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萌发的蒺藜苜蓿种子在失去和重新建立脱水耐受性过程中DNA和微管的变化

Changes in DNA and microtubules during loss and re-establishment of desiccation tolerance in germinating Medicago truncatula seeds.

作者信息

Faria José M R, Buitink Julia, van Lammeren André A M, Hilhorst Henk W M

机构信息

Laboratory of Plant Physiology, Wageningen University, Arboretumlaan 4, 6703 BD Wageningen, The Netherlands.

出版信息

J Exp Bot. 2005 Aug;56(418):2119-30. doi: 10.1093/jxb/eri210. Epub 2005 Jun 20.

Abstract

Desiccation tolerance (DT) in orthodox seeds is acquired during seed development and lost upon imbibition/germination, purportedly upon the resumption of DNA synthesis in the radicle cells. In the present study, flow cytometric analyses and visualization of microtubules (MTs) in radicle cells of seedlings of Medicago truncatula showed that up to a radicle length of 2 mm, there is neither DNA synthesis nor cell division, which were first detected in radicles with a length of 3 mm. However, DT started to be lost well before the resumption of DNA synthesis, when germinating seeds were dried back. By applying an osmotic treatment with polyethylene glycol (PEG) before dehydration, it was possible to re-establish DT in seedlings with a radicle up to 2 mm long. Dehydration of seedlings with a 2 mm radicle, with or without PEG treatment, caused disassembly of MTs and appearance of tubulin granules. Subsequent pre-humidification led to an almost complete disappearance of both MTs and tubulin granules. Upon rehydration, neither MTs nor tubulin granules were detected in radicle cells of untreated seedlings, while PEG-treated seedlings were able to reconstitute the microtubular cytoskeleton and continue their normal development. Dehydration of untreated seedlings also led to an apoptotic-like DNA fragmentation in radicle cells, while in PEG-treated seedlings DNA integrity was maintained. The results showed that for different cellular components, desiccation-tolerant seedlings may apply distinct strategies to survive dehydration, either by avoidance or further repair of the damages.

摘要

正统种子的耐干性(DT)在种子发育过程中获得,并在吸胀/萌发时丧失,据推测是在胚根细胞中DNA合成恢复时丧失。在本研究中,对蒺藜苜蓿幼苗胚根细胞进行的流式细胞术分析和微管(MTs)可视化显示,在胚根长度达到2 mm之前,既没有DNA合成也没有细胞分裂,而在长度为3 mm的胚根中首次检测到DNA合成和细胞分裂。然而,当萌发种子回干时,DT早在DNA合成恢复之前就开始丧失。通过在脱水前用聚乙二醇(PEG)进行渗透处理,有可能在胚根长度达2 mm的幼苗中重新建立DT。对胚根长2 mm的幼苗进行脱水处理,无论是否经过PEG处理,都会导致MTs解聚和微管蛋白颗粒出现。随后的预湿化导致MTs和微管蛋白颗粒几乎完全消失。复水后,未处理幼苗的胚根细胞中未检测到MTs和微管蛋白颗粒,而经过PEG处理的幼苗能够重新构建微管细胞骨架并继续正常发育。未处理幼苗的脱水还导致胚根细胞中出现凋亡样DNA片段化,而经过PEG处理的幼苗中DNA完整性得以维持。结果表明,对于不同的细胞成分,耐干燥的幼苗可能采用不同的策略来在脱水后存活,要么通过避免损伤,要么通过进一步修复损伤。

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