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组织因子快速有效地掺入脂质体。

Rapid and efficient incorporation of tissue factor into liposomes.

作者信息

Smith S A, Morrissey J H

机构信息

Department of Biochemistry, University of Illinois at Urbana-Champaign, Urbana, IL 61801, USA.

出版信息

J Thromb Haemost. 2004 Jul;2(7):1155-62. doi: 10.1111/j.1538-7836.2004.00772.x.

Abstract

Tissue factor (TF), the physiological trigger of the blood clotting cascade, is also the active ingredient in thromboplastin preparations which are widely used in clotting assays such as the prothrombin time (PT) test. A type I integral membrane protein, TF must be incorporated into suitable phospholipid membranes for full procoagulant activity. Several methods exist for incorporating TF into phospholipid vesicles, typically employing the formation of mixed micelles containing detergent, phospholipid and TF, followed by detergent removal or dilution below the critical micelle concentration (CMC). These methods have certain drawbacks: they may take several days to complete, employ expensive detergents, are difficult to scale up, and do not always result in complete detergent removal. In this study we have investigated the use of a variety of detergents [Triton X-100, octaethylene glycol monododecyl ether (C(12)E(8)), cholate, deoxycholate, and n-octyl-beta-D-glucopyranoside], and the use of adsorbent beads (Bio-Beads SM-2) for removing detergent, in processes to incorporate TF into proteoliposomes with high specific activity in coagulation assays. The method we have developed is rapid and readily scalable, yielding thromboplastin preparations with specific activities in plasma clotting assays that are at least as high as those made with detergent dialysis.

摘要

组织因子(TF)是血液凝固级联反应的生理触发因素,也是凝血活酶制剂中的活性成分,凝血活酶制剂广泛用于诸如凝血酶原时间(PT)测试等凝血试验中。作为一种I型整合膜蛋白,TF必须整合到合适的磷脂膜中才能具有完全的促凝血活性。存在几种将TF整合到磷脂囊泡中的方法,通常是利用含有去污剂、磷脂和TF的混合胶束的形成,然后将去污剂去除或稀释至临界胶束浓度(CMC)以下。这些方法有一定的缺点:它们可能需要几天才能完成,使用昂贵的去污剂,难以扩大规模,并且并不总是能完全去除去污剂。在本研究中,我们研究了多种去污剂[ Triton X-100、八乙二醇单十二烷基醚(C(12)E(8))、胆酸盐、脱氧胆酸盐和正辛基-β-D-葡萄糖苷]的使用,以及使用吸附珠(Bio-Beads SM-2)去除去污剂,以便在凝血试验中将TF整合到具有高比活性的蛋白脂质体中。我们开发的方法快速且易于扩大规模,所产生的凝血活酶制剂在血浆凝血试验中的比活性至少与通过去污剂透析制备的制剂一样高。

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