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一种新型甘露糖结合凝集素相关丝氨酸蛋白酶1/3基因变体。

A novel mannose-binding lectin-associated serine protease 1/3 gene variant.

作者信息

Weiss G, Madsen H O, Garred P

机构信息

Tissue Typing Laboratory-7631, Department of Clinical Immunology, Rigshospitalet, University of Copenhagen, Copenhagen, Denmark.

出版信息

Scand J Immunol. 2007 May;65(5):430-4. doi: 10.1111/j.1365-3083.2007.01925.x.

DOI:10.1111/j.1365-3083.2007.01925.x
PMID:17444953
Abstract

The ficolins and mannose-binding lectin (MBL) create complexes with three different serine proteases (MASP-1, MASP-2 and MASP-3) and a truncated non-enzymatic form of MASP-2 (sMAP). MASP-2 is able to activate complement by cleavage of C4 and C2, while the physiological functions of MASP-1, MASP-3 and sMAP still are debated. MASP-1 and MASP-3 are alternative spliced forms of the same MASP gene. To gain insight in the molecular variation in the MASP-1/3 gene, we undertook a systematic study of the protein coding sequences of the MASP-1/3 gene. The coding regions of the MASP-1/3 gene were sequenced in 92 healthy Caucasian donors. A total of six nucleotide substitutions were detected. Five were detected only once. One polymorphism identified in exon 10 at position +50074 (rs 38343199) relative to the transcription start site resulting in the amino acid substitution of a glycine (GGG) with a glutamic acid residue (GAG) in the second complement control protein domain was observed. The frequency of this allele in 305 blood donors, 90 patients with systemic lupus erythematosus and 234 patients with the systemic inflammatory response syndrome (SIRS) and/or sepsis was 0.03, 0.017 and 0.03 respectively. No significant differences in genotype frequencies between the groups were observed (P > 0.45). However, the SIRS/sepsis group deviated from the Hardy-Weinberg expectations due to one variant allele homozygote (P = 0.07), which was not observed in the other groups. In conclusion, the MASP1/3 gene harbours a low-frequent polymorphic site resulting in an amino acid substitution, which may influence the function of the gene product.

摘要

纤维胶凝蛋白和甘露糖结合凝集素(MBL)与三种不同的丝氨酸蛋白酶(MASP-1、MASP-2和MASP-3)以及一种截短的非酶形式的MASP-2(sMAP)形成复合物。MASP-2能够通过切割C4和C2来激活补体,而MASP-1、MASP-3和sMAP的生理功能仍存在争议。MASP-1和MASP-3是同一MASP基因的可变剪接形式。为了深入了解MASP-1/3基因的分子变异,我们对MASP-1/3基因的蛋白质编码序列进行了系统研究。在92名健康的白种人供体中对MASP-1/3基因的编码区进行了测序。共检测到六个核苷酸替换。其中五个仅被检测到一次。观察到在相对于转录起始位点的第10外显子+50074位置(rs 38343199)鉴定出一个多态性,导致在第二个补体控制蛋白结构域中甘氨酸(GGG)被谷氨酸残基(GAG)替换。该等位基因在305名献血者、90名系统性红斑狼疮患者和234名全身性炎症反应综合征(SIRS)和/或脓毒症患者中的频率分别为0.03、0.017和0.03。各群体之间的基因型频率未观察到显著差异(P>0.45)。然而,SIRS/脓毒症组由于一个变异等位基因纯合子而偏离了哈迪-温伯格预期(P = 0.07),这在其他组中未观察到。总之,MASP1/3基因含有一个低频多态性位点,导致氨基酸替换,这可能会影响基因产物的功能。

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