钙诱导人血浆因子 XIII 的解离及催化活性的出现。

Calcium-induced dissociation of human plasma factor XIII and the appearance of catalytic activity.

作者信息

Cooke R D

出版信息

Biochem J. 1974 Sep;141(3):683-91. doi: 10.1042/bj1410683.

DOI:10.1042/bj1410683

PMID:4463958

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1168173/

Abstract

The Ca(2+) dependence of the activity of plasma Factor XIII(a) was studied by using the continuous assay based on the incorporation of dansylcadaverine into dephosphorylated acetylated beta-casein (beta-substrate). The K(m) for Ca(2+) is about 0.170mm. 2. At low concentrations of Ca(2+) there was a lag in attaining the steady-state rate. The size of the lag was decreased and eventually abolished if the enzyme was preincubated with a high concentration of Ca(2+) before assay. The concentration of Ca(2+) required to decrease the lag phase by 50% in 10min depended on the protein concentration: at 0.87mg of protein/ml it required 17mm-Ca(2+) and at 0.44mg/ml it needed 10mm-Ca(2+). 3. The concentrations of Ca(2+) required either to abolish the lag phase in the appearance of enzyme activity or to activate the essential thiol for reaction with 5,5'-dithiobis-(2-nitrobenzoate) in 10min incubation were similar at the same protein concentration. This indicated that Ca(2+) induces a conformation change that is responsible for both phenomena. A model is proposed that links this conformation change to the dissociation of the tetrameric enzyme. 4. This was supported by the observation that the addition of excess of b chains to the Factor XIII(a) (a'(2)b(2)) increased the concentration of Ca(2+) required to expose the reactive thiol, and inhibited the Ca(2+)-dependent aggregation of a' chains. 5. Platelet Factor XIII(a) (a'(2)) was inhibited by 5,5'-dithiobis-(2-nitrobenzoate) in the absence of Ca(2+), and no lag phases were observed in attaining the steady-state rate at low Ca(2+) concentrations, thus confirming the model for the activation of the plasma enzyme. 6. The Ca(2+) dependence of platelet Factor XIII(a) indicated that Ca(2+) has an additional role in the enzyme mechanism of the plasma enzyme, perhaps being involved in substrate binding. 7. The dependence of the stability of plasma Factor XIII(a) on Ca(2+) and protein concentration indicates that the decay in activity is related to the tetramer dissociation. 8. beta-Substrate decreased the Ca(2+) concentration required for (1) abolition of the lag phase and (2) enzyme inhibition by thiol reagents. The effect on the former is greater than on the latter. 9. The role of the b chains of the plasma Factor and the evolutionary significance of the plasma and platelet Factors are considered.

摘要

通过基于将丹磺酰尸胺掺入去磷酸化乙酰化β-酪蛋白（β-底物）的连续测定法，研究了血浆因子XIII(a)活性对Ca(2+)的依赖性。Ca(2+)的K(m)约为0.170mmol/L。2. 在低浓度Ca(2+)时，达到稳态速率存在滞后现象。如果在测定前将酶与高浓度Ca(2+)预孵育，滞后的大小会减小并最终消除。在10分钟内使滞后阶段减少50%所需的Ca(2+)浓度取决于蛋白质浓度：在0.87mg蛋白质/ml时需要17mmol/L的Ca(2+)，在0.44mg/ml时需要10mmol/L的Ca(2+)。3. 在相同蛋白质浓度下，在10分钟孵育中消除酶活性出现时的滞后阶段或激活与5,5'-二硫代双-(2-硝基苯甲酸)反应的必需巯基所需的Ca(2+)浓度相似。这表明Ca(2+)诱导了一种构象变化，这两种现象均由此引起。提出了一个将这种构象变化与四聚体酶的解离联系起来的模型。4. 观察到向因子XIII(a)（a'(2)b(2)）中添加过量的b链会增加暴露反应性巯基所需的Ca(2+)浓度，并抑制a'链的Ca(2+)依赖性聚集，这支持了上述观点。5. 在没有Ca(2+)的情况下，血小板因子XIII(a)（a'(2)）被5,5'-二硫代双-(2-硝基苯甲酸)抑制，并且在低Ca(2+)浓度下达到稳态速率时未观察到滞后阶段，从而证实了血浆酶激活的模型。6. 血小板因子XIII(a)对Ca(2+)的依赖性表明Ca(2+)在血浆酶的酶促机制中具有额外作用，可能参与底物结合。7. 血浆因子XIII(a)稳定性对Ca(2+)和蛋白质浓度的依赖性表明活性的衰减与四聚体解离有关。8. β-底物降低了（1）消除滞后阶段和（2）巯基试剂对酶抑制所需的Ca(2+)浓度。对前者的影响大于对后者的影响。9. 考虑了血浆因子b链的作用以及血浆和血小板因子的进化意义。