical features of the brain with current routine techniques as well as explore light sheet microscopy for large scale quantitative reconstructions of rodent brains. Integration efforts of the cortical column model of the Blue Brain project into more detailed cortical circuitry sparked the search of acute slice preparations suitable for long range electrophysiology. Serial section reconstruction of the rat S1 hindlimb anterograde projections was performed with special attention to the anatomical relationship between S1 hindlimb region and VPL nucleus of thalamus. It was found that a functional electrophysiological slice preparation between S1-HL and VPL is feasible. The subsequent experimental exploration proved the intact fiber path in acute slice preparations based on the morphometric measurements of the previous serial sectioning reconstruction. Another mesoscale trait investigated was the excitatory to inhibitory ratio of the juvenile rat cortex. The measured numbers for the cellular density are higher than previously published. Cellular density for S1-HL is 84535$\pm$4400 neurons/mm$^{3}$ high with an E-I ratio of 8.3. Like in other brains the cellular density is a continuously adapting function of the distance from pia and the current brain region. In the second part of this dissertation Selective Plane Illumination Microscopy(SPIM) and tissue clearing are evaluated as novel tools for whole mount rodent brain scanning, with emphasis on somata, fibers and vasculature as quantifiable brain features. Clearing methods are evaluated and a novel embedding medium for cleared tissues is presented: Thiodiethanol(TDE). Index matched brains with TDE show high degree of fluorescence conservation and transparency. Whole mount mouse and rat brains are imaged and reconstructed. The results show that whole mount microscopy is a potent tool that allows routine quantification of anatomic features on a whole brain level.

46. Using Light Sheet Fluorescence Microscopy to Image Zebrafish Eye Development

Author

Stephan Preibisch, Jaroslav Icha, Jaydeep Sidhaye, Pavel Tomancak, Christopher Schmied, and Caren Norden

Subjects

0301 basic medicine, retina, Open-source, Embryo, Nonmammalian, Light, General Chemical Engineering, Embryonic Development, Troubleshooting, Biology, Eye, Multiview Deconvolution, General Biochemistry, Genetics and Molecular Biology, Issue 110, 03 medical and health sciences, Animals, sample mounting, Fiji, Computer vision, Protocol (object-oriented programming), Bead based Registration, Zebrafish, BigDataViewer, General Immunology and Microbiology, business.industry, General Neuroscience, Multiview Reconstruction, Light Sheet Fluorescence Microscopy, Pipeline (software), 030104 developmental biology, Open source, Microscopy, Fluorescence, Light sheet fluorescence microscopy, Zebrafish embryo, Artificial intelligence, business, Multiple view, Selective Plane Illumination Microscopy, Developmental Biology

Abstract

Light sheet fluorescence microscopy (LSFM) is gaining more and more popularity as a method to image embryonic development. The main advantages of LSFM compared to confocal systems are its low phototoxicity, gentle mounting strategies, fast acquisition with high signal to noise ratio and the possibility of imaging samples from various angles (views) for long periods of time. Imaging from multiple views unleashes the full potential of LSFM, but at the same time it can create terabyte-sized datasets. Processing such datasets is the biggest challenge of using LSFM. In this protocol we outline some solutions to this problem. Until recently, LSFM was mostly performed in laboratories that had the expertise to build and operate their own light sheet microscopes. However, in the last three years several commercial implementations of LSFM became available, which are multipurpose and easy to use for any developmental biologist. This article is primarily directed to those researchers, who are not LSFM technology developers, but want to employ LSFM as a tool to answer specific developmental biology questions. Here, we use imaging of zebrafish eye development as an example to introduce the reader to LSFM technology and we demonstrate applications of LSFM across multiple spatial and temporal scales. This article describes a complete experimental protocol starting with the mounting of zebrafish embryos for LSFM. We then outline the options for imaging using the commercially available light sheet microscope. Importantly, we also explain a pipeline for subsequent registration and fusion of multiview datasets using an open source solution implemented as a Fiji plugin. While this protocol focuses on imaging the developing zebrafish eye and processing data from a particular imaging setup, most of the insights and troubleshooting suggestions presented here are of general use and the protocol can be adapted to a variety of light sheet microscopy experiments.