2001
DOI: 10.1177/002215540104901201
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Enzyme Cytochemical Techniques for Metabolic Mapping in Living Cells, with Special Reference to Proteolysis

Abstract: Specific enzymes play key roles in many pathophysiological processes and therefore are targets for therapeutic strategies. The activity of most enzymes is largely determined by many factors at the post-translational level. Therefore, it is essential to study the activity of target enzymes in living cells and tissues in a quantitative manner in relation to pathophysiological processes to understand its relevance and the potential impact of its targeting by drugs. Proteases, in particular, are crucial in every a… Show more

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Cited by 75 publications
(88 citation statements)
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“…Labeling stoichiometries were determined from the ratio of absorption in the visible (462 nm for proflavin, 512 nm for rhodamine 110) to that at 260 nm for tRNA (corrected for a contribution from the dye). The lower stoichiometry in the case of rhodamine may be due to its expected lower nucleophilicity as compared with proflavin, given its much lower pK a value (rhodamine 110, 4.3 [Boonacker and Van Noorden, 2001]; proflavin, 9.6 [Horobin et al 2006]) and its more hindered primary amine.…”
Section: Fluorescent Labeling Of D-containing Trnasmentioning
confidence: 99%
“…Labeling stoichiometries were determined from the ratio of absorption in the visible (462 nm for proflavin, 512 nm for rhodamine 110) to that at 260 nm for tRNA (corrected for a contribution from the dye). The lower stoichiometry in the case of rhodamine may be due to its expected lower nucleophilicity as compared with proflavin, given its much lower pK a value (rhodamine 110, 4.3 [Boonacker and Van Noorden, 2001]; proflavin, 9.6 [Horobin et al 2006]) and its more hindered primary amine.…”
Section: Fluorescent Labeling Of D-containing Trnasmentioning
confidence: 99%
“…To quantify overall protease activity, a microplate assay kit (Molecular Probes, Eugene, Oreg.) was utilized as previously described (4). Protease activ-ity was slightly decreased in the agr mutant (ϳ0.8-fold) but significantly increased in the sarA mutant (three-to fivefold; P Ͻ 0.05) compared to the parental strain (Fig.…”
mentioning
confidence: 95%
“…Excitation for cresyl violet was performed at 591 nm with a slit width of 10 nm and emission was detected at 628 nm with a slit width of 10 nm (Boonacker and Van Noorden 2001). Rhodamine 110 was excited at 491 nm with a slit width of 10 nm and emission was detected at 529 nm with a slit width of 10 nm (Boonacker and Van Noorden 2001). Fluorescence was measured continuously during the first 4 min of incubation.…”
Section: Fluorospectrometric Analysis Of Dppiv Activitymentioning
confidence: 99%