Salih E, Malthouse J P, Kowlessur D, Jarvis M, O'Driscoll M, Brocklehurst K
Department of Biochemistry, St. Bartholomew's Hospital Medical College, University of London, U.K.
Biochem J. 1987 Oct 1;247(1):181-93. doi: 10.1042/bj2470181.
The characteristics of actinidin (EC 3.4.22.14) and papain (EC 3.4.22.2), two cysteine proteinases whose catalytic-site regions appear to superimpose to a degree that approaches atomic co-ordinate accuracy of both crystal structures, were evaluated by determining (a) the pH-dependence in acid media of the acylation process of the catalytic act (k+2/Ks) using N alpha-benzoyl-L-arginine p-nitroanilide (L-Bz-Arg-Nan) as substrate and (b) the sensitivity of the reactivity of the catalytic-site thiol group and its pH-dependence to structural change in small, thiol-specific, two-protonic-state reactivity probes (2,2'-dipyridyl disulphide and methyl 2-pyridyl disulphide) where enzyme-probe contacts should be restricted to areas close to the catalytic site. Distortion of the catalytic sites of the two enzymes at pH less than 4 was evaluated over time-scales appropriate for both stopped-flow reactivity probe kinetics (less than or equal to 1-2 s) and steady-state substrate catalysis kinetics (3-5 min) by using the 2,2'-dipyridyl disulphide monocation as a titrant for non-distorted catalytic sites. This permitted a lower pH limit to be defined for valid kinetic analysis of both types. The behaviour of the enzymes at pH less than 4 requires a kinetic model in which the apparently biomolecular reaction of enzyme with probe reagent is separated from the process leading to loss of conformational integrity by a potentially reversible step. The acylation of actinidin with L-Bz-Arg-Nan in acidic media occurs in two protonic states, one produced by raising the pH across pKa less than 4 which probably characterizes the formation of -S-/-ImH+ ion pair (pKa approx. 3) and the other, of higher reactivity, produced by raising the pH across pKa 5.5, which may characterize rearrangement of catalytic-site geometry. The pH-dependence of the acylation of papain by L-Bz-Arg-Nan is quite different and is not influenced by protonic dissociation with pKa values in the range 5-6. The earlier conclusion that the acylation of papain depends on two protonic dissociations each with pKa approx. 4 was confirmed. This argument is now more firmly based because titration with 2,2'-dipyridyl disulphide permits the loss of conformational integrity to be taken into account in the analysis of the kinetic data at very low pH. Methyl 2-pyridyl disulphide was synthesized by reaction of pyridine-2-thione with methyl methanethiolsulphonate and its pKa at I = 0.1 was determined by spectral analysis at 307 nm to be 2.8.(ABSTRACT TRUNCATED AT 400 WORDS)
对肌动蛋白酶(EC 3.4.22.14)和木瓜蛋白酶(EC 3.4.22.2)这两种半胱氨酸蛋白酶的特性进行了评估。这两种酶催化位点区域似乎在一定程度上相互重叠,接近两种晶体结构的原子坐标精度。评估方法如下:(a)以Nα-苯甲酰-L-精氨酸对硝基苯胺(L-Bz-Arg-Nan)为底物,测定催化行为(k+2/Ks)在酸性介质中酰化过程的pH依赖性;(b)在小的、硫醇特异性的双质子态反应性探针(2,2'-二吡啶二硫化物和2-吡啶基甲基二硫化物)中,测定催化位点硫醇基团反应性的敏感性及其pH依赖性,其中酶与探针的接触应限于靠近催化位点的区域。通过使用2,2'-二吡啶二硫化物单阳离子作为未变形催化位点的滴定剂,在适合停流反应性探针动力学(小于或等于1 - 2秒)和稳态底物催化动力学(3 - 5分钟)的时间尺度上,评估了两种酶在pH小于4时催化位点的变形情况。这为两种类型的有效动力学分析确定了较低的pH极限。酶在pH小于4时的行为需要一个动力学模型,其中酶与探针试剂的表观双分子反应通过一个潜在的可逆步骤与导致构象完整性丧失的过程分开。在酸性介质中,肌动蛋白酶与L-Bz-Arg-Nan的酰化反应发生在两种质子态下,一种是通过将pH升高超过pKa小于4产生的,这可能表征-S-/-ImH+离子对的形成(pKa约为3),另一种反应性较高,是通过将pH升高超过pKa 5.5产生的,这可能表征催化位点几何结构的重排。L-Bz-Arg-Nan对木瓜蛋白酶的酰化反应的pH依赖性则大不相同,不受pKa值在5 - 6范围内的质子解离影响。早期关于木瓜蛋白酶酰化反应依赖于两个pKa约为4的质子解离的结论得到了证实。现在这个论点有了更坚实的基础,因为用2,2'-二吡啶二硫化物滴定可以在极低pH下分析动力学数据时考虑构象完整性的丧失。2-吡啶基甲基二硫化物是通过吡啶-2-硫酮与甲硫醇磺酸甲酯反应合成的,通过在307 nm处的光谱分析确定其在I = 0.1时的pKa为2.8。(摘要截短于400字)
