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小鼠金属硫蛋白表达的个体发生:与甲胎蛋白基因的比较。

The ontogeny of expression of murine metallothionein: comparison with the alpha-fetoprotein gene.

作者信息

Andrews G K, Adamson E D, Gedamu L

出版信息

Dev Biol. 1984 Jun;103(2):294-303. doi: 10.1016/0012-1606(84)90317-8.

Abstract

The ontogeny of expression of mouse metallothionein was studied by RNA dot and Northern blot hybridization using a cloned cDNA probe. In some instances the synthesis of metallothionein was analyzed by cell-free translation of RNA as well as pulse-labeling of proteins in short-term organ cultures followed by polyacrylamide gel electrophoresis. Interesting parallels between metallothionein and alpha-fetoprotein gene expression during development were noted. Like alpha-fetoprotein mRNA ( Dziadek and Andrews, 1983), metallothionein mRNA was found to be abundant in developing liver as well as in visceral yolk sac endoderm. In addition, metallothionein mRNA was abundant in parietal yolk sac. During liver development metallothionein and alpha-fetoprotein mRNAs were abundant by Day 12 of gestation, increasing to maximal levels on Day 16 and decreasing during late fetal and neonatal life to basal levels in adult. Metallothionein mRNA increased in maternal liver and was also abundant in certain hepatomas. Synthesis of metallothionein and levels of metallothionein mRNA in visceral yolk sac increased from Day 9 of gestation to maximal levels on Days 11-12 and then decreased abruptly after Day 15. RNA from differentiated teratocarcinoma cells with primitive, parietal or visceral endoderm characteristics each contained high levels of metallothionein mRNA, whereas, levels of this mRNA varied widely among embryonal carcinoma stem cell lines. alpha-Fetoprotein mRNA was not detected in embryonal carcinoma cells but was expressed in visceral endoderm-like differentiated cells. These results indicate that parietal and visceral endoderm cells actively express the metallothionein gene and further suggest that expression may be initiated at the earlier stage of primitive endoderm.

摘要

利用克隆的cDNA探针,通过RNA斑点杂交和Northern印迹杂交研究了小鼠金属硫蛋白表达的个体发生。在某些情况下,通过RNA的无细胞翻译以及短期器官培养中蛋白质的脉冲标记,随后进行聚丙烯酰胺凝胶电泳,分析了金属硫蛋白的合成。注意到在发育过程中金属硫蛋白和甲胎蛋白基因表达之间有趣的相似之处。与甲胎蛋白mRNA一样(Dziadek和Andrews,1983),发现金属硫蛋白mRNA在发育中的肝脏以及内脏卵黄囊内胚层中含量丰富。此外,金属硫蛋白mRNA在壁层卵黄囊中含量丰富。在肝脏发育过程中,金属硫蛋白和甲胎蛋白mRNA在妊娠第12天时含量丰富,在第16天增加到最高水平,并在胎儿后期和新生儿期减少至成年期的基础水平。金属硫蛋白mRNA在母体肝脏中增加,并且在某些肝癌中也含量丰富。内脏卵黄囊中金属硫蛋白的合成和金属硫蛋白mRNA水平从妊娠第9天增加到第11 - 12天的最高水平,然后在第15天后突然下降。来自具有原始、壁层或内脏内胚层特征的分化畸胎瘤细胞的RNA各自含有高水平的金属硫蛋白mRNA,而这种mRNA的水平在胚胎癌细胞系中差异很大。在胚胎癌细胞中未检测到甲胎蛋白mRNA,但在内脏内胚层样分化细胞中表达。这些结果表明壁层和内脏内胚层细胞积极表达金属硫蛋白基因,并进一步表明表达可能在原始内胚层的早期阶段开始。

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