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Analysis of the Functional Interaction of Arabidopsis Starch Synthase and Branching Enzyme Isoforms Reveals that the Cooperative Action of SSI and BEs Results in Glucans with Polymodal Chain Length Distribution Similar to Amylopectin

机译:拟南芥淀粉合酶和分支酶同工型的功能相互作用的分析表明SSI和BEs的协同作用导致葡聚糖具有类似于支链淀粉的多峰链长分布。

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摘要

Starch synthase (SS) and branching enzyme (BE) establish the two glycosidic linkages existing in starch. Both enzymes exist as several isoforms. Enzymes derived from several species were studied extensively both in vivo and in vitro over the last years, however, analyses of a functional interaction of SS and BE isoforms are missing so far. Here, we present data from in vitro studies including both interaction of leaf derived and heterologously expressed SS and BE isoforms. We found that SSI activity in native PAGE without addition of glucans was dependent on at least one of the two BE isoforms active in Arabidopsis leaves. This interaction is most likely not based on a physical association of the enzymes, as demonstrated by immunodetection and native PAGE mobility analysis of SSI, BE2, and BE3. The glucans formed by the action of SSI/BEs were analysed using leaf protein extracts from wild type and be single mutants (Atbe2 and Atbe3 mutant lines) and by different combinations of recombinant proteins. Chain length distribution (CLD) patterns of the formed glucans were irrespective of SSI and BE isoforms origin and still independent of assay conditions. Furthermore, we show that all SS isoforms (SSI-SSIV) were able to interact with BEs and form branched glucans. However, only SSI/BEs generated a polymodal distribution of glucans which was similar to CLD pattern detected in amylopectin of Arabidopsis leaf starch. We discuss the impact of the SSI/BEs interplay for the CLD pattern of amylopectin.
机译:淀粉合酶(SS)和分支酶(BE)建立淀粉中存在的两个糖苷键。两种酶都以几种同工型存在。在过去的几年中,在体内和体外对源自几种物种的酶进行了广泛的研究,但是,到目前为止,对SS和BE同工型的功能相互作用的分析尚不完善。在这里,我们提供了来自体外研究的数据,包括叶衍生的和异源表达的SS和BE同种型的相互作用。我们发现,不添加葡聚糖的天然PAGE中的SSI活性取决于拟南芥叶片中有活性的两种BE异构体中的至少一种。正如SSI,BE2和BE3的免疫检测和天然PAGE迁移分析所证明的,这种相互作用很可能不是基于酶的物理结合。使用来自野生型且为单一突变体(Atbe2和Atbe3突变体系)的叶蛋白提取物,以及重组蛋白的不同组合,分析了由SSI / BEs作用形成的葡聚糖。所形成的葡聚糖的链长分布(CLD)模式与SSI和BE同工型的来源无关,并且仍与测定条件无关。此外,我们显示所有SS同工型(SSI-SSIV)都能够与BE相互作用并形成支链葡聚糖。然而,只有SSI / BEs产生了葡聚糖的多峰分布,这与拟南芥叶淀粉支链淀粉中检测到的CLD模式相似。我们讨论了SSI / BE相互作用对支链淀粉CLD模式的影响。

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