首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Genotyping of Madurella mycetomatis by Selective Amplification of Restriction Fragments (Amplified Fragment Length Polymorphism) and Subtype Correlation with Geographical Origin and Lesion Size
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Genotyping of Madurella mycetomatis by Selective Amplification of Restriction Fragments (Amplified Fragment Length Polymorphism) and Subtype Correlation with Geographical Origin and Lesion Size

机译:通过选择性扩增限制性片段(扩增的片段长度多态性)以及分型与地理起源和病变大小的相关性,对食小孔虫进行基因分型

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摘要

One of the causative organisms of mycetoma is the fungus Madurella mycetomatis. Previously, extensive molecular typing studies identified Sudanese isolates of this fungus as clonal, but polymorphic genetic markers have not yet been identified. Here, we report on the selective amplification of restriction fragment (AFLP) analysis of 37 Sudanese clinical isolates of M. mycetomatis. Of 93 AFLP fragments generated, 25 were polymorphic, and 12 of these 25 polymorphic fragments were found in a large fraction of the strains. Comparative analysis resulted into a tree, composed of two main (clusters I and II) and one minor cluster (cluster III). Seventy-five percent of the strains found in cluster I originated from central Sudan, while the origin of the strains in cluster II was more heterogeneous. Furthermore, the strains found in cluster I were generally obtained from lesions larger than those from which the strains found in cluster II were obtained (chi-square test for trend, P = 0.03). Among the 12 more commonly found polymorphisms, 4 showed sequence homology with known genes. Marker A7 was homologous to an endo-1,4-beta-glucanase from Aspergillus oryzae, 97% identical markers A12 and B3 matched a hypothetical protein from Gibberella zeae, and marker B4 was homologous to casein kinase I from Danio rerio. The last marker seemed to be associated with strains originating from central Sudan (P = 0.001). This is the first report on a genotypic study where genetic markers which may be used to study pathogenicity in M. mycetomatis were obtained.
机译:菌丝瘤的致病生物之一是真菌霉菌。以前,广泛的分子分型研究将苏丹分离的这种真菌鉴定为克隆,但尚未鉴定出多态性遗传标记。在这里,我们报告了37例苏丹分枝杆菌的临床分离株的限制性片段的选择性扩增(AFLP)分析。在产生的93个AFLP片段中,有25个是多态片段,在这25个多态片段中,有12个在很大一部分菌株中被发现。比较分析得出一棵树,该树由两个主要群集(群集I和II)和一个较小群集(群集III)组成。在第一类中发现的菌株中有百分之七十五来自苏丹中部,而第二类中的菌株起源更为异质。此外,在群集I中发现的菌株通常来自比在群集II中发现的菌株更大的病变(卡方检验趋势,P = 0.03)。在12种较常见的多态性中,有4种与已知基因具有序列同源性。标记A7与米曲霉的内切1,4-β-葡聚糖酶同源,97%相同的标记A12和B3与来自玉米赤霉菌的假定蛋白匹配,标记B4与来自达尼奥里奥的酪蛋白激酶I同源。最后一个标记似乎与源自苏丹中部的菌株有关(P = 0.001)。这是有关基因型研究的第一份报告,其中获得了可用于研究食管分枝杆菌致病性的遗传标记。

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