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减数分裂过程中着丝粒组蛋白H3变体的装载——它与有丝分裂有何不同?

Loading of the centromeric histone H3 variant during meiosis-how does it differ from mitosis?

作者信息

Schubert Veit, Lermontova Inna, Schubert Ingo

机构信息

Leibniz Institute of Plant Genetics and Crop Plant Research (IPK), 06466, Gatersleben, Germany,

出版信息

Chromosoma. 2014 Oct;123(5):491-7. doi: 10.1007/s00412-014-0466-9. Epub 2014 May 8.

Abstract

In eukaryotic phyla studied so far, the essential centromeric histone H3 variant (CENH3) is loaded to centromeric nucleosomes after S-phase (except for yeast) but before mitotic segregation (except for metazoan). While the C-terminal part of CENH3 seems to be sufficient for mitotic centromere function in plants, meiotic centromeres neither load nor tolerate impaired CENH3 molecules. However, details about CENH3 deposition in meiocytes are unknown (except for Drosophila). Therefore, we quantified fluorescence signals after the immunostaining of CENH3 along meiotic and mitotic nuclear division cycles of rye, a monocotyledonous plant. One peak of fluorescence intensity appeared in the early meiotic prophase of pollen mother cells and a second one during interkinesis, both followed by a decrease of CENH3. Then, the next loading occurred in the male gametophyte before its first mitotic division. These data indicate that CENH3 loading differs between mitotic and meiotic nuclei. Contrary to the situation in mitotic cycles, CENH3 deposition is biphasic during meiosis and apparently linked with a quality check, a removal of impaired CENH3 molecules, and a general loss of CENH3 after each loading phase. These steps ensure an endowment of centromeres with a sufficient amount of correct CENH3 molecules as a prerequisite for centromere maintenance during mitotic cycles of the microgametophyte and the progeny. From a comparison with data available for Drosophila, we hypothesise that the post-divisional mitotic CENH3 loading in metazoans is evolutionarily derived from the post-divisional meiotic loading phase, while the pre-divisional first meiotic loading has been conserved among eukaryotes.

摘要

在迄今为止研究的真核生物门类中,必需的着丝粒组蛋白H3变体(CENH3)在S期之后(酵母除外)但在有丝分裂分离之前(后生动物除外)加载到着丝粒核小体上。虽然CENH3的C末端部分似乎足以在植物中发挥有丝分裂着丝粒功能,但减数分裂着丝粒既不加载也不容忍受损的CENH3分子。然而,关于CENH3在减数分裂细胞中的沉积细节尚不清楚(果蝇除外)。因此,我们对单子叶植物黑麦减数分裂和有丝分裂核分裂周期中CENH3进行免疫染色后的荧光信号进行了定量。花粉母细胞减数分裂前期早期出现一个荧光强度峰值,在减数分裂间期出现第二个峰值,随后CENH3含量下降。然后,下一次加载发生在雄配子体的第一次有丝分裂之前。这些数据表明,CENH3在有丝分裂和减数分裂细胞核中的加载情况不同。与有丝分裂周期的情况相反,CENH3在减数分裂过程中是双相沉积的,显然与质量检查、受损CENH3分子的去除以及每个加载阶段后CENH3的总体损失有关。这些步骤确保着丝粒拥有足够数量的正确CENH3分子,这是在小配子体及其后代的有丝分裂周期中维持着丝粒的先决条件。通过与果蝇的现有数据进行比较,我们假设后生动物中分裂后有丝分裂CENH3的加载在进化上源自分裂后减数分裂加载阶段,而分裂前的第一次减数分裂加载在真核生物中得以保留。

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