ABSTRACT
Cartilage is a vital organ to maintain joint function. Upon arthritis, proteolytic enzymes initiate degradation of cartilage extracellular matrix (ECM) resulting in eventual loss of joint function. However, there are only limited ways of non-invasively monitoring early chemical changes in cartilage matrix. Here we report that the autofluorescence decay profiles of cartilage tissue are significantly affected by proteolytic degradation of cartilage ECM and can be characterised by measurements of the autofluorescence lifetime (AFL). A compact multidimensional fluorometer coupled to a fibre-optic probe was developed for single point measurements of AFL and applied to cartilage that was treated with different proteinases. Upon treating cartilage with bacterial collagenase, trypsin or matrix metalloproteinase 1, a significant dose and time dependent decrease of AFL was observed. Our data suggest that AFL of cartilage tissue is a potential non-invasive readout to monitor cartilage matrix integrity that may contribute to future diagnosis of cartilage defects as well as monitoring the efficacy of anti-joint therapeutic agents.
Subject(s)
Biomarkers/metabolism , Cartilage/physiopathology , Extracellular Matrix Proteins/metabolism , Extracellular Matrix/pathology , Optical Imaging/methods , Proteolysis , Animals , Cartilage/metabolism , Cattle , Collagenases , Extracellular Matrix/metabolism , Fluorometry/methods , Swine , TrypsinABSTRACT
We performed analyses of the molecular mechanisms involved in the regulation of phospholipase Cγ2 (PLCγ2). We identified several regions in the PLCγ-specific array, γSA, that contribute to autoinhibition in the basal state by occlusion of the catalytic domain. While the activation of PLCγ2 by Rac2 requires stable translocation to the membrane, the removal of the domains required for membrane translocation in the context of an enzyme with impaired autoinhibition generated constitutive, highly active PLC in cells. We further tested the possibility that the interaction of PLCγ2 with its activator protein Rac2 was sufficient for activation through the release of autoinhibition. However, we found that Rac2 binding in the absence of lipid surfaces was not able to activate PLCγ2. Together with other observations, these data suggest that an important consequence of Rac2 binding and translocation to the membrane is that membrane proximity, on its own or together with Rac2, has a role in the release of autoinhibition, resulting in interfacial activation.
Subject(s)
Cell Membrane/metabolism , Enzyme Activation , Phospholipase C gamma/metabolism , rac GTP-Binding Proteins/metabolism , Animals , COS Cells , Cell Line , Chlorocebus aethiops , Humans , Phospholipase C gamma/chemistry , Protein Binding , Protein Structure, Tertiary , Protein TransportABSTRACT
We applied fluorescence lifetime imaging microscopy to map the microenvironment of the myosin essential light chain (ELC) in permeabilized skeletal muscle fibers. Four ELC mutants containing a single cysteine residue at different positions in the C-terminal half of the protein (ELC-127, ELC-142, ELC-160, and ELC-180) were generated by site-directed mutagenesis, labeled with 7-diethylamino-3-((((2-iodoacetamido)ethyl)amino)carbonyl)coumarin, and introduced into permeabilized rabbit psoas fibers. Binding to the myosin heavy chain was associated with a large conformational change in the ELC. When the fibers were moved from relaxation to rigor, the fluorescence lifetime increased for all label positions. However, when 1% stretch was applied to the rigor fibers, the lifetime decreased for ELC-127 and ELC-180 but did not change for ELC-142 and ELC-160. The differential change of fluorescence lifetime demonstrates the shift in position of the C-terminal domain of ELC with respect to the heavy chain and reveals specific locations in the lever arm region sensitive to the mechanical strain propagating from the actin-binding site to the lever arm.
Subject(s)
Microscopy, Fluorescence/methods , Muscle Fibers, Skeletal/metabolism , Myosin Light Chains/chemistry , Myosin Light Chains/metabolism , Animals , Biomechanical Phenomena , Fluorescent Dyes/metabolism , Humans , Models, Molecular , Muscle Fibers, Skeletal/chemistry , Muscle Relaxation , Myosin Heavy Chains/metabolism , Permeability , Protein Conformation , RabbitsABSTRACT
We describe a fluorescence lifetime imaging endomicroscope employing a fibre bundle probe and time correlated single photon counting. Preliminary images of stained pollen grains, eGFP-labelled cells exhibiting Förster resonant energy transfer and tissue autofluorescence are presented.
Subject(s)
Endoscopes , Endoscopy/methods , Microscopy, Confocal/instrumentation , Microscopy, Fluorescence/instrumentation , Animals , COS Cells , Chlorocebus aethiops , Fluorescence , Green Fluorescent Proteins/metabolism , Photons , Pollen , Rats , Tendons/anatomy & histology , Time FactorsABSTRACT
OBJECTIVE: A hallmark of rheumatoid arthritis (RA) is invasion of the synovial pannus into cartilage, and this process requires degradation of the collagen matrix. The aim of this study was to explore the role of one of the collagen-degrading matrix metalloproteinases (MMPs), membrane type 1 MMP (MT1-MMP), in synovial pannus invasiveness. METHODS: The expression and localization of MT1-MMP in human RA pannus were investigated by Western blot analysis of primary synovial cells and immunohistochemical analysis of RA joint specimens. The functional role of MT1-MMP was analyzed by 3-dimensional (3-D) collagen invasion assays and a cartilage invasion assay in the presence or absence of tissue inhibitor of metalloproteinases 1 (TIMP-1), TIMP-2, or GM6001. The effect of adenoviral expression of a dominant-negative MT1-MMP construct lacking a catalytic domain was also examined. RESULTS: MT1-MMP was highly expressed at the pannus-cartilage junction in RA joints. Freshly isolated rheumatoid synovial tissue and isolated RA synovial fibroblasts invaded into a 3-D collagen matrix in an MT1-MMP-dependent manner. Invasion was blocked by TIMP-2 and GM6001 but not by TIMP-1. Invasion was also inhibited by the overexpression of a dominant-negative MT1-MMP, which inhibits collagenolytic activity and proMMP-2 activation by MT1-MMP on the cell surface. Synovial fibroblasts also invaded into cartilage in an MT1-MMP-dependent manner. This process was further enhanced by removing aggrecan from the cartilage matrix. CONCLUSION: MT1-MMP serves as an essential collagen-degrading proteinase during pannus invasion in human RA. Specific inhibition of MT1-MMP-dependent invasion may represent a novel therapeutic strategy for RA.
Subject(s)
Arthritis, Rheumatoid/metabolism , Arthritis, Rheumatoid/pathology , Cell Movement/physiology , Matrix Metalloproteinase 14/metabolism , Synovial Membrane/metabolism , Synovial Membrane/pathology , Cell Movement/drug effects , Cells, Cultured , Collagen/metabolism , Dipeptides/pharmacology , Dose-Response Relationship, Drug , Humans , Protease Inhibitors/pharmacology , Synovial Membrane/drug effects , Tissue Inhibitor of Metalloproteinase-1/pharmacology , Tissue Inhibitor of Metalloproteinase-2/pharmacologyABSTRACT
We describe a simple implementation of a slit scanning confocal microscope to obtain an axial resolution better than that of a point-scanning confocal microscope. Under slit illumination, images of a fluorescent object are captured using an array detector instead of a line detector so that out-of-focus light is recorded and then subtracted from the adjacent images. Axial resolution after background subtraction is 2.2 times better than the slit confocal resolution, and out-of-focus image suppression is calculated to attenuate with defocus faster by 1 order of magnitude than in the point confocal case.
Subject(s)
Image Processing, Computer-Assisted/methods , Microscopy, Confocal/instrumentation , Microscopy, Confocal/methods , Algorithms , Equipment Design , Fluorescence , Fluorescent Dyes/pharmacology , Models, Statistical , Pollen/chemistry , Reproducibility of Results , Subtraction TechniqueABSTRACT
Fluorescence lifetime imaging (FLIM) is used to quantitatively map the concentration of a small molecule in three dimensions in a microfluidic mixing device. The resulting experimental data are compared with computational fluid-dynamics (CFD) simulations. A line-scanning semiconfocal FLIM microscope allows the full mixing profile to be imaged in a single scan with submicrometer resolution over an arbitrary channel length from the point of confluence. Following experimental and CFD optimization, mixing times down to 1.3+/-0.4 ms were achieved with the single-layer microfluidic device.
Subject(s)
Microfluidics , Microscopy, Fluorescence/methods , Calibration , Equipment Design , Fluorescence , Imaging, Three-Dimensional , Kinetics , Microfluidic Analytical Techniques/instrumentation , Microscopy, Fluorescence/instrumentation , Time FactorsABSTRACT
We report a novel, compact and automated multidimensional spectrofluorometer that exploits a fibre-laser-pumped ultrafast supercontinuum source to provide resolution with respect to intensity, excitation and emission wavelength, decay time and polarisation. This instrument has been applied to study the photophysics of the phase-sensitive membrane probe di-4-ANEPPDHQ and to characterise protein-protein interactions via Förster resonance energy transfer. It can be applied to in situ measurements via a fibre-optic probe in medical and other contexts and is demonstrated here to provide a comprehensive characterisation of tissue autofluorescence.
Subject(s)
Spectrometry, Fluorescence/instrumentation , Cartilage/chemistry , Cell Membrane/chemistry , Equipment Design , Fluorescence Resonance Energy Transfer/instrumentation , Fluorescent Dyes , Humans , In Vitro Techniques , Lipid Bilayers/chemistry , Microscopy, Fluorescence, Multiphoton/instrumentation , Optical Fibers , Photochemical Processes , Protein Interaction Mapping/instrumentation , Pyridinium Compounds/chemistryABSTRACT
We present a time-gated, optically sectioned, hyperspectral fluorescence lifetime imaging (FLIM) microscope incorporating a tunable supercontinuum excitation source extending into the UV. The system is capable of resolving the excitation spectrum, emission spectrum, and fluorescence decays in an optically sectioned image.
Subject(s)
Image Processing, Computer-Assisted/methods , Microscopy, Fluorescence/methods , Animals , Collagen/chemistry , Collagen/ultrastructure , Convallaria/cytology , Image Processing, Computer-Assisted/instrumentation , Microscopy, Fluorescence/instrumentation , Microscopy, Ultraviolet/instrumentation , Microscopy, Ultraviolet/methods , Rats , Tail/cytologyABSTRACT
We report a rapid hyperspectral fluorescence lifetime imaging (FLIM) instrument that exploits high-speed FLIM technology in a line-scanning microscope. We demonstrate the acquisition of whole-field optically sectioned hyperspectral fluorescence lifetime image stacks (with 32 spectral bins) in less than 40 s and illustrate its application to unstained biological tissue.
