首页> 外文期刊>Journal of Clinical Microbiology >Preliminary study using species-specific oligonucleotide probe for rRNA of Bilophila wadsworthia.
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Preliminary study using species-specific oligonucleotide probe for rRNA of Bilophila wadsworthia.

机译:使用物种特异性寡核苷酸探针对Badophila wadsworthia的rRNA进行的初步研究。

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Portions of the 16S RNA from a urease-positive Bilophila wadsworthia strain were sequenced, and a probe was constructed. The probe was end labeled with [32P]ATP and polynucleotide kinase and hybridized on a nylon filter (by dot blot hybridization) to the immobilized rRNA of 12 B. wadsworthia strains and eight other anaerobic isolates. The probe efficiently hybridized only to the Bilophila strains. Cross-reactivity at high RNA levels (2,000 ng) was observed with one strain of Bacteroides thetaiotamicron and one strain of Bacteroides fragilis (with 10x SET buffer [20x SET buffer is 0.5 M NaCl, 0.03 M Tris, and 2 mM EDTA]) but was not seen at lower RNA levels or with 5x SET buffer. When tested against mixed cultures of aerobic and anaerobic isolates representative of appendiceal abscess flora, the probe did not react with mixed cultures containing no Bilophila cells and could detect > or = 10(5) Bilophila CFU/ml when the mixture was seeded with Bilophila cells. This probe is of potential use in the rapid identification of pure isolates and in the direct identification of B. wadsworthia in clinical specimens.
机译:对来自尿素酶阳性的嗜酸性双歧杆菌沃兹沃氏菌株的16S RNA的部分进行测序,并构建了探针。该探针末端用[32P] ATP和多核苷酸激酶标记,并在尼龙滤膜上杂交(通过斑点印迹杂交)到12个B. wadsworthia菌株和其他八个厌氧菌的固定rRNA上。该探针仅有效地与嗜盐菌菌株杂交。在一株拟杆菌(Theactotaides thetaiotamicron)和一株脆弱拟杆菌(Bacteroides the gilgilis)(使用10x SET缓冲液[20x SET缓冲液为0.5 M NaCl,0.03 M Tris和2 mM EDTA])中观察到了在高RNA水平(2,000 ng)下的交叉反应。在较低的RNA水平或使用5x SET缓冲液时未见到。当针对代表阑尾脓肿菌群的需氧和厌氧分离株的混合培养物进行测试时,该探针不与不包含Bilophila细胞的混合培养物反应,并且当将混合物接种Bilophila细胞时,可以检测到> = 10(5)Bilophila CFU / ml 。该探针可用于快速鉴定纯分离物和直接鉴定临床标本中的沃兹沃德氏菌。

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