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α2,8-多聚唾液酸转移酶II/STX和IV/PST参与虹鳟卵巢O-连接糖蛋白上多聚唾液酸链的生物合成。

Involvement of the alpha2,8-polysialyltransferases II/STX and IV/PST in the biosynthesis of polysialic acid chains on the O-linked glycoproteins in rainbow trout ovary.

作者信息

Asahina Shinji, Sato Chihiro, Matsuno Midori, Matsuda Tsukasa, Colley Karen, Kitajima Ken

机构信息

Laboratory of Animal Cell Function, Bioscience and Biotechnology Center, Department of Bioengineering Sciences, Nagoya University, Nagoya 464-8601.

出版信息

J Biochem. 2006 Nov;140(5):687-701. doi: 10.1093/jb/mvj200. Epub 2006 Oct 5.

Abstract

Polysialoglycoprotein (PSGP) in salmonid fish egg is a unique glycoprotein bearing alpha2,8-linked polysialic acid (polySia) on its O-linked glycans. Biosynthesis of the polySia chains is developmentally regulated and only occurs at later stage of oogenesis. Two alpha2,8-polysialyltransferases (alpha2,8-polySTs), PST (ST8Sia IV) and STX (ST8Sia II), responsible for the biosynthesis of polySia on N-glycans of glycoproteins, are known in mammals. However, nothing has been known about which alpha2,8-polySTs are involved in the biosynthesis of polySia on O-linked glycans in any glycoproteins. We thus sought to identify cDNA encoding the alpha2,8-polyST involved in polysialylation of PSGP. A clone for PST orthologue, rtPST, and two clones for the STX orthologue, rtSTX-ov and rtSTX-em, were identified in rainbow trout. The deduced amino acid sequence of rtPST shows a high identity (72-77%) to other vertebrate PSTs, while that of rtSTX-ov shows 92% identity with rtSTX-em and a significant identity (63-76%) to other vertebrate STXs. The rtPST exhibited the in vivo alpha2,8-polyST activity, although its in vitro activity was low. However, the rtSTXs showed no in vivo and very low in vitro activities. Interestingly, co-existence of rtPST and rSTX-ov in the reaction mixture synergistically enhanced the alpha2,8-polyST activity. During oogenesis, rtPST was constantly expressed, while the expression of rtSTX-ov was not increased until polySia chain is abundantly biosynthesized in the later stage. rtSTX-em was not expressed in ovary. These results suggest that the enhanced expression of rtSTX-ov under the co-expression with rtPST may be important for the biosynthesis of polySia on O-linked glycans of PSGP.

摘要

鲑鱼卵中的多唾液酸糖蛋白(PSGP)是一种独特的糖蛋白,其O-连接聚糖上带有α2,8-连接的多唾液酸(polySia)。多唾液酸链的生物合成受发育调控,仅在卵子发生的后期发生。在哺乳动物中,已知两种α2,8-多唾液酸转移酶(α2,8-polySTs),即PST(ST8Sia IV)和STX(ST8Sia II),负责糖蛋白N-聚糖上多唾液酸的生物合成。然而,对于任何糖蛋白中O-连接聚糖上多唾液酸的生物合成涉及哪些α2,8-polySTs,人们一无所知。因此,我们试图鉴定编码参与PSGP多唾液酸化的α2,8-polyST的cDNA。在虹鳟鱼中鉴定出了PST同源物rtPST的一个克隆,以及STX同源物rtSTX-ov和rtSTX-em的两个克隆。rtPST推导的氨基酸序列与其他脊椎动物的PST具有高度同一性(72-77%),而rtSTX-ov与rtSTX-em具有92%的同一性,与其他脊椎动物的STX具有显著同一性(63-76%)。rtPST表现出体内α2,8-多唾液酸转移酶活性,尽管其体外活性较低。然而,rtSTXs在体内没有活性,体外活性也非常低。有趣的是,反应混合物中rtPST和rSTX-ov的共存协同增强了α2,8-多唾液酸转移酶活性。在卵子发生过程中,rtPST持续表达,而rtSTX-ov的表达直到后期多唾液酸链大量生物合成时才增加。rtSTX-em在卵巢中不表达。这些结果表明,rtSTX-ov与rtPST共表达时的增强表达可能对PSGP的O-连接聚糖上多唾液酸的生物合成很重要。

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