阿拉拉特小麦(Triticum araraticum)抗白粉病基因向普通小麦转移 Ⅰ.阿拉拉特小麦与普通小麦杂种后代的细胞遗传研究及抗性鉴定

配制了普通小麦与阿拉拉特小麦的正、反交组合２０个,杂交结实率为４．９％～３３．６％。不同组合杂种Ｆ１每个ＰＭＣ平均的单价体为１５．２０～１８．５５,二价体为７．０３～９．０２,三价体和四价体分别为０．３６～１．１５和０．０１～０．０２。通过对杂种后代连续２年成株期混合菌种抗性鉴定和苗期分小种分菌系鉴定表明,从普通小麦中国春与阿拉拉特小麦的杂种Ｆ３和Ｆ４代已选择到对白粉病高抗～免疫的单株,它们具有４２条染色体,在ＰＭＣ′ｓＭＩ形成０．００～０．４６个单价体,２０．７７～２１．００个二价体,０．００～０．０６个四价体,在细胞学上已稳定。与已知白粉病抗性基因比较的抗谱分析表明,阿拉拉特小麦携有主效抗病基因Ｐｍ２,在上述的杂交选择过程中,已通过遗传重组将Ｐｍ２基因导入到中国春中。     

Identification and Mapping of Two New Genes Conferring Resistance to Powdery Mildew from Aegilops tauschii （Coss,） Schmal

Two powdery mildew resistance genes were Identified from Aegilops tauschll accessions Y201 and Y212 and mapped using two different F2 populations derived from the crosses between susceptible accession Y2272 and Y201, and susceptible accession Y2263 and Y212. Genetic analysis of resistance to powdery mildew Indicated that the resistance of Y201 was controlled by a single dominant gene, whereas the resistance of Y212 was controlled by a single recessive gene. We have temporarily designated these genes as PmY201 and PmY212, respectively. By bulk segregation analysis, six mlcrosatelllte markers Including Xgwm174, cfd26, cfd57, cfdl02, Xgwm583 and Xgwm639 were found to be linked to PraY201 with genetic distances of 5.2, 7.7, 9.6, 12.5, 20.2 and 22.1 cM, respectively. Five SSR markers, including cfd57, Xgwm182, cfd7, cfd102, and cfd12, were found to be linked to PmY212 with distances of 5.6, 7.2, 11.5, 14.7, and 18.5 cM, respectively. According to the locations of the linked markers, the two resistance genes were located In the 5DL region. Based on the chromosomal locations and the resistance patterns of the two genes, we propose that PmY201 and PmY212 are two novel powdery mildew resistance genes, and are suitable for marker-assisted selection.     

Genome-Wide Association Study of Powdery Mildew Resistance in Russian Spring Wheat (T. aestivum L.) Varieties

Russian Journal of Genetics - Powdery mildew caused by the fungal pathogen Blumeria graminis f. sp. tritici (Bgt) is an econo-mically important disease of common wheat T. aestivum L. One of the...     

Genome-Wide Identification and Characterization of Germin and Germin-Like Proteins (GLPs) and Their Response Under Powdery Mildew Stress in Wheat (Triticum aestivum L.)

Plant Molecular Biology Reporter - Germin and germin-like proteins (GLPs) play multifaceted roles in plants and participate in signaling processes associated with host–pathogen interactions...     

小麦抗倒性研究进展

倒伏是严重影响小麦子粒产量和品质的一个重要因素。本文系统阐述了小麦茎秆形态和结构特性、茎秆化学成分与抗倒伏关系以及抗倒性的遗传和分子标记等方面的最新研究进展。株高、基部节间长度与抗倒性呈负相关;而基部节间粗度、秆壁厚、单位长度干重与抗倒性呈正相关。茎秆机械组织细胞层数、厚度,维管束数目、面积以及髓腔大小与抗倒性密切相关。茎秆化学成分中纤维素、木质素以及碳水化合物含量和硅、钾元素含量与抗倒性呈正相关。小麦抗倒性呈数量性状遗传特征,除受多对主基因控制外,可能还受微效修饰基因作用。采用分子标记技术已将抗倒性以及与抗倒性相关的茎秆形态性状进行了QTL定位。     

Genetics and Resistance Mechanism of the Cucumber (Cucumis sativus L.) Against Powdery Mildew

Journal of Plant Growth Regulation - Powdery mildew (PM) is one of the most severe foliar diseases in cucumbers (Cucumis sativus L.), but the inheritance of PM resistance remains unclear. The...     

含有抗白粉病基因的黑麦染色体小片段向小麦的转移

利用感白粉病的小麦品种绵阳11的纯系和黑麦自交系R12杂交, 在其单体附加系自交后代的BC₁F₅株系中选择小麦－黑麦异源易位系。根据已报道的黑麦特异重复序列pSc20H设计了一对特异引物, 用PCR方法鉴定了300个单体附加系的自交BC₁F₅株系,发现其中70个株系含有黑麦染色体成分。一个来源于6R单体附加系的小麦株系96Ⅱ691-830-98表现了对白粉病的高度抗性, PCR方法鉴定证明其含有黑麦染色体成分。对该株系作进一步的基因组原位杂交(GISH)鉴定, 证明它的一对染色体的端部含有黑麦染色体的小片段。这一结果指出, 含有抗白粉病基因的黑麦染色体6R小片段被引入了小麦。研究表明利用单体附加诱导染色体小片段易位是一种有效的方法。利用PCR和GISH原位杂交相结合的方法可提高检测外源染色体小片段的准确性和选择效率。     

Resistance of bread wheat (Triticum aestivum L.) to preharvest sprouting: An association analysis

A statistical analysis of the data about 1422 bread wheat accessions with estimated preharvest sprouting was carried out. Close associations of preharvest sprouting resistance with the grain color and with resistance to Fusarium head blight were revealed, as well as weak, but statistically significant, associations with the habit, awnedness, and reduced height genes Rht-B1 and Rht-D1 (insensitive to gibberellin GA3). The pedigree analysis showed that the cluster structures of the gene pools of the North American red-grained and white-grained varieties are practically identical. In both groups, varieties that are resistant to preharvest sprouting differ from susceptible ones in the percentage of the contributions of the Crimean and Mediterranean landraces. Resistance is associated with a high contribution by the Crimean landrace and susceptibility is associated with a high contribution by the Mediterranean landrace.     

小麦高分子量麦谷蛋白亚基1Dx5启动子驱动外源基因的表达

将小麦高分子量麦谷蛋白亚基(HMW-GS)基因的胚乳组织特异性表达启动子驱动的外源突变型1Dx5基因和gus基因导入小麦中.对其转基因植株连续3代的跟踪研究表明,突变型1Dx5基因的重复序列导致其表达蛋白分子量增大,并影响其它1Bx17 1By18亚基基因的表达.组织化学分析观察到gus基因在1Dx5基因启动子驱动下的表达表现出胚乳组织特异性,在开花2周后开始表达,表达量呈持续上升,至腊熟期达到最高,其次为籽粒成熟期.     

Plant regeneration from coleoptile tissue of wheat (Triticum aestivum L.)

Plant regeneration was achieved from coleoptile tissue of wheat (Triticum aestivum L. cv. Kharachia-65). Coleoptiles (1.0 - 3.5 cm long) were excised from 2- to 5-d-old seedlings and cultured on Murashige and Skoog's (MS) medium supplemented with 2,4-dichlorophenoxyacetic acid (2,4-D - 0.5, 2.5, and 5.0 mg dm^-3). Cream, friable callus was obtained after 6 weeks of inoculation. This callus was sub-cultured on MS medium supplemented with 2,4-D (2.5 mg dm^-3) and 5 % coconut water. After 6 weeks of sub-culturing white, cream or pale, friable, nodular callus was obtained. Plant regeneration occurred when this callus was sub-cultured on MS medium supplemented with 0.2 mg dm^-3 1-naphthalene acetic acid + 1.0 mg dm^-3 6-benzylaminopurine. For rooting, regenerated shoots or plantlets were transferred on MS medium supplemented with 0.5 mg dm^-3 indole-3-acetic acid. Rooted plantlets were directly transferred into pots and grown under field conditions. Seed setting invariably occurred in all plants. This revised version was published online in July 2006 with corrections to the Cover Date.     

Purification and Characterization of Lipase from Wheat (Triticum aestivum L.) Germ

A method of isolation and purification of lipase (EC 3.1.1.3) from the germ of wheat (Triticum aestivumL.) is described. An electrophoretically homogeneous preparation of the enzyme (specific activity, 622.5 × 10^–3 mol/min per mg protein) was obtained after 61-fold purification. The molecular weight of the enzyme, determined by gel chromatography, was 143 ± 2 kDa. The optimal conditions for the enzyme were 37°C and pH 8.0. The homogeneous preparation of the lipase exhibited high thermal stability: over 20% of the original activity was retained after incubation of the preparation at high temperatures (60–90°C) for 1 h at pH 8.0.     

A new flavone O-glycoside and other constituents from wheat leaves (Triticum aestivum L.)

From leaves of Triticum aestivum a new O-glycosylflavone has been isolated together with chlorogenic acid and its 3'-methyl ether and 6 C-glycosylflavones. The structure of the new flavonoid was determined by 1D and 2D NMR techniques and other spectral evidence as 5,7-dihydroxy-3',4',5'-trimethoxyflavone-7-O-beta-rutinoside.     

小麦异交群体连续歧化选择的RAPD分析

利用太谷核不育基因构建的遗传变异丰富的基础群体DNS2,进行了连续5轮歧化选择。本论文从不同的世代中,选择了10个子群体进行RAPD分析。采用7个引物扩增出116个位点,从基因频率和表型带两个角度的分析都表明,群体具有丰富的遗传变异。整个群体总的多态位点百分率达88.79,总杂合度为0.3143。子群体内（间）遗传距离的结果显示：子群体内的遗传差异小于子群体间的遗传差异;各选择子群体与未选群体间都有较大的遗传距离;随着选择轮次的增加,株高选择子群体间的遗传距离逐渐增大;对同一性状进行选择的子群体间世代内（间）平均遗传距离小于对不同性状进行选择的子群体内（间）的遗传距离。RAPD分子聚类结果显示出对同一性状进行选择的子群体聚在一起,反映了对株高选高的选择效果比较明显。 Abstract:A base population was established through multi-parent random crossing by using Taigu dominant male-sterile wheat,and then five cycles of 2-way selection for four quantitative characters were conducted.The dynamic changes of genetic structures in the open-pollinated wheat population were examined by RAPD technique.Seven primers in RAPD analysis amplified 116 sites.The results of gene frequencies and phenotypic bands showed abundant genetic variations existed in the population.The percentage of polymorphic loci was 8879,and the average heterozygosity was 0.3143 in the whole population.The genetic distance of RAPD showed as follows :① The genetic distance within a subpopulation was lower than that between every two subpopulations.② Each subpopulation had considerable divergence compared with unselected population.③ The genetic distances between the subpopulations which were selected for plant height gradually increased accompanied with the selection.④The genetic distance between subpopulations which were selected for the same character was lower than that were selected for different characters both in the same generation and among different generations.The cluster results of RAPD genetic distance demonstrated that the subpopulations selected for the same character going to one cluster.It also showed that the selective effect of increasing plant height was obvious.     

A Study of Floret Development in Wheat (Triticum aestivum L.)

Plants of wheat (Triticum aestlvum L.) cv. Aotea were grownat high or low nitrogen levels and in a natural photoperiodor continuous light. Starting 17–21 days from the double-ridgestage, eight plants from each treatment were sampled every 3days until anthesis, and the two basal, the sixth, and the terminalspikelets were sectioned longitudinally. A developmental scorewas assigned to each floret and rates of development calculated.Continuous light hastened development but reduced the numberof spikelets per ear, while high nitrogen delayed developmentbut increased spikelet numbers. The number of florets initiatedin each spikelet varied within narrow limits, but grain settingdepended strongly on spikelet position and on treatment. Althoughflorets were initiated in acropetal succession, the rate ofdevelopment tended to increase up to floret 4 but then declinedmarkedly. As a result grain setting was confined to basal floretpositions, although the two basal spikelets developed so slowlythat they contributed relatively little to grain yield. Distalflorets degenerated almost simultaneously at or before ear emergence,but those in intermediate positions continued to develop untilafter fertilization in the lower florets. It is argued thatthe spikelet is an integrated system in which correlative mechanismsplay a part throughout the development of the florets.     

RELP markers linked to two Hessian fly-resistance genes in wheat (Triticum aestivum L.) from Triticum tauschii (coss.) Schmal

Summary Restriction fragment length polymorphism (RFLP) markers linked to genes controlling Hessian fly resistance from Triticum tauschii (Coss.) Schmal. were identified for two wheat (Triticum aestivum L.) germ plasm lines KS89WGRC3 (C3) and KS89WGRC6 (C6). Forty-six clones with loci on chromosomes of homoeologous group 3 and 28 clones on those of group 6 were surveyed for polymorphisms. Eleven and 12 clones detected T. tauschii loci in the two lines, respectively. Analysis of F₂ progenies indicated that the Hessian fly resistance gene H23 identified in C3 is linked to XksuH4 (6.9 cM) and XksuG48 (A) (15.6 cM), located on 6D. The resistance gene H24 in C6 is linked to XcnlBCD451 (5.9 cM), XcnlCD0482 (5.9 cM) and XksuG48 (B) (12.9 cM), located on 3DL.Paper No. 810 of the Cornell Plant Breeding Series     

Characterization of cytosolic phosphoglucoisomerase from immature wheat (Triticum aestivum L.) endosperm

Phosphoglucoisomerase from cytosol of immature wheat endosperm was purified 650-fold by ammonium sulphate fractionation, isopropyl alcohol precipitation, DEAE-cellulose chromatography and gel filtration through Sepharose CL-6B. The enzyme, with a molecular weight of about 130,000, exhibited maximum activity at pH 8.1. It showed typical hyperbolic kinetics with both fructose 6-P and glucose 6-P withK _m of 0.18 mM and 0.44mM respectively. On either side of the optimum pH, the enzyme had lower affinity for the substrates. Using glucose 6-P as the substrate, the equilibrium was reached at 27% fructose 6-P and 73% glucose 6-P with an equilibrium constant of 2.7. The ΔF calculated from the apparent equilibrium constant was +597 cal mol^-1. The activation energy calculated from the Arrhenius plot was 5500 cal mol^-1. The enzyme was completely inhibited by ribose 5-P, ribulose 5-P and 6-phosphogluconate, withK _i values of 0.17, 0.25 and 0.14 mM respectively. The probable role of the enzyme in starch biosynthesis is discussed.