HMW-GS和LMW-GS组成对小麦加工品质的影响

高分子量麦谷蛋白亚基(HMW-GS)和低分子量麦谷蛋白亚基(LMW-GS)是决定小麦加工品质的重要因素。以小麦品种PH82-2(亚基组成1, 14+15, 2+12和Glu-A3d, Glu-B3d, Glu-D3c)和内乡188(亚基组成1, 7+9, 5+10和 Glu-A3a, Glu-B3j, Glu-D3b)的242份F₃和F₄株系(试验I)和91份产量比较试验材料(试验II)研究了贮藏蛋白组成对小麦加工品质的影响。结果表明,HMW-GS和LMW-GS等位变异对籽粒蛋白质含量的影响不大,但对加工品质均有极显著影响(P<1%)。就位点的效应而言,Glu-D1位点对加工品质的效应较大,而Glu-D3位点的效应较小。就单个亚基而言,在Glu-B1位点,14+15<7+9;在Glu-D3位点,Glu-D3c>Glu-D3b。1B/1R易位系的部分品质性状,如和面时间、曲线下降斜度和峰积分好于非1B/1R易位系。     

麦谷蛋白亚基Clu-1和Glu-3位点基因等位变异对小麦品质特性的影响

甲单向一步SDS-PAGE方法分析表明亲本品种Suneca和Cook在麦谷蛋白亚基的5个位点(Glu-B1,Glu-D1,Glu-A3,Glu-B3和Glu-D3)均含不同等位基因。本研究重点对Suneca×Cook的F_4代群体中在麦谷蛋白亚基位点均为纯合基因的60个系的出粉率(FY),面粉蛋白质含量(FP)及和面时间(PTM)进行了分析,以研究麦谷蛋白各亚基位点等位基因变异及位点间互作对小麦品质特性的影响。结果表明,不同基因型间出粉率无显著差异,Glu-D1位点等位基因d和a对FP的效应存在显著差异,Glu-Dld基因(编码5 10亚基)的正效应显著高于Glu-Dla基因(编码2 12亚基);Glu-D1、Glu-A3和Glu-B3位点上基因的等位变异对PTM有显著和极显著影响,含Glu-Dld、Glu-A3b和Glu-B3b基因的系分别比含Glu-Dla,Glu-A3d和Glu-B3h基因的系有较长的和面时间;Glu-B1位点上等位变异i和u以及Glu-D3位点等位基因b和e分别对PTM无明显影响。在这种遗传背景下,麦谷蛋白亚基位点对PTM的效应大小依次排列为Glu-D1>Glu-B3>Glu-A3>GIu-B1=Glu-D3。Glu-1位点和Glu-3位点间对和面特性的影响存在累加效应和互作效应。     

低分子量谷蛋白亚基GlU-A3和GlU-B3位点对小麦面筋强度和烘焙特性影响

低分子量谷蛋白亚基是小麦谷蛋白亚基的重要组成部分,黄淮麦区小麦低分子量谷蛋白亚基组成对品质的效应尚缺乏系统的研究。本研究采用SDS-PAGE方法,鉴定了黄淮麦区42个小麦品种的Glu-A3位点和Glu-B3位点低分子量谷蛋白亚基组成,分析了低分子量谷蛋白亚基对小麦面筋强度和烘烤品质的影响。结果表明,在Glu-A3位点,对面筋强度和面包烘焙品质正向效应为:d,b>a,e;在Glu-B3位点,对面筋强度正效应为:h,d>f>g,b,j,对面包烘焙品质正向效应为:h>f,d>g,b,j。Glu-A3d/Glu-B3h亚基组合具有较好的面筋强度和烘焙品质。就低分子量谷蛋白亚基单个变异位点对品质综合效应而言,Glu-B3位点对品质作用比较大,与Glu-B1位点相近,同时,高低分子量谷蛋白亚基之间存在着互作效应,以Glu-B1/Glu-A3和Glu-D1/Glu-B3位点的互作效应比较显著。Glu-A3和Glu-B3位点及其所编码的不同亚基种类对品质的效应差异显著,并且与高分子量谷蛋白亚基位点存在互作,对不同位点优质亚基的聚合将有助于小麦品质的遗传改良。     

四川藏区小麦地方品种高分子量谷蛋白亚基组成分析

利用SDS-PAGE分析检测了36份四川藏区小麦地方品种的高分子量谷蛋白亚基组成,从中可检测到7种亚基组合类型.其中,Null、7+8、2+12为四川藏区小麦的优势亚基组合,其频率高达58.33%.在Glu-A 1、Glu-B 1和Glu.D 1位点中,分别有3,5和3种等位变异类型,各位点出现频率最高的亚基分别是Null、7+8和2+12,频率分别为86.11%、63.89%和94.44%.在WL25的Glu-B 1位点发现了一个未知的y型亚基,其迁移率比By 8慢,与Bx7以亚基组合形式同时出现.在wL 16的Glu-D 1位点,Dx亚基沉默,而仅表达了Dy 12亚基.参试材料的面包品质评分为4-8分,无评分达9分以上的品种.     

小麦Glu-1位点变异和1B/1R易位对谷蛋白亚基表达量和面包加工品质的影响

选用北方冬麦区近年来育成的优质强筋品种及山东省主栽品种共42份, 采用反相高效液相色谱法(RP-HPLC)和凝胶色谱法(SE-HPLC)对小麦贮藏蛋白组分进行量化, 分析了不同高分子量谷蛋白亚基(HMW-GS)组成对其表达量、面团流变学特性和面包加工品质的影响。结果表明, Glu-D1位点对谷蛋白亚基含量和加工品质的加性效应最大, 达5%显著水平, 贡献率为28.5%~71.3%。在Glu-A1和Glu-D1位点, 单个亚基对谷蛋白亚基含量和加工品质的贡献分别为1>2*>N和5+10>2+12>4+12, 而在Glu-B1位点, 则表现为差异不显著。不同亚基组合的HMW–GS表达量差异达5%显著水平, 相同亚基组合的品种间贮藏蛋白组分表达量的变异较大, 亚基表达量的差异可能是导致品种间品质差异的重要原因。1B/1R易位显著降低LMW-GS、谷蛋白总量和%UPP, 导致加工品质变劣。选择具有优质亚基组合, 且谷蛋白亚基表达量高的类型, 是有效改良面筋强度, 进一步提高优质新品种选育的有效途径。     

新疆奎屯地区小麦高分子量谷蛋白亚基组成分析

应用SDS-PAGE方法对24份外引品种和31份品种(系)的HMW-GS组成与分布进行分析。结果表明,HMWGS分别具有17种带型组合;3个位点共发现14个等位基因。Glu-A1、Glu-B1和Glu-D1分别有3、7和4个变异位点;亚基Null、1、7+9、7+8、2+12和5+10是主要的HWM-GS类型,频率分别为61.8%、36.4%、20.0%、45.5%、56.4%和36.4%。     

二系杂交小麦HMW-GS组成与品质关系的初步研究

为了研究二系杂交小麦HMW-GS类型与蛋白质含量、沉淀值、面团形成时间和衰弱角斜率等品质性状的关系,采用SDS-PAGE方法分析了杂交种的高分子量麦谷蛋白亚基(HMW-GS)的组成.结果表明,在试验材料中普遍存在有劣质亚基N和2+12,它们的频率分别是60.4%,83.0%.在HMW-GS与F1籽粒品质性状关系的研究中发现,各位点对蛋白质含量的贡献率是Glu-B1>Glu-A1>Glu-D1;对沉淀值贡献率是Glu-B1>Glu-D1>Glu-A1;对形成时间和衰落角斜率的贡献率是Glu-D1>Glu-B1>Glu-A1.总体来说,位点按对品质的贡献率大小依次为Glu-B1>Glu-D1>Glu-A1.就单个亚基而言Glu-D1位点,杂合2+12/5+10>纯合2+12;Glu-A1位点蛋白质含量、SDS沉淀值和形成时间均为N/N>N/1;在Glu-B1位点,蛋白质含量是7+8/17+18=7+9/17+18=7+8/7+9=7+8/7+8>7+9/7+9;沉淀值的大小依次为7+8/17+18≥7+9/17+18=7+8/7+9=7+8/7+8≥7+9/7+9;形成时间是7+8/17+18>7+9/17+18＝7+8/7+9＝7+8/7+8＝7+9/7+9;衰弱角斜率大小是7+9/17+18≥7+8/17+18＝7+9/7+9≥7+8/7+9=7+8/7+8.在不同亚基组合中,具有N/N,7+8/7+8,2+12/5+10亚基的品质最好.杂合位点5+10亚基对2+12亚基的品质具有补偿效应.     

利用RIL群体分析HMW-GS对小麦品质性状的量化效应

利用重组自交系群体——RIL-8群体的131个系及其亲本为材料,分析了高分子量麦谷蛋白亚基及亚基组合对10个小麦品质性状的量化效应及其差异。结果表明,RIL-8群体Glu-A1、Glu-B1、Glu-D1位点编码的亚基分别为 1、N,7+9、7+8和5+10、2+12,主要存在7种亚基组合类型。同一位点不同亚基对面粉吸水率、Zeleny沉淀值、面团形成时     

引进小麦种质材料的高分子量谷蛋白亚基分析

为了有效利用多年来引自俄罗斯及中亚地区的小麦资源,了解引进材料的遗传基础,特别是品质基础,采用SDS-PAGE技术对102份小麦材料的高分子量谷蛋白亚基（HMW-GS）组成进行了分析。结果表明,参试材料中共检测到11种HMW-GS类型,Glu-A1位点上有1、2＊、Null,Null位点相对比较多,为40.20%;Glu-B1位点上有7、7＋8、7＋9、6＋8、17＋18,以7＋9为主要类型（59.80%）;Glu-D1位点有2＋12、2＋12’、5＋10三种类型,其中5＋10所占比例为51.96%。参试材料共检测到16种亚基组合,其中＂Null,7＋9,2＋12＂所占比例较大,为25.5%。值得一提的是,参试材料中品质评分为10分的材料有22个,9分的有29个。这些材料有可能会成为比较有价值的品质改良中间材料。     

小麦Glu-1位点变异和1B/1R易位对谷蛋白亚基表达量和面包加工品质的影响

选用北方冬麦区近年来育成的优质强筋品种及山东省主栽品种共42份, 采用反相高效液相色谱法(RP-HPLC)和凝胶色谱法(SE-HPLC)对小麦贮藏蛋白组分进行量化, 分析了不同高分子量谷蛋白亚基(HMW-GS)组成对其表达量、面团流变学特性和面包加工品质的影响。结果表明, Glu-D1位点对谷蛋白亚基含量和加工品质的加性效应最大, 达5%显著水平, 贡献率为28.5%~71.3%。在Glu-A1和Glu-D1位点, 单个亚基对谷蛋白亚基含量和加工品质的贡献分别为1>2*>N和5+10>2+12>4+12, 而在Glu-B1位点, 则表现为差异不显著。不同亚基组合的HMW–GS表达量差异达5%显著水平, 相同亚基组合的品种间贮藏蛋白组分表达量的变异较大, 亚基表达量的差异可能是导致品种间品质差异的重要原因。1B/1R易位显著降低LMW-GS、谷蛋白总量和%UPP, 导致加工品质变劣。选择具有优质亚基组合, 且谷蛋白亚基表达量高的类型, 是有效改良面筋强度, 进一步提高优质新品种选育的有效途径。     

Allelic variation and composition of HMW-GS in advanced lines derived from d-genome synthetic hexaploid / bread wheat (<Emphasis Type="Italic">Triticum aestivum</Emphasis> L.)

The objective of this study was to identify allelic variations at Glu-1 loci of wheat (Triticum aestivum L.) advanced lines derived from hybridization of bread wheat and synthetic hexaploid wheats (2n = 6x = 42; AABBDD). Locally adapted wheat genotypes were crossed with synthetic hexaploid wheats. From the 134 different cross combinations made, 202 F₈ advanced lines were selected and their HMW-GS composition was studied using SDS-PAGE. In total, 24 allelic variants and 68 HMW-GS combinations were observed at Glu-A1, Glu-B1, and Glu-D1 loci. In bread wheat, the Glu-D1 locus is usually characterized by subunits 1Dx2+1Dy12 and 1Dx5+1Dy10 with the latter having a stronger effect on bread-making quality. The subunit 1Dx5+1Dy10 was predominantly observed in these advanced lines. The inferior subunit 1Dx2+1Dy12, predominant in adapted wheat germplasm showed a comparative low frequency in the derived advanced breeding lines. Its successful replacement is due to the other better allelic variants at the Glu-D1 locus inherited in these synthetic hexaploid wheats from Aegilops tauschii (2n = 2x = 14; DD).     

Glu-1位点等位变异及表达量对麦谷蛋白聚合体粒度分布的影响

选用我国春播麦区23份(试验I)和北部冬麦区21份(试验II)品种(系),研究了Glu-1位点等位变异及其亚基表达量对谷蛋白聚合体粒度分布的影响。结果表明,Glu-1位点等位变异及其亚基表达量显著影响谷蛋白聚合体的粒度分布,且影响程度受蛋白质含量,尤其是高分子量谷蛋白总量水平的影响。在高分子量谷蛋白总量较低时(试验I),Glu-B1和Glu-D1位点对不溶性谷蛋白大聚体含量(UPP)及其占聚合体蛋白总量的百分比(%UPP)的加性效应都达1%显著水平;Glu-B1和Glu-D1位点单个亚基对两者的贡献分别为7^OE+8^* >7+9 >17+18 >7+8和5+10 >2+12,具有5+10亚基组合的%UPP显著高于具有2+12的亚基组合。高分子量谷蛋白的亚基表达量与UPP含量呈高度正相关,相关系数为0.79~0.93(P < 0.01)。而在高分子量谷蛋白总量较高时(试验II),仅Glu-D1位点对%UPP的加性效应达5%显著水平,5+10亚基对%UPP的贡献显著高于2+12和4+12;亚基组合间的聚合体粒度分布无显著差异。高分子量谷蛋白的亚基表达量与UPP含量的相关系数为0.42~0.86(P < 0.05或0.01)。结合高分子量谷蛋白表达量和优质亚基进行选择,能有效提高不溶性谷蛋白大聚体的含量和相对比例,有利于面筋强度和加工品质的进一步提高。     

Introduction to bread wheat (Triticum aestivum L.) and assessment for bread-making quality of alleles from T. boeoticum Boiss. ssp. thaoudar at Glu-A1 encoding two high-molecular-weight subunits of glutenin

Two alleles, Glu-A1r encoding high-molecular-weight (HMW) glutenin subunits 39+40 and Glu-A1s encoding HMW glutenin subunits 41+42, were introgressed to bread wheat (Triticum aestivum L.) cv. Sicco from two accessions of T. boeoticum Boiss. ssp. thaoudar (A genome species, 2n=2x=14). Alleles at Glu-A1 in current commercial bread wheats encode zero or one subunit, and alleles at the homoeoloci Glu-B1 and Glu-D1 encode a maximum of two subunits; hence the maximum number of subunits found in commercial wheats is five, whereas the lines incorporating Glu-A1r and Glu-A1s carry six. Using near-isogenic lines, the current results demonstrated that the introduction of Glu-A1r resulted in diminished dough stickiness and improved stability during mixing compared with Glu-A1a encoding subunit 1, and a small improvement in gluten strength as shown by the SDS- sedimentation test. The introduction of Glu-A1a also resulted in a small improvement in gluten strength predicted by the SDS-sedimentation test. Thus the alleles are of potential value in breeding programmes designed to improve bread-making quality.     

Biochemical and molecular characterisation of Glu-1 loci in Argentinean wheat cultivars

The high molecular weight glutenin subunit (HMW-GS) composition of acollection of 107 Argentinean bread wheat cultivars was analysed bysodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE).Allelic variation at the Glu-1 loci was identified and its frequencycalculated. Eleven alleles were detected, three encoded at the Glu-A1locus, six at the Glu-B1 locus and two at the Glu-D1 locus. Alow frequency of the null allele at the Glu-A1 locus and a highfrequency of subunits 5+10 at the Glu-D1 locus were observed.Reversed phase-high performance liquid chromatography (RP-HPLC)analysis was used to further characterise HMW-GS. Two different types ofBx subunit 8 (named subunits 8 and 8) were detected, the latterhaving shorter elution time. Subunit 8 was not identifiable bySDS-PAGE. According to quantification by RP-HPLC analysis, two groupsof subunit 7 were observed. One group, with a relatively high proportionof subunit 7 (approximately 39% of the total amount of HMW-GS)appeared in cultivars with allele 7+8 at the Glu-B1 locus; asecond group of subunit 7 (around 24% of the total amount ofHMW-GS), was found in alleles 7+8, 7+8 and 7+9. Restrictionfragment length polymorphisms (RFLP) analyses of HMW-GS genes werealso carried out after digestion of genomic DNA with HindIII andTaqI restriction enzymes. The relationship between DNA fragment sizeand glutenin subunits, as estimated by electrophoretic mobility inSDS-PAGE, was also examined. The restriction enzyme TaqIdemonstrated to be a useful tool to detect homozygous plants in selectionprograms against the Glu-A1 null allele.     

The high and low molecular weight glutenin subunits and ω-gliadin composition of bread and durum wheats commonly grown in Portugal

A collection of 63 bread wheats (Triticum aestivum L.) and 21 durum wheats (Triticum durum Desf.) commonly grown in Portugal since 1982 were characterized for the composition of wheat storage proteins (WSP), high molecular weight glutenin subunits (HMW-GS), low molecular weight glutenin subunits (LMW-GS) and ω-gliadins. The composition of HMW-GS, LMW-GS and &-gliadins, encoded at loci Glu-1, Glu-3 and Gli-1, respectively, was revealed by sodium dodecyl sulphate polyacrylamide gel electrophoresis. WSP allelic compositions of bread and durum wheat patterns were given. In the bread wheats, a total of 24, 24 and 18 patterns were observed for HMW-GS, LMW-GS and ω-gliadins, respectively. Forty-two different alleles were identified for the nine loci studied, Glu-A1 (3), Glu-B1 (7), Glu-D1 (4), Glu-A3 (5), Glu-B1 (7), Glu-D3 (2), Gli-A1 (2), Gli-B1 (8) and Gli-D1 (4). In the case of durum wheats, 19 alleles were identified: one allele at Glu-A1, two at Glu-B3, Glu-B2 and Gli-A1, three at Glu-B1, four at Glu-A3 and five at Gli-B1. For HMW-GS, LMW-GS and ω-gliadins, three, six and six different patterns were revealed, respectively. This study represents the first attempt to discriminate the bread and durum wheat varieties commonly grown in Portugal by the allelic variation of storage proteins. The database is useful for varietal identification and for plant breeders who seek to devise effective programmes aimed at improving wheat quality.     

黄淮麦区小麦品种高分子量谷蛋白亚基位点 与品质性状的数量分析

对黄淮麦区77个不同品种高分子量谷蛋白亚基及亚其组成与蛋白质含量和沉降值关系，通过回归、相关分析，结果表明：Glu-1三个位点对蛋白质含量和沉降值的回归、通径效应均可表示为：Glu-D1＞Glu-B1＞Glu-A1。其中，Glu-D1、Glu-B1与蛋白质含量和沉降值均相关显著。Glu-1三个位点亚基与蛋白质含量和沉降值的效应可分别表示为：1＞2*＞Null，14+15＞7+8＞17+18＞7，5+10＞2+12＞4+10。通过品种的亚基组成对其蛋白质含量和沉降值进行回归预测，结果可行，可靠性达显著水平。     

The effect ofGlu-B1 high molecular weight glutenin subunits on biscuit-making quality of wheat

Summary The aim of this study was to assess the effect of specificGlu-B1 HMW-GS on biscuit-making quality. Three soft spring wheat cultivars with the sameGlu-A1 andGlu-D1 HMW-GS, but differentGlu-B1 HMW-GS were used in crosses. F₂₄ derived lines were developed from these crosses.Glu-B1 HMW-GS 6+8 and 17+18; and 7+9 and 17+18 were compared. Lines with HMW-GS 6+8 versus those with HMW-GS 17+18 had a higher flour protein- and alveograph P/L ratio, shorter mixograph mixing time, more vitreous kernels, and a lower alveograph distensibility and strength (all values significant at p=0.05). Lines with HMW-GS 7+9 compared to those with 17+18 showed significant differences for flour extraction and biscuit diameter. The presence of HMW-GS 17+18 was significantly correlated with several biscuit-making quality characteristics in the Dirkwin/Zaragosa F₂₄ lines but not in the Waverley/Zaragosa F₂₄ lines, therefore the effect of HMW-GS 17+18 was modified by the genetic background in which they were expressed.