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基于iTRAQ的粳稻灌浆初期颖花上下位颖蛋白质组图谱分析

iTRAQ-based proteome profile analysis of superior and inferior Spikelets at early grain filling stage in japonica Rice.

作者信息

You Cuicui, Chen Lin, He Haibing, Wu Liquan, Wang Shaohua, Ding Yanfeng, Ma Chuanxi

机构信息

College of Agronomy, Anhui Agricultural University, Hefei, 230036, People's Republic of China.

College of Agronomy, Nanjing Agricultural University/Key Laboratory of Crop Physiology Ecology and Production Management, Ministry of Agriculture, Nanjing, 210095, People's Republic of China.

出版信息

BMC Plant Biol. 2017 Jun 7;17(1):100. doi: 10.1186/s12870-017-1050-2.

Abstract

BACKGROUND

Large-panicle rice varieties often fail to achieve their yield potential due to poor grain filling of late-flowering inferior spikelets (IS). The physiological and molecular mechanisms of poor IS grain filling, and whether an increase in assimilate supply could regulate protein abundance and consequently improve IS grain filling for japonica rice with large panicles is still partially understood.

RESULTS

A field experiment was performed with two spikelet removal treatments at anthesis in the large-panicle japonica rice line W1844, including removal of the top 1/3 of spikelets (T1) and removal of the top 2/3 of spikelets (T2), with no spikelet removal as a control (T0). The size, weight, setting rate, and grain filling rate of IS were significantly increased after spikelet removing. The biological functions of the differentially expressed proteins (DEPs) between superior and inferior spikelets as well as the response of IS to the removal of superior spikelets (SS) were investigated by using iTRAQ at 10 days post anthesis. A total of 159, 87, and 28 DEPs were identified from group A (T0-SS/T0-IS), group B (T0-SS/T2-IS), and group C (T2-IS/T0-IS), respectively. Among these, 104, 63, and 22 proteins were up-regulated, and 55, 24, and 6 proteins were down-regulated, respectively. Approximately half of these DEPs were involved in carbohydrate metabolism (sucrose-to-starch metabolism and energy metabolism) and protein metabolism (protein synthesis, folding, degradation, and storage).

CONCLUSIONS

Reduced endosperm cell division and decreased activities of key enzymes associated with sucrose-starch metabolism and nitrogen metabolism are mainly attributed to the poor sink strength of IS. In addition, due to weakened photosynthesis and respiration, IS are unable to obtain a timely supply of materials and energy after fertilization, which might be resulted in the stagnation of IS development. Finally, an increased abundance of 14-3-3 protein in IS could be involved in the inhibition of starch synthesis. The removal of SS contributed to transfer of assimilates to IS and enhanced enzymatic activities of carbon metabolism (sucrose synthase, starch branching enzyme, soluble starch synthase, and pullulanase) and nitrogen metabolism (aspartate amino transferase and alanine amino transferase), promoting starch and protein synthesis in IS. In addition, improvements in energy metabolism (greater abundance of pyrophosphate-fructose 6-phosphate 1-phosphotransferase) might be played a vital role in inducing the initiation of grain filling. These results collectively demonstrate that carbohydrate supply is the main cause of poor IS grain filling.

摘要

背景

大穗型水稻品种常常因迟开花的弱势小穗灌浆不良而无法实现其产量潜力。弱势小穗灌浆不良的生理和分子机制,以及增加同化物供应是否能够调节蛋白质丰度从而改善大穗型粳稻弱势小穗的灌浆情况,目前仍部分未知。

结果

在大穗型粳稻品系W1844开花期进行了两种小穗去除处理的田间试验,包括去除顶部1/3小穗(T1)和去除顶部2/3小穗(T2),以不去除小穗作为对照(T0)。去除小穗后,弱势小穗的大小、重量、结实率和灌浆速率均显著增加。在开花后10天,利用iTRAQ技术研究了强势小穗和弱势小穗之间差异表达蛋白(DEPs)的生物学功能以及弱势小穗对去除强势小穗的响应。分别从A组(T0 - SS/T0 - IS)、B组(T0 - SS/T2 - IS)和C组(T2 - IS/T0 - IS)中鉴定出159、87和28个DEPs。其中,分别有104、63和22个蛋白上调,55、24和6个蛋白下调。这些DEPs中约一半参与碳水化合物代谢(蔗糖 - 淀粉代谢和能量代谢)和蛋白质代谢(蛋白质合成、折叠、降解和储存)。

结论

胚乳细胞分裂减少以及与蔗糖 - 淀粉代谢和氮代谢相关的关键酶活性降低主要归因于弱势小穗的库强不足。此外,由于光合作用和呼吸作用减弱,弱势小穗在受精后无法及时获得物质和能量供应,这可能导致弱势小穗发育停滞。最后,弱势小穗中14 - 3 - 3蛋白丰度增加可能参与抑制淀粉合成。去除强势小穗有助于同化物向弱势小穗转移,并增强碳代谢(蔗糖合酶、淀粉分支酶、可溶性淀粉合酶和支链淀粉酶)和氮代谢(天冬氨酸氨基转移酶和丙氨酸氨基转移酶)的酶活性,促进弱势小穗中淀粉和蛋白质的合成。此外,能量代谢的改善(磷酸果糖激酶 - 6 - 磷酸 - 1 - 磷酸转移酶丰度增加)可能在诱导灌浆启动中起关键作用。这些结果共同表明碳水化合物供应是弱势小穗灌浆不良的主要原因。

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