Single objective light-sheet microscopy for high-speed whole-cell 3D super-resolution

Marjolein B. M. Meddens; Sheng Liu; Patrick S. Finnegan; Thayne L. Edwards; Conrad D. James; Keith A. Lidke

doi:10.1364/boe.7.002219

Single Objective Light-Sheet Microscopy for High-Speed Whole-Cell 3D Super-Resolution

Biophysical Journal ◽

10.1016/j.bpj.2016.11.1035 ◽

2017 ◽

Vol 112 (3) ◽

pp. 187a ◽

Cited By ~ 1

Author(s):

Marjolein B.M. Meddens ◽

Sheng Liu ◽

Patrick S. Finnegan ◽

Thayne L. Edwards ◽

Conrad D. James ◽

...

Keyword(s):

High Speed ◽

Super Resolution ◽

Light Sheet ◽

Whole Cell ◽

Light Sheet Microscopy ◽

Single Objective

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Reflected Beam Light-Sheet Microscopy for Whole-Cell 3D Super-Resolution Imaging

Biophysical Journal ◽

10.1016/j.bpj.2014.11.218 ◽

2015 ◽

Vol 108 (2) ◽

pp. 35a

Author(s):

Marjolein B.M. Meddens ◽

Sheng Liu ◽

Conrad D. James ◽

Keith A. Lidke

Keyword(s):

Super Resolution ◽

Light Sheet ◽

Whole Cell ◽

Light Sheet Microscopy ◽

Resolution Imaging

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High-speed panoramic light-sheet microscopy reveals global endodermal cell dynamics

Nature Communications ◽

10.1038/ncomms3207 ◽

2013 ◽

Vol 4 (1) ◽

Cited By ~ 117

Author(s):

Benjamin Schmid ◽

Gopi Shah ◽

Nico Scherf ◽

Michael Weber ◽

Konstantin Thierbach ◽

...

Keyword(s):

High Speed ◽

Light Sheet ◽

Endodermal Cell ◽

Cell Dynamics ◽

Light Sheet Microscopy

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Circumvention of common labeling artifacts using secondary nanobodies

10.1101/818351 ◽

2019 ◽

Author(s):

Shama Sograte-Idrissi ◽

Thomas Schlichthaerle ◽

Carlos J. Duque-Afonso ◽

Mihai Alevra ◽

Sebastian Strauss ◽

...

Keyword(s):

Super Resolution ◽

Light Sheet ◽

Common Procedure ◽

Tissue Samples ◽

Localization Accuracy ◽

Light Sheet Microscopy ◽

Large Size ◽

Resolution Imaging ◽

Single Domain Antibodies ◽

Secondary Antibodies

AbstractThe most common procedure to reveal the location of specific (sub)cellular elements in biological samples is via immunostaining followed by optical imaging. This is typically performed with target-specific primary antibodies (1.Abs), which are revealed by fluorophore-conjugated secondary antibodies (2.Abs). However, at high resolution this methodology can induce a series of artifacts due to the large size of antibodies, their bivalency, and their polyclonality. Here we use STED and DNA-PAINT super-resolution microscopy or light sheet microscopy on cleared tissue to show how monovalent secondary reagents based on camelid single-domain antibodies (nanobodies; 2.Nbs) attenuate these artifacts. We demonstrate that monovalent 2.Nbs have four additional advantages: 1) they increase localization accuracy with respect to 2.Abs; 2) they allow direct pre-mixing with 1.Abs before staining, reducing experimental time, and enabling the use of multiple 1.Abs from the same species; 3) they penetrate thick tissues efficiently; and 4) they avoid the artificial clustering seen with 2.Abs both in live and in poorly fixed samples. Altogether, this suggests that 2.Nbs are a valuable alternative to 2.Abs, especially when super-resolution imaging or staining of thick tissue samples are involved.

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Quantitative high-speed imaging of entire developing embryos with simultaneous multiview light-sheet microscopy

Nature Methods ◽

10.1038/nmeth.2062 ◽

2012 ◽

Vol 9 (7) ◽

pp. 755-763 ◽

Cited By ~ 347

Author(s):

Raju Tomer ◽

Khaled Khairy ◽

Fernando Amat ◽

Philipp J Keller

Keyword(s):

High Speed ◽

Light Sheet ◽

High Speed Imaging ◽

Light Sheet Microscopy

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Digital Spindle: A New Way to Explore Mitotic Functions by Whole Cell Data Collection and a Computational Approach

Cells ◽

10.3390/cells9051255 ◽

2020 ◽

Vol 9 (5) ◽

pp. 1255

Author(s):

Norio Yamashita ◽

Masahiko Morita ◽

Hideo Yokota ◽

Yuko Mimori-Kiyosue

Keyword(s):

Cell Biology ◽

Information Science ◽

Three Dimensional ◽

Light Sheet ◽

Live Imaging ◽

Three Dimensions ◽

Complex Data ◽

Spatiotemporal Resolution ◽

Whole Cell ◽

Light Sheet Microscopy

From cells to organisms, every living system is three-dimensional (3D), but the performance of fluorescence microscopy has been largely limited when attempting to obtain an overview of systems’ dynamic processes in three dimensions. Recently, advanced light-sheet illumination technologies, allowing drastic improvement in spatial discrimination, volumetric imaging times, and phototoxicity/photobleaching, have been making live imaging to collect precise and reliable 3D information increasingly feasible. In particular, lattice light-sheet microscopy (LLSM), using an ultrathin light-sheet, enables whole-cell 3D live imaging of cellular processes, including mitosis, at unprecedented spatiotemporal resolution for extended periods of time. This technology produces immense and complex data, including a significant amount of information, raising new challenges for big image data analysis and new possibilities for data utilization. Once the data are digitally archived in a computer, the data can be reused for various purposes by anyone at any time. Such an information science approach has the potential to revolutionize the use of bioimage data, and provides an alternative method for cell biology research in a data-driven manner. In this article, we introduce examples of analyzing digital mitotic spindles and discuss future perspectives in cell biology.

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Rapid Whole Cell Imaging Reveals A Calcium-APPL1-Dynein Nexus That Regulates Cohort Trafficking of Stimulated EGF Receptors

10.1101/481796 ◽

2018 ◽

Author(s):

H M York ◽

A Patil ◽

U K Moorthi ◽

A Kaur ◽

A Bhowmik ◽

...

Keyword(s):

Signal Processing ◽

Cell Imaging ◽

Light Sheet ◽

Endosomal Trafficking ◽

Egf Receptors ◽

Whole Cell ◽

Cellular Processes ◽

Light Sheet Microscopy ◽

Signaling Receptors ◽

Cell Surface Signaling

ABSTRACTMulticellular life processes such as proliferation and differentiation depend on cell surface signaling receptors that bind ligands generally referred to as growth factors. Recently, it has emerged that the endosomal system provides rich signal processing capabilities for responses elicited by these factors [1-3]. At the single cell level, endosomal trafficking becomes a critical component of signal processing, as exemplified by the epidermal growth factor (EGF) receptors of the receptor tyrosine kinase family. EGFRs, once activated by EGF, are robustly trafficked to the phosphatase-enriched peri-nuclear region (PNR), where they are dephosphorylated [4-8]. However, the details of the mechanisms regulating the movements of stimulated EGFR in time and space, i.e., towards the PNR, are not known. What endosomal regulators provide specificity to EGFR? Do modifications to the receptor upon stimulation regulate its trafficking? To understand the events leading to EGFR translocation, and especially the early endosomal dynamics that immediately follow EGFR internalization, requires the real-time, long-term, whole-cell imaging of multiple elements. Here, exploiting the advantages of lattice light-sheet microscopy [9], we show that the binding of EGF by its receptor, EGFR, triggers a transient calcium increase that peaks by 30 s, causing the desorption of APPL1 from pre-existing endosomes within one minute, the rebinding of liberated APPL1 to EGFR within three minutes, and the dynein-dependent translocation of APPL1-EGF-bearing endosomes to the PNR within five minutes. The novel, cell spanning, fast acting network that we reveal integrates a cascade of events dedicated to the cohort movement of activated EGFR receptors. Our findings support the intriguing proposal that certain endosomal pathways have shed some of the stochastic strategies of traditional trafficking, and have evolved behaviors whose predictability is better suited to signaling [10, 11]. Work presented here demonstrates that our whole cell imaging approach can be a powerful tool in revealing critical transient interactions in key cellular processes such as receptor trafficking.

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Reflective imaging improves resolution, speed, and collection efficiency in light sheet microscopy

10.1101/154807 ◽

2017 ◽

Author(s):

Yicong Wu ◽

Abhishek Kumar ◽

Corey Smith ◽

Evan Ardiel ◽

Panagiotis Chandris ◽

...

Keyword(s):

High Resolution ◽

High Speed ◽

Collection Efficiency ◽

Single Cells ◽

Numerical Aperture ◽

Light Sheet ◽

Three Dimensions ◽

Spatiotemporal Resolution ◽

Light Sheet Microscopy ◽

Simultaneous Acquisition

AbstractLight-sheet fluorescence microscopy (LSFM) enables high-speed, high-resolution, gentle imaging of live biological specimens over extended periods. Here we describe a technique that improves the spatiotemporal resolution and collection efficiency of LSFM without modifying the underlying microscope. By imaging samples on reflective coverslips, we enable simultaneous collection of multiple views, obtaining 4 complementary views in 250 ms, half the period it would otherwise take to collect only two views in symmetric dual-view selective plane illumination microscopy (diSPIM). We also report a modified deconvolution algorithm that removes the associated epifluorescence contamination and fuses all views for resolution recovery. Furthermore, we enhance spatial resolution (to < 300 nm in all three dimensions) by applying our method to a new asymmetric diSPIM, permitting simultaneous acquisition of two high-resolution views otherwise difficult to obtain due to steric constraints at high numerical aperture (NA). We demonstrate the broad applicability of our method in a variety of samples of moderate (< 50 μm) thickness, studying mitochondrial, membrane, Golgi, and microtubule dynamics in single cells and calcium activity in nematode embryos.

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High-Resolution, Large Field-of-View, and Multi-View Single Objective Light-Sheet Microscopy

10.1101/2020.09.22.309229 ◽

2020 ◽

Author(s):

Bin Yang ◽

Alfred Millett-Sikking ◽

Merlin Lange ◽

Ahmet Can Solak ◽

Hirofumi Kobayashi ◽

...

Keyword(s):

High Resolution ◽

Light Sheet ◽

Field Of View ◽

Large Field ◽

Sample Rotation ◽

Light Sheet Microscopy ◽

Spatio Temporal ◽

Large Living ◽

Single Objective ◽

Imaging Speed

Light-sheet microscopy has become the preferred method for long-term imaging of large living samples because of its low photo-invasiveness and good optical sectioning capabilities. Unfortunately, refraction and scattering often pose obstacles to light-sheet propagation and limit imaging depth. This is typically addressed by imaging multiple complementary views to obtain high and uniform image quality throughout the sample. However, multi-view imaging often requires complex multi-objective configurations that complicate sample mounting, or sample rotation that decreases imaging speed. Recent developments in single-objective light-sheet microscopy have shown that it is possible to achieve high spatio-temporal resolution with a single objective for both illumination and detection. Here we describe a single-objective light-sheet microscope that achieves: (i) high-resolution and large field-of-view imaging via a custom remote focusing objective; (ii) simpler design and ergonomics by remote placement of coverslips; (iii) fast volumetric imaging by means of light-sheet stabilised stage scanning – a novel scanning modality that extends the imaging volume without compromising imaging speed nor quality; (iv) multi-view imaging by means of dual orthogonal light-sheet illumination. Finally, we demonstrate the speed, field of view and resolution of our novel instrument by imaging zebrafish tail development.

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Dual-view light-sheet imaging through tilted glass interface using a deformable mirror

10.1101/2020.10.20.345306 ◽

2020 ◽

Author(s):

N Vladimirov ◽

F Preusser ◽

J Wisniewski ◽

Z Yaniv ◽

RA Desai ◽

...

Keyword(s):

Adaptive Optics ◽

High Speed ◽

Microfluidic Channel ◽

Microfluidic Devices ◽

Light Sheet ◽

Stochastic Gradient Descent ◽

Deformable Mirror ◽

Optical Aberrations ◽

Light Sheet Microscopy ◽

Gradient Descent Algorithm

AbstractLight-sheet microscopy has become one of the primary tools for imaging live developing organisms because of its high speed, low phototoxicity, and optical sectioning capabilities. Detection from multiple sides (multi-view imaging) additionally allows nearly isotropic resolution via computational merging of the views. However, conventional light-sheet microscopes require that the sample is suspended in a gel to allow optical access from two or more sides. At the same time, the use of microfluidic devices is highly desirable for many experiments, but geometric constrains and strong optical aberrations caused by the coverslip titled relative to objectives make the use of multi-view lightsheet challenging for microfluidics.In this paper we describe the use of adaptive optics (AO) to enable multi-view light-sheet microscopy in such microfluidic setup by correcting optical aberrations introduced by the tilted coverslip. The optimal shape of deformable mirror is computed by an iterative stochastic gradient-descent algorithm that optimizes PSF in two orthogonal planes simultaneously. Simultaneous AO correction in two optical arms is achieved via a knife-edge mirror that splits excitation path and combines the detection path.We characterize the performance of this novel microscope setup and, by dual-view light-sheet imaging of C.elegans inside a microfluidic channel, demonstrate a drastic improvement of image quality due to AO and dual-view reconstruction. Our microscope design allows multi-view light-sheet microscopy with microfluidic devices for precisely controlled experimental conditions and high-content screening.

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