黄河中游地区节节麦抗穗发芽的鉴定与分析

小麦穗发芽是小麦生产中的主要灾害和重要问题,在普通小麦中缺乏抗穗发芽的品种资源。本试验通过对35份黄河中游地区节节麦、14份国外节节麦及部分小麦品种的发芽率的测定及抗性多样性分析,综合评价了黄河中游地区节节麦的穗发芽抗性状况。结果表明,节节麦穗发芽抗性普遍高于小麦品种,黄河中游地区节节麦的抗穗发芽能力优于国外材料,其中以T005、T007、T008、T016、T030、T062、T065、T068、T069、T072和T085等11个材料的抗穗发芽能力最强,是小麦穗发芽改良优异的抗源材料。     

小麦抗穗发芽研究进展

穗发芽严重影响小麦品质和产量。种子自身休眠特性、α-淀粉酶活性、α-淀粉酶抑制剂、迟熟α-淀粉酶活性、种皮颜色、颖壳抑制物以及穗部形态等,均是影响小麦穗发芽的重要因素,其中对子粒休眠特性和α-淀粉酶活性的研究较为深入。位于第3染色体组上的R基因、休眠基因以及4AL上的Phs基因均与小麦穗发芽密切相关。已开发出一些与穗发芽抗性相关的分子标记,其中位于第3部分同源群的三重R基因和位于3B染色体的STS标记Vp1B3,以及位于3A染色体的主效QTL位点QPhs.ccsu-3A.1均可直接用于穗发芽抗性的筛选。本文对以上内容进行了详细论述,并就今后如何提高小麦穗发芽抗性进行了讨论。     

冬小麦穗发芽抗性及其遗传研究

1987—1989年在人工模拟降雨室对123个小麦品种进行了成熟期穗发芽抗性鉴定。重点研究了13个品种的穗发芽率、籽粒发芽率、籽粒含水量,籽粒吸水速率和α-淀粉酶活性的动态变化。并通过6个抗性不同品种的双列杂交,初步探讨了穗发芽抗性的遗传特点。结果表明:红粒品种普遍抗穗发芽,但白粒品种中也存在不少抗源;开花后35—40天是鉴定穗发芽抗性的适宜时期;这个对期的仔粒吸水速率阳α-淀汾酶活性是抗性鉴定的可靠指标;穗发芽抗性是遗传性状,存在母、子体抗性因子互作效应。     

不同生态区小麦品种的穗发芽抗性评价

本研究对来自不同生态区的137个小麦品种进行穗发芽抗性鉴定,计算相对发芽指数,并分析这些品种穗部籽粒性状、品质指标、吸胀萌发后0～72 h α-淀粉酶活性及其基因表达量与穗发芽抗性之间的关系。结果表明: 长江中下游麦区小麦的平均发芽指数最低,抗穗发芽品种最多,其次是长江上游麦区,黄淮麦区抗穗发芽品种相对较少。红粒品种小麦的相对发芽指数低于白粒品种,相对发芽指数与籽粒长度、宽度呈极显著正相关,与小穗数呈显著正相关,与穗型、穗色、穗长、小穗密度、穗粒数、千粒重无显著相关性。相对发芽指数与容重呈极显著负相关,与面团形成时间和出粉率呈显著负相关,与蛋白质含量、湿面筋含量、吸水率、稳定时间、沉降值、拉伸面积、延展性、最大阻力无显著相关性。不同品种的α-淀粉酶活性随吸胀萌发时间的延长呈上升趋势,萌发24～72 h的相对发芽指数与α-淀粉酶活性呈极显著正相关,穗发芽中抗以上品种萌发48 h后α-淀粉酶活性聚类分析结果与穗发芽鉴定结果一致。萌发后各时段α-淀粉酶基因表达量与相对发芽指数呈极显著正相关。     

小麦Vp-1基因RNA干扰表达载体的构建及遗传转化

小麦成熟期穗发芽是世界性的自然灾害,严重影响小麦的产量和品质.Viviparous-1(Vp-1)是促进胚成熟和休眠的主要转录调节因子,与小麦穗发芽抗性有着密切的关系.本实验根据小麦Vp-1基因序列,以植物表达载体pAHC25为基础,成功构建了含有反向重复序列的RNA干扰表达载体pAHC-WVpRi.采用基因枪法轰击小麦品种新春9号幼胚材料1825个,共获得34株T0再生植株.利用Bar基因引物和干扰片段特异引物对再生植株进行PCR检测,获得Bar基因和干扰片段均为阳性的植株3株,转化率为0.16%.本研究为深入分析Vp-1基因功能,进而通过分子育种进行小麦穗发芽抗性的遗传改良提供了科学依据.     

RSP抗穗发芽基因育种利用研究初报

利用农艺性状优良、优质的红粒小麦品种绵阳11以及2个白粒、极易穗发芽(常年穗发芽在50%以上)的小麦品系YY2和88-1643与穗发芽抗性来源于长休眠节节麦的人工合成小麦RSP杂交,对3个组合的F2单株和F3株系的穗发芽测试,从RSP×绵阳11中筛选出15个与RSP相当的纯合抗性株系和27份穗发芽接近0的F3单株;从RSP×YY2和RSP×88-1643组合中共筛选出5份穗发芽在7%以下的白粒株系.这些株系或单株相对于RSP的高秆、晚熟等不利性状已有较大改良,为节节麦抗穗发芽基因向优质或白粒小麦转移研制出了更容易利用的中间材料.     

小麦抗穗发芽生理

本文介绍近年来小麦抗穗发芽生理研究的进展,包括温度、水分、穗部及籽粒性状,酶、激素和发芽抑制物等因素对穗发芽的影响,并对今后的研究提出一些看法。     

转反义trxs基因小麦株系01TY18遗传分析及抗穗发芽特性

以豫麦18为受体导入反义trxs基因获得的株系01TY18(T0)为材料,运用PCR、实时荧光RT-PCR以及离体整穗发芽的方法,对反义trxs基因在转基因小麦中的遗传稳定性、基因表达和抗穗发芽特性进行了研究.结果表明,8个T1代转基因株系中有6个株系目的基因检测呈阳性,且在以后的世代中能够稳定遗传并呈典型的孟德尔单基因3∶1分离规律;反义trxs基因在6个转基因株系中能够正常表达且表现出显著的抗穗发芽特性.与非转基因对照相比,转基因株系穗粒发芽率和穗发芽度平均分别降低62%(P<0.01)和50.8%(P<0.01).     

转反义trxs基因小麦株系00T89分子鉴定及抗穗发芽特性研究

以皖麦48为受体导入反义trxs基因已获得00T89第4代(T4)转基因株系,对其进行反义基因的PCR鉴定、相对定量RT-PCR基因表达检测以及抗穗发芽特性研究。结果表明,18个T4代转基因株系中,13个株系目的基因检测呈阳性;成熟期籽粒萌发过程中,8个株系转录水平上mRNA丰度极显著降低(P<0·01),mRNA丰度与穗发芽指标呈显著和极显著的相关性(r=0·7181)。其中6个株系在开花后30d至成熟后10d表现出明显的抗穗发芽特性。与非转基因对照相比,平均穗开始发芽时间推迟2·7d(P<0·01),穗粒发芽率和穗发芽度分别降低35·5%(P<0·01)和47·5%(P<0·01),成熟后25d这些株系又逐渐恢复发芽特性,无显著差异(P>0·05)。     

转反义trxs基因小麦株系00T89分子鉴定及抗穗发芽特性研究

以皖麦48为受体导入反义trxs基因已获得00T89第4代（T₄）转基因株系,对其进行反义基因的PCR鉴定、相对定量RT-PCR基因表达检测以及抗穗发芽特性研究。结果表明,18个T₄代转基因株系中,13个株系目的基因检测呈阳性;成熟期籽粒萌发过程中,8个株系转录水平上mRNA丰度极显著降低（P<0.01）,mRNA丰度与穗发芽指标呈显著和极显著的相关性（r=0.7181）。其中6个株系在开花后30d至成熟后10d表现出明显的抗穗发芽特性。与非转基因对照相比,平均穗开始发芽时间推迟2.7d（P<0.01）,穗粒发芽率和穗发芽度分别降低35.5%（P<0.01）和47.5%（P<0.01）,成熟后25d这些株系又逐渐恢复发芽特性,无显著差异（P>0.05）。     

Inheritance of seed dormancy in Tibetan semi-wild wheat accession Q1028

Tibetan semi-wild wheat (Triticum aestivum ssp. tibetanum Shao) is one of the Chinese endemic hexaploid wheat genetic resources, distributed only in the Qinghai-Xizang Plateau of China. It has special characters, such as a hulled glume and spike disarticulation. However, seed dormancy, another important character for wheat resistance to pre-harvest sprouting, was rarely reported. Seed dormancy of more than 10 Tibetan semi-wild wheat accessions was evaluated, and their germinations were 0% or near 0% with both treatments of threshed seeds and intact spikes at hard dough stage. Tibetan semi-wild wheat accession Q1028 was investigated for its seed dormant characters by testing the seed germination percentages of intact spikes, seeds with bract powder, normal seeds, seeds with pierced coat, and sectioned embryos. It was observed that embryo dormancy of Q1028 accounted for its seed dormancy. Using threshed seeds and intact spikes at hard dough stage, the inheritance of seed dormancy was carried out using the F1, F2, F3 and F2BC1 populations of the cross between Q1028 and a wheat line 88-1643, susceptible to preharvest sprouting. The germinations of seeds and intact spikes in F1 plants were 1.0% and 0.9%, respectively. It indicated that seed dormancy of Q1028 was inherited as a dominant trait. From the genetic analysis of the F2, F3 and F2BC1 populations it was found that the strong seed dormancy of Q1028 was controlled by two dominant genes.     

Dormancy and germination: How does the crop seed decide?

Whether seeds germinate or maintain dormancy is decided upon through very intricate physiological processes. Correct timing of these processes is most important for the plants life cycle. If moist conditions are encountered, a low dormancy level causes pre‐harvest sprouting in various crop species, such as wheat, corn and rice, this decreases crop yield and negatively impacts downstream industrial processing. In contrast, a deep level of seed dormancy prevents normal germination even under favourable conditions, resulting in a low emergence rate during agricultural production. Therefore, an optimal seed dormancy level is valuable for modern mechanised agricultural systems. Over the past several years, numerous studies have demonstrated that diverse endogenous and environmental factors regulate the balance between dormancy and germination, such as light, temperature, water status and bacteria in soil, and phytohormones such as ABA (abscisic acid) and GA (gibberellic acid). In this updated review, we highlight recent advances regarding the molecular mechanisms underlying regulation of seed dormancy and germination processes, including the external environmental and internal hormonal cues, and primarily focusing on the staple crop species. Furthermore, future challenges and research directions for developing a full understanding of crop seed dormancy and germination are also discussed.     

Polymorphic Homoeolog of Key Gene of RdDM Pathway,ARGONAUTE4_9 class Is Associated with Pre-Harvest Sprouting in Wheat (Triticum aestivum L.)

Resistance to pre-harvest sprouting (PHS) is an important objective for the genetic improvement of many cereal crops, including wheat. Resistance, or susceptibility, to PHS is mainly influenced by seed dormancy, a complex trait. Reduced seed dormancy is the most important aspect of seed germination on a spike prior to harvesting, but it is influenced by various environmental factors including light, temperature and abiotic stresses. The basic genetic framework of seed dormancy depends on the antagonistic action of abscisic acid (ABA) and gibberellic acid (GA) to promote dormancy and germination. Recent studies have revealed a role for epigenetic changes, predominantly histone modifications, in controlling seed dormancy. To investigate the role of DNA methylation in seed dormancy, we explored the role of ARGONAUTE4_9 class genes in seed development and dormancy in wheat. Our results indicate that the two wheat AGO4_9 class genes i.e. AGO802 and AGO804 map to chromosomes 3S and 1S are preferentially expressed in the embryos of developing seeds. Differential expressions of AGO802-B in the embryos of PHS resistant and susceptible varieties also relates with DNA polymorphism in various wheat varieties due to an insertion of a SINE-like element into this gene. DNA methylation patterns of the embryonic tissue from six PHS resistant and susceptible varieties demonstrate a correlation with this polymorphism. These results suggest a possible role for AGO802-B in seed dormancy and PHS resistance through the modulation of DNA methylation.     

Genes controlling seed dormancy and pre-harvest sprouting in a rice-wheat-barley comparison

Pre-harvest sprouting results in significant economic loss for the grain industry around the world. Lack of adequate seed dormancy is the major reason for pre-harvest sprouting in the field under wet weather conditions. Although this trait is governed by multiple genes it is also highly heritable. A major QTL controlling both pre-harvest sprouting and seed dormancy has been identified on the long arm of barley chromosome 5H, and it explains over 70% of the phenotypic variation. Comparative genomics approaches among barley, wheat and rice were used to identify candidate gene(s) controlling seed dormancy and hence one aspect of pre-harvest sprouting. The barley seed dormancy/pre-harvest sprouting QTL was located in a region that showed good synteny with the terminal end of the long arm of rice chromosome 3. The rice DNA sequences were annotated and a gene encoding GA20-oxidase was identified as a candidate gene controlling the seed dormancy/pre-harvest sprouting QTL on 5HL. This chromosomal region also shared synteny with the telomere region of wheat chromosome 4AL, but was located outside of the QTL reported for seed dormancy in wheat. The wheat chromosome 4AL QTL region for seed dormancy was syntenic to both rice chromosome 3 and 11. In both cases, corresponding QTLs for seed dormancy have been mapped in rice.C. Li and P. Ni contributed equally to this work     

A major QTL controlling seed dormancy and pre-harvest sprouting resistance on chromosome 4A in a Chinese wheat landrace

Wheat pre-harvest sprouting (PHS) can cause significant reduction in yield and end-use quality of wheat grains in many wheat-growing areas worldwide. To identify a quantitative trait locus (QTL) for PHS resistance in wheat, seed dormancy and sprouting of matured spikes were investigated in a population of 162 recombinant inbred lines (RILs) derived from a cross between the white PHS-resistant Chinese landrace Totoumai A and the white PHS-susceptible cultivar Siyang 936. Following screening of 1,125 SSR primers, 236 were found to be polymorphic between parents, and were used to screen the mapping population. Both seed dormancy and PHS of matured spikes were evaluated by the percentage of germinated kernels under controlled moist conditions. Twelve SSR markers associated with both PHS and seed dormancy were located on the long arm of chromosome 4A. One QTL for both seed dormancy and PHS resistance was detected on chromosome 4AL. Two SSR markers, Xbarc 170 and Xgwm 397, are 9.14 cM apart, and flanked the QTL that explained 28.3% of the phenotypic variation for seed dormancy and 30.6% for PHS resistance. This QTL most likely contributed to both long seed dormancy period and enhanced PHS resistance. Therefore, this QTL is most likely responsible for both seed dormancy and PHS resistance. The SSR markers linked to the QTL can be used for marker-assisted selection of PHS-resistant white wheat cultivars. Shi-Bin Cai and Cui-Xia Chen contributed equally to this work.     

A new PCR-based marker on chromosome 4AL for resistance to pre-harvest sprouting in wheat (<Emphasis Type="Italic">Triticum aestivum</Emphasis> L.)

Pre-harvest sprouting (PHS) is a complex trait controlled by multiple genes with strong interaction between environment and genotype that makes it difficult to select breeding materials by phenotypic assessment. One of the most important genes for pre-harvest sprouting resistance is consistently identified on the long arm of chromosome 4A. The 4AL PHS tolerance gene has therefore been targeted by Australian white-grained wheat breeders. A new robust PCR marker for the PHS QTL on wheat chromosome 4AL based on candidate genes search was developed in this study. The new marker was mapped on 4AL deletion bin 13-0.59-0.66 using 4AL deletion lines derived from Chinese Spring. This marker is located on 4AL between molecular markers Xbarc170 and Xwg622 in the doubled-haploid wheat population Cranbrook × Halberd. It was mapped between molecular markers Xbarc170 and Xgwm269 that have been previously shown to be closely linked to grain dormancy in the doubled haploid wheat population SW95-50213 × Cunningham and was co-located with Xgwm269 in population Janz × AUS1408. This marker offers an additional efficient tool for marker-assisted selection of dormancy for white-grained wheat breeding. Comparative analysis indicated that the wheat chromosome 4AL QTL for seed dormancy and PHS resistance is homologous with the barley QTL on chromosome 5HL controlling seed dormancy and PHS resistance. This marker will facilitate identification of the gene associated with the 4A QTL that controls a major component of grain dormancy and PHS resistance.     

Genetic and QTL analyses of seed dormancy and preharvest sprouting resistance in the wheat germplasm CN10955

The inheritance and genetic linkage analysis for seed dormancy and preharvest sprouting (PHS) resistance were carried out in an F₈ recombinant inbred lines (RILs) derived from the cross between “CN19055” (white-grained, PHS-resistant) with locally adapted Australian cultivar “Annuello” (white-grained, PHS-susceptible). Seed dormancy was assessed as germination index (GI7) while assessment for preharvest sprouting resistance was based on whole head assay (sprouting index, SI) and visibly sprouted seeds (VI). Segregation analysis of the F₂, F₃ data from the glasshouse and the RIL population in 2004 and 2005 field data sets indicated that seed dormancy and PHS resistance in CN19055 is controlled by at least two genes. Heritabilities for GI7 and VI were high and moderate for SI. The most accurate method for assessing PHS resistance was achieved using VI and GI7 while SI exhibited large genotype by environment interaction. Two quantitative trait loci (QTLs) QPhs.dpivic.4A.1 and QPhs.dpivic.4A.2 were identified. On pooled data across four environments, the major QTL, QPhs.dpivic.4A.2, explained 45% of phenotypic variation for GI7, 43% for VI and 20% for SI, respectively. On the other hand, QPhs.dpivic.4A.1 which accounted for 31% of the phenotypic variation in GI7 in 2004 Horsham field trial, was not stable across environments. Physical mapping of two SSR markers, Xgwm937 and Xgwm894 linked to the major QTL for PHS resistance, using Chinese Spring deletions lines for chromosome 4AS and 4AL revealed that the markers were located in the deletion bins 4AL-12 and 4AL-13. The newly identified SSR markers (Xgwm937/Xgwm894) showed strong association with seed dormancy and PHS resistance in a range of wheat lines reputed to possess PHS resistance. The results suggest that Xgwm937/Xgwm894 could be used in marker-assisted selection (MAS) for incorporating preharvest sprouting resistance into elite wheat cultivars susceptible to PHS.     

Mapping quantitative trait loci for preharvest sprouting resistance in white wheat

The premature germination of seeds before harvest, known as preharvest sprouting (PHS), is a serious problem in all wheat growing regions of the world. In order to determine genetic control of PHS resistance in white wheat from the relatively uncharacterized North American germplasm, a doubled haploid population consisting of 209 lines from a cross between the PHS resistant variety Cayuga and the PHS susceptible variety Caledonia was used for QTL mapping. A total of 16 environments were used to detect 15 different PHS QTL including a major QTL, QPhs.cnl-2B.1, that was significant in all environments tested and explained from 5 to 31% of the trait variation in a given environment. Three other QTL QPhs.cnl-2D.1, QPhs.cnl-3D.1, and QPhs.cnl-6D.1 were detected in six, four, and ten environments, respectively. The potentially related traits of heading date (HD), plant height (HT), seed dormancy (DOR), and rate of germination (ROG) were also recorded in a limited number of environments. HD was found to be significantly negatively correlated with PHS score in most environments, likely due to a major HD QTL, QHd.cnl-2B.1, found to be tightly linked to the PHS QTL QPhs.cnl-2B.1. Using greenhouse grown material no overlap was found between seed dormancy and the four most consistent PHS QTL, suggesting that greenhouse environments are not representative of field environments. This study provides valuable information for marker-assisted breeding for PHS resistance, future haplotyping studies, and research into seed dormancy.     

Characterization of quantitative trait loci controlling genetic variation for preharvest sprouting in synthetic backcross-derived wheat lines

Aegilops tauschii, the wild relative of wheat, has stronger seed dormancy, a major component of preharvest sprouting resistance (PHSR), than bread wheat. A diploid Ae. tauschii accession (AUS18836) and a tetraploid (Triticum turgidum L. ssp. durum var. Altar84) wheat were used to construct a synthetic wheat (Syn37). The genetic architecture of PHS was investigated in 271 BC(1)F(7) synthetic backcross lines (SBLs) derived from Syn37/2*Janz (resistant/susceptible). The SBLs were evaluated in three environments over 2 years and PHS was assessed by way of three measures: the germination index (GI), which measures grain dormancy, the whole spike assay (SI), which takes into account all spike morphology, and counted visually sprouted seeds out of 200 (VI). Grain color was measured using both Chroma Meter- and NaOH-based approaches. QTL for PHSR and grain color were mapped and their additive and epistatic effects as well as their interactions with environment were estimated by a mixed linear-model approach. Single-locus analysis following composite interval mapping revealed four QTL for GI, two QTL for SI, and four QTL for VI on chromosomes 3DL and 4AL. The locus QPhs.dpiv-3D.1 on chromosome 3DL was tightly linked to the red grain color (RGC) at a distance of 5 cM. The other locus on chromosome 3D, "QPhs.dpiv-3D.2" was independent of RGC locus. Two-locus analysis detected nine QTL with main effects and 18 additive x additive interactions for GI, SI, and VI. Two of the nine main effects QTL and two epistatic QTL showed significant interactions with environments. Both additive and epistatic effects contributed to phenotypic variance in PHSR and the identified markers are potential candidates for marker-assisted selection of favorable alleles at multiple loci. SBLs derived from Ae. tauschii proved to be a promising tool to dissect, introgress, and pyramid different PHSR genes into adapted wheat genetic backgrounds. The enhanced expression of PHS resistance in SBLs enabled us to develop white PHS-resistant wheat germplasm from the red-grained Ae. tauschii accession.