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肝细胞癌相关去γ-羧基凝血酶原的γ-羧基谷氨酸含量

gamma-Carboxyglutamic acid content of hepatocellular carcinoma-associated des-gamma-carboxy prothrombin.

作者信息

Naraki Toru, Kohno Noriatsu, Saito Hiroyuki, Fujimoto Yoshinori, Ohhira Motoyuki, Morita Takashi, Kohgo Yutaka

机构信息

Tsukuba Research Laboratories, Eisai Co., Ltd., 1-3 Tokodai 5-chome, Ibaraki 300-2635, Japan.

出版信息

Biochim Biophys Acta. 2002 Apr 24;1586(3):287-98. doi: 10.1016/s0925-4439(01)00107-7.

DOI:10.1016/s0925-4439(01)00107-7
PMID:11997080
Abstract

Serum des-gamma-carboxy prothrombin (DCP) is a useful marker for the diagnosis of hepatocellular carcinoma (HCC), but the exact mechanism of its synthesis and its structural properties in liver diseases are unknown. DCP is measured by the monoclonal antibody MU-3. The purpose of this study was to examine the epitope of MU-3 and to characterize the differences in DCP between HCC and benign liver diseases. The epitope of MU-3 was examined by ELISA using prothrombin Gla domain polypeptides and was determined to be amino acid residues 17-27 of the prothrombin Gla domain, which has four gamma-carboxyglutamic acid residues (Gla) at positions 19, 20, 25 and 26. Peptides having a glutamic acid residue (Glu) at these positions reacted strongly to MU-3 but lost reactivity when Glu 19 or 20 was changed to Gla. In the order of gamma-carboxylation, MU-3 reacted strongly to DCP containing 0-1 Gla, weakly to 2-4 Gla and not at all to DCP containing more than five Gla. After adsorbing normal prothrombin with barium carbonate, DCP reaction to MU-3 was measured by determining the amount of DCP that was adsorbed by MU-3-coated beads. The proportion of DCP reacting to MU-3 in HCC was 41.0-76.8%, whereas in patients with benign liver diseases, only 0-42.1% reacted to MU-3. These results indicate that DCP variants preferentially synthesized in HCC have less than four Gla, which are restricted to positions 16, 25, 26 and 29, whereas DCP variants in benign liver diseases have more than five Gla.

摘要

血清去γ-羧基凝血酶原(DCP)是诊断肝细胞癌(HCC)的一种有用标志物,但在肝脏疾病中其合成的确切机制及其结构特性尚不清楚。DCP通过单克隆抗体MU-3进行检测。本研究的目的是检测MU-3的表位,并表征HCC与良性肝脏疾病之间DCP的差异。使用凝血酶原γ-羧基谷氨酸结构域多肽通过酶联免疫吸附测定(ELISA)检测MU-3的表位,确定其为凝血酶原γ-羧基谷氨酸结构域的第17 - 27位氨基酸残基,该结构域在第19、20、25和26位有四个γ-羧基谷氨酸残基(Gla)。在这些位置具有谷氨酸残基(Glu)的肽与MU-3强烈反应,但当Glu 19或20变为Gla时失去反应性。按照γ-羧化顺序,MU-3与含0 - 1个Gla的DCP强烈反应,与含2 - 4个Gla的DCP反应较弱,与含超过5个Gla的DCP完全不反应。用碳酸钡吸附正常凝血酶后,通过测定被包被MU-3的磁珠吸附的DCP量来检测DCP与MU-3的反应。HCC中与MU-3反应的DCP比例为41.0 - 76.8%,而在良性肝脏疾病患者中,只有0 - 42.1%的DCP与MU-3反应。这些结果表明,在HCC中优先合成的DCP变体具有少于四个Gla,这些Gla限于第16、25、26和29位,而良性肝脏疾病中的DCP变体具有超过五个Gla。

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