Publications

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A novel hyperspectral fluorescence microscope for high-resolution 3D optical sectioning of cells and other structures has been designed, constructed, and used to investigate a number of different problems. We have significantly extended new multivariate curve resolution (MCR) data analysis methods to deconvolve the hyperspectral image data and to rapidly extract quantitative 3D concentration distribution maps of all emitting species. The imaging system has many advantages over current confocal imaging systems including simultaneous monitoring of numerous highly overlapped fluorophores, immunity to autofluorescence or impurity fluorescence, enhanced sensitivity, and dramatically improved accuracy, reliability, and dynamic range. Efficient data compression in the spectral dimension has allowed personal computers to perform quantitative analysis of hyperspectral images of large size without loss of image quality. We have also developed and tested software to perform analysis of time resolved hyperspectral images using trilinear multivariate analysis methods. The new imaging system is an enabling technology for numerous applications including (1) 3D composition mapping analysis of multicomponent processes occurring during host-pathogen interactions, (2) monitoring microfluidic processes, (3) imaging of molecular motors and (4) understanding photosynthetic processes in wild type and mutant Synechocystis cyanobacteria.

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Multivariate data analysis applied to hyperspectral images offers the unique opportunity to dramatically increase the amount of information gained from a single biological sample. Numerous fluorescent tags can be used to perform multiple studies in parallel from a single hyperspectral image scan. Highly spatially and spectrally overlapping fluorophores can be separated even amidst a large autofluorescence background with the use of multivariate curve resolution methods. The results of two biological samples with multiple fluorescent labels are shown and compared to a traditional filter-based multispectral system. These examples illustrate the combined power of the hyperspectral microscope hardware and the multivariate image analysis software for biomedical imaging. This technique has the potential to be applied to a broad array of biological applications where fluorescent tags are a central and ubiquitous tool, and to biomedical areas that focus on the discovery and identification of weak, broad spectrum native fluorescence. © 2006 IEEE.

We have developed a new, high performance, hyperspectral microscope for biological and other applications. For each voxel within a three-dimensional specimen, the microscope simultaneously records the emission spectrum from 500 nm to 800 nm, with better than 3 nm spectral resolution. The microscope features a fully confocal design to ensure high spatial resolution and high quality optical sectioning. Optical throughput and detection efficiency are maximized through the use of a custom prism spectrometer and a backside thinned electron multiplying charge coupled device (EMCCD) array. A custom readout mode and synchronization scheme enable 512-point spectra to be recorded at a rate of 8300 spectra per second. In addition, the EMCCD readout mode eliminates curvature and keystone artifacts that often plague spectral imaging systems. The architecture of the new microscope is described in detail, and hyperspectral images from several specimens are presented.

Hyperspectral imaging provides complex image data with spectral information from many fluorescent species contained within the sample such as the fluorescent labels and cellular or pigment autofluorescence. To maximize the utility of this spectral imaging technique it is necessary to couple hyperspectral imaging with sophisticated multivariate analysis methods to extract meaningful relationships from the overlapped spectra. Many commonly employed multivariate analysis techniques require the identity of the emission spectra of each component to be known or pure component pixels within the image, a condition rarely met in biological samples. Multivariate curve resolution (MCR) has proven extremely useful for analyzing hyperspectral and multispectral images of biological specimens because it can operate with little or no a priori information about the emitting species, making it appropriate for interrogating samples containing autofluorescence and unanticipated contaminating fluorescence. To demonstrate the unique ability of our hyperspectral imaging system coupled with MCR analysis techniques we will analyze hyperspectral images of four-color in-situ hybridized rat brain tissue containing 455 spectral pixels from 550 - 850 nm. Even though there were only four colors imparted onto the tissue in this case, analysis revealed seven fluorescent species, including contributions from cellular autofluorescence and the tissue mounting media. Spectral image analysis will be presented along with a detailed discussion of the origin of the fluorescence and specific illustrations of the adverse effects of ignoring these additional fluorescent species in a traditional microscopy experiment and a hyperspectral imaging system.

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Basic research is needed to better understand the potential risk of dangerous biological agents that are unintentionally or intentionally introduced into a water distribution system. We report on our capabilities to conduct such studies and our preliminary investigations. In 2004, the Biofilms Laboratory was initiated for the purpose of conducting applied research related to biofilms with a focus on application, application testing and system-scale research. Capabilities within the laboratory are the ability to grow biofilms formed from known bacteria or biofilms from drinking water. Biofilms can be grown quickly in drip-flow reactors or under conditions more analogous to drinking-water distribution systems in annular reactors. Biofilms can be assessed through standard microbiological techniques (i .e, aerobic plate counts) or with various visualization techniques including epifluorescent and confocal laser scanning microscopy and confocal fluorescence hyperspectral imaging with multivariate analysis. We have demonstrated the ability to grow reproducible Pseudomonas fluorescens biofilms in the annular reactor with plate counts on the order of 10{sup 5} and 10{sup 6} CFU/cm{sup 2}. Stationary phase growth is typically reached 5 to 10 days after inoculation. We have also conducted a series of pathogen-introduction experiments, where we have observed that both polystyrene microspheres and Bacillus cereus (as a surrogate for B. anthracis) stay incorporated in the biofilms for the duration of our experiments, which lasted as long as 36 days. These results indicated that biofilms may act as a safe harbor for bio-pathogens in drinking water systems, making it difficult to decontaminate the systems.

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