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苔藓原丝体中的细胞分化:一项形态学与实验研究

Cellular differentiation in moss protonemata: a morphological and experimental study.

作者信息

Pressel Silvia, Ligrone Roberto, Duckett Jeffrey G

机构信息

School of Biological and Chemical Sciences, Queen Mary University of London, Mile End Road, London, E1 4NS, UK.

出版信息

Ann Bot. 2008 Aug;102(2):227-45. doi: 10.1093/aob/mcn080. Epub 2008 May 27.

Abstract

BACKGROUND AND AIMS

Previous studies of protonemal morphogenesis in mosses have focused on the cytoskeletal basis of tip growth and the production of asexual propagules. This study provides the first comprehensive description of the differentiation of caulonemata and rhizoids, which share the same cytology, and the roles of the cytoskeleton in organelle shaping and spatial arrangement.

METHODS

Light and electron microscope observations were carried out on in vitro cultured and wild protonemata from over 200 moss species. Oryzalin and cytochalasin D were used to investigate the role of the cytoskeleton in the cytological organization of fully differentiated protonemal cells; time-lapse photography was employed to monitor organelle positions.

KEY RESULTS

The onset of differentiation in initially highly vacuolate subapical cells is marked by the appearance of tubular endoplasmic reticulum (ER) profiles with crystalline inclusions, closely followed by an increase in rough endoplasmic reticulum (RER). The tonoplast disintegrates and the original vacuole is replaced by a population of vesicles and small vacuoles originating de novo from RER. The cytoplasm then becomes distributed throughout the cell lumen, an event closely followed by the appearance of endoplasmic microtubules (MTs) in association with sheets of ER, stacks of vesicles that subsequently disperse, elongate mitochondria and chloroplasts and long tubular extensions at both poles of the nucleus. The production of large vesicles by previously inactive dictysomes coincides with the deposition of additional cell wall layers. At maturity, the numbers of endoplasmic microtubules decline, dictyosomes become inactive and the ER is predominantly smooth. Fully developed cells remain largely unaffected by cytochalasin; oryzalin elicits profound cytological changes. Both inhibitors elicit the formation of giant plastids. The plastids and other organelles in fully developed cells are largely stationary.

CONCLUSIONS

Differentiation of caulonemata and rhizoids involves a remarkable series of cytological changes, some of which closely recall major events in sieve element ontogeny in tracheophytes. The cytology of fully differentiated cells is remarkably similar to that of moss food-conducting cells and, in both, is dependent on an intact microtubule cytoskeleton. The disappearance of the major vacuolar apparatus is probably related to the function of caulonema and rhizoids in solute transport. Failure of fully differentiated caulonema and rhizoid cells to regenerate is attributed to a combination of endo-reduplication and irreversible tonoplast fragmentation. The formation of giant plastids, most likely by fusion, following both oryzalin and cytochalasin treatments, suggests key roles for both microtubules and microfilaments in the spatial arrangement and replication of plastids.

摘要

背景与目的

以往对苔藓原丝体形态发生的研究主要集中在顶端生长的细胞骨架基础以及无性繁殖体的产生。本研究首次全面描述了具有相同细胞学特征的茎丝和假根的分化过程,以及细胞骨架在细胞器塑形和空间排列中的作用。

方法

对200多种苔藓的体外培养和野生原丝体进行了光学显微镜和电子显微镜观察。使用oryzalin和细胞松弛素D研究细胞骨架在完全分化的原丝体细胞细胞学组织中的作用;采用延时摄影监测细胞器位置。

关键结果

最初高度液泡化的亚顶端细胞开始分化时,出现带有晶体包涵体的管状内质网(ER)轮廓,随后粗面内质网(RER)增加。液泡膜解体,原来的液泡被大量从头起源于RER的小泡和小液泡取代。细胞质随后分布于整个细胞腔,紧接着内质微管(MTs)与内质网片层、随后分散的小泡堆叠、伸长的线粒体和叶绿体以及细胞核两极的长管状延伸物一起出现。先前不活跃的高尔基体产生大泡与额外细胞壁层的沉积同时发生。成熟时,内质微管数量减少,高尔基体变得不活跃,内质网主要为光滑型。完全发育的细胞在很大程度上不受细胞松弛素影响;oryzalin引发深刻的细胞学变化。两种抑制剂都引发巨大质体的形成。完全发育细胞中的质体和其他细胞器在很大程度上是静止的。

结论

茎丝和假根的分化涉及一系列显著的细胞学变化,其中一些变化与维管植物筛管分子个体发育中的主要事件极为相似。完全分化细胞 的细胞学与苔藓营养传导细胞的细胞学非常相似,并且在这两种细胞中,都依赖于完整的微管细胞骨架。主要液泡结构的消失可能与茎丝和假根在溶质运输中的功能有关。完全分化的茎丝细胞和假根细胞无法再生归因于核内复制和不可逆的液泡膜碎片化的共同作用。oryzalin和细胞松弛素处理后形成巨大质体,最有可能是通过融合形成,这表明微管和微丝在质体的空间排列和复制中起关键作用。

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