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从富含禽生长板软骨基质小泡的微粒体中分离出两种糖基化形式的膜结合碱性磷酸酶。

Isolation of two glycosylated forms of membrane-bound alkaline phosphatase from avian growth plate cartilage matrix vesicle-enriched microsomes.

作者信息

Wu L N, Valhmu W B, Lloyd G C, Genge B R, Wuthier R E

机构信息

Department of Chemistry, University of South Carolina, Columbia 29208.

出版信息

Bone Miner. 1989 Sep;7(2):113-25. doi: 10.1016/0169-6009(89)90069-x.

Abstract

Isolation of two membrane-bound alkaline phosphatase (AP) species from avian growth plate cartilage matrix vesicle (MV) fractions is described. AP was first released from the membranes by phosphatidylinositol-specific phospholipase C (PIase C), followed by chromatography on DEAE-Bio-Gel A and Reactive-Red agarose. Two AP species having apparent Mr of 81.5 and 77 kDa by SDS-PAGE were purified in high yield and specific activity by this simple method. Treatment with neuraminidase to remove sialic acid residues reduced their size slightly, but did not diminish the difference in Mr between the two species. Digestion with N-glycanase, however, decreased both AP species to a common size of 59 kDa. This reveals that both enzymes are highly glycosylated and suggests that the two forms may result from differences in degree of glycation. The amino acid compositions of the two avian enzyme forms are very similar, but are markedly enriched in serine, glycine and glutamate when compared to those reported for mammalian liver-kidney-bone AP. Possible differences in amino acid sequence between the two avian forms have not been excluded. The cross-reactivity of polyclonal antibodies to these enzymes with bovine kidney, but not intestinal AP, indicate that the avian cartilage APs are of the liver-kidney-bone isozyme type.

摘要

本文描述了从禽生长板软骨基质小泡(MV)组分中分离出两种膜结合碱性磷酸酶(AP)的方法。AP首先通过磷脂酰肌醇特异性磷脂酶C(PIase C)从膜上释放出来,然后在DEAE-生物凝胶A和活性红琼脂糖上进行层析。通过这种简单的方法,以高产率和比活性纯化了两种经SDS-PAGE测定表观分子量分别为81.5 kDa和77 kDa的AP。用神经氨酸酶处理以去除唾液酸残基,使其大小略有减小,但并未消除这两种AP分子量的差异。然而,用N-聚糖酶消化后,两种AP的分子量均降至共同的59 kDa。这表明这两种酶都高度糖基化,并提示这两种形式可能是由于糖基化程度不同所致。这两种禽酶形式的氨基酸组成非常相似,但与报道的哺乳动物肝-肾-骨AP相比,丝氨酸、甘氨酸和谷氨酸含量明显富集。尚未排除这两种禽酶形式在氨基酸序列上可能存在的差异。针对这些酶的多克隆抗体与牛肾AP有交叉反应,但与肠AP无交叉反应,这表明禽软骨AP属于肝-肾-骨同工酶类型。

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