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Cloning and sequencing of the breakpoint regions of inversion 5g fixed in Drosophila buzzatii

机译:固定于果蝇的5g倒位断裂点的克隆与序列分析

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Chromosomal inversions are ubiquitous in Drosophila both as intraspecific polymorphisms and interspecific differences. Many gaps still remain in our understanding of the mechanisms that generate them. Previous work has shown that in Drosophila buzzatii, three polymorphic inversions were generated by ectopic recombination between copies of the transposon Galileo. In this study, we have characterized the breakpoint regions of inversion 5g, fixed in D. buzzatii and absent in Drosophila koepferae and other closely related species. A novel approach comprising four experimental steps was used. First, D. buzzatii BAC clones encompassing the breakpoints were identified and their ends sequenced. Then, breakpoint regions were mapped at high resolution in the Drosophila mojavensis genome sequence. Finally, breakpoint regions were isolated by polymerase chain reaction in D. buzzatii and D. koepferae and sequenced. Our aim was to shed light on the mechanism that generated inversion 5g and specifically to test for an implication of the transposon Galileo. No evidence implicates Galileo or other transposable elements in the origin of inversion 5g that was generated most likely by two independent breaks and non-homologous end-joining repair. Our results show that different inversion-generating mechanisms may coexist within the same lineage and suggest a hypothesis for the evolutionary time and mode of their operation. Communicated by B. Calvi
机译:染色体倒置在果蝇中普遍存在,既有种内多态性,又有种间差异。我们对产生这些差异的机制的理解仍然存在许多差距。先前的研究表明,在果蝇中,通过转座子伽利略的拷贝之间的异位重组产生了三个多态性倒置。在这项研究中,我们已经确定了倒置5g的断点区域的特征,该断点固定在Buzzatii中,而果蝇和其他紧密相关的物种中则不存在。使用了包括四个实验步骤的新颖方法。首先,鉴定了包含断点的巴氏梭状芽胞杆菌BAC克隆并对其末端进行测序。然后,在果蝇基因组序列中高分辨率定位断点区域。最终,通过聚合酶链反应在巴氏梭菌和科氏杆菌中分离出断点区域并测序。我们的目的是阐明产生5g倒置的机制,特别是测试转座子Galileo的含义。没有证据表明伽利略或其他转座因子可能是由两次独立断裂和非同源末端连接修复最有可能产生的5g反转源。我们的研究结果表明,不同的反转产生机制可能在同一谱系中共存,并为它们的进化时间和模式提出了假设。由B. Calvi传达

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