小麦种质资源苗期耐盐性鉴定评价

土壤盐渍化是影响小麦生长的重要非生物胁迫之一,筛选培育耐盐小麦种质资源对开展盐碱地综合利用具有重要意义。本研究以19份杂交小麦和2份常规品种为试验材料,以蛭石为培养基质,设置NaCl含量分别为0、0.4%、0.8%、1.2%、1.6%、2.0%的6个处理,从播种时开始盐胁迫处理,分析测定生长相关的11项指标。采用多元统计分析方法对小麦种质资源进行苗期耐盐性评价,结果表明,在1.2%盐处理下,小麦种质资源大多数指标的耐盐系数四分位差最大,因此,1.2%盐被认为是耐盐鉴定最适浓度;利用主成分分析方法可将11项调查指标的耐盐系数简化为3个主成分;通过主成分贡献率和隶属函数分析进一步将3个主成分值简化成综合评价指标D值;根据D值利用聚类分析将21份小麦种质资源划分为5类,对应高耐、耐盐、中耐、敏感和高敏5个耐盐级别,苗期耐盐鉴定表明13份杂交小麦的综合评价D值高于捷麦19与济麦22;结合逐步回归分析获得11个调查指标耐盐系数与D值的最优回归方程:D=–0.743+0.779×PLL+0.372×TNL+1.273×PH+0.336×PLC+0.279×RL+0.558×RDW,由此回归方程可知倒二叶叶长(PLL)、总叶片数(TNL)、株高(PH)、倒二叶叶绿素(PLC)、根长(RL)和根干重(RDW)可作为1.2%持续盐胁迫下小麦种质资源苗期鉴定评价指标。

我国部分审定小麦品种的品质性状及基因型分析

为了解我国小麦品种的品质相关基因分布及品质性状表现,本研究针对近年来我国审定的530份小麦品种,进行容重、粗蛋白质含量、湿面筋含量、吸水率和稳定时间等性状的分析,同时利用13个品质相关的KASP标记检测基因型,明析不同的品质种植区域内的审定品种优异品质基因等位变异的分布及聚合情况。检测的优异品质基因等位变异在不同区域间的分布不均衡,其中1BL/1RS(-)、1Ax 1/1Ax 2*、Pinb-D1b和Pinb-B2b优异等位变异在品质区域间分布频率呈显著性差异,而1Bx17+1By18、TaPsy-D1a和TaPod-A1b等优异等位变异的分布在区域间无差异;同时进行多个优异等位变异聚合情况分析发现:5个面筋质量相关基因中筛选出同时含有1B/1R(-)、1Ax 1/1Ax 2*,1Dx5+1Dy10、glu-B3g+4个优异等位变异的材料12份;3个籽粒硬度相关基因中未检测到同时含有Pina-D1b、Pinb-D1b和Pinb-B2b的材料,检测到含有Pina-D1b/Pinb-B2b组合的材料16份,含有Pinb-D1b/Pinb-B2b组合的材料88份。5个籽粒颜色相关基因中同时聚合5个优异等位变异的材料10份。检测的13个品质相关基因KASP标记中,未发现聚合11个以上优异等位变异基因的材料,聚合10个优异等位变异基因的材料有4份,聚合9个优异等位变异的材料有16份。品质分析结果显示:不同区域间品质指标值也存在区域性的差异,且稳定时间与蛋白质含量和湿面筋含量指标不协调。面筋品质相关基因优异等位变异1BL/1RS(-)、1Ax1/1Ax2*和1Dx5+1Dy10在强筋,中强筋和中筋品种间的分布频率呈极显著差异,且与品质表现呈极显著正相关。

外引小麦种质资源HMW-GS组成及品质评价

为有效利用外引小麦种质资源,本研究对引自国际玉米小麦改良中心、法国、巴基斯坦等区域的393份小麦种质资源进行高分子量麦谷蛋白亚基组成及品质性状的分析,结果表明,在供试材料中共检测到23种亚基类型和50种亚基组合类型;资源品质评分在4~10分之间,平均为7.68分,其中品质评分为10分、9分、8分的材料分别有74份、76份、96份,包含的亚基组合类型分别有8种、2种、14种,品质评分为8分及以上的材料共计246份,占总材料的62.6%;此外,9份材料检测出新的亚基及组合类型:F14(2*,14*+15*/6*+16*,Null)、F33(2*,14*+15*/6*+16*,Null)、C119(1,7*+16*,5+10)、C120(Null,7*+16*,5+10)、C125(2*,7+8,5′+10)、C51(2*,7+9,5′+10)、O13(2*,7+16,2+12)、O17(2*,7+16,2+12)和P27(2*,7+18,2+12)。总体上这些外引材料优质亚基分布频率高、组合类型丰富,可作为优异资源进一步开发利用,并为我国小麦品质改良提供材料基础及理论依据。

小麦TaPIP1基因克隆及其在花药开裂中潜在功能分析

二系杂交小麦育种是小麦产量提高的重要途径之一。光温敏雄性不育小麦生殖生长过程中花药的发育及开裂情况直接影响杂交小麦的制种效率和产量。植物花药的开裂与脱水活动紧密相关。水通道蛋白(aquaporins,AQPs)是高效转运水分及特异小分子的膜内在蛋白,其中质膜内在蛋白(plasma membrane intrinsic proteins,PIPs)在水分的吸收与外排中发挥着重要作用。为进一步了解水通道蛋白在小麦光温敏核雄性不育系花药开裂中的作用提供理论基础。本研究以不育系BS366花药的cDNA为模板,克隆获得了TaPIP1基因。利用生物信息学软件对TaPIP1进行分析,该基因包含一个879 bp的开放阅读框,编码292个氨基酸。TaPIP1的启动子区存在赤霉素、脱落酸、茉莉酸和光等响应元件。TaPIP1属于MIP超家族,具有典型的NPA保守结构域,亚细胞定位于细胞质膜与核膜上。miRNA互作预测发现TaPIP1受tae-miR1131与tae-miR408的剪切抑制,表明TaPIP1可能和与植物的抗氧化能力相关。通过蛋白互作预测及qPCR实验,表明TaPIP1可与热激蛋白(heat shock protein 90,TaHSP90)相互作用,在高温和干旱复合胁迫下,参与花药细胞壁膨压调控,进而调控花药的开裂。

Molecular Mapping of Two Novel Stripe Rust Resistant Genes YrTp1 and YrTp2 in A-3 Derived from Triticum aestivum × Thinopyrum ponticum

Loss of variety resistance to stripe rust （Puccinia striiformis Westend f. sp.tritici） is an important factor causing massive periodical epidemic of rust in wheat production. Creation and development of new races of rust pathogen have led to serious crisis of resistance loss in widely planted varieties. This has quickened the search for new resistance resources. Molecular marker could facilitate the identification of the location of novel genes. A line A-3 with high resistance （immune） to currently epidemic yellow rust races （CY29, 31, 32） was screened out in offspring of Triticum aestivura x Thinopyrum ponticum. Segregation in F2 and BC1 populations indicated that the resistance was controlled by two independent genes： one dominant and one recessive. SSR markers were employed to map the two resistant genes in the F2 and BC1 populations. A marker WMC477-167bp located on 2BS was linked to the dominant gene with genetic distance of 0.4 cM. Another marker WMC364-2os bp located on 7BS was linked to the recessive-resistant gene with genetic distance of 5.8 cM. The two genes identified in this paper might be two novel stripe rust resistant genes, which were temporarily designated as YrTpl and YrTp2, respectively. The tightly linking markers facilitate transfer of the two resistant genes into the new varieties to control epidemic of yellow rust.

Assessment of wheat variety distinctness using SSR markers

Assessment of variety distinctness is important for both the registration and the protection of particular variety. However, the current testing system, which assesses a range of morphological characters of each pair of varieties grown side-by-side, is time-consuming and is not suitable for the assessment of hundreds of samples. The objective of this study was to develop a procedure for the assessment of wheat variety distinctness using simple sequence repeat（SSR） markers. A comparison between the molecular and morphological profile of 797 varieties was made. On the basis of the comparison, pairs of varieties with a genetic similarity value（GSV） ≤90% were deemed to be distinct, accounting for ~85% of varieties assessed in wheat regional trials. For the remaining ~15% of varieties, GSVs between different varieties were 〉90%, among which ~35% were not distinct and the other ~65% were distinct. Therefore, if given a GSV〉90%, the pairs of varieties should be morphologically assessed in the field. To avoid any errors in the assessments, we proposed the elimination of contaminant plants from the sample before comparing the varietal genotypes, scoring of the genotype at each locus with a pair of allele numbers when constructing a molecular profile, and faithfully recording two alleles at a non-homozygous locus. To reduce the workload and cost, a three-grade markers comparison among varieties is suggested. In addition, 80 SSR markers and a technical procedure for assessment of wheat variety distinctness have been proposed. Based on the procedure, the distinctness assessment of ~85% of all wheat varieties is completed in our laboratory annually. Consequently, total field assessment has been reduced considerably.