Application: CSU-X1, CSU22, CSU10
- Vesicle trafficking
- Cell Division
- FRET Imaging
- Calcium Imaging
- in vivo imaging
- Multi-color imaging
- Long-term, multi-dimensional live-cell imaging
- Micro PIV
Vesicle trafficking
*Movies from Indiana Center for Biological Microscopy, taken by Kenneth Dunn, Ph.D. (movies of Vesicle trafficking)
All images were collected using the system described below:
Nikon TE 2000U inverted microscope, using Nikon 60 or 100 NA 1.4, oil-immersion plan apochromatic objectives, with a Hamamatsu Orca-ER CCD system
GFP labeled tubulin in living Madin-Darby canine kidney cells
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GFP labeled Rab7 and GFP labeled tubulin microtubules in living Madin-Darby canine kidney cells, 380 frames collected at 18fps, the movie plays back at 2x speed
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GFP labeled tubulin in living Madin-Darby canine kidney cells, images collected at 2fps for 60 seconds, the movie plays back at 15x speed
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GFP labeled Rab7 and GFP labeled tubulin in living Madin-Darby canine kidney cells
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GFP labeled tubulin in living Madin-Darby canine kidney cells, rendered using our Voxx software
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GFP labeled tubulin in living Chinese Hamster Ovary Cells, rendered using our Voxx software
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Cell Division
Cell Division of an LLCPK1 cell
*Movies from Patricia Wadsworth’s laboratory
Cell Division of an LLCPK1 cell expressing GFP-tagged EB1, a microtubule plus-end binding protein (kind gift of Lynne Cassimeris).
(All movies were taken by Dr. U. Serdar Tulu by using a MicroMax camera on a Nikon TE-300 inverted microscope coupled to a Yokogawa spinning disc confocal unit (Perkin Elmer Life & Analytical Sciences. )and are shown at the speed of 10 frames/sec.)
Interphase-1 movie:
The cell is in the G1/S phase, which is characterized by the presence of one centrosome. Images were recorded every 4 seconds for a total of 3 min with 600 msec exposure-time
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Interphase-2 movie
The cell is in the G2 phase, which is characterized by the presence of two centrosomes. Images were recorded every 4 seconds for a total of 3 min with 600 msec exposure-time
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Metaphase movie:
Images were recorded every 2 seconds for a total of 2 min with 600 msec exposure time.
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Cell Division
*Movies by Drs. Jonathan M. Scholey& David J. Sharp
Interphase S2 cell expressing EGFP-tubulin
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Mitotic S2 cell expressing EGFP-tubulin
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Mitotic S2 cell expressing EGFP-EB1
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Drosophila syncytial blastoderm-stage embryo injected with rhodamine tubulin and expressing GFP-histone.
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Intravital Molecular Imaging
Movies by Paul Maddox, Ludwig Inst. of Cancer Research Time-lapse images were acquired by using a CSU10 Yokogawa spinning-disk confocal system (Perkin-Elmer Life Sciences Wallac) mounted on a Nikon Eclipse TE300 inverted microscope (Nikon Instrument Group). The specimens were illuminated at 488 nm with an air-cooled Ar/Kr laser (60mW, Melles Griot). Digital images were acquired with an Orca ER, Hamamatsu 16-bit cooled CCD camera (Hamamatsu Photonics), providing the goa-1 and gpa-16 DNA constructs, Stephan Grill, and the acquisition system was controlled by MetaMorph software (Universal Imaging). Fluorescence images were acquired with 350 ms exposure at 2- or 5-s intervals by using a Plan Apochromat 100_/1.4 NA objective and 2 _ 2 binning in the camera. Images were analyzed by using MetaMorph software and Microsoft Excel (Microsoft) and were processed with Adobe Photoshop (Adobe Systems)
Drosophila embryo expressing GFP-centromere protein & injected with X-rhodamine tubulin, Maddox et.al. Current Biology(2002)
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GFP-Histone & GFP spindle poles in C. elegans embryo.
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GFP tubulin in C. elegans embryo.
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Hela_yfp_cenpa_control1 : HeLa cell expressing YFP-CENP-A(kinetochore specific protein) with DIC.
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C. elegans embryo
*Movies by Fumio Motegi & Asako Sugimoto
(Laboratory for Developmental Genomics, RIKEN Center for Developmental Biology)
Dynamics of GFP-EBP-1 (a homolog of EB1, a microtubule plus-end binding protein) during the first cell division of a C. elegans embryo. Images were acquired with a 1-s exposure time at 2-s intervals.
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Dynamics of GFP-RHO-1 at the cell cortex during the establishment of anterior-posterior polarity in a C. elegans one-cell embryo. Images were acquired with a 0.5-s exposure time at 5-s intervals. The embryo is oriented with the anterior pole to the left.
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Tobacco BY-2 cell
*Movies by Takumi Higaki & Seiichiro Hasezawa
Laboratory of Plant Cell Biology in Totipotency,
Department of Integrated Bioscience, Graduate school of Frontier Science, The University of Tokyo
Cell division of tobacco BY-2 cell
Red: chromosome(RFP-HistoneH2B)
Green: microtubule(GFP-tubulin),
Blue: cell plate(FM4-64)
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Localization of actin microfilaments
Left: Control
Right: BA treatment
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Time-lapse imaging of neural progenitor cells during cortical development
Tangential time-lapse monitoring of all cell-cell borders, about 5 µm from the apical surface, in a cortical wall prepared from E13 Lyn-Venus transgenic mouse Data : Mayumi Okamoto, Ph.D., Department of Anatomy and Cell Biology,
Nagoya University Graduate School of Medicine
Blue: Neural progenitor cell(M phase), Magenta: Daughter cell
Reference:
Okamoto, M., Namba, T., Shinoda, T., Kondo, T., Watanabe, T., Inoue, Y., Takeuchi, K., Enomoto, Y., Ota, K., Oda, K., Wada, Y., Sagou, K., Saito, K., Sakakibara, A., Kawaguchi, A., Nakajima, K., Adachi, T., Fujimori, T., Ueda, M. Hayashi, S., Kaibuchi, K., Miyata, T.
TAG-1–assisted progenitor elongation streamlines nuclear migration to optimize subapical crowding. Nat. Neurosci., 16: 1556-1566 (2013) DOI: 10.1038/nn.3525
FRET Imaging
Real-time/real-color FRET imaging/Yellow Cameleon
Takeharu Nagai, and Atsushi Miyawaki A real-time movie of confocal real color images and corresponding pseudocolored ratio images showing Ca2+ waves inside cells, which were evoked by histamine, in HeLa cells expressing YC3.60(Yellow Cameleon). The images were taken at video rate (30 Hz) using a color 3CCD camera for simultaneous acquisition of CFP (cyan-emitting mutant of GFP) and YFP (yellow-emitting mutant of GFP) images. To improve z-axis resolution, a spinning disk confocal unit was placed in front of the camera. Ten micromolar histamines was added to the recording medium to activate receptor-evoked Ca2+ release from the endoplasmic reticulum.
Left: A real-time movie of confocal real color images
Right: Corresponding pseudocolored ratio images
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Real-time/real-color FRET imaging/Yellow Cameleon
A real-time movie of confocal images and corresponding pseudocolored ratio images showing Ca2+ waves inside cells, which were evoked by histamine, in HeLa cells expressing YC3.60(Yellow Cameleon).
Left: A real-time movie of confocal image of YFP channel
Right: Corresponding pseudocolored ratio images
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Calcium Imaging
Real-time intracellular calcium dynamics of the Purkinje fibers in the perfused rat heart
*Movies from Tetsuro Takamatsu’s laboratory (In Japanese)
The fluo3-fluorescence (8 bits, pseudo-color image) of the perfused rat heart was visualized by the CSU-based real-time confocal microscopy at 30 frames/s.
Pixels 205 x 230. The scale bar denotes 50 m.
Microscope: BX50WI, Olympus、Objective lens: LUMIPlan FL x20, Olympus, with CSU-21,
CCD camera: ES310 Turbo, Roper Scientific & Image intensifier: VS4-1845, Videoscope.
Spatially uniform Ca2+ transients are identified in Purkinje fibers on the ventricular septal wall.
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Simultaneous imaging of phosphatidylinositol metabolism and Ca2+ levels in PC12h cells
BBRC 308 (2003) 673-678
Mitsuhiro Morita, Fumito Yoshiki, and Yoshihisa Kudo
Laboratory of Cellular Neurobiology, School of Life Science, Tokyo University of Pharmacy and Life Science (in Japanese)
Relationship between phosphatidylinositol metabolism and Ca 2+ level was analyzed with high spatial resolution at video rate in PC12h cells double-labeled with GFP fused with the pleckstrin homology domain and FuraRed,
CSU10, C6790 CCD camera, and W-View; simultaneous dual-color imaging system (Hamamatsu), Nikon E600FN microscope with Fluor 40X/0.8W.
Left: EGFP
Right: FraRed
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Functional multineuron calcium imaging
Yuji Ikegaya
Laboratory of Chemical Pharmacology, Graduate school of Pharmaceutical Sciences, The University of Tokyo.
fMCI is a functional imaging technique with multicell loading of calcium fluorophores. fMCI has unique advantages, including: i) recording en masse from hundreds of neurons in a wide area, ii) single-cell resolution, iii) identifiable location of neurons, and iv) detection of non-active neurons during the observation period
Spontaneous firing-induced somatic calcium spikes of CA3 pyramidal cells in a rat hippocampal slice culture loaded with Oregon Green 488 BAPTA-1AM
High-speed calcium imaging
Data: Yuji Ikegaya Ph.D., Graduate School of Pharmaceutical Sciences at the University of Tokyo
Cell assemblies in spontaneous activity of a CA3 neuron population
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Clustered synaptic inputs in a spontaneously active CA3 neuron
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in vivo imaging
Intravital Molecular Imaging
Satoshi Nishimura
Department of Cardiovascular Medicine, Graduate School of Medicine, The University of Tokyo
Dr. Satoshi Nishimura is a world-renowned expert of intravital molecular imaging; which means in vivo imaging of microcirculation and molecular dynamics in living animals with high spatiotemporal resolution.
Intravital Molecular imaging is a powerful tool to elucidate not only vascular pathological conditions such as arteriosclerosis but also to study molecular mechanisms of pathological conditions caused by complicated and multi-cellular abnormal interactions, such as cancer or metabolic syndrome.
He has developed an imaging system based on highly spatiotemporal imaging with the CSU and visualized microcirculation, vascular functions, and multi-cellular dynamics of target molecules in real-time and in three dimensions, in vivo.
Using this technique, he successfully elucidated how obese adipose tissue played a bad role in obesity.
An example of real-time movie of microcirculation in mice, which clearly shows dynamic movement and interactions among leukocytes, platelets, macrophages, and endothelium.
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Cellular kinetics in microcirculation
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Deformed erythrocyte and platelets in microcirculation
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Long-time, 4 colors, and 3D in vivo imaging.
Mikala Egeblad, Andrew Ewald, Zena Werb., UCSF, Dept of Anatomy
Researchers at UCSF developed in vivo imaging system capable of multicolor, 3D imaging at multi-points to observe tumor microenvironment in the same live mouse for a long time, by using the CSU.
Nuclear EGFP in Foxp3+ Tregs in a tumor within a live MMTVPyMT; ACTB-ECFP; Foxp3EGFP mouse.
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Membrane EGFP in CD11c+ dendritic-like cells in a tumor within a live MMTVPyMT; ACTB-ECFP; CD11-DTR-EGFP mouse.
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Example of migration of two myeloid cells at the border of a late carcinoma – a low-migratory, dextran-ingesting cell and a high-migratory, dextran-negative cell.
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Dynamics of several types of stromal cells in the different tumor micro environment for up to 12 hours to find different behaviors of each stromal cell
Green: c-fms-EGFP
Blue: ACTB-ECFP
Red: 10 kDa dextran
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Multi-color imaging
Multi-color imaging of live cells and tissues
Satoshi Nishimura
Department of Cardiovascular Medicine, Graduate School of Medicine, The University of Tokyo
3D Reconstruction image of intact mouse adipose tissues
Blue / adipocytes: BODIPY
Green / Nuclei: Hoechst33342
Red / collagen: isolectin Gs-IB4
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3D Reconstruction image of a blood vessel in mouse adipose tissues.
Blue / adipocytes: BODIPY
Green / Nuclei: Hoechst33342
Red/endothelial cells: isolectin Gs-IB4
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Escape of intracellular vesicles induced by mechanical stress
(By courtesy of Dr. Satoshi Nishimura, Department of Cardiovascular Medicine, Graduate School of Medicine, The University of Tokyo and Dr. Seiryo Sugiura, Department of Human and Engineered Environmental Studies, Graduate School of Frontier Sciences, The University of Tokyo.)
Cultured NIH3T3 cells, excerpt from time-lapse images taken at 3.6 sec. interval.
Blue / Nuclei: Hoechst33342
Green / eGFP-Actin
Red / Vesicles: Cholera Toxin
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3D reconstruction image of blood vessels in mouse adipose tissues (unfixed)
(By courtesy of Dr. Satoshi Nishimura, Department of Cardiovascular Medicine, Graduate School of Medicine, The University of Tokyo and Dr. Seiryo Sugiura, Department of Human and Engineered Environmental Studies, Graduate School of Frontier Sciences, The University of Tokyo.)
Blue / Nuclei: Hoechst33342
Green / actin rhodamine
Red / eGFP-GULT4
Long-term,multi-dimensional livecell imaging
Long-term, Six-dimensional Live-cell Imaging
Kazuo Yamagata, PhD, Wakayama Lab (Laboratory for Genomic Reprogramming), Center for Developmental Biology, RIKEN
(Present post: Research Institute for Microbial Diseases, Osaka University)
IVF embryos were injected with a mixture of mRNAs for EGFP-α -tublin (Tublin, green) and H2B-mRFP1(H2B, red). The embryos were imaged by being exposed to two different wavelengths of excitation(488 and 561 nm) at 7.5min intervals for about 70h and 51 images were acqired in the Z axis at each time point( total of 56,814 fluorescent images). As a result of transplanting the embryos after imaging, all the pups were healthy, reproductively normal, and not transgenic. Thus, this live-cell imaging technology is safe for full-term mouse development.
IVF: in vitro fretilization
Left: DIC
Right: Confocal
Tubulin: Green
(EGFP- α -tubulin)
Null: Red
(H2B-mRFP1)
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Micro PIV
Visualization of the warped interface between two fluids at a curve downstream of the Y junction
(By courtesy of Seika Corporation (Japanese content). This experiment was done in the collaboration of the Oshima Laboratory, Institute of Industrial Science, The University of Tokyo.)
Curved micro-channel (width 100um × depth 50um)
Shape analysis by volume rendering.
Instantaneous velocity distribution analysis of fluid flow in a round shape microchannel (width 100um × depth 50um)
(By courtesy of Seika Corporation (Japanese content). This experiment was done in the collaboration of the Oshima Laboratory, Institute of Industrial Science, The University of Tokyo.)
Curved micro-channel
(width 100um×depth 50um)
Shape analysis by volume rendering.
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Spinning Disk Confocal CSU
Using our proprietary dual spinning disk design, Yokogawa’s confocal scanner units transform optical microscopes by enabling real-time live cell imaging.