Tang J C, Li S, McGray P, Vecchio A
Ann N Y Acad Sci. 1984;434:536-40. doi: 10.1111/j.1749-6632.1984.tb29889.x.
Tissue plasminogen activator (TPA) is a serine protease involved in the fibrinolytic system that dissolves blood clots. The enzyme catalyzes the conversion of a zymogen, plasminogen, to the enzymatically active form, plasmin, by limited proteolysis. In the course of searching for specific activity assays that might be useful in monitoring the purification of TPA, we have developed several coupled photometric assays. In addition, radioactive, agarose-plate, and other activity assays have also been considered and investigated for this purpose (Table 1). We have previously reported the one-step photometric procedure consisting of a thioester, thiobenzyl benzyloxycarbonyl-lysine (Z-Lys-S-Bzl) and fibrinogen-coated plates. It is simpler and more sensitive than the old two-step method without using immobilized fibrinogen. The new assay has been used successfully for protein purification and can be easily adapted to automated processes. Recently, other chromogenic substrates, D-Val-L-Leu-L-Lys-p-nitroanilide (Val-Leu-Lys-pNA) and D-Ile-L-Pro-L-Arg-p-nitroanilide (Ile-Pro-Arg-pNA) were also used in the one-step assay. It is found that TPA activity is greatly enhanced by immobilized fibrinogen and free fibrinogen when either the thioester. Val-Leu-Lys-pNA, or Ile-Pro-Arg-pNA were used in the colorimetric assay (Fig. 1, A-D). Enzyme kinetics studies indicate that the Km for plasminogen assayed on the thioester and fibrinogen-coated plates is 1.5 micrograms per ml, which is substantially lower than that observed in untreated plates (4.8 micrograms per ml). This is not due to the effect of fibrinogen on the second step of the coupled photometric assay because there is no change in the plasmin activity under these conditions (Fig. 1E). Similar results in TPA activation have also been observed, when fibrin-coated plates were used. Free fibrinogen, which is an activator of TPA, has been included in the standard assay mixture. We are able to detect less than 1 ng of TPA activity within a one-hour incubation time at 20 degrees C (Fig. 2A). In the thioester assay, however, high concentrations of reducing agents and nonspecific proteins cause significant background due to the interaction of DTNB with these reagents. 125I-labeled fibrin-coated plates had been extensively used in the past for urokinase and TPA assays. Although the sensitivity of the radioactive procedure is equivalent to that of the thioester photometric method, it appears that the kinetics of the enzyme are not easy to follow nor is the reproducibility great.(ABSTRACT TRUNCATED AT 400 WORDS)
组织型纤溶酶原激活剂(TPA)是一种参与溶解血凝块的纤维蛋白溶解系统的丝氨酸蛋白酶。该酶通过有限的蛋白水解作用催化酶原纤溶酶原转化为具有酶活性的形式——纤溶酶。在寻找可能有助于监测TPA纯化的特异性活性测定方法的过程中,我们开发了几种偶联光度测定法。此外,还为此考虑并研究了放射性、琼脂糖平板和其他活性测定法(表1)。我们之前报道了一种一步光度法,该方法由硫酯、硫代苄基苄氧羰基赖氨酸(Z-Lys-S-Bzl)和纤维蛋白原包被的平板组成。它比旧的两步法更简单、更灵敏,且无需使用固定化纤维蛋白原。这种新的测定法已成功用于蛋白质纯化,并且可以很容易地适用于自动化过程。最近,其他生色底物,如D-缬氨酸-L-亮氨酸-L-赖氨酸-对硝基苯胺(Val-Leu-Lys-pNA)和D-异亮氨酸-L-脯氨酸-L-精氨酸-对硝基苯胺(Ile-Pro-Arg-pNA)也被用于一步测定法中。发现在比色测定中,当使用硫酯、Val-Leu-Lys-pNA或Ile-Pro-Arg-pNA时,固定化纤维蛋白原和游离纤维蛋白原可大大增强TPA活性(图1,A-D)。酶动力学研究表明,在硫酯和纤维蛋白原包被的平板上测定纤溶酶原的Km为每毫升1.5微克,这大大低于在未处理平板上观察到的Km(每毫升4.8微克)。这不是由于纤维蛋白原对偶联光度测定法第二步的影响,因为在这些条件下纤溶酶活性没有变化(图1E)。当使用纤维蛋白包被的平板时,也观察到了TPA激活的类似结果。游离纤维蛋白原是TPA的激活剂,已包含在标准测定混合物中。在20℃孵育1小时内,我们能够检测到低于1纳克的TPA活性(图2A)。然而,在硫酯测定中,由于DTNB与这些试剂的相互作用,高浓度的还原剂和非特异性蛋白质会导致显著的背景。过去,125I标记的纤维蛋白包被平板已广泛用于尿激酶和TPA测定。尽管放射性方法的灵敏度与硫酯光度法相当,但似乎酶的动力学不容易跟踪,重复性也不太好。(摘要截短至400字)
