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Detection of cell type and marker specificity of nuclear binding sites for anionic carbohydrate ligands
Authors:M Chovanec  K Smetana Jr  T Purkrábková  Z Holíková  B Dvoránková  S André
Affiliation:1. Institute of Anatomy, Charles University, 1st Faculty of Medicine, U nemocnice 3, 128 00, Prague, 2, Czech Republic;2. Department of Otorhinolaryngology, Head and Neck Surgery, V úvalu 84, 150 06, Prague, 5, Czech Republicksmet@lf1.cuni.cz;4. 2nd Faculty of Medicine, Center of Cell Therapy and Tissue Repair, V úvalu 84, 150 06, Prague, 5, Czech Republic;5. Institute of Macromolecular Chemistry, Academy of Sciences of the Czech Republic, Heyrovského námestí 6, 162 06, Prague, 6, Czech Republic;6. Clinical Department of Hematology and Nephrology, U nemocnice 2 128 08, Prague, Czech Republic;7. 2nd Faculty of Medicine, Center of Cell Therapy and Tissue Repair, V úvalu 84, 150 06, Prague, 5, Czech Republic;8. 3rd Faculty of Medicine, Department of Burn Surgery, ?robárova 1150, 100 34, Prague, 10, Czech Republic;9. Institute of Macromolecular Chemistry, Academy of Sciences of the Czech Republic, Heyrovského námestí 6, 162 06, Prague, 6, Czech Republic
Abstract:The emerging functionality of glycosaminoglycan chains engenders interest in localizing specific binding sites using cytochemical tools. We investigated nuclear binding of labeled heparin, heparan sulfate, a sulfated fucan, chondroitin sulfate, and hyaluronic acid in epidermal keratinocytes, bone marrow stromal cells, 3T3 fibroblasts and glioma cells using chemically prepared biotinylated probes. Binding of the markers was cell-type specific and influenced by extraction of histones, but was not markedly affected by degree of proliferation, differentiation or malignancy. Cell uptake of labeled heparin and other selected probes and their transport into the nucleus also was monitored. Differences between keratinocytes and bone marrow stromal cells were found. Preincubation of permeabilized bone marrow stromal cells with label-free heparin reduced the binding of carrier-immobilized hydrocortisone to its nuclear receptors. Thus, these tools enabled binding sites for glycosaminoglycans to be monitored in routine assays.
Keywords:chromatin-fibroblast growth factor  glycohistochemistry  heparin  histones  hyaluronic acid  steroid hormones
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