Your search keyword '"Multiphoton Fluorescence Microscopy"' showing total 14 results

1. Real-time interactive two-photon photoconversion of recirculating lymphocytes for discontinuous cell tracking in live adult mice.

Author

Chtanova T, Hampton HR, Waterhouse LA, Wood K, Tomura M, Miwa Y, Mackay CR, Brink R, and Phan TG

Subjects

Animals, Luminescent Proteins metabolism, Lymphocytes metabolism, Mice, Cell Tracking methods, Lymphocytes cytology, Microscopy methods, Photons

Abstract

The potential usefulness of intravital two-photon microscopy for fate mapping is limited by its inability to track cells beyond the confines of the imaging volume. Therefore, we have developed and validated a novel method for in vivo photolabelling of spatially-restricted cells expressing the Kaede optical highlighter by two-photon excitation. This has allowed us to optically mark a cohort of follicular B cells and track their dissemination from the original imaging volume in the lymph node to the spleen and contralateral lymph node. We also present the first demonstration, to our knowledge, of in vivo photoconversion of a freely moving single cell in a live adult animal. This method of `discontinuous' cell tracking therefore significantly extends the fate mapping capabilities of two-photon microscopy to delineate the spatiotemporal dynamics of cellular processes that span multiple anatomical sites at the single cell level., (Copyright © 2014 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2014

2. Two-Photon Fluorescence Microscopy and Applications in Angiogenesis and Related Molecular Events

Author

Sathya Kannan, Rosa Vinicius, Gopu Sriram, Tong Cao, Jerry Y. H. Fuh, Marcus Jin Fu Lee, Wen Feng Lu, and Muniraj Giridharan

Subjects

Microscope, Angiogenesis, Biomedical Engineering, Bioengineering, Biology, Regenerative Medicine, Two photon fluorescence, Biochemistry, Regenerative medicine, Multiphoton Fluorescence Microscopy, law.invention, Cell biology, Biomaterials, Cross-Sectional Studies, Microscopy, Fluorescence, Multiphoton, Microscopy, Fluorescence, law, Microscopy, Fluorescence microscope, Animals

Abstract

The role of angiogenesis in health and disease have gained considerable momentum in recent years. Visualizing angiogenic patterns and associated events of surrounding vascular beds in response to therapeutic and laboratory-grade biomolecules have become a commonplace in regenerative medicine and the biosciences. To aid imaging investigations in angiogenesis, the two-photon excitation fluorescence microscopy (2PEF), or multiphoton fluorescence microscopy is increasingly utilized in scientific investigations. The 2PEF microscope confers several distinct imaging advantages over other fluorescence excitation microscopy techniques - for the observation of in-depth, three-dimensional vascularity in a variety of tissue formats, including fixed tissue specimens and in vivo vasculature in live specimens. Understanding morphological and subcellular changes that occur in cells and tissues during angiogenesis will provide insights to behavioral responses in diseased states, advance the engineering of physiologically-relevant tissue models and provide biochemical clues for the design of therapeutic strategies. We review the applicability and limitations of the 2PEF microscope on the biophysical and molecular-level signatures of angiogenesis in various tissue models. Imaging techniques and strategies for best practices in 2PEF microscopy will be reviewed.

Published

2022

3. Integrated multimodal optical microscopy for structural and functional imaging of engineered and natural skin.

Author

Zhao, Youbo, Graf, Benedikt W., Chaney, Eric J., Mahmassani, Ziad, Antoniadou, Eleni, DeVolder, Ross, Kong, Hyunjoon, Boppart, Marni D., and Boppart, Stephen A.

Abstract

An integrated multimodal optical microscope is demonstrated for high-resolution, structural and functional imaging of engineered and natural skin. This microscope incorporates multiple imaging modalities including optical coherence (OCM), multi-photon (MPM), and fluorescence lifetime imaging microscopy (FLIM), enabling simultaneous visualization of multiple contrast sources and mechanisms from cells and tissues. Spatially co-registered OCM/MPM/FLIM images of multi-layered skin tissues are obtained, which are formed based on complementary information provided by different modalities, i.e., scattering information from OCM, molecular information from MPM, and functional cellular metabolism states from FLIM. Cellular structures in both the dermis and epidermis, especially different morphological and physiological states of keratinocytes from different epidermal layers, are revealed by mutually-validating images. In vivo imaging of human skin is also investigated, which demonstrates the potential of multimodal microscopy for in vivo investigation during engineered skin engraftment. This integrated imaging technique and microscope show the potential for investigating cellular dynamics in developing engineered skin and following in vivo grafting, which will help refine the control and culturing conditions necessary to obtain more robust and physiologically-relevant engineered skin substitutes. (© 2012 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim) [ABSTRACT FROM AUTHOR]

Published

2012

4. Two-photon microscopic analysis of acetylcholine-induced mucus secretion in guinea pig nasal glands.

Author

Oshima, Akihiro, Kojima, Tatsuya, Dejima, Kenji, Hisa, Yasuo, Kasai, Haruo, and Nemoto, Tomomi

Subjects

MUCUS, ACETYLCHOLINE, CALCIUM, MICROSCOPY, CELL physiology, BIOLOGICAL transport, GUINEA pigs as laboratory animals

Abstract

Abstract: The spatiotemporal changes in intracellular free Ca2+ concentration ([Ca2+]i) as well as fluid secretion and exocytosis induced by acetylcholine (ACh) in intact acini of guinea pig nasal glands were investigated by two-photon excitation imaging. Cross-sectional images of acini loaded with the fluorescent Ca2+ indicator fura-2 revealed that the ACh-evoked increase in [Ca2+]i was immediate and spread from the apical region (the secretory pole) of acinar cells to the basal region. Immersion of acini in a solution containing a fluorescent polar tracer, sulforhodamine B (SRB), revealed that fluid secretion, detected as a rapid disappearance of SRB fluorescence from the extracellular space, occurred exclusively in the luminal region and was accompanied by a reduction in acinar cell volume. Individual exocytic events were also visualized with SRB as the formation of Ω-shaped profiles at the apical membrane. In contrast to the rapidity of fluid secretion, exocytosis of secretory granules occurred with a delay of ∼70s relative to the increase in [Ca2+]i. Exocytic events also occurred deep within the cytoplasm in a sequential manner with the latency of secondary exocytosis being greatly reduced compared with that of primary exocytosis. The delay in sequential compound exocytosis relative to fluid secretion may be important for release of the viscous contents of secretory granules into the nasal cavity. [Copyright &y& Elsevier]

Published

2005

5. A stage-scanning two-photon microscope equipped with a temporal and a spatial pulse shaper

Author

Frederik Büchau, Yang Yang, Albrecht Lindinger, Alexander Patas, and Karsten Heyne

Subjects

Materials science, Microscope, 02 engineering and technology, 01 natural sciences, law.invention, 010309 optics, Optics, law, 0103 physical sciences, Microscopy, Chirp, Instrumentation, Two-photon excitation microscopy, Wavefront, Spatial light modulator, business.industry, Optical modulators, Feedback control system, 021001 nanoscience & nanotechnology, Laser, Pulse shaping, Multiphoton fluorescence microscopy, Coherent control, 0210 nano-technology, business

Abstract

Here, we present a stage-scanning two-photon microscope (2PM) equipped with a temporal pulse shaper and a spatial light modulator enabling full control over spectral and spatial phases of the exciting laser pulse. We demonstrate the capability of correcting wavefronts and temporal pulse distortions without cross-dependencies induced by optical elements at the same time enhancing the fluorescence signal. We implemented phase resolved interferometric spectral modulation for temporal pulse shaping and the iterative feedback adaptive compensation technique for spatial pulse modulation as iterative techniques. Sample distortions were simulated by cover glass plates in the optical path and by chirping the exciting laser pulses. Optimization of the spectral and spatial phases results in a signal increase of 30% and nearly complete recovery of the losses. Applying a measured spatial compensation phase within a real leaf sample shows the enhancement in contrast due to wavefront shaping with local fluorescence increase up to 75%. The setup allows full independent control over spatial and spectral phases keeping or improving the spatial resolution of our microscope and provides the optimal tool for sensitive non-linear and coherent control microscopy.

Published

2018

6. Multiphoton microscopy: a personal historical review, with some future predictions

Author

Colin J. R. Sheppard

Subjects

Paper, two-photon fluorescence, Microscope, Materials science, Biomedical Engineering, Nanotechnology, History, 21st Century, 01 natural sciences, Multiphoton Fluorescence Microscopy, law.invention, 010309 optics, Biomaterials, Special Section Celebrating Thirty Years of Multiphoton Microscopy in the Biomedical Sciences, Signal strength, law, Confocal microscopy, 0103 physical sciences, Microscopy, Humans, focal modulation microscopy, image scanning microscopy, fungi, Pulse duration, Second-harmonic generation, History, 20th Century, Atomic and Molecular Physics, and Optics, Electronic, Optical and Magnetic Materials, Microscopy, Fluorescence, Multiphoton, Multiphoton fluorescence microscope, Microscopy, Fluorescence, multiphoton microscopy, Forecasting, second-harmonic generation

Abstract

The historical development of multiphoton microscopy is described, starting with a review of two-photon absorption, and including two- and three-photon fluorescence microscopies, and second- and third-harmonic generation microscopies. The effects of pulse length on signal strength and breakdown are considered. Different contrast mechanisms, including use of nanoparticles, are discussed. Two new promising techniques that can be applied to multiphoton microscopy are described.

Published

2020

7. Mapping of hemoglobin in erythrocytes and erythrocyte ghosts using two photon excitation fluorescence microscopy

Author

Branislav M. Jelenkovic, Aleksandar J. Krmpot, Ana Stancic, Svetlana Z. Jovanić, Branko Bugarski, Dejan Pantelić, Ivana Drvenica, Mihailo D. Rabasović, Katarina Bukara, and Vesna Ilić

Subjects

0301 basic medicine, Erythrocytes, Swine, Echinocyte, Biomedical Engineering, 01 natural sciences, 010309 optics, Biomaterials, 03 medical and health sciences, Hemoglobins, Optics, Two-photon excitation microscopy, 0103 physical sciences, Microscopy, erythrocyte ghosts, medicine, Fluorescence microscope, Animals, Humans, business.industry, Chemistry, multiphoton fluorescence microscopy, Erythrocyte Membrane, hemoglobin, medicine.disease, Fluorescence, Atomic and Molecular Physics, and Optics, Hemolysis, Electronic, Optical and Magnetic Materials, Autofluorescence, 030104 developmental biology, Microscopy, Fluorescence, erythrocytes, Biophysics, Hemoglobin, ultrafast lasers, business, label-free imaging

Abstract

The present study describes utilization of two photon excitation fluorescence (2PE) microscopy for visualization of the hemoglobin in human and porcine erythrocytes and their empty membranes (i.e., ghosts). High-quality, label- and fixation-free visualization of hemoglobin was achieved at excitation wavelength 730 nm by detecting visible autofluorescence. Localization in the suspension and spatial distribution (i.e., mapping) of residual hemoglobin in erythrocyte ghosts has been resolved by 2PE. Prior to the 2PE mapping, the presence of residual hemoglobin in the bulk suspension of erythrocyte ghosts was confirmed by cyanmethemoglobin assay. 2PE analysis revealed that the distribution of hemoglobin in intact erythrocytes follows the cells’ shape. Two types of erythrocytes, human and porcine, characterized with discocyte and echinocyte morphology, respectively, showed significant differences in hemoglobin distribution. The 2PE images have revealed that despite an extensive washing out procedure after gradual hypotonic hemolysis, a certain amount of hemoglobin localized on the intracellular side always remains bound to the membrane and cannot be eliminated. The obtained results open the possibility to use 2PE microscopy to examine hemoglobin distribution in erythrocytes and estimate the purity level of erythrocyte ghosts in biotechnological processes.

Published

2016

8. Second harmonic generation microscopy in zebrafish

Author

Jayne M. Squirrell, Kevin W. Eliceiri, Anna Huttenlocher, and Danny C. LeBert

Subjects

0301 basic medicine, Microscopy, Wound Healing, Embryo, Nonmammalian, animal structures, Optical Imaging, fungi, Second-harmonic generation, Anatomy, Biology, Second Harmonic Generation Microscopy, biology.organism_classification, Multiphoton Fluorescence Microscopy, Article, 03 medical and health sciences, 030104 developmental biology, Optical imaging, Larva, Temporal resolution, Biophysics, Animals, Wound healing, Zebrafish

Abstract

Modern optical imaging has progressed rapidly with the ability to non-invasively image cellular and subcellular phenomena with high spatial and temporal resolution. In particular, emerging techniques such as Second Harmonic Generation Microscopy (SHG) can allow for the monitoring of intrinsic contrast, such as that from collagen, in live and fixed samples. When coupled with multiphoton fluorescence microscopy, SHG can be used to image interactions between cells and the surrounding extracellular environment. There is recent interest in using these approaches to study inflammation and wound healing in zebrafish, an important model for studying these processes. In this chapter we present the practical aspects of using second harmonic generation to image interactions between leukocytes and collagen during wound healing in zebrafish.

Published

2016

9. Point Spread Function Engineering for Super-Resolution Single-Photon and Multiphoton Fluorescence Microscopy

Author

Alberto Diaspro, Partha Pratim Mondal, and Hawkes, PW

Subjects

Point spread function, Photon, business.industry, Aperture, Computer science, Super-resolution microscopy, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Superresolution, Multiphoton Fluorescence Microscopy, Depth imaging, Optics, Microscopy, Instrumentation Appiled Physics, business

Abstract

Super-resolution imaging techniques are of paramount interest for applications in bioimaging and fluorescence microscopy. Recent advances in bioimaging demand application-tailored point spread functions. Here, we present some approaches for generating application-tailored point spread functions along with fast imaging capabilities. Aperture engineering techniques provide interesting solutions for obtaining desired system point spread functions. Specially designed spatial filters—realized by optical mask—are outlined both in a single-lens and 4Pi configuration. Applications include depth imaging, multifocal imaging, and super-resolution imaging. Such an approach is suitable for fruitful integration with most existing state-of-art imaging microscopy modalities.

Published

2013

10. Multiphoton histology of entire intact mouse organs

Author

Thomas H. Chia, Sonia Parra, Michael J. Levene, and Joseph P. Zinter

Subjects

Pathology, medicine.medical_specialty, Multiphoton fluorescence microscope, Microscopy, Second-harmonic imaging microscopy, Fluorescence microscope, medicine, Histology, sense organs, Biology, Multiphoton Fluorescence Microscopy, Mouse Intestine, Clearance

Abstract

We present multiphoton fluorescence microscopy and second harmonic imaging of entire intact, fixed and optically cleared mouse organs. We achieved imaging depths of several millimeters in mouse intestine, heart, lung, brain and other organs.

Published

2010

11. Three-dimensional multi-modal microscopy

Author

Charles A. DiMarzio

Subjects

Computer science, business.industry, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Process (computing), Multiphoton Fluorescence Microscopy, Laser technology, Modal, Microscopy, Microscopic imaging, Computer vision, Artificial intelligence, business, Epi fluorescence microscopy, Laser beams

Abstract

Advances in lasers in recent decades have led to novel techniques of microscopy that are only possible with powerful coherent sources. Modern electronic cameras and computers have made it possible to capture, process, and display the resulting images. The continued growth in computing power now makes it possible to combine images from different microscopic imaging modalities.

Published

2009

12. Principles of multiphoton microscopy

Author

Pamela A. Young and Kenneth W. Dunn

Subjects

Fluorescence-lifetime imaging microscopy, Pathology, medicine.medical_specialty, Materials science, Biomedical Research, Physiology, Context (language use), General Medicine, Kidney, Multiphoton Fluorescence Microscopy, Multiphoton fluorescence microscope, Microscopy, Fluorescence, Multiphoton, Tissue optics, Nephrology, Microscopy, Genetics, Fluorescence microscope, medicine, Animals, Preclinical imaging, Biomedical engineering

Abstract

Multiphoton fluorescence microscopy is a powerful, important tool in biomedical research that offers low photon toxicity and higher spatial and temporal resolution than other in vivo imaging modalities. The capability to collect images hundreds of micrometers into biological tissues provides an invaluable tool for studying cellular and subcellular processes in the context of tissues and organs in living animals. Multiphoton microscopy is based upon two-photon excitation of fluorescence that occurs only in a sub-femtoliter volume at the focus; by scanning the focus through a sample, 2- and 3-dimensional images can be collected. The complex 3-dimensional organization of the kidney makes it especially appropriate for multiphoton microscopic analysis, which has been used to characterize numerous aspects of renal physiology and pathophysiology in living rats and mice. However, the ability to collect fluorescence images deep into biological tissues raises unique problems not encountered in other forms of optical microscopy, including issues of probe access, and tissue optics. Future improvements in multiphoton fluorescence microscopy will involve optimizing objectives for the unique characteristics of multiphoton fluorescence imaging, improving the speed at which images may be collected and extending the depth to which imaging may be conducted.

Published

2006

13. Multiphoton fluorescence and second harmonic generation microscopy of different skin states

Author

Wen Lo, Chen-Yuan Dong, Sung-Jan Lin, Shiou-Hwa Jee, and Yen Sun

Subjects

Multiphoton fluorescence microscope, Optics, Materials science, integumentary system, Image quality, business.industry, Microscopy, High harmonic generation, Second-harmonic generation, Second Harmonic Generation Microscopy, business, Fluorescence, Multiphoton Fluorescence Microscopy

Abstract

In recent years, non-linear imaging techniques such as multiphoton fluorescence and harmonic generation microscopy have been successfully applied to dermatological imaging. Confocal-like image quality, enhanced depth penetration, and non-linear spectral signatures are among the main advantages of this family of techniques. In this presentation, we will focus on the applications of multiphoton microscopy to skin specimens in different physiological states. Images of normal and diseased tissue specimens will be presented and spectrally characterized. Our work has potential applications in developing multiphoton microscopy into a clinically applicable diagnostic tool.

Published

2005

14. Monitoring the transdermal delivery of fluorescent nanoparticles using multiphoton fluorescence microscopy

Author

Shiou-Hwa Jee, Chun Chai Yeh, Chen-Yuan Dong, Chia Chun Chen, Sung-Jan Lin, Pei Yue Huang, Chien Hsin Tso, Tze Lung Hsu, and Wen Lo

Subjects

Materials science, integumentary system, Quantum dot, fungi, Microscopy, food and beverages, Nanoparticle, Nanotechnology, Nanometre, Luminescence, Fluorescence, Multiphoton Fluorescence Microscopy, Transdermal

Abstract

An interesting area of applying multiphoton fluorescence microscopy is in investigating the delivery of fluorescent nanoparticles (quantum dots) across biological barriers such as the skin. Fluorescence nanoparticles are nanometer in size and understanding the delivery mechanisms of these materials across the skin can be important in understanding the delivery of important biological macromolecules for therapeutic purposes. In addition, pathological diagnosis can be performed with the successful delivery of fluorescent nanoparticles.

Published

2004