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Identification and characterisation of functional expressed sequence tags-derived simple sequence repeat (eSSR) markers for genetic linkage mapping of Schistosoma mansoni juvenile resistance and susceptibility loci in Biomphalaria glabrata

机译:功能性表达序列标签衍生的简单序列重复(eSSR)标记的鉴定和表征用于曼氏血吸虫幼虫抗性和易感基因座的遗传连锁作图

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摘要

Biomphalaria glabrata susceptibility to Schistosoma mansoni has a strong genetic component, offering the possibility for investigating host–parasite interactions at the molecular level, perhaps leading to novel control approaches. The identification, mapping and molecular characterisation of genes that influence the outcome of parasitic infection in the intermediate snail host is, therefore, seen as fundamental to the control of schistosomiasis. To better understand the evolutionary processes driving disease resistance/susceptibility phenotypes, we previously identified polymorphic random amplification of polymorphic DNA and genomic simple sequence repeats from B. glabrata. In the present study we identified and characterised polymorphic expressed simple sequence repeats markers (Bg-eSSR) from existing B. glabrata expressed sequence tags. Using these markers, and with previously identified genomic simple sequence repeats, genetic linkage mapping for parasite refractory and susceptibility phenotypes, the first known for B. glabrata, was initiated. Data mining of 54,309 expressed sequence tag, produced 660 expressed simple sequence repeats of which dinucleotide motifs (TA)n were the most common (37.88%), followed by trinucleotide (29.55%), mononucleotide (18.64%) and tetranucleotide (10.15%). Penta- and hexanucleotide motifs represented <3% of the Bg-eSSRs identified. While the majority (71%) of Bg-eSSRs were monomorphic between resistant and susceptible snails, several were, however, useful for the construction of a genetic linkage map based on their inheritance in segregating F2 progeny snails derived from crossing juvenile BS-90 and NMRI snails. Polymorphic Bg-eSSRs assorted into six linkage groups at a logarithm of odds score of 3. Interestingly, the heritability of four markers (Prim1_910, Prim1_771, Prim6_1024 and Prim7_823) with juvenile snail resistance were, by t-test, significant (P < 0.05) while an allelic marker, Prim24_524, showed linkage with the juvenile snail susceptibility phenotype. On the basis of our results it is possible that the gene(s) controlling juvenile resistance and susceptibility to S. mansoni infection in B. glabrata are not only on the same linkage group but lie within a short distance (42 cM) of each other.
机译:曼氏血吸虫的光滑小球菌具有很强的遗传成分,为在分子水平上研究宿主-寄生虫的相互作用提供了可能性,也许导致了新的控制方法。因此,影响中间蜗牛宿主寄生虫感染结果的基因的鉴定,作图和分子表征被认为是控制血吸虫病的基础。为了更好地理解驱动疾病抗性/敏感性表型的进化过程,我们先前鉴定了多态性DNA的多态性随机扩增和光滑双歧杆菌的基因组简单序列重复。在本研究中,我们从现有的光滑小球藻表达序列标签中鉴定并鉴定了多态表达的简单序列重复标记(Bg-eSSR)。使用这些标记物,并利用先前鉴定的基因组简单序列重复序列,开始了针对首次发现于光滑芽孢杆菌的寄生虫难治性和易感性表型的遗传连锁作图。数据挖掘54,309个表达的序列标签,产生660个表达的简单序列重复,其中最常见的是二核苷酸基序(TA)n(37.88%),其次是三核苷酸(29.55%),单核苷酸(18.64%)和四核苷酸(10.15%) 。五核苷酸和六核苷酸基序占所鉴定Bg-eSSR的<3%。虽然大多数(71%)Bg-eSSRs在抗性和易感蜗牛之间是单态的,但是,基于它们的遗传分离来自杂交幼体BS-90和F2后代的F2后代蜗牛,其中的一些对构建遗传连锁图很有用。 NMRI蜗牛。通过t检验,多态性Bg-eSSRs以3的对数比值对数分为6个连锁组,有趣的是,通过t检验,四个标记(Prim1_910,Prim1_771,Prim6_1024和Prim7_823)的遗传力显着(P <0.05) ),而等位基因标记Prim24_524显示与少年蜗牛敏感性表型相关。根据我们的研究结果,可能有一个基因控制着光滑芽孢杆菌中的少年抗性和对曼氏沙门氏菌感染的易感性,这些基因不仅在同一连接基团上,而且彼此之间的距离很短(42 cM) 。

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