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首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Analysis of the Type IV Fimbrial-Subunit Gene fimA of Xanthomonas hyacinthi: Application in PCR-Mediated Detection of Yellow Disease in Hyacinths
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Analysis of the Type IV Fimbrial-Subunit Gene fimA of Xanthomonas hyacinthi: Application in PCR-Mediated Detection of Yellow Disease in Hyacinths

机译:风信子黄单胞菌IV型纤维亚基基因fimA的分析:在PCR介导的风信子黄病检测中的应用

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A sensitive and specific detection method was developed for Xanthomonas hyacinthi; this method was based on amplification of a subsequence of the type IV fimbrial-subunit gene fimA from strain S148. The fimA gene was amplified by PCR with degenerate DNA primers designed by using the N-terminal and C-terminal amino acid sequences of trypsin fragments of FimA. The nucleotide sequence of fimA was determined and compared with the nucleotide sequences coding for the fimbrial subunits in other type IV fimbria-producing bacteria, such as Xanthomonas campestris pv. vesicatoria, Neisseria gonorrhoeae, and Moraxella bovis. In a PCR internal primers JAAN and JARA, designed by using the nucleotide sequences of the variable central and C-terminal region of fimA, amplified a 226-bp DNA fragment in all X. hyacinthi isolates. This PCR was shown to be pathovar specific, as assessed by testing 71 Xanthomonas pathovars and bacterial isolates belonging to other genera, such as Erwinia and Pseudomonas. Southern hybridization experiments performed with the labelled 226-bp DNA amplicon as a probe suggested that there is only one structural type IV fimbrial-gene cluster in X. hyacinthi. Only two Xanthomonas translucens pathovars cross-reacted weakly in PCR. Primers amplifying a subsequence of the fimA gene of X. campestris pv. vesicatoria (T. Ojanen-Reuhs, N. Kalkkinen, B. Westerlund-Wikström, J. van Doorn, K. Haahtela, E.-L. Nurmiaho-Lassila, K. Wengelink, U. Bonas, and T. K. Korhonen, J. Bacteriol. 179: 1280–1290, 1997) were shown to be pathovar specific, indicating that the fimbrial-subunit sequences are more generally applicable in xanthomonads for detection purposes. Under laboratory conditions, approximately 1,000 CFU of X. hyacinthi per ml could be detected. In inoculated leaves of hyacinths the threshold was 5,000 CFU/ml. The results indicated that infected hyacinths with early symptoms could be successfully screened for X. hyacinthi with PCR.
机译:开发了一种灵敏且特异的检测方法,用于Xanthomonas hyacinthi。该方法基于扩增菌株S148的IV型纤维亚基基因fimA的子序列。使用简并DNA引物通过PCR扩增fimA基因,简并DNA引物是使用FimA胰蛋白酶片段的N端和C端氨基酸序列设计的。确定了fimA的核苷酸序列,并将其与编码其他IV型产菌细菌例如坎氏单胞菌(Xanthomonas campestris pv)中的纤维亚基的核苷酸序列进行比较。 vesicatoria,淋病奈瑟菌和牛莫拉氏菌。在PCR中,通过使用fimA可变的中央和C端区域的核苷酸序列设计的内部引物JAAN和JARA,在所有X. hyacinthi分离物中扩增了226 bp的DNA片段。通过测试71个Xanthomonas病原菌和属于其他属(如欧文氏菌和假单胞菌)的细菌分离物,该PCR被证明是特定于病原菌的。用标记的226-bp DNA扩增子作为探针进行的Southern杂交实验表明,在X. hyacinthi中只有一个结构IV型纤维基因簇。在PCR中,只有两个Xanthomonas转透明质致病病原体交叉反应较弱。引物可扩增喜树耶尔森氏菌pv的fimA基因的亚序列。 vesicatoria(T. Ojanen-Reuhs,N.Kalkkinen,B.Westerlund-Wikström,J.van Doorn,K. Bacteriol。179:1280-1290,1997)被证明是病原体特异性的,表明该纤维亚基序列更普遍地应用于黄单胞菌中以进行检测。在实验室条件下,大约1000 CFU的X。每毫升可检测到hyacinthi 。在风信子的接种叶片中,阈值为5,000 CFU / ml。结果表明,具有早期症状的受感染风信子可以成功地筛查 X。 hyacinthi 进行PCR。

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