首页> 外文期刊>Soil Biology & Biochemistry >Quantification of Wautersia [Ralstonia] basilensis in the mycorrhizosphere of Pinus thunbergii Parl. and its effect on mycorrhizal formation
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Quantification of Wautersia [Ralstonia] basilensis in the mycorrhizosphere of Pinus thunbergii Parl. and its effect on mycorrhizal formation

机译:松柏菌根体内的Walutersia [Ralstonia] basilensis的定量。及其对菌根形成的影响

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The bacterium Wautersia [Ralstonia] basilensis has been shown to enhance the mycorrhizal symbiosis between Suillus granulatus and Pinus thunbergii (Japanese black pine). However, no information is available about this bacterium under field conditions. The objectives of this study were to detect W. basilensis in bulk and mycorhizosphere soils in a Japanese pine plantation in the Tottori Sand Dunes, determine the density of W. basilensis in soil, and determine the optimal cell density of W. basilensis for mycorrhizal formation in pine seedlings. We designed and validated 16S rRNA gene-targeted specific primers for detection and quantification of W. basilensis. SYBR Green I real-time PCR assay was used. A standard curve relating cultured W. basilensis cell density (10(3)10(8) cells ml1) to amplification of DNA showed a strong linear relationship (R = 0.9968). The specificity of the reaction was confirmed by analyzing DNA melting curves and sequencing of the amplicon. The average cell density of W. basilensis was >4.8 c 10(7) cells g1 of soil in the mycorrhizosphere and 7.0 c 10(6) cells g1 in the bulk soil. We evaluated the W. basilensis cell density required for mycorrhizal formation using an in vitro microcosm with various inoculum densities ranging from 10(2) to 10(7) cells g1 soil (10(4)10(9) cells ml1). Cell densities of W. basilensis of >10(6) cells g1 of soil were required to stimulate mycorrhizal formation. In vivo and in vitro experiments showed that W. basilensis was sufficiently abundant to enhance mycorrhizal formation in the mycorrhizosphere of Japanese black pine sampled from the Tottori Sand Dunes.
机译:业已证明,瓦特氏菌[Ralstonia] basilensis可以增强粒状牛肝菌和黑松(日本黑松)之间的菌根共生。但是,在田间条件下没有有关该细菌的信息。这项研究的目的是在鸟取沙丘的日本松树人工林中检测散装和根际土壤中的W.basilensis,确定土壤中的W.basilensis密度,并确定用于菌根形成的W.basilensis的最佳细胞密度。在松树苗中。我们设计和验证了16S rRNA基因靶向的特异性引物,用于W.basilensis的检测和定量。使用SYBR Green I实时PCR测定。有关培养的W.basilensis细胞密度(10(3)10(8)细胞ml1)与DNA扩增的标准曲线显示出很强的线性关系(R = 0.9968)。通过分析DNA解链曲线和扩增子的测序证实了反应的特异性。菌根土壤中W.basilensis的平均细胞密度> 4.8 c 10(7)g1,散装土壤中7.0 c 10(6)g1。我们使用体外接种物评估了菌根形成所需的W.basilensis细胞密度,该接种物具有从10(2)到10(7)细胞g1土壤(10(4)10(9)细胞ml1)的各种接种物密度。刺激土壤中菌根形成需要W.basilensis的细胞密度> 10(6)个细胞g1。体内和体外实验表明,从鸟取沙丘采集的日本黑松菌根中,W。basilensis足够丰富,可以增强菌根形成。

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