Übersetzung für "Enzymology" in Deutsch

So she applied for the international doctoral programme Molecular Enzymology at TU Graz.

Coursework includes instruction in organic chemistry, protein chemistry, bioanalytical chemistry, enzymology, and others.

He investigated the regulation of the metabolism and the cell cycle and focussed on molecular biological and endocrinological topics as well as enzymology and the differentiation of the parenchyma of the liver.

From 1982 till 1993 he worked at the Institute of Applied Enzymology in Vilnius.

For some years, in histo- and cytochemical enzymology, detection methods have found a firm place which depends upon the esterolytic activity of the enzymes present in the systems to be determined (cf., for example, A. G. E. Pearse, Histochemistry, Theoretical and Applied).

The carrier-bound nucleic acid or protein fraction is now used as a column filling for affinity chromatography (see P. Cuatrecasas: Affinity Chromatography of Macromolecules: Advances in Enzymology.

Examples for components of this kind are substrates (for example alanine, aspartate, glutamate, pyruvate, 2-oxobutyrate, 2-oxoglutarate), auxiliary enzymes (for example malate dehydrogenase, lactate dehydrogenase, urease, glutamate dehydrogenase), other coenzymes such as adenosine diphosphate or adenosine triphosphate, or buffer substances that are common in enzymology, such as trishydroxymethylaminomethane-HCl and others as specified above.

The properties of the proteolytic enzymes, in particular their biochemical actions, are described in the following literature: G. E. Perlmann and L. Lorand, Methods in Enzymology, 19 (1970) 199 to 215;

The bifunctional reagents used are built up either symmetrically or unsymmetrically (F. Wold, Methods in Enzymology 11, page 617 et seq.

The oligosaccharides formed are determined with 3,5-dinitrosalicylic acid in accordance with the method of P. Berenfeld (Methods in Enzymology, Volume I, 149, Academic Press, 1955).

The maltose formed was determined with 3,5-dinitrosalicylic acid by the method of P. Berenfeld (Methods in Enzymology, Volume 5, 149;

Furthermore, by variation of the phosphate-trimethylammonium distance in the phosphaditylcholines, a breakdown by phospholipase C and D can, as desired, be slowed down or completely suppressed (Eibl and Kovatchev, Methods of Enzymology (1981), 72, 632).

Various metoods for the detection of proteases and esterases are also known from histochemical and cytochemical enzymology (compare, for example, A.G.E. Pearse, Histochemistry, Theoretical and Applied, 3rd edition, Churchill Livingstone, Edinburgh-London-New York 1968).

Various methods for the detection of proteases and esterases are also known from histochemical and cytochemical enzymology (compare, for example, A. G. E. Pearse, Histochemistry, Theoretical and Applied, 3rd edition, Churchill Livingstone, Edinburgh-London-New York 1968).

U.S. Pat. Nos. 4,626,506, 4,680,264 and 4,686,184 (Puhler et al.) and Simon et al. (Biotechnology, November, 1983 and Methods in Enzymology, vol. 118, pp. 640-659) teach the mutagenesis of gram-negative bacteria using mobilizable E. coli vectors.

Other vectors, such as pSUP102 or pSUP205, are known from the literature and are obtained according to analogous methods from known vectors (Simon et al., Methods of Enzymology 118 640 fl. (1986) and Biotechnology, November, 1983).

According to KISIEL and DAVIE's method (KISIEL, W. and DAVIE, E. W. Protein C. Methods in Enzymology 80, 320-332 (1981)), protein C is assayed in chromatographic fractions using the kaolin-cephalin clotting time of human citrated plasma as the indicator reaction.

Thus, for example, appropriate processes for the synthesis of the ether-glycero- and acyl-glycerophosphocholines are described in Methods in Enzymology, 98, 623/1983 and in Biochim.

A good overview of the current state-of-the-art in the purification of 5'-FMN is given in the reviews by P. Nielsen et al in Methods in Enzymology, 122 (1986), 209-220, and by R. Hausinger et al in ibid. 122 (1986), 199-208.