Your search keyword '"Issue 30"' showing total 2 results

1. Mesoscopic fluorescence tomography for in-vivo imaging of developing Drosophila

Author

Vinegoni, C., Razansky, D., Pitsouli, Chrysoula, Perrimon, N., Ntziachristos, V., Weissleder, R., and Pitsouli, Chrysoula [0000-0003-4074-9684]

Subjects

growth, development and aging, three dimensional imaging, article, methodology, tomography, Optical imaging, Scattering, Drosophila melanogaster, Imaging, Three-Dimensional, Animals, animal, Drosophila, fluorescence, Diffusion tomography, Fluorescence tomography, Issue 30, Mesoscopic imaging, Developmental Biology

Abstract

Visualizing developing organ formation as well as progession and treatment of disease often heavily relies on the ability to optically interrogate molecular and functional changes in intact living organisms. Most existing optical imaging methods are inadequate for imaging at dimensions that lie between the penetration limits of modern optical microscopy (0.5-1mm) and the diffusion-imposed limits of optical macroscopy (>1cm) [1]. Thus, many important model organisms, e.g. insects, animal embryos or small animal extremities, remain inaccessible for in-vivo optical imaging. Although there is increasing interest towards the development of nanometer-resolution optical imaging methods, there have not been many successful efforts in improving the imaging penetration depth. The ability to perform in-vivo imaging beyond microscopy limits is in fact met with the difficulties associated with photon scattering present in tissues. Recent efforts to image entire embryos for example [2,3] require special chemical treatment of the specimen, to clear them from scattering, a procedure that makes them suitable only for post-mortem imaging. These methods however evidence the need for imaging larger specimens than the ones usually allowed by two-photon or confocal microscopy, especially in developmental biology and in drug discovery. We have developed a new optical imaging technique named Mesoscopic Fluorescence Tomography [4], which appropriate for non-invasive in-vivo imaging at dimensions of 1mm-5mm. The method exchanges resolution for penetration depth, but offers unprecedented tomographic imaging performance and it has been developed to add time as a new dimension in developmental biology observations (and possibly other areas of biological research) by imparting the ability to image the evolution of fluorescence-tagged responses over time. As such it can accelerate studies of morphological or functional dependencies on gene mutations or external stimuli, and can importantly, capture the complete picture of development or tissue function by allowing longitudinal time-lapse visualization of the same, developing organism. The technique utilizes a modified laboratory microscope and multi-projection illumination to collect data at 360-degree projections. It applies the Fermi simplification to Fokker-Plank solution of the photon transport equation, combined with geometrical optics principles in order to build a realistic inversion scheme suitable for mesoscopic range. This allows in-vivo whole-body visualization of non-transparent three-dimensional structures in samples up to several millimeters in size. We have demonstrated the in-vivo performance of the technique by imaging three-dimensional structures of developing Drosophila tissues in-vivo and by following the morphogenesis of the wings in the opaque Drosophila pupae in real time over six consecutive hours. © JoVE 2006-2011 All Rights Reserved. Cited By :8

Published

2009

2. Combining QD-FRET and microfluidics to monitor DNA nanocomplex self-assembly in real-time

Author

Kam W. Leong, Yi-Ping Ho, Tza-Huei Wang, and Hunter H. Chen

Subjects

General Chemical Engineering, Microfluidics, Biomedical Engineering, fluorescence resonance energy transfer, quantum dots, Nanotechnology, 02 engineering and technology, Gene delivery, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, chemistry.chemical_compound, Fluorescence Resonance Energy Transfer, Plasmids, Microfluidics, Nanostructures, Dna, Quantum Dots, nanocomplexes, gene delivery, Issue 30, Microscale chemistry, 030304 developmental biology, 0303 health sciences, General Immunology and Microbiology, Chemistry, General Neuroscience, Rational design, DNA, self-assembly, 021001 nanoscience & nanotechnology, Molecular biology, Nanostructures, Förster resonance energy transfer, Self-assembly, Microreactor, 0210 nano-technology, Plasmids

Abstract

Advances in genomics continue to fuel the development of therapeutics that can target pathogenesis at the cellular and molecular level. Typically functional inside the cell, nucleic acid-based therapeutics require an efficient intracellular delivery system. One widely adopted approach is to complex DNA with a gene carrier to form nanocomplexes via electrostatic self-assembly, facilitating cellular uptake of DNA while protecting it against degradation. The challenge lies in the rational design of efficient gene carriers, since premature dissociation or overly stable binding would be detrimental to the cellular uptake and therapeutic efficacy. Nanocomplexes synthesized by bulk mixing showed a diverse range of intracellular unpacking and trafficking behavior, which was attributed to the heterogeneity in size and stability of nanocomplexes. Such heterogeneity hinders the accurate assessment of the self-assembly kinetics and adds to the difficulty in correlating their physical properties to transfection efficiencies or bioactivities. We present a novel convergence of nanophotonics (i.e. QD-FRET) and microfluidics to characterize the real-time kinetics of the nanocomplex self-assembly under laminar flow. QD-FRET provides a highly sensitive indication of the onset of molecular interactions and quantitative measure throughout the synthesis process, whereas microfluidics offers a well-controlled microenvironment to spatially analyze the process with high temporal resolution (~milliseconds). For the model system of polymeric nanocomplexes, two distinct stages in the self-assembly process were captured by this analytic platform. The kinetic aspect of the self-assembly process obtained at the microscale would be particularly valuable for microreactor-based reactions which are relevant to many micro- and nano-scale applications. Further, nanocomplexes may be customized through proper design of microfludic devices, and the resulting QD-FRET polymeric DNA nanocomplexes could be readily applied for establishing structure-function relationships.

Published

2009