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非洲爪蟾精子中高度甲基化的核糖体DNA在卵母细胞中的转录。

Transcription in oocytes of highly methylated rDNA from Xenopus laevis sperm.

作者信息

Macleod D, Bird A

出版信息

Nature. 1983;306(5939):200-3. doi: 10.1038/306200a0.

Abstract

The genes for ribosomal RNA exist as multiple copies in the genome. Each repeated unit comprises a region that codes for the 40S rRNA precursor, and a spacer region of uncertain function (Fig. 1a). In Xenopus laevis there are about 1,000 copies of the dinucleotide sequence C-G in each repeat unit, and of these about 250 can be tested for the presence of 5-methylcytosine using restriction endonucleases. Most of the detectable C-Gs are heavily methylated, but in somatic cells unmethylated C-Gs occur in a 60 base pair (bp) sequence (NTS-60) that is repeated in the spacer. In contrast, the spacer of sperm rDNA is heavily methylated at these and all other testable C-Gs. Loss of methylation at NTS-60 takes place during the first day of embryonic development, near the time when rDNA transcription begins. In an attempt to assess the significance of this developmental change in methylation, we have isolated sperm rDNA and investigated whether it can be transcribed in oocytes. We have found that sperm rDNA is transcribed as efficiently as cloned rDNA, although no loss of methylation was detectable. Direct sequencing of sperm rDNA showed that all 19 C-GS in the promoter are highly methylated. Thus, in the case of rDNA injected into oocytes, loss of methylation is unnecessary for effective transcription.

摘要

核糖体RNA基因在基因组中以多拷贝形式存在。每个重复单元包含一个编码40S rRNA前体的区域和一个功能不明的间隔区(图1a)。在非洲爪蟾中,每个重复单元约有1000个二核苷酸序列C-G,其中约250个可以用限制性内切酶检测5-甲基胞嘧啶的存在。大多数可检测到的C-G都高度甲基化,但在体细胞中,未甲基化的C-G出现在间隔区重复的60个碱基对(bp)序列(NTS-60)中。相比之下,精子rDNA的间隔区在这些以及所有其他可检测的C-G处都高度甲基化。NTS-60处的甲基化缺失发生在胚胎发育的第一天,接近rDNA转录开始的时间。为了评估这种甲基化发育变化的意义,我们分离了精子rDNA并研究了它是否能在卵母细胞中被转录。我们发现精子rDNA的转录效率与克隆的rDNA一样高,尽管没有检测到甲基化的缺失。精子rDNA的直接测序表明,启动子中的所有19个C-G都高度甲基化。因此,在将rDNA注入卵母细胞的情况下,甲基化的缺失对于有效转录是不必要的。

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