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两栖类灯刷染色体的电子显微镜原位杂交

Electron microscopic in situ hybridization in amphibian lampbrush chromosomes.

作者信息

Bonnanfant-Jaïs M L, Penrad-Mobayed M, Angelier N

机构信息

Centre de Biologie Cellulaire, Ivry-sur-Seine/France.

出版信息

Eur J Cell Biol. 1993 Aug;61(2):362-8.

PMID:7693473
Abstract

Electron microscopy RNA/RNA in situ hybridization was adjusted to Pleurodeles lampbrush chromosomes. The cRNA probe used was synthesized from genomic DNA sequences which were proven to be moderately repetitive. Preembedding hybridization was performed on lampbrush chromosome preparations, and several fixation and hybridization conditions were tested. Paraformaldehyde and glutaraldehyde were used as fixatives at various concentrations and durations. Hybridization was then performed with or without formamide for various times of incubation. The best results were obtained when hybridization was carried out for 4 h at 42 degrees C in the presence of formamide, with lampbrush chromosomes having been previously fixed overnight in a mixture of paraformaldehyde/glutaraldehyde. Due to the excellent preservation of the ultrastructure and specificity of the signal obtained under these conditions, we were able to demonstrate, at the ultrastructural level, that such RNA expression occurs in two types of lampbrush loop ribonucleoprotein matrices showing a different morphology of their transcripts. Furthermore, a different mapping of the same sequence along the loop DNA axes is strongly suggested by a different labeling distribution in these loops.

摘要

电子显微镜RNA/RNA原位杂交技术已应用于有尾目动物的灯刷染色体。所用的cRNA探针是由经证实为中度重复的基因组DNA序列合成的。在灯刷染色体标本上进行包埋前杂交,并测试了几种固定和杂交条件。使用不同浓度和时间的多聚甲醛和戊二醛作为固定剂。然后在有或没有甲酰胺的情况下进行不同时间的杂交孵育。当在甲酰胺存在的情况下于42℃进行4小时杂交时,获得了最佳结果,此前灯刷染色体已在多聚甲醛/戊二醛混合物中固定过夜。由于在这些条件下获得的超微结构保存良好且信号具有特异性,我们能够在超微结构水平上证明,这种RNA表达发生在两种类型的灯刷环核糖核蛋白基质中,它们的转录本具有不同的形态。此外,这些环中不同的标记分布强烈表明同一序列沿环DNA轴的定位不同。

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