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Subtle Regulation of Potato Acid Invertase Activity by a Protein Complex of Invertase, Invertase Inhibitor, and SUCROSE NONFERMENTING1-RELATED PROTEIN KINASE

机译:转化酶,转化酶抑制剂和蔗糖非发酵1相关蛋白激酶蛋白复合物对马铃薯酸性转化酶活性的微妙调节

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摘要

Slowing down cold-induced sweetening (CIS) of potato (Solanum tuberosum) tubers is of economic importance for the potato industry to ensure high-quality products. The conversion of sucrose to reducing sugars by the acid invertase StvacINV1 is thought to be critical for CIS. Identification of the specific StvacINV1 inhibitor StInvInh2B and the alpha- and beta-subunits of the interacting protein SUCROSE NONFERMENTING1-RELATED PROTEIN KINASE from the wild potato species Solanum berthaultii (SbSnRK1) has led to speculation that invertase activity may be regulated via a posttranslational mechanism that remains to be elucidated. Using bimolecular fluorescence complementation assays, this study confirmed the protein complex by pairwise interactions. In vitro kinase assays and protein phosphorylation analysis revealed that phosphorylation of SbSnRK1 alpha is causal for StvacINV1 activity and that its active form blocks the inhibition of StInvInh2B by SbSnRK1 beta, whereas its inactive form restores the function of SbSnRK1 beta that prevents StInvInh2B from repressing StvacINV1. Overexpression of SbSnRK1 alpha in CIS-sensitive potato confirmed that SbSnRK1 alpha has significant effects on acid invertase-associated sucrose degradation. A higher level of SbSnRK1 alpha expression was accompanied by elevated SbSnRK1 alpha phosphorylation, reduced acid invertase activity, a higher sucrose-hexose ratio, and improved chip color. Our results lend new insights into a subtle regulatory mode of invertase activity and provide a novel approach for potato CIS improvement.
机译:减慢马铃薯(Solanum tuberosum)块茎的冷诱导甜化(CIS)对确保马铃薯行业高质量产品具有重要的经济意义。酸性转化酶StvacINV1将蔗糖转化为还原糖被认为对CIS至关重要。从野生马铃薯Solnum berthaultii(SbSnRK1)对特定StvacINV1抑制剂StInvInh2B以及相互作用蛋白SUCROSE NONFERMENTING1相关蛋白激酶的α-和β-亚基的鉴定导致人们推测,转化酶活性可能是通过翻译后机制调节的有待阐明。使用双分子荧光互补测定法,该研究通过成对相互作用证实了蛋白质复合物。体外激酶测定和蛋白质磷酸化分析表明,SbSnRK1 alpha的磷酸化是StvacINV1活性的原因,并且其活性形式阻止了SbSnRK1 beta对StInvInh2B的抑制作用,而其非活性形式恢复了SbSnRK1 beta的功能,该功能阻止了StInvInh2B抑制StInvInh2B抑制StvacINV1。 SbSnRK1 alpha在CIS敏感马铃薯中的过表达证实SbSnRK1 alpha对酸转化酶相关的蔗糖降解具有显着影响。 SbSnRK1α的较高表达水平伴随着SbSnRK1α的磷酸化升高,酸转化酶活性降低,蔗糖-己糖比更高以及芯片颜色得到改善。我们的结果为转化酶活性的微调模式提供了新的见解,并为马铃薯CIS改良提供了一种新颖的方法。

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