Ugarova N N, Rozhkova G D, Berezin I V
Biokhimiia. 1978 Aug;43(8):1382-9.
Thermostability of horseradish peroxidase modified by acetic, propionic, butyric, valeric and succinic anhydrides and trinitrobenzolsulfonic acid (TNBS) is studied within the temperature range of 56-80 degrees C. Acylation of 4 amino groups and arylation of 3 amino groups with TNBS are found to stabilize the enzyme, while modification of 6 groups decreases the enzyme stability. Chemical modification of peroxidase does not change its pH-dependence with respect to enzyme thermostability. Thermodynamic activation parameters of irreversible thermoinactivation are determined for native and modified peroxidase. Native peroxidase has deltaH not equal to = 30+/-1 kcal/mole and deltaS not equal to = 14 e. e.; modified by acid anhydrides peroxidase has deltaH not equal to within 64-87 kcal/mole and deltaS not equal to within 110-178 e. e. depending on the nature of a modifying agent. The effect of the structure of a radical introduced into the enzyme molecule, and of a number of modified epsilon-amino groups on thermoinactivation deltaH not equal to and deltaS not equal to values is discussed.
研究了经乙酸酐、丙酸酐、丁酸酐、戊酸酐和琥珀酸酐以及三硝基苯磺酸(TNBS)修饰的辣根过氧化物酶在56 - 80摄氏度温度范围内的热稳定性。发现4个氨基的酰化和3个氨基与TNBS的芳基化可使酶稳定,而6个基团的修饰则会降低酶的稳定性。过氧化物酶的化学修饰在酶热稳定性方面并未改变其pH依赖性。测定了天然和修饰过氧化物酶不可逆热失活的热力学活化参数。天然过氧化物酶的ΔH≠ = 30±1千卡/摩尔,ΔS≠ = 14 e.e.;经酸酐修饰的过氧化物酶,根据修饰剂的性质,ΔH≠在64 - 87千卡/摩尔范围内,ΔS≠在110 - 178 e.e.范围内。讨论了引入酶分子中的自由基结构以及修饰的ε - 氨基数量对热失活ΔH≠和ΔS≠值的影响。
