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Oligonucleotide Probes That Hybridize with rRNA as a Tool To Study Frankia Strains in Root Nodules

机译:与rRNA杂交的寡核苷酸探针作为研究根瘤中Frankia菌株的工具

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Oligonucleotide probes that hybridize with specific sequences in variable regions of the 16S rRNA of the nitrogen-fixing actinomycete Frankia were used for the identification of Frankia strains in nodules. Frankia cells were released from plant tissue by grinding glutaraldehyde-fixed root nodules in guanidine hydrochloride solution. rRNA was obtained after sonication, precipitation with ethanol, and purification by phenolchloroform extraction. Degradation of rRNA, evident in Northern blots, did not affect hybridization with the oligonucleotides. Nodules of about 1 mg (fresh weight) provided sufficient rRNA for reliable detection of the Frankia strain. The utility of this rRNA extraction method was tested in a competition experiment between two effective Frankia strains on cloned Alnus glutinosa plants.
机译:与固氮放线菌弗兰克菌的16S rRNA可变区中的特定序列杂交的寡核苷酸探针用于鉴定结核中的弗兰克菌菌株。通过在盐酸胍溶液中研磨戊二醛固定的根瘤,从植物组织中释放Frankia细胞。超声处理,乙醇沉淀并通过苯酚氯仿萃取纯化后,得到rRNA。在RNA印迹中明显的rRNA的降解不影响与寡核苷酸的杂交。约1 mg(鲜重)的结节提供了足够的rRNA,可以可靠地检测Frankia菌株。这种rRNA提取方法的效用在克隆的Alnus glutinosa植物上的两个有效Frankia菌株之间的竞争实验中进行了测试。

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