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肌苷单磷酸脱氢酶在豇豆(菜豆)固氮根瘤中尿囊素形成中的作用。

Role of Inosine Monophosphate Oxidoreductase in the Formation of Ureides in Nitrogen-Fixing Nodules of Cowpea (Vigna unguiculata L. Walp.).

机构信息

Botany Department, University of Western Australia, Nedlands WA 6009 Australia.

出版信息

Plant Physiol. 1983 Aug;72(4):1029-34. doi: 10.1104/pp.72.4.1029.

Abstract

Cell-free extracts from nodules of cowpea (Vigna unguiculata L. (Walp.) cv Caloona:Rhizobium strain CB756) prepared in the presence of 15% (v/v) glycerol showed high rates (30 to 60 nanomoles NAD reduced per minute per gram fresh weight nodule) of inosine monophosphate oxidoreductase (EC 1.2.1.14) activity. The enzyme was labile (half-life of activity less than 3 hours) but could be stabilized for up to 18 hours by inclusion of the substrates NAD and inosine monophosphate in the breaking media. Activity showed a broad pH optimum between 8.5 and 9.5, had an apparent K(m) (inosine monophosphate) of 4 and 12 micromolar at pH 7.5 and 9.0, respectively, and was largely (96%) associated with the plant cell cytosol fraction of the nodule.Metabolism of [8-(14)C]inosine monophosphate and [1-(14)C]glycine by the cell-free system showed two pathways for purine base production from inosine monophosphate, one via xanthosine monophosphate, xanthosine, and xanthine, the other via inosine and hypoxanthine. The proportion of inosine monophosphate utilized by inosine monophosphate oxidoreductase and the xanthine-based pathway was increased from 30% at 0.5 millimolar to 80% at 0.01 millimolar inosine monophosphate. The data are interpreted to indicate that in vivo inosine monophosphate oxidation rather than dephosphorylation is the predominant metabolic route leading to ureide synthesis and that inosine monophosphate provides the link between de novo purine nucleotide synthesis in the plastid and ureide production in the plant cell cytosol.

摘要

无细胞提取物从豆科植物根瘤(Vigna unguiculata L.(Walp.)cv Caloona:根瘤菌菌株 CB756)在 15%(v/v)甘油存在下制备,显示出高肌苷单磷酸氧化还原酶(EC 1.2.1.14)活性(每分钟每克新鲜重的根瘤 30 至 60 毫摩尔 NAD 还原)。该酶不稳定(半衰期小于 3 小时),但在破碎介质中包含 NAD 和肌苷单磷酸可以将其稳定 18 小时。活性在 8.5 和 9.5 之间具有广泛的 pH 最佳值,在 pH 7.5 和 9.0 时分别具有 4 和 12 微摩尔的表观 K(m)(肌苷单磷酸),并且主要(96%)与植物细胞胞质溶胶部分的根瘤相关。细胞无细胞系统对 [8-(14)C]肌苷单磷酸和 [1-(14)C]甘氨酸的代谢显示了从肌苷单磷酸产生嘌呤碱的两种途径,一种途径是通过黄苷单磷酸,黄嘌呤核苷和黄嘌呤,另一种途径是通过肌苷和次黄嘌呤。在 0.5 毫摩尔肌苷单磷酸时,肌苷单磷酸氧化还原酶和基于黄嘌呤的途径利用的肌苷单磷酸的比例从 30%增加到 0.01 毫摩尔肌苷单磷酸时的 80%。数据解释表明,在体内肌苷单磷酸氧化而不是磷酸化是导致脲合成的主要代谢途径,并且肌苷单磷酸提供了质体中新嘌呤核苷酸合成与植物细胞胞质溶胶中脲生产之间的联系。

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