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High-Density Detection of Restriction-Site-Associated DNA Markers for Rapid Mapping of Mutated Loci in Neurospora

机译:限制性位点相关DNA标记的高密度检测用于快速定位神经孢菌中的突变基因座

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摘要

The wealth of sequence information available for Neurospora crassa and other fungi has greatly facilitated evolutionary and molecular analyses of this group. Although “reverse” genetics, in which genes are first identified by their sequence rather than by their mutant phenotypes, serves as a valuable new approach for elucidating biological processes, classical “forward” genetic analysis is still extremely useful. Unfortunately, mapping mutations and identifying the corresponding genes has typically been slow and laborious. To facilitate forward genetics in Neurospora, we have adapted microarray-based restriction-site-associated DNA (RAD) mapping for use with N. crassa oligonucleotide microarrays. This technique was used to simultaneously detect an unprecedented number of genomewide restriction site polymorphisms from two N. crassa strains: Mauriceville and Oak Ridge. Furthermore, RAD mapping was used to quickly map a previously unknown gene, defective in methylation-7 (dim-7).
机译:可用于crusspora crassa和其他真菌的大量序列信息极大地促进了该组的进化和分子分析。尽管首先通过序列而非突变表型鉴定基因的“反向”遗传学是阐明生物学过程的有价值的新方法,但经典的“正向”遗传分析仍然非常有用。不幸的是,定位突变和鉴定相应的基因通常是缓慢而费力的。为了促进Neurospora中的正向遗传学,我们调整了基于微阵列的限制位点相关的DNA(RAD)定位图,以与N. crassa寡核苷酸微阵列一起使用。这项技术用于同时检测来自两个猪笼草的两个基因组:莫里斯维尔(Mauriceville)和橡树岭(Oak Ridge)的前所未有的全基因组限制位点多态性。此外,RAD定位用于快速定位甲基化7(dim-7)有缺陷的先前未知的基因。

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