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脲酶阳性嗜热弯曲菌(UPTC)基因组DNA的首次限制性内切酶分析和基因图谱绘制,以及小限制性片段测序。

First restriction and genetic mapping of the genomic DNA of urease-positive thermophilic campylobacters (UPTC), and small restriction fragment sequencing.

作者信息

Aritomi T, Sekizuka T, Imamaki R, Murayama O, Millar B C, Moore J E, Matsuda M

机构信息

Laboratory of Molecular Biology, School of Environmental Health Sciences, Azabu University, Sagamihara, Japan.

出版信息

Br J Biomed Sci. 2006;63(2):63-7. doi: 10.1080/09674845.2006.11732722.

Abstract

A restriction and genetic map of urease-positive thermophilic campylobacter (UPTC) CF89-12 genome DNA is constructed using a pulsed-field gel electrophoresis procedure after digestion with SalI and SmaI and Southern blot hybridisation. Each of the six gene fragments (flaA, glyA, lysS, recA, sodB and ureAB) selected are mapped in only a fragment on the restriction map. Three DNA fragments for rrn operon probes are mapped in multiple regions on the map. When two SmaI-digested neighbouring small fragments hybridised with rrn probes are cloned and sequenced, a total sequence length of 7487 bp is determined. In the sequence, part of the pnp gene (734 bp) bearing a p-independent transcriptional termination region, a cluster of five tRNA genes including the putative promoter region, a hypothetical Cj0171-like 507-bp sequence containing an internal termination codon, and a part of the rrn operon including the putative promoter region (4700 bp) are identified. The 507 bp sequence carried both putative transcriptional promoter sequences, including a ribosome binding site upstream of the ATG start codon and a characteristic G9 structure, and a possible p-independent transcriptional termination region. A hypothetical Cj0170-like 204-bp sequence containing an internal termination codon also occurred, overlapping partly with the Cj0171-like sequence. Based on nucleotide sequence alignment analysis between the UPTC rrn operon examined here and the previously reported one, two different 16S-23S ribosomal DNA (rDNA) internal spacer regions are shown to exist.

摘要

用脉冲场凝胶电泳法,在经SalI和SmaI酶切及Southern印迹杂交后,构建了脲酶阳性嗜热弯曲杆菌(UPTC)CF89 - 12基因组DNA的限制性内切酶图谱和遗传图谱。所选择的六个基因片段(flaA、glyA、lysS、recA、sodB和ureAB)中的每一个都仅定位在限制性内切酶图谱的一个片段上。rrn操纵子探针的三个DNA片段定位在图谱的多个区域。当克隆并测序与rrn探针杂交的两个经SmaI酶切的相邻小片段时,确定了总序列长度为7487 bp。在该序列中,鉴定出带有不依赖于p的转录终止区的pnp基因的一部分(734 bp)、包括假定启动子区的五个tRNA基因簇、含有内部终止密码子且长度为507 bp的假定Cj0171样序列,以及包括假定启动子区的rrn操纵子的一部分(4700 bp)。507 bp序列同时携带假定的转录启动子序列,包括ATG起始密码子上游的核糖体结合位点和特征性G9结构,以及可能的不依赖于p的转录终止区。还出现了一个含有内部终止密码子且长度为204 bp的假定Cj0170样序列,它与Cj0171样序列部分重叠。基于此处检测的UPTC rrn操纵子与先前报道的rrn操纵子之间的核苷酸序列比对分析,显示存在两个不同的16S - 23S核糖体DNA(rDNA)内部间隔区。

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