Fluorescent cytochemistry of acid phosphatase and demonstration of fluid-phase endocytosis using an azo dye method

Espada, Jesús; Horobin, Richard W.; Stockert, Juan C.

doi:10.1007/s004180050188

Cited by 13 publications

(9 citation statements)

References 32 publications

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“…Likewise, some reports on the subcellular localization of porphycenes are not based on their direct visualization by fluorescence microscopy, but on the observation of PStreated cells that are also labelled with fluorescent organelle probes, i.e., a colocalization strategy is used. On the other hand, although filamentous organelles such as mitochondria are easily identified in living cells, granular components are more heterogeneous, involving a wide spectrum of ATP-dependent acidic organelles, which comprise not only endosomes and lysosomes [256,257], but also all types of zymogen granules [258,259], vacuoles [260], clathrin-coated vesicles, multivesicular bodies, and Golgi components [261].…”

Section: Subcellular Localizationmentioning

confidence: 99%

Porphycenes: Facts and Prospects in Photodynamic Therapy of Cancer

Stockert¹,

Cañete²,

Juarranz³

et al. 2007

CMC

177

130

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The photodynamic process induces cell damage and death by the combined effect of a photosensitizer (PS), visible light, and molecular oxygen, which generate singlet oxygen ((1)O(2)) and other reactive oxygen species that are responsible for cytotoxicity. The most important application of this process with increasing biomedical interest is the photodynamic therapy (PDT) of cancer. In addition to hematoporphyrin-based drugs, 2nd generation PSs with better photochemical properties are now studied using cell cultures, experimental tumors and clinical trials. Porphycene is a structural isomer of porphyrin and constitutes an interesting new class of PS. Porphycene derivatives show higher absorption than porphyrins in the red spectral region (lambda > 600 nm, epsilon > 50000 M-(1)cm(-1)) owing to the lower molecular symmetry. Photophysical and photobiological properties of porphycenes make them excellent candidates as PSs, showing fast uptake and diverse subcellular localizations (mainly membranous organelles). Several tetraalkylporphycenes and the tetraphenyl derivative (TPPo) induce photodamage and cell death in vitro. Photodynamic treatments of cultured tumor cells with TPPo and its palladium(II) complex induce cytoskeletal changes, mitotic blockage, and dose-dependent apoptotic or necrotic cell death. Some pharmacokinetic and phototherapeutic studies on experimental tumors after intravenous or topical application of lipophilic alkyl-substituted porphycene derivatives are known. Taking into account all these features, porphycene PSs should be very useful for PDT of cancer and other biomedical applications.

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Section: Subcellular Localizationmentioning

confidence: 99%

Porphycenes: Facts and Prospects in Photodynamic Therapy of Cancer

Stockert¹,

Cañete²,

Juarranz³

et al. 2007

CMC

177

130

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“…Mechanisms for uptake and accumulation of fluorescent probes and drugs in the cytosol, endoplasmic reticulum, Golgi apparatus, lysosome, mitochondrium, and nucleus have been described (Espada et al 1997, Horobin 2001, Colston et al 2003, Horobin et al 2006, D'Souza et al 2008.…”

mentioning

confidence: 99%

Improving images of fluorescent cell labeling by background signal subtraction

Stockert

Villanueva

Cristóbal

et al. 2009

Biotechnic & Histochemistry

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The uptake and selective accumulation of fluorescent labels and drugs into organelles of cultured cells currently are widely investigated in biomedical research. In such studies, co-localization procedures are frequently used to identify the accumulation sites of compounds with biological activity. A drawback with fluorescent labeling is the autofluorescence of some cell organelles, which can hinder the precise assessment of co-localization. We report here labeling of the Golgi apparatus of A-549 cells using the photosensitizer zinc(II)-phthalocyanine (ZnPc) and co-localization with the Golgi probe NBD C6-ceramide. The blue autofluorescence signal of mitochondria can be subtracted easily from the original picture by image processing, after which the co-localization of the isolated red ZnPc signal with the green signal from the Golgi probe is considerably improved.

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“…Minimal autofluorescence and negligible fading rate are useful features of EY, AF and XP when excited by green light. It must be emphasized that, in this case, the red colour detected by fluorescence microscopy is due to the spectral profile of the barrier filter, which allows only the far red emission of fluorescent dyes to be observed ( Espada et al ., 1997 ).…”

Section: Discussionmentioning

confidence: 99%

“…Analytical and microscopical reactions based on fluorescence emission can be at least two orders of magnitude more sensitive than those based on light absorption ( Guilbault, 1973). Therefore, there is a growing interest in converting classical staining methods for bright‐field illumination into their corresponding counterparts for fluorescence microscopy ( Ferrer et al ., 1983 ; Molero et al ., 1986 ; Raap, 1986; Espada et al ., 1993 , 1997; Stockert & Trigoso, 1994). In this connection, the main advantages of using the emission properties of EY, AF and XP (from routinely HE‐ or MT‐stained tissues) are the higher sensitivity of selective fluorescence reactions, as well as possibilities for prolonged observation, re‐evaluation of the customary histological image of archive sections, and easy recognition of specific protein structures in embryonic tissues by fluorescence microscopy.…”

Section: Discussionmentioning

confidence: 99%

“…Spectrofluorometric studies were performed with 0.1 mg mL −1 solutions of EY, XP or AF, in either distilled water or 90% glycerol, using a Perkin‐Elmer fluorescence spectrophotometer 650‐10S, equipped with a 150‐W xenon lamp and the R 372 F photomultiplier detector. To compare spectroscopic and microscopic features of the fluorescent dyes, emission spectra were also recorded through the barrier filter (BF 590) corresponding to the microscopical green excitation, which was placed between the cuvette and the detector window ( Espada et al ., 1997 ). The Raman scattering of solvents was subtracted from emission spectra.…”

Section: Methodsmentioning

confidence: 99%

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Fluorescence microscopy of rat embryo sections stained with haematoxylin–eosin and Masson's trichrome method

Apgar

Juarranz

Espada

et al. 1998

Journal of Microscopy

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The fluorescence pattern induced by haematoxylin-eosin (HE) and Masson's trichrome (MT) staining methods on paraffin sections of rat embryos (from 13 to 18 days old) has been studied. Using optimal excitation (green light, 545 nm), HE- or MT-stained sections showed a selective red emission of the acidophilic tissue components, which was due to eosin Y in the case of HE and to acid fuchsin and/or xylidine ponceau in the case of MT. The fluorescence intensity induced by these anionic dyes was variable and related to the substrate nature and the embryo age. Whereas in young embryos only the immature red blood cells showed a noticeable fluorescence, in the oldest embryos there were also other tissue components that selectively fluoresced with these dyes, in particular fibre lens cells, elastic fibres, zymogen granules and muscle cells. Spectrofluorometric studies on free dyes and densitometric analysis of protein blots confirmed microscopical observations. Our results indicate that the standard HE and MT staining methods can be used in recognizing the appearance of specific protein structures in embryonic tissues by means of fluorescence microscopy.

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Fluorescent cytochemistry of acid phosphatase and demonstration of fluid-phase endocytosis using an azo dye method

Cited by 13 publications

References 32 publications

Porphycenes: Facts and Prospects in Photodynamic Therapy of Cancer

Porphycenes: Facts and Prospects in Photodynamic Therapy of Cancer

Improving images of fluorescent cell labeling by background signal subtraction

Fluorescence microscopy of rat embryo sections stained with haematoxylin–eosin and Masson's trichrome method

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