Ito Y, Kaku H, Shibuya N
Department of Biotechnology, National Institute of Agrobiological Resources, Ibaraki, Japan.
Plant J. 1997 Aug;12(2):347-56. doi: 10.1046/j.1365-313x.1997.12020347.x.
A high-affinity binding protein for the N-acetylchito-oligosaccharide elicitor of phytoalexin biosynthesis was identified by photoaffinity labeling and affinity cross-linking in the plasma membrane of suspension-cultured rice cells. Both a [125I]-labeled photolabile 2-(4-azidophenyl)ethylamino conjugate ([125I]-GN8-AzPEA) and a [125I]-labeled 2-(4-aminophenyl)ethylamino conjugate ([125]-GN8-APEA) of N-acetylchito-octaose were synthesized. The two conjugates were separately incubated with the plasma membrane prepared by aqueous two-phase partitioning, and covalently cross-linked to the elicitor binding site by irradiation with UV light or treatment with the cross-linking agent glutaraldehyde, respectively. Autoradiography of the SDS-PAGE gel of the solubilized membrane proteins revealed the labeling of a single 75 kDa band in both cases. The incorporation of the radiolabeled ligands into the 75 kDa protein showed a saturable mode of binding, with half-maximal incorporation at 45 and 52 nM for photoaffinity labeling and affinity cross-linking, respectively. The labeling of the 75 kDa protein was inhibited by N-acetylchito-oligosaccharides in a size-dependent manner, and N-acetylchito-octaose (GlcNAc)8 showed a half-maximal inhibition at concentrations of the order of 10 nM. However, neither chito-octaose (GlcN)8, cellopentaose nor alpha-1,4 linked N-acetylgalactosamine octamer (GalNAc)8 at concentrations as high as 25 microM inhibited the labeling of the 75 kDa protein. These results are in good agreement with the sensitivity and the specificity of the 'high-affinity binding site' previously identified by binding assays, as well as with the activities of these oligosaccharides in the induction of phytoalexin biosynthesis and other cellular responses. These results suggest that the 75 kDa protein identified by the affinity labeling represents a functional receptor for this elicitor.
通过光亲和标记和亲和交联法,在悬浮培养的水稻细胞的质膜中鉴定出一种与植物抗毒素生物合成的N-乙酰几丁寡糖诱导子具有高亲和力的结合蛋白。合成了N-乙酰几丁八糖的[125I]标记的光不稳定2-(4-叠氮苯基)乙氨基偶联物([125I]-GN8-AzPEA)和[125I]标记的2-(4-氨基苯基)乙氨基偶联物([125I]-GN8-APEA)。将这两种偶联物分别与通过双水相分配制备的质膜一起温育,并分别通过紫外线照射或用交联剂戊二醛处理,使其与诱导子结合位点共价交联。对溶解的膜蛋白进行SDS-PAGE凝胶放射自显影,结果显示在两种情况下均标记出一条单一的75 kDa条带。放射性标记配体掺入75 kDa蛋白呈现出饱和结合模式,光亲和标记和亲和交联的半数最大掺入量分别为45和52 nM。N-乙酰几丁寡糖以大小依赖的方式抑制75 kDa蛋白的标记,N-乙酰几丁八糖(GlcNAc)8在10 nM左右的浓度下表现出半数最大抑制作用。然而,浓度高达25 μM的几丁八糖(GlcN)8、纤维五糖或α-1,4连接的N-乙酰半乳糖胺八聚体(GalNAc)8均未抑制75 kDa蛋白的标记。这些结果与先前通过结合试验鉴定的“高亲和力结合位点”的敏感性和特异性以及这些寡糖在诱导植物抗毒素生物合成和其他细胞反应中的活性高度一致。这些结果表明,通过亲和标记鉴定的75 kDa蛋白代表了这种诱导子的功能性受体。
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