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MBL/ficolin 相关蛋白-1 的血清浓度和相互作用特性。

Serum concentration and interaction properties of MBL/ficolin associated protein-1.

机构信息

Laboratory of Molecular Medicine, Department of Clinical Immunology, Sect 7631, Rigshospitalet, Faculty of Health Sciences, University Hospital of Copenhagen, Denmark.

出版信息

Immunobiology. 2011 May;216(5):625-32. doi: 10.1016/j.imbio.2010.09.011. Epub 2010 Sep 24.

DOI:10.1016/j.imbio.2010.09.011
PMID:21035894
Abstract

Recently, a novel protein named MBL/ficolin associated protein-1 (MAP-1) derived from the MASP1 gene through differential splicing was identified. In the present study, we established biochemical characteristics, determined the serum level and assessed the interactions between the lectin complement pathway (LCP) recognition molecules and MAP-1. We expressed recombinant MAP-1 in CHO DG44 cells, developed a quantitative ELISA assay based on a MAP-1 specific monoclonal capture antibody and measured the serum levels in 100 Danish blood donors. In addition we assessed the association properties between MAP-1 and Ficolin-2, -3 and MBL in serum using ELISA and density gradient ultra centrifugation. When recombinant MAP-1 was subjected to N-glycosidase F treatment the molecular mass decreased from ∼45 kDa to ∼40 kDa equivalent with the calculated molecular mass from the deduced amino acid sequence without the signal peptide. We found that serum MAP-1 was very stable when subjected to repeated freeze and thaw cycles. The mean serum concentration of MAP-1 was found to be 240 ng/ml (range: 115-466 ng/ml). MAP-1 was predominantly found in complex with Ficolin-3 and to a lesser degree with Ficolin-2 and MBL and by use of density gradient ultra centrifugation we could show that the major part of serum MAP-1 circulates in complex with the LCP molecules. In conclusion, these results show that MAP-1 is a highly stable glycosylated human serum protein found in complex with Ficolin-3, Ficolin-2 and MBL.

摘要

最近,一种新型蛋白质被鉴定为 MBL/ficolin 相关蛋白-1(MAP-1),它是通过差异剪接从 MASP1 基因衍生而来。在本研究中,我们建立了生化特征,测定了血清水平,并评估了凝集素补体途径(LCP)识别分子与 MAP-1 之间的相互作用。我们在 CHO DG44 细胞中表达重组 MAP-1,开发了一种基于 MAP-1 特异性单克隆捕获抗体的定量 ELISA 检测方法,并测量了 100 名丹麦献血者的血清水平。此外,我们使用 ELISA 和密度梯度超速离心评估了 MAP-1 与 Ficolin-2、-3 和 MBL 在血清中的结合特性。当重组 MAP-1 接受 N-糖苷酶 F 处理时,其分子量从约 45 kDa 降低至约 40 kDa,与推导的氨基酸序列的计算分子量相当,而没有信号肽。我们发现,当血清 MAP-1 经受反复冷冻和解冻循环时,非常稳定。发现 MAP-1 的平均血清浓度为 240 ng/ml(范围:115-466 ng/ml)。MAP-1 主要与 Ficolin-3 形成复合物,其次与 Ficolin-2 和 MBL 形成复合物,并且通过使用密度梯度超速离心,我们可以证明血清 MAP-1 的主要部分与 LCP 分子形成复合物循环。总之,这些结果表明 MAP-1 是一种高度稳定的糖基化人血清蛋白,与 Ficolin-3、Ficolin-2 和 MBL 形成复合物。

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