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一种用于检测ADAMTS-13的快速酶联检测法。

A rapid enzyme-linked assay for ADAMTS-13.

作者信息

Wu J-J, Fujikawa K, Lian E C, McMullen B A, Kulman J D, Chung D W

机构信息

Department of Biochemistry, University of Washington, Seattle, WA 98195, USA.

出版信息

J Thromb Haemost. 2006 Jan;4(1):129-36. doi: 10.1111/j.1538-7836.2005.01677.x.

DOI:10.1111/j.1538-7836.2005.01677.x
PMID:16409462
Abstract

BACKGROUND

A deficiency in the plasma metalloprotease ADAMTS-13 is associated with deposition of microvascular thrombi that cause thrombotic thrombocytopenic purpura. Current assays for ADAMTS-13 are technically complex and time-consuming. The objective of this study is to devise a rapid and sensitive assay for ADAMTS-13 activity in plasma and verify the site of cleavage.

METHOD

A new enzyme-linked substrate, which contains a core ADAMTS-13-specific peptide conjugated to horseradish peroxidase (HRP) at the N-terminus, and labeled with biotin at the C-terminus, was constructed. After cleavage of this substrate by plasma ADAMTS-13 and removal of uncleaved substrate by adsorption with streptavidin-agarose, ADAMTS-13 activity was quantitated by determining the unadsorbed HRP activity remaining in solution. Levels of inhibitory antibodies in test plasma were also determined by measuring the residual ADAMTS-13 activity after varying amounts of test plasma were incubated with a known amount of ADAMTS-13.

RESULTS

Plasma ADAMTS-13 activity was readily determined in approximately 60 min (coefficient of variation 5.8%) using 1 microL of test plasma. Amino acid sequencing of the cleavage product confirmed that cleavage occurred at the Tyr1605-Met1606 bond in the substrate. ADAMTS-13 activities in the plasma of five TTP patients were below 2%. Inhibitory antibody titers in these samples varied from undetectable to 81 BU mL(-1).

CONCLUSION

The HRP-linked substrate provides a rapid, sensitive, and reproducible way of determining the levels of ADAMTS-13 activity and inhibitory antibodies in plasma.

摘要

背景

血浆金属蛋白酶ADAMTS - 13缺乏与微血管血栓形成有关,微血管血栓会导致血栓性血小板减少性紫癜。目前检测ADAMTS - 13的方法技术复杂且耗时。本研究的目的是设计一种快速、灵敏的检测血浆中ADAMTS - 13活性的方法,并验证其切割位点。

方法

构建了一种新的酶联底物,该底物在N端含有与辣根过氧化物酶(HRP)偶联的ADAMTS - 13特异性核心肽,在C端用生物素标记。血浆ADAMTS - 13切割该底物后,通过与链霉亲和素琼脂糖吸附去除未切割的底物,通过测定溶液中剩余的未吸附HRP活性来定量ADAMTS - 13活性。通过测量不同量的测试血浆与已知量的ADAMTS - 13孵育后剩余的ADAMTS - 13活性,还可确定测试血浆中抑制性抗体的水平。

结果

使用1微升测试血浆,约60分钟内即可轻松测定血浆ADAMTS - 13活性(变异系数为5.8%)。切割产物的氨基酸测序证实切割发生在底物的Tyr1605 - Met1606键处。5例血栓性血小板减少性紫癜患者血浆中的ADAMTS - 13活性均低于2%。这些样本中的抑制性抗体滴度从无法检测到81 BU mL(-1)不等。

结论

HRP连接的底物为测定血浆中ADAMTS - 13活性和抑制性抗体水平提供了一种快速、灵敏且可重复的方法。

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