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   English Wikipedia
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  lüll Current cytochemical techniques for the investigation of peroxisomes  A review Fahimi HD; Baumgart EJ Histochem Cytochem  1999[Oct]; 47 (10): 1219-32The past decade has witnessed unprecedented progress in elucidation of the  complex problems of the biogenesis of peroxisomes and related human disorders,  with further deepening of our understanding of the metabolic role of this  ubiquitous cell organelle. There have been many recent reviews on biochemical and  molecular biological aspects of peroxisomes, with the morphology and  cytochemistry receiving little attention. This review focuses on the  state-of-the-art cytochemical techniques available for investigation of  peroxisomes. After a brief introduction into the use of the 3,3'-diaminobenzidine  method for localization of catalase, which is still most commonly used for  identification of peroxisomes, the cerium technique for detection of peroxisomal  oxidases is discussed. The influence of the buffer used in the incubation medium  on the ultrastructural pattern obtained in rat liver peroxisomes in conjunction  with the localization of urate oxidase in their crystalline cores is discussed,  particularly since Tris-maleate buffer inhibits the enzyme activity. In  immunocytochemistry, quantitation of immunogold labeling by automatic image  analysis enables quantitative assessment of alterations of proteins in the matrix  of peroxisomes. This provides a highly sensitive approach for analysis of  peroxisomal responses to metabolic alterations or to xenobiotics. The recent  evidence suggesting the involvement of ER in the biogenesis of "preperoxisomes"  is mentioned and the potential role of preembedding immunocytochemistry for  identification of ER-derived early peroxisomes is emphasized. The use of GFP  expressed with a peroxisomal targeting signal for the investigation of  peroxisomes in living cells is briefly discussed. Finally, the application of in  situ hybridization for detection of peroxisomal mRNAs is reviewed, with emphasis  on a recent protocol using perfusion-fixation, paraffin embedding, and  digoxigenin-labeled cRNA probes, which provides a highly sensitive method for  detection of both high- and low-abundance mRNAs encoding peroxisomal proteins. (J  Histochem Cytochem 47:1219-1232, 1999)|Animals[MESH]|Catalase/metabolism[MESH]|Cerium/chemistry[MESH]|Histocytochemistry/*methods[MESH]|Immunoenzyme Techniques[MESH]|In Situ Hybridization[MESH]|Microbodies/*enzymology/*ultrastructure[MESH]|Microscopy, Fluorescence[MESH]|Microscopy, Immunoelectron[MESH]|Oxidoreductases/metabolism[MESH] |