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核糖体蛋白mRNA的组织特异性积累与rRNA转录不同步,且先于海胆长腕幼虫的生长。

Tissue-restricted accumulation of a ribosomal protein mRNA is not coordinated with rRNA transcription and precedes growth of the sea urchin pluteus larva.

作者信息

Angerer L M, Yang Q, Liesveld J, Kingsley P D, Angerer R C

机构信息

Department of Biology, University of Rochester, New York 14627.

出版信息

Dev Biol. 1992 Jan;149(1):27-40. doi: 10.1016/0012-1606(92)90261-e.

Abstract

We have identified an mRNA that encodes a protein, SpS24, of the small ribosomal subunit in the sea urchin, Strongylocentrotus purpuratus. RNA blot and in situ hybridization analyses show that the SpS24 gene is active during early oogenesis, downregulated in the mature egg and during cleavage, and reactivated in the early blastula. The mRNA then increases in abundance at least 100-fold. Later in development, expression of SpS24 mRNA becomes restricted primarily to cells in the oral ectoderm and endoderm of the pluteus larva, and the message is undetectable in aboral ectoderm cells and most mesenchyme cells. To determine whether transcription of the ribosomal RNA genes occurs at a higher rate in oral ectoderm and endoderm tissues, a probe for the transcribed spacer was used in RNase protection and in situ hybridization assays. High concentrations of rRNA-processing intermediates were observed in unfertilized eggs and shown to reside primarily, if not exclusively, in the cytoplasm. The spatial and temporal distributions of these sequences strongly suggest that they are associated with heavy bodies. New embryonic rRNA transcripts are first detectable at the very early blastula stage. In later embryos, the content of this transcribed spacer sequence is similar in all but a few cells, which implies that they synthesize rRNA at a similar low rate. Comparison of available estimates of rRNA transcription rate with the potential rate of SpS24 protein synthesis, calculated from SpS24 mRNA prevalence, shows that oral ectoderm and endoderm cells have the capacity to synthesize 15- to 30-fold more SpS24 protein than is required to keep pace with rRNA synthesis in these cells. Because the sea urchin embryo develops from an egg to a pluteus larva in the absence of growth, this stockpiling of SpS24 mRNA anticipates rather than accompanies the onset of growth, which does not begin until after feeding. Upregulation of this gene is therefore part of the developmental program, rather than a physiological response to nutrient availability.

摘要

我们已经鉴定出一种信使核糖核酸(mRNA),它编码海胆紫海胆小核糖体亚基中的一种蛋白质SpS24。RNA印迹和原位杂交分析表明,SpS24基因在卵子发生早期是活跃的,在成熟卵子和卵裂期间表达下调,并在囊胚早期重新激活。然后,该mRNA的丰度至少增加100倍。在发育后期,SpS24 mRNA的表达主要局限于长腕幼虫口外胚层和内胚层的细胞,而在反口外胚层细胞和大多数间充质细胞中检测不到该信使核糖核酸。为了确定核糖体RNA基因在口外胚层和内胚层组织中的转录速率是否更高,在核糖核酸酶保护和原位杂交试验中使用了转录间隔区的探针。在未受精卵中观察到高浓度的rRNA加工中间体,并且显示这些中间体主要(如果不是唯一的话)存在于细胞质中。这些序列的时空分布强烈表明它们与多核糖体相关。新的胚胎rRNA转录本最早在囊胚早期可以检测到。在后期胚胎中,除少数细胞外,所有细胞中这种转录间隔区序列的含量相似,这意味着它们以相似的低速率合成rRNA。将rRNA转录速率的现有估计值与根据SpS24 mRNA丰度计算的SpS24蛋白质合成潜在速率进行比较,结果表明,口外胚层和内胚层细胞合成SpS24蛋白质的能力比这些细胞中与rRNA合成同步所需的能力高15至30倍。由于海胆胚胎在没有生长的情况下从卵子发育成长腕幼虫,SpS24 mRNA的这种储备是预期而非伴随生长开始的,生长直到摄食后才开始。因此,该基因的上调是发育程序的一部分,而不是对营养可用性的生理反应。

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