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多头绒泡菌中核糖体基因对微球菌核酸酶的可及性。

Accessibility of the ribosomal genes to micrococcal nuclease in Physarum polycephalum.

作者信息

Stalder J, Seebeck T, Braun R

出版信息

Biochim Biophys Acta. 1979 Feb 27;561(2):452-63. doi: 10.1016/0005-2787(79)90153-9.

Abstract

In Physarum polycephalum most genes coding for ribosomal RNA are not integrated in chromosomes, but are located in many copies in the nucleolus as plasmid-like palindromic DNA molecules. To find out whether coding sequences of rDNA are organized in a chromatin-like structure similar to that of bulk chromatin, nuclei were treated with micrococcal nuclease and DNA fragments were isolated. From bulk chromatin multimers of a basic unit of 170-180 base pairs were obtained. Nuclease fragmented DNA hybridized with labelled 19-S + 26-S rRNA was found to give the same saturation value as did unfragmented control DNA. No preferential degradation of ribosomal genes to acid soluble products was observed. A more detailed analysis of the nuclease degradation products was carried out with fragments separated by preparative gel electrophoresis. DNA eluted from the gels was hybridized in solution with labelled 19-S + 26-S rRNA. The coding sequences of rRNA were found to be degraded to approximately nucleosome size slightly more quickly than was the DNA of bulk chromatin. However, the distribution of the rDNA fragments on the gels did not coincide with the distribution of the fragments derived from bulk chromatin nucleosomes and their oligomers. The amount of rDNA in the interband regions was about intermediate between that found in the two adjacent bands. These results lead to the conclusion that the ribosomal genes, most of which are presumably active during rapid growth, are protected by proteins, probably histones. However, the ribosomal genes are present in a structure differing in some way from that of bulk chromatin.

摘要

在多头绒泡菌中,大多数编码核糖体RNA的基因并未整合到染色体中,而是以质粒样回文DNA分子的形式大量存在于核仁中。为了弄清楚核糖体DNA(rDNA)的编码序列是否以类似于整体染色质的染色质样结构组织,用微球菌核酸酶处理细胞核并分离DNA片段。从整体染色质中获得了170 - 180个碱基对基本单位的多聚体。发现与标记的19 - S + 26 - S rRNA杂交的核酸酶切割后的DNA与未切割的对照DNA具有相同的饱和度值。未观察到核糖体基因优先降解为酸溶性产物。用制备性凝胶电泳分离的片段对核酸酶降解产物进行了更详细的分析。从凝胶上洗脱的DNA在溶液中与标记的19 - S + 26 - S rRNA杂交。发现rRNA的编码序列降解速度比整体染色质的DNA略快,降解产物大小约为核小体大小。然而,凝胶上rDNA片段的分布与源自整体染色质核小体及其寡聚体的片段分布不一致。带间区域的rDNA量约介于两个相邻带中的量之间。这些结果得出结论,大多数核糖体基因可能在快速生长期间处于活跃状态,它们受到蛋白质(可能是组蛋白)的保护。然而,核糖体基因以某种方式存在于与整体染色质不同的结构中。

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