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Search: WFRF:(Sjöstrand Johan 1936) > (1995-1999) > Proteolysis in huma...

Proteolysis in human lens epithelium determined by a cell-permeable substrate

Karlsson, Jan-Olof, 1944 (author)
Gothenburg University,Göteborgs universitet,Institutionen för anatomi och cellbiologi,Institute of Anatomy and Cell Biology
Andersson, Madeleine (author)
Gothenburg University,Göteborgs universitet,Institutionen för klinisk neurovetenskap, Sektionen för oftalmologi,Institute of Clinical Neurosciences, Section of Ophtalmology
Kling-Petersen, Anne, 1962 (author)
Gothenburg University,Göteborgs universitet,Institutionen för anatomi och cellbiologi,Institute of Anatomy and Cell Biology
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Sjöstrand, Johan, 1936 (author)
Gothenburg University,Göteborgs universitet,Institutionen för klinisk neurovetenskap, Sektionen för oftalmologi,Institute of Clinical Neurosciences, Section of Ophtalmology
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 (creator_code:org_t)
1999
1999
English.
In: Invest Ophthalmol Vis Sci. ; 40:1, s. 261-4
  • Journal article (peer-reviewed)
Abstract Subject headings
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  • PURPOSE: To develop a system for continuous evaluation of proteolytic activity in human lens epithelium and to characterize factors of importance for the regulation of proteolytic activity in lens epithelial cells. METHODS: Human lens epithelial cells were obtained during cataract surgery. Capsule epithelium specimens consisted of the central parts of the anterior capsule and the underlying lens epithelium. The sample, with the cell-permeable substrate Suc-Leu-Leu-Val-Tyr-7-amino-4-methylcoumarin, was placed in a chamber, which was placed in a thermostat-controlled aluminum block. Fluorescence changes were continuously measured by the fiber optics of the luminometer, which was placed 5 mm above the buffer surface. RESULTS: After administration of substrate to the medium overlying the cells, the substrate was degraded at a relatively slow rate. Approximately 10 picomoles of amino-4-methylcoumarin were formed per minute. A significant increase of proteolytic activity could be observed after application of 1 microM ionomycin or 2 microM thapsigargin. No leakage of lactate dehydrogenase from the cells was observed during these procedures. Basal proteolytic activity was totally inhibited by the proteasome inhibitor lactacystin. Lactacystin also attenuated the response to ionomycin and thapsigargin. CONCLUSIONS: Human lens epithelium responds to increased Ca levels from external or internal stores with an increased proteolytic activity that may be mediated by calpain, by the proteasome, or by both. This calcium-dependent change in proteolytic activity may be of importance in the development of cataract.

Subject headings

MEDICIN OCH HÄLSOVETENSKAP  -- Medicinska och farmaceutiska grundvetenskaper -- Cell- och molekylärbiologi (hsv//swe)
MEDICAL AND HEALTH SCIENCES  -- Basic Medicine -- Cell and Molecular Biology (hsv//eng)

Keyword

derivatives/pharmacology
Calcium/metabolism
Calpain/*metabolism
*Cell Membrane Permeability
Cell Survival
Coumarins/*metabolism
Cysteine Endopeptidases/*metabolism
Enzyme Inhibitors/pharmacology
Epithelium/drug effects/enzymology
Human
Ionomycin/pharmacology
Lactate Dehydrogenase/metabolism
Lens
Crystalline/drug effects/*enzymology
Multienzyme Complexes/*metabolism
Oligopeptides/*metabolism
Substrate Specificity
Support
Non-U.S. Gov't
Thapsigargin/pharmacology

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art (subject category)

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MEDICAL AND HEAL ...
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University of Gothenburg

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