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大麦4H染色体短臂端粒附近麦芽品质数量性状基因座复合体的精细定位

Fine mapping of a malting-quality QTL complex near the chromosome 4H S telomere in barley.

作者信息

Gao W, Clancy J A, Han F, Jones B L, Budde A, Wesenberg D M, Kleinhofs A, Ullrich S E

机构信息

Department of Crop and Soil Sciences, Washington State University, Pullman, WA 99164-6420, USA.

出版信息

Theor Appl Genet. 2004 Aug;109(4):750-60. doi: 10.1007/s00122-004-1688-7.

Abstract

Malting quality has long been an active objective in barley (Hordeum vulgare L.) breeding programs.However, it is difficult for breeders to manipulate malting-quality traits because of inheritance complexity and difficulty in evaluation of these quantitative traits. Quantitative trait locus (QTL) mapping provides breeders a promising basis with which to manipulate quantitative trait genes. A malting-quality QTL complex, QTL2, was mapped previously to a 30-cM interval in the short-arm telomere region of barley chromosome 4H in a "Step-toe"/"Morex" doubled haploid population by the North American Barley Genome Project, using an interval mapping method with a relatively low-resolution genetic map. The QTL2 complex has moderate effects on several malting-quality traits, including malt extract percentage(ME), a-amylase activity (AA), diastatic power (DP), malt 13-glucan content (BG), and seed dormancy, which makes it a promising candidate gene source in malting barley-cultivar development. Fine mapping QTL2 is desirable for precisely studying barley malting-quality trait inheritance and for efficiently manipulating QTL2 in breeding. A reciprocal-substitution mapping method was employed to fine map QTL2. Molecular marker-assisted backcrossing was used to facilitate the generation of isolines. Fourteen different types of "Steptoe" isolines, including regenerated "Steptoe" and 13 different types of "Morex" isolines,including regenerated "Morex", were made within a 41.5-cM interval between MWG634 and BCD265B on chromosome 4H. Duplicates were identified for 12 "Steptoe" and 12 "Morex" isoline types. The isolines together with "Steptoe" and "Morex" were grown variously at three locations in 2 years for a total of five field environments.Four malting-quality traits were measured: ME, DP, AA,and BG. Few significant differences were found between duplicate isolines for these traits. A total of 15 putative QTLs were mapped; three for ME, four for DP, six for AA,and two for BG. Background genotype seemed to make a difference in expression/detection of QTLs. Of the 15 QTLs identified, ten were from the "Morex" and only five from the "Steptoe" background. By combining the results from different years, field environments, and genetic backgrounds and taking into account overlapping QTLsegments, six QTLs can be conservatively estimated: two each for ME and AA and one each for DP and BG with chromosome segments ranging from 0.7 cM to 27.9 cM. A segment of 15.8 cM from the telomere (MWG634-CDO669) includes all or a portion of all QTLs identified. Further study and marker-assisted breeding should focus on this 15.8-cM chromosome region.

摘要

长期以来,麦芽品质一直是大麦(Hordeum vulgare L.)育种计划中的一个重要目标。然而,由于这些数量性状的遗传复杂性和评估难度,育种者很难操控麦芽品质性状。数量性状位点(QTL)定位为育种者操控数量性状基因提供了一个有前景的基础。一个麦芽品质QTL复合体QTL2,先前由北美大麦基因组计划在一个“Step-toe”/“Morex”双单倍体群体中,使用分辨率相对较低的遗传图谱通过区间作图法定位到了大麦4H染色体短臂端粒区域的一个30厘摩区间内。QTL2复合体对几个麦芽品质性状有中等效应,包括麦芽浸出率(ME)、α-淀粉酶活性(AA)、糖化力(DP)、麦芽β-葡聚糖含量(BG)和种子休眠,这使其成为麦芽大麦品种培育中有前景的候选基因来源。精确绘制QTL2图谱对于准确研究大麦麦芽品质性状遗传以及在育种中有效操控QTL2是很有必要的。采用相互替代作图法对QTL2进行精细定位。利用分子标记辅助回交来促进近等基因系的产生。在4H染色体上MWG634和BCD265B之间41.5厘摩的区间内,构建了14种不同类型的“Steptoe”近等基因系,包括再生的“Steptoe”,以及13种不同类型的“Morex”近等基因系,包括再生的“Morex”。确定了12种“Steptoe”和12种“Morex”近等基因系类型的重复系。这些近等基因系与“Steptoe”和“Morex”一起在2年中的3个地点种植,共形成5个田间环境。测定了4个麦芽品质性状:ME、DP、AA和BG。在这些性状的重复近等基因系之间未发现显著差异。共定位到15个推定的QTL;3个与ME相关,4个与DP相关,6个与AA相关,2个与BG相关。背景基因型似乎对QTL的表达/检测有影响。在鉴定出的15个QTL中,10个来自“Morex”背景,只有5个来自“Steptoe”背景。通过综合不同年份、田间环境和遗传背景的结果,并考虑重叠的QTL区段,可以保守估计有6个QTL:ME和AA各2个,DP和BG各1个,染色体区段范围从0.7厘摩到27.9厘摩。来自端粒的一段15.8厘摩(MWG634-CDO669)包含了所有已鉴定QTL的全部或部分。进一步的研究和标记辅助育种应聚焦于这个15.8厘摩的染色体区域。

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