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针对基因组的组蛋白滴定设定了非洲爪蟾中囊胚转换的DNA与细胞质阈值。

Histone titration against the genome sets the DNA-to-cytoplasm threshold for the Xenopus midblastula transition.

作者信息

Amodeo Amanda A, Jukam David, Straight Aaron F, Skotheim Jan M

机构信息

Departments of Biology and.

Biochemistry, Stanford University, Stanford, CA 94305

出版信息

Proc Natl Acad Sci U S A. 2015 Mar 10;112(10):E1086-95. doi: 10.1073/pnas.1413990112. Epub 2015 Feb 23.

Abstract

During early development, animal embryos depend on maternally deposited RNA until zygotic genes become transcriptionally active. Before this maternal-to-zygotic transition, many species execute rapid and synchronous cell divisions without growth phases or cell cycle checkpoints. The coordinated onset of transcription, cell cycle lengthening, and cell cycle checkpoints comprise the midblastula transition (MBT). A long-standing model in the frog, Xenopus laevis, posits that MBT timing is controlled by a maternally loaded inhibitory factor that is titrated against the exponentially increasing amount of DNA. To identify MBT regulators, we developed an assay using Xenopus egg extract that recapitulates the activation of transcription only above the DNA-to-cytoplasm ratio found in embryos at the MBT. We used this system to biochemically purify factors responsible for inhibiting transcription below the threshold DNA-to-cytoplasm ratio. This unbiased approach identified histones H3 and H4 as concentration-dependent inhibitory factors. Addition or depletion of H3/H4 from the extract quantitatively shifted the amount of DNA required for transcriptional activation in vitro. Moreover, reduction of H3 protein in embryos induced premature transcriptional activation and cell cycle lengthening, and the addition of H3/H4 shortened post-MBT cell cycles. Our observations support a model for MBT regulation by DNA-based titration and suggest that depletion of free histones regulates the MBT. More broadly, our work shows how a constant concentration DNA binding molecule can effectively measure the amount of cytoplasm per genome to coordinate division, growth, and development.

摘要

在早期发育过程中,动物胚胎依赖母源沉积的RNA,直到合子基因转录激活。在母源-合子转变之前,许多物种进行快速同步的细胞分裂,没有生长阶段或细胞周期检查点。转录的协调起始、细胞周期延长和细胞周期检查点构成了中囊胚转变(MBT)。在非洲爪蟾(Xenopus laevis)中,一个长期存在的模型认为,MBT的时间是由母源加载的抑制因子控制的,该因子会与指数增加的DNA量进行滴定。为了鉴定MBT调节因子,我们开发了一种利用非洲爪蟾卵提取物的检测方法,该方法仅在MBT时胚胎中发现的DNA与细胞质比例以上才能重现转录激活。我们使用这个系统对低于阈值DNA与细胞质比例时负责抑制转录的因子进行生化纯化。这种无偏差的方法确定组蛋白H3和H4是浓度依赖性抑制因子。从提取物中添加或去除H3/H4会定量改变体外转录激活所需的DNA量。此外,胚胎中H3蛋白的减少会诱导过早的转录激活和细胞周期延长,而添加H3/H4会缩短MBT后的细胞周期。我们的观察结果支持了一种基于DNA滴定的MBT调节模型,并表明游离组蛋白的消耗调节MBT。更广泛地说,我们的工作展示了一种恒定浓度的DNA结合分子如何有效地测量每个基因组的细胞质量,以协调分裂、生长和发育。

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