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Pyruvate kinase activity determination using

Creatine kinase was purified from rabbit muscle by the method of Kuby et al, (4). Rabbit muscle pyruvate kinase was purchased from Boehringer. Porcine muscle adenylate kinase was purchased from Sigma, and was further purified by gel filtration on Sephadex G-50. The enzymes were homogeneous as judged by their specific activities and by their migration as single components in sodium dodecyl sulfate gel electrophoresis. Proton NMR spectra at 250 MHz of 0.5-2.0 mM enzyme sites in 0 solution were obtained with a Bruker WM 250 MHz pulse FT spectrometer at 25°. At least 256 transients were accumulated over 8192 data points using 16 bit A/D conversion. Relaxation rates and histidine pK values were determined by standard NMR methods (5, 6),... [Pg.125]

The lactate oxidation catalyzed by LMO forms the basis of several other multienzyme electrodes (Fig. 86). The LDH-LMO sensor has also been used to assay the activity of alanine aminotransferase (ALAT, EC 2.6.1.2) and pyruvate kinase (PK, EC 2.7.1.40) (Weigelt 1987 Weigelt et al., 1988). The sample was added to the NADH-containing measuring solution and when the steady state signal for endogenous lactate and pyruvate was attained the substrates of the enzyme to be determined... [Pg.201]

Pyruvate kinase (PK) activity in hemolyzed erythrocytes has been determined by using an LDH-lactate monooxygenase sequence electrode (Weigelt et al., 1988). The enzymes were immobilized in gelatin and attached to an oxygen probe. Since the sample material contains only... [Pg.309]

It was found that the enzyme is specific for (/ )-ATPaS but does not react with (S)-ATPaS. As shown in Scheme 43, when (/ )-ATPatS and l70-acetate are used as substrates, the 170 from acetate will be incorporated into the pro-5 position of AMPS if the reaction proceeds with retention of configuration or into the pro-/ position if inversion occurs. To determine the configuration of the 170-labeled AMPS (compound type 4), it is converted to (S)-ATPoS by stereospecific phosphorylation at the pro-/ oxygen catalyzed by adenylate kinase, followed by a second phosphorylation catalyzed by pyruvate kinase (144,145). By such a conversion, 170 should be incorporated into the nonbridging position of (5)-ATPaS if the step of acetate activation proceeds with retention of configuration. On the other hand, 170 should be located at the P—O—P bridging... [Pg.310]

N.m.r. has been used to study the active site of other zinc-containing enzymes. In bovine carbonic anhydrase there is a single zinc co-ordination site available for Cl interaction, and the latter can be inhibited by CN and acetazolamide. C1 Resonance has also been used to investigate the environmental diflFerences of the zinc in carbonic anhydrase isozymes and the activation of pyruvate kinase with zinc, and to determine the pJ values in cobalt(u)-carbonic anhydrase. It is suggested that, although the TpK of aquozinc is about 9, the environment of the zinc ion in carbonic anhydrase B greatly increases the tendency of a zinc-bound water molecule... [Pg.248]


See other pages where Pyruvate kinase activity determination using is mentioned: [Pg.95]    [Pg.190]    [Pg.826]    [Pg.115]    [Pg.346]    [Pg.235]    [Pg.35]    [Pg.111]    [Pg.763]    [Pg.496]    [Pg.105]    [Pg.616]    [Pg.230]    [Pg.234]   


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