Lane D A, Olds R R, Thein S L
Department of Haematology, Charing Cross and Westminster Medical School, Hammersmith, London.
Blood Coagul Fibrinolysis. 1992 Jun;3(3):315-41. doi: 10.1097/00001721-199206000-00012.
Antithrombin is the most important physiological proteinase inhibitor of thrombin and other coagulation proteinases. It is a single chain glycoprotein of MW 58,200 which has sequence homology with alpha 1-antitrypsin and other members of the serpin superfamily of inhibitors. Two functional domains of importance have been identified, the reactive centre that interacts with the proteinase and a heparin binding domain. Failure to maintain an adequate level of functional antithrombin in plasma results in an increased risk of thromboembolism: deficiency can be inherited or acquired. There is still uncertainty regarding the prevalence of inherited deficiency and the prevalence of thrombosis in affected individuals. The production of antithrombin is under the control of a single gene which is localized on chromosome 1q 23-25. Characterization of the coding sequence, which is distributed over seven exons, has allowed the analysis of the molecular basis for inherited antithrombin deficiency. To date more than 100 cases have been successfully investigated at the gene and/or protein sequence level and 40 novel mutations have been identified. Mutations causing amino acid substitutions solely affecting the heparin binding site have thus far been located primarily at the N-terminal region of the molecule, residues 7-129; this region has been postulated to align as a positive groove in the molecule that forms the primary contact region for the essential antithrombin binding pentasaccharide of heparin. Not all the residues in which substitutions have been found are basic and some serve to maintain the conformation of nearby basic regions. Examples of this are provided by the Pro-41 to Leu mutation and a recently investigated mutant, Leu-99 to Phe. The reactive site defects are an interesting group, including those that alter P1, P1' and P12-P10 residues. Perhaps more remote mutations can also be included such as Pro-429 to Leu. The P1 and P1' mutations directly block interaction of the proteinase with anti-thrombin, while P12-P10 mutants (which have mutations affecting serpin strand s4A) enable the substrate reaction to proceed to completion, i.e. the antithrombin-thrombin complex is not stabilized and the mutant inhibitor is transformed into a substrate. The effect of the Pro-429 to Leu substitution is impairment of the reactive site and heparin binding, and the finding that this variant is not completely recognized by some MAbs implies a conformational change at the C terminus. Another group (nine cases) of interesting mutations is emerging, that has its primary defect in or near serpin strand 1C, amino acid sequence 402-407.(ABSTRACT TRUNCATED AT 400 WORDS)
抗凝血酶是凝血酶和其他凝血蛋白酶最重要的生理性蛋白酶抑制剂。它是一种分子量为58,200的单链糖蛋白,与α1 -抗胰蛋白酶及丝氨酸蛋白酶抑制剂超家族的其他成员具有序列同源性。已确定了两个重要的功能结构域,即与蛋白酶相互作用的反应中心和肝素结合结构域。血浆中未能维持足够水平的功能性抗凝血酶会导致血栓栓塞风险增加:缺乏症可遗传或后天获得。关于遗传性缺乏症的患病率以及受影响个体中血栓形成的患病率仍存在不确定性。抗凝血酶的产生受位于1号染色体1q 23 - 25上的单个基因控制。对分布在7个外显子上的编码序列进行表征,有助于分析遗传性抗凝血酶缺乏症的分子基础。迄今为止,已在基因和/或蛋白质序列水平成功研究了100多例病例,并鉴定出40种新的突变。迄今为止,仅影响肝素结合位点的氨基酸替代突变主要位于分子的N端区域,即第7 - 129位残基;该区域被推测在分子中排列为一个正性凹槽,形成抗凝血酶与肝素必需结合五糖的主要接触区域。并非所有发现有替代的残基都是碱性的,有些残基用于维持附近碱性区域的构象。Pro - 41突变为Leu以及最近研究的Leu - 99突变为Phe就是这样的例子。反应位点缺陷是一个有趣的类别,包括那些改变P1、P1'以及P12 - P10残基的突变。也许更远端的突变也可包括在内,如Pro - 429突变为Leu。P1和P1'突变直接阻断蛋白酶与抗凝血酶的相互作用,而P12 - P10突变体(其突变影响丝氨酸蛋白酶抑制剂链s4A)使底物反应能够进行到底,即抗凝血酶 - 凝血酶复合物不稳定,突变抑制剂转化为底物。Pro - 429突变为Leu的替代效应是反应位点和肝素结合受损,并且该变体未被某些单克隆抗体完全识别这一发现意味着C端存在构象变化。另一组(9例)有趣的突变正在出现,其主要缺陷位于丝氨酸蛋白酶抑制剂链1C或其附近,氨基酸序列为402 - 407。(摘要截短至400字)
