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Evidence for unlinked rrn operons in the Planctomycete Pirellula marina.

机译:在Planctomycete Pirellula码头上无关联的rrn操纵子的证据。

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摘要

Southern hybridization of rRNAs to chromosomal BamHI-digested DNA of the eubacterium Pirellula marina revealed the presence of two sets of 16S and 23S rRNA genes. The two copies of the 23S rRNA genes, located on 11- and about 13-kilobase (kb) inserts, were isolated from a lambda bacteriophage Charon 35 library. The 11-kb fragment was cloned directly into pBR322, while a 5.4-kb BamHI-PstI rDNA subfragment of the approximately 13-kb insert was cloned into pUC18. Both recombinant plasmids, pPI1100 and pPI540, were characterized by restriction enzyme mapping and Southern hybridization with the large rRNA species. Restriction fragments from both inserts were subcloned into phage M13 mp18 and mp19. Correlation of genomic hybridization data with physical characterization of recombinant plasmids showed that, in contrast to the general organization of rrn operons in eubacteria, the 16S rRNA genes of P. marina are separated by at least 8.5 (pPI540) and 4.4 (pPI1100) kb, respectively, from the closely linked 23S-5S rRNA genes. Comparison of the flanking regions from both 23S-5S rRNA genes with published consensus sequences of structural elements indicates the presence of putative transcription signals, i.e., a single Pribnow box, discriminator, antitermination boxes A, B, and C, and a Rho-independent terminator.
机译:rRNA与真细菌Pirellula marina的染色体BamHI消化的DNA的Southern杂交显示存在两组16S和23S rRNA基因。从Lambda噬菌体Charon 35文库中分离了位于11碱基和大约13碱基(kb)插入片段上的23S rRNA基因的两个拷贝。将11kb片段直接克隆到pBR322中,而将大约13kb插入片段的5.4kb BamHI-PstI rDNA亚片段克隆到pUC18中。重组质粒pPI1100和pPI540均通过限制性酶切图谱和与大型rRNA的Southern杂交来表征。来自两个插入片段的限制性片段被亚克隆到噬菌体M13 mp18和mp19中。基因组杂交数据与重组质粒物理特性的相关性表明,与真细菌中rrn操纵子的一般组织形成对比,滨海假单胞菌的16S rRNA基因至少相距8.5(pPI540)和4.4(pPI1100)kb,分别来自紧密相连的23S-5S rRNA基因。将两个23S-5S rRNA基因的侧翼区域与已发表的结构元件共有序列进行比较,表明存在假定的转录信号,即单个Pribnow框,鉴别子,抗终止框A,B和C,以及Rho独立终结者。

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