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Structural characterization of human and bovine lung surfactant protein D.

机译:人和牛肺表面活性物质D的结构表征

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摘要

Human and bovine surfactant proteins D (SP-D) were purified from late amniotic fluid and bronchioalveolar lavage on the basis of its Ca(2+)-dependent affinity for maltose. The molecular mass of a trimeric subunit was determined by matrix-assisted laser desorption ionization MS to lie in the range 115-125 kDa for human SP-D and 110-123 kDa for bovine SP-D. A single polypeptide chain was determined at 37-41 and 36-40 kDa for the human and bovine species respectively. The major parts of the primary structures of both SP-D molecules were determined by a combination of MS and Edman degradation. The heterogeneity in SP-D was caused mainly by a high number of post-translational modifications in the collagen-like region. Proline and lysine residues were partly hydroxylated and lysine residues were further O-glycosylated with the disaccharide galactose-glucose. A partly occupied N-linked glycosylation site was characterized in human SP-D. The carbohydrate was determined as a complex type bi-antennary structure, with a small content of mono-antennary and tri-antennary structures. No sialic acid residues were present on the glycan, but some had an attached fucose and/or an N-acetylglucosamine residue linked to the core. Bovine SP-D was determined as having a similar structure.
机译:人和牛表面活性剂蛋白D(SP-D)是从晚期羊水和支气管肺泡灌洗液中纯化的,基于其对麦芽糖的Ca(2+)依赖性。通过基质辅助激光解吸电离质谱法确定三聚体亚基的分子量在人SP-D范围内为115-125 kDa,在牛SP-D范围内为110-123 kDa。对于人和牛,分别在37-41和36-40kDa处确定了一条多肽链。两个SP-D分子一级结构的主要部分由MS和Edman降解的组合确定。 SP-D中的异质性主要是由胶原样区域中大量的翻译后修饰引起的。脯氨酸和赖氨酸残基被部分羟基化,赖氨酸残基被二糖半乳糖-葡萄糖进一步O-糖基化。在人SP-D中表征了部分占据的N-连接的糖基化位点。碳水化合物被确定为具有少量单触角和三触角结构的复杂类型的双触角结构。在聚糖上不存在唾液酸残基,但是一些残基具有连接到核心的连接的岩藻糖和/或N-乙酰氨基葡糖残基。确定牛SP-D具有相似的结构。

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