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对主要效应贡献者进行顺序剔除,可鉴定出调控酵母高温生长的其他数量性状基因座。

Sequential elimination of major-effect contributors identifies additional quantitative trait loci conditioning high-temperature growth in yeast.

作者信息

Sinha Himanshu, David Lior, Pascon Renata C, Clauder-Münster Sandra, Krishnakumar Sujatha, Nguyen Michelle, Shi Getao, Dean Jed, Davis Ronald W, Oefner Peter J, McCusker John H, Steinmetz Lars M

机构信息

European Molecular Biology Laboratory, Heidelberg, Germany.

出版信息

Genetics. 2008 Nov;180(3):1661-70. doi: 10.1534/genetics.108.092932. Epub 2008 Sep 9.

Abstract

Several quantitative trait loci (QTL) mapping strategies can successfully identify major-effect loci, but often have poor success detecting loci with minor effects, potentially due to the confounding effects of major loci, epistasis, and limited sample sizes. To overcome such difficulties, we used a targeted backcross mapping strategy that genetically eliminated the effect of a previously identified major QTL underlying high-temperature growth (Htg) in yeast. This strategy facilitated the mapping of three novel QTL contributing to Htg of a clinically derived yeast strain. One QTL, which is linked to the previously identified major-effect QTL, was dissected, and NCS2 was identified as the causative gene. The interaction of the NCS2 QTL with the first major-effect QTL was background dependent, revealing a complex QTL architecture spanning these two linked loci. Such complex architecture suggests that more genes than can be predicted are likely to contribute to quantitative traits. The targeted backcrossing approach overcomes the difficulties posed by sample size, genetic linkage, and epistatic effects and facilitates identification of additional alleles with smaller contributions to complex traits.

摘要

几种数量性状基因座(QTL)定位策略能够成功识别主效基因座,但在检测微效基因座时往往成功率较低,这可能是由于主基因座的混杂效应、上位性以及样本量有限所致。为克服这些困难,我们采用了一种定向回交定位策略,该策略从基因层面消除了先前鉴定出的酵母高温生长(Htg)相关主QTL的影响。此策略有助于定位对临床来源酵母菌株的Htg有贡献的三个新QTL。其中一个与先前鉴定的主效QTL连锁的QTL被剖析,NCS2被确定为致病基因。NCS2 QTL与第一个主效QTL的相互作用依赖于遗传背景,揭示了跨越这两个连锁基因座的复杂QTL结构。这种复杂结构表明,可能有比预期更多的基因对数量性状有贡献。定向回交方法克服了样本量、遗传连锁和上位性效应带来的困难,并有助于识别对复杂性状贡献较小的其他等位基因。

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