Genetic diversity of Datisca cannabina-compatible Frankia strains as determined by sequence analysis of the PCR-amplified 16S rRNA gene.

M S Mirza; S Hameed; A D Akkermans

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Genetic diversity of Datisca cannabina-compatible Frankia strains as determined by sequence analysis of the PCR-amplified 16S rRNA gene.

机译：通过PCR扩增的16S rRNA基因的序列分析确定了与Datisca canabina兼容的Frankia菌株的遗传多样性。

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The presence of Frankia strains in soil samples collected from northern areas of Pakistan was detected by inoculating Coriaria nepalensis and Datisca cannabina plants. The abundance of compatible Frankia strains in some areas was indicated by profuse nodulation of the host plants, whereas soil samples from other localities failed to result in nodulation. An oligonucleotide probe (COR/DAT) directed against the 16S rRNA gene of the endophytes of Coriaria and Datisca spp. that did not cross-react with the RNA gene of Frankia strains isolated from other hosts was developed. Genetic diversity among Frankia strains nodulating D. cannabina was determined by sequence analysis of the partial 16S rRNA gene amplified from nodules induced by soil samples from different localities by PCR. Four types of Frankia sequences and one non-Frankia sequence were detected by hybridization with a Frankia genus probe and the COR/DAT probe as well as by sequence analysis of the cloned PCR products.

机译：通过接种尼泊尔海i和Datisca cannabina植物，可以检测到从巴基斯坦北部地区收集的土壤样品中存在Frankia菌株。寄主植物的结瘤表明某些地区有足够的相容性Frankia菌株，而其他地区的土壤样品未能结瘤。针对Coriaria和Datisca spp内生菌的16S rRNA基因的寡核苷酸探针（COR / DAT）。与其他宿主分离的Frankia菌株的RNA基因没有交叉反应。通过PCR分析不同地方土壤样品诱导的结节中扩增的部分16S rRNA基因的序列，从而确定了根瘤菌D. cannabina的Frankia菌株之间的遗传多样性。通过与Frankia属探针和COR / DAT探针杂交以及对克隆的PCR产物进行序列分析，检测到四种类型的Frankia序列和一种非Frankia序列。

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《Applied and Environmental Microbiology》 |1994年第7期|共6页
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M S Mirza; S Hameed; A D Akkermans;
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中图分类植物学;
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6. Genetic diversity of Datisca cannabina-compatible Frankia strains as determined by sequence analysis of the PCR-amplified 16S rRNA gene. [O] . M S Mirza, S Hameed, A D Akkermans 1994

机译：通过PCR扩增的16S rRNA基因的序列分析确定了与Datisca canabina兼容的Frankia菌株的遗传多样性。
7. Genetic diversity of Pasteurella multocida fowl cholera isolates as demonstrated by ribotyping and 16S rRNA and partial atpD sequence comparisons The GenBank accession numbers for the 16S rRNA sequences of strain HIM 830-7T (NCTC 10204T) and 77179 of P. multocida subsp. gallicida and HIM 746-6T (NCTC 11619T) of P. multocida subsp. septica are AF326323, AF326324 and AF326325, respectively; those for the atpD nucleotide sequences are in Fig. 3. [O] . Kamille D Petersen, Henrik Christensen, Magne Bisgaard, 2001

机译：通过核划分和16S rRNA和部分ATPD序列所证明的巴斯氏菌和部分ATPD序列的遗传多样性与16S rRNA和部分ATPD序列的菌株对菌株630-7T（NCTC 10204T）和77179的P. Multocida Subsp进行比较。 Gallicida和他746-6T（NCTC 11619T）的P. Multocida Subsp。 Septica分别是AF326323，AF326324和AF326325;用于ATPD核苷酸序列的那些在图2中。3。

Genetic diversity of Datisca cannabina-compatible Frankia strains as determined by sequence analysis of the PCR-amplified 16S rRNA gene.

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