Masters Advice Forum

Masters Discussion Forum

The following thread is brought to you by our sister Web site PostgraduateForum.com. If you wish to reply or post your own thread, you will be redirected to this site.

Search Forum Post new topic

Post reply on Postgrad Forum | Sort latest to earliest | Back to topics

Author	Message
eading [Registered User] 16 May 2013 09:08	Article Request from ScienceDirevt User: eading - 16 May 2013 09:08 Title : Catalase in vitro Authors : Hugo Aebi Journal : Methods in Enzymology Publication Date : 1984 Direct Link : "www.sciencedirect.com/science/article/pii/S0076687984050163" Abstract : Catalase exerts a dual function: (1) decomposition of H2O2 to give H2O and O2 (catalytic activity) and (2) oxidation of H donors, for example, methanol, ethanol, formic acid, phenols, with the consumption of 1 mol of peroxide (peroxide activity). The kinetics of catalase does not obey the normal pattern. Measurements of enzyme activity at substrate saturation or determination of the Ks is therefore impossible. In contrast to reactions proceeding at substrate saturation, the enzymic decomposition of H2O2 is a first-order reaction, the rate of which is always proportional to the peroxide concentration present. Consequently, to avoid a rapid decrease in the initial rate of the reaction, the assay must be carried out with relatively low concentrations of H2O2 (about 0.01 M). This chapter discusses the catalytic activity of catalase. The method of choice for biological material, however, is ultraviolet (UV) spectrophotometry. Titrimetric methods are suitable for comparative studies. For large series of measurements, there are either simple screening tests, which give a quick indication of the approximative catalase activity, or automated methods.
eading [Registered User] 16 May 2013 11:42	User: eading - 16 May 2013 11:42 My deepest thanks to you, Memo...

Author

Message

eading

[Registered User]
16 May 2013 09:08

Article Request from ScienceDirevt

User: eading - 16 May 2013 09:08

Title : Catalase in vitro
Authors : Hugo Aebi
Journal : Methods in Enzymology
Publication Date : 1984
Direct Link : "www.sciencedirect.com/science/article/pii/S0076687984050163"
Abstract :
Catalase exerts a dual function: (1) decomposition of H2O2 to give H2O and O2 (catalytic activity) and (2) oxidation of H donors, for example, methanol, ethanol, formic acid, phenols, with the consumption of 1 mol of peroxide (peroxide activity). The kinetics of catalase does not obey the normal pattern. Measurements of enzyme activity at substrate saturation or determination of the Ks is therefore impossible. In contrast to reactions proceeding at substrate saturation, the enzymic decomposition of H2O2 is a first-order reaction, the rate of which is always proportional to the peroxide concentration present. Consequently, to avoid a rapid decrease in the initial rate of the reaction, the assay must be carried out with relatively low concentrations of H2O2 (about 0.01 M). This chapter discusses the catalytic activity of catalase. The method of choice for biological material, however, is ultraviolet (UV) spectrophotometry. Titrimetric methods are suitable for comparative studies. For large series of measurements, there are either simple screening tests, which give a quick indication of the approximative catalase activity, or automated methods.