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酿酒酵母细胞粘附分子α-凝集素亚基内功能区域的描绘。

Delineation of functional regions within the subunits of the Saccharomyces cerevisiae cell adhesion molecule a-agglutinin.

作者信息

Shen Z M, Wang L, Pike J, Jue C K, Zhao H, de Nobel H, Kurjan J, Lipke P N

机构信息

Department of Biological Sciences and the Institute for Biomolecular Structure and Function, Hunter College of the City University of New York, New York 10021, USA.

出版信息

J Biol Chem. 2001 May 11;276(19):15768-75. doi: 10.1074/jbc.M010421200. Epub 2001 Feb 5.

DOI:10.1074/jbc.M010421200
PMID:11278672
Abstract

a-Agglutinin from Saccharomyces cerevisiae is a cell adhesion glycoprotein expressed on the surface of cells of a mating type and consists of an anchorage subunit Aga1p and a receptor binding subunit Aga2p. Cell wall attachment of Aga2p is mediated through two disulfide bonds to Aga1p (Cappellaro, C., Baldermann, C., Rachel, R., and Tanner, W. (1994) EMBO J. 13, 4737-4744). We report here that purified Aga2p was unstable and had low molar specific activity relative to its receptor alpha-agglutinin. Aga2p co-expressed with a 149-residue fragment of Aga1p formed a disulfide-linked complex with specific activity 43-fold higher than Aga2p expressed alone. Circular dichroism of the complex revealed a mixed alpha/beta structure, whereas Aga2p alone had no periodic secondary structure. A 30-residue Cys-rich Aga1p fragment was partially active in stabilization of Aga2p activity. Mutation of either or both Aga2p cysteine residues eliminated stabilization of Aga2p. Thus the roles of Aga1p include both cell wall anchorage and cysteine-dependent conformational restriction of the binding subunit Aga2p. Mutagenesis of AGA2 identified only C-terminal residues of Aga2p as being essential for binding activity. Aga2p residues 45-72 are similar to sequences in soybean Nod genes, and include residues implicated in interactions with both Aga1p (including Cys(68)) and alpha-agglutinin.

摘要

来自酿酒酵母的α-凝集素是一种细胞粘附糖蛋白,表达于a交配型细胞表面,由一个锚定亚基Aga1p和一个受体结合亚基Aga2p组成。Aga2p与细胞壁的附着是通过两个二硫键介导至Aga1p(卡佩拉罗,C.,巴尔德曼,C.,雷切尔,R.,和坦纳,W.(1994年)《欧洲分子生物学组织杂志》13卷,4737 - 4744页)。我们在此报告,纯化的Aga2p不稳定,相对于其受体α-凝集素,其摩尔比活性较低。与Aga1p的149个残基片段共表达的Aga2p形成了一种二硫键连接的复合物,其比活性比单独表达的Aga2p高43倍。该复合物的圆二色性显示出α/β混合结构,而单独的Aga2p没有周期性二级结构。一个富含30个残基的Aga1p半胱氨酸片段在稳定Aga2p活性方面部分有效。Aga2p的一个或两个半胱氨酸残基发生突变会消除对Aga2p的稳定作用。因此,Aga1p的作用包括细胞壁锚定以及对结合亚基Aga2p的半胱氨酸依赖性构象限制。对AGA2进行诱变发现,只有Aga2p的C末端残基对于结合活性是必不可少的。Aga2p的45 - 72位残基与大豆结瘤基因中的序列相似,并且包括与Aga1p(包括Cys(68))和α-凝集素相互作用所涉及的残基。

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Delineation of functional regions within the subunits of the Saccharomyces cerevisiae cell adhesion molecule a-agglutinin.酿酒酵母细胞粘附分子α-凝集素亚基内功能区域的描绘。
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