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Starch Granule Biosynthesis in Arabidopsis Is Abolished by Removal of All Debranching Enzymes but Restored by the Subsequent Removal of an Endoamylase

机译:去除所有脱支酶后拟南芥淀粉颗粒的生物合成被取消但随后去除内淀粉酶则恢复了淀粉颗粒的生物合成。

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摘要

Several studies have suggested that debranching enzymes (DBEs) are involved in the biosynthesis of amylopectin, the major constituent of starch granules. Our systematic analysis of all DBE mutants of Arabidopsis thaliana demonstrates that when any DBE activity remains, starch granules are still synthesized, albeit with altered amylopectin structure. Quadruple mutants lacking all four DBE proteins (Isoamylase1 [ISA1], ISA2, and ISA3, and Limit-Dextrinase) are devoid of starch granules and instead accumulate highly branched glucans, distinct from amylopectin and from previously described phytoglycogen. A fraction of these glucans are present as discrete, insoluble, nanometer-scale particles, but the structure and properties of this material are radically altered compared with wild-type amylopectin. Superficially, these data support the hypothesis that debranching is required for amylopectin synthesis. However, our analyses show that soluble glucans in the quadruple DBE mutant are degraded by α- and β-amylases during periods of net accumulation, giving rise to maltose and branched malto-oligosaccharides. The additional loss of the chloroplastic α-amylase AMY3 partially reverts the phenotype of the quadruple DBE mutant, restoring starch granule biosynthesis. We propose that DBEs function in normal amylopectin synthesis by promoting amylopectin crystallization but conclude that they are not mandatory for starch granule synthesis.
机译:几项研究表明,脱支酶(DBE)参与了支链淀粉的生物合成,支链淀粉是淀粉颗粒的主要成分。我们对拟南芥所有DBE突变体的系统分析表明,当保留任何DBE活性时,尽管支链淀粉的结构发生了改变,淀粉颗粒仍可以合成。缺少所有四个DBE蛋白(异淀粉酶1 [ISA1],ISA2和ISA3以及极限糊精酶)的四重突变体没有淀粉颗粒,而是积聚了高度分支的葡聚糖,与支链淀粉和前述植物糖原不同。这些葡聚糖的一部分以离散,不溶的纳米级颗粒形式存在,但与野生型支链淀粉相比,这种材料的结构和性质发生了根本性的变化。从表面上看,这些数据支持支链淀粉合成需要脱支这一假设。但是,我们的分析表明,四倍DBE突变体中的可溶性葡聚糖在净积累期间会被α-和β-淀粉酶降解,从而产生麦芽糖和分支的麦芽低聚糖。叶绿体α-淀粉酶AMY3的额外损失部分恢复了四倍DBE突变体的表型,从而恢复了淀粉颗粒的生物合成。我们建议DBEs通过促进支链淀粉的结晶在正常支链淀粉的合成中起作用,但是得出结论,它们不是淀粉颗粒合成所必需的。

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