Urea inhibits the activity of alkaline phosphatase during the reaction course. The
inactivation is progressively stronger for the placental, intestinal and renal subforms.
Influence of reaction temperature, pH, type and molarity of buffer, magnesium chloride, albumin
and enzyme concentration on the inactivation mechanism is evaluated. In all experimental
conditions the process follows pseudofirst-order kinetics and the inactivation profiles are
distinct and typical for each enzymatic subform. With a simple graphical analysis, a single
inactivation curve in controlled experimental conditions, allows the identification of each
isoenzyme from the slope and the calculation of the respective fractional amount from the
intercept of the time-activity plot.
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