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A more sensitive modification of the catalase assay with the Clark oxygen electrode: Application to the kinetic study of the pea leaf enzyme

✍ Scribed by Luís A. del Río; M.Gómez Ortega; A.Leal López; J.López Gorgé

Publisher: Elsevier Science
Year: 1977
Tongue: English
Weight: 390 KB
Volume: 80
Category: Article
ISSN: 0003-2697
DOI: 10.1016/0003-2697(77)90662-5

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✦ Synopsis

A modification of the method of catalase determination by means of the Clark oxygen electrode is described. The assay is based on measurement of the initial rate at which oxygen is released by catalase in an oxygen-free buffer. Displacement of oxygen was brought about by flushing with nitrogen, and the substrate used was hydrogen peroxide at a 33.5 mM final concentration. The method is rapid and can be used with crude catalase preparations. Its sensitivity is at least 20 times higher than that of previous methods; it has an interval of measurable activity of about 0.01-8.4 pmol of O,/min and, therefore, is applicable to an 840-fold range of catalase concentrations. This modification was applied to the kinetic study of crude extracts of pea leaf catalase. An apparent K, of 0.190 M was calculated.

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✍ Laura Escobar; Carolina Salvador; Martha Contreras; J. Edgardo Escamilla 📂 Article 📅 1990 🏛 Elsevier Science 🌐 English ⚖ 678 KB

A method for recording O2 concentrations in nonconducting organic media with the Clark oxygen electrode was developed. Spontaneous oxidation of Na2S2O4 and the enzymatic reduction of NaBO3 or H2O2 by bovine liver catalase trapped in hydrated micelles of dioctylsulfosuccinate (AOT)/toluene were used