利用AABBDDDD八倍体培育小麦一簇毛麦二体附加系的研究

对普通小麦（Ｔｒｉｔｉｃｕｍ ａｅｓｔｉｖｕｍ）－节节麦（Ａｅｇｉｌｏｐｓ ｓｑｕａｒｒｏｓａ）八倍体（２ｎ＝８ｘ＝５６,ＡＡＢＢＤＤＤＤ）与硬粒小麦（Ｔｒｉｔｉｃｕｍ ｄｕｒｕｍ）－簇毛麦９Ｈａｙｎａｌｄｉａ ｖｉｌｌｏｓａ）六倍体（２ｎ＝６ｘ＝４２,ＡＡＢＢＶＶ）杂交后,将所得七倍体杂种（ＡＡＢＢＤＤＶ）进行连续自交,在Ｆ４代中利用Ｃ－分带鉴定出可能的簇毛麦６Ｖ二体附加系９５－７和２Ｖ二体附加     

筛选利用小麦微卫星标记追踪簇毛麦各条染色体

选用定位于普通小麦7个部分同源群上的276对微卫星引物对普通小麦中同春和簇毛麦的基因组DNA进行扩增分析,有148对引物可在两个物种间检测到多态性。利用上述显示多态性的引物进一步对7个中国春-簇毛麦二体附加系进行扩增分析,筛选出分别可用来追踪簇毛麦1V至7V染色体的引物wmc49（1BS）、wmc25（2BS）、gdm36（3DS）、gdml45（4AL）、wmc233（5DS）、wmc256（6AL）和gwm344（7BL）。此外还发现6DS上的微卫星引物gwm469可以用来追踪簇毛麦的2V染色体;2DS上的微卫星引物gdm107可用来追踪簇毛麦的6V染色体。进一步用涉及不同簇毛麦和小麦背景的小麦一簇毛麦染色体附加系、代换系和易位系进行扩增分析,这些微卫星标记也可用来鉴定簇毛麦的各条染色体。因此,这然簇毛麦染色体特异的微卫星标记可用来追踪普通小麦背景中的簇毛麦染色体。     

簇毛麦染色体组特异性RAPD标记的筛选、定位和应用

以普通小麦中国春、中国春－簇毛麦二体附加系以及不同来源的簇毛麦为材料,用100个10碱基随机引物进行RAPD扩增。引物OPF02能在不同来源的簇毛麦及所有中国春－簇毛麦二体附加系中扩增出一条长约750bp的片段OPF02 750。普通小麦和硬粒小麦不能扩增出该片段。因此,OPF02 750为分布于簇毛麦所有染色体上的一个簇毛麦染色体组特异片段。用引物OPF02对普通小麦－簇毛麦双二倍体、硬粒小麦－簇毛麦双二倍体以及几个普通小麦的簇毛麦二体代换系、二体附加系进行检测,发现NAU302已经丢失了其所附加的簇毛麦3V染色体。     

利用离果山羊草3C染色体诱导簇毛麦4V染色体结构变异

通过普通小麦农林26-离果山羊草3C异附加系与普通小麦-簇毛麦4V（4D）代换系杂交,杂交F1代与普通小麦回交,综合运用染色体构型分析、C-分带和荧光原位杂交等技术从BC1F2、BC1F3代中鉴定出涉及簇毛麦4V染色体的易位系、端体、等臂染色体系等变异植株,表明离果山羊草3C染色体可有效诱发簇毛麦4V染色体结构变异,是创造小麦-簇毛麦4V易位系的一种有效途径。     

用分子原位杂交（GISH）鉴定小麦－簇毛麦双倍体、附加系、代换系和易位系

用生物素标记的簇毛麦（Ｈａｙｎａｌｄｉａｖｉｌｌｏｓａ）染色体组ＤＮＡ（ｔｏｔａｌｇｅｎｏｍｉｃＤＮＡ）作探针,以普通小麦染色体组ＤＮＡ作遮盖（用量１：２００左右）,进行有丝分裂中期和减数分裂中期Ｉ染色体的分子原位杂交（ＧＩＳＨ）,经抗生物素蛋白－辣根过氧化物酶复合物（ｂｉｏ－ｓｔｒｅｐｔａｖｉｄｉｎ－ｈｏｒｓｅｒａｄｉｓｈｐｅｒｏｘｉｄａｓｅ）和联苯胺四盐酸（ＤＡＢ）检测显色后,小麦－簇毛麦双倍体、附加系、代换系和易位系中的簇毛麦染色体及染色体片段显棕色,与显浅蓝色的小麦染色体可明显区分。用ＧＩＳＨ不仅可以检测导入小麦中的簇毛麦染色质,而且可以清楚地显示出易位染色体断裂点的确切位置。将ＧＩＳＨ用于减数分裂期染色体配对分析,还可以清晰形象地显示出同源和非同源染色体之间的配对和分离情况。     

簇毛麦端体6VS的显微切割及其专化DNA序列的克隆和分析

从簇毛麦（Haynaldia villosa (L.)Schur.)组合CA9211／RW15（6D／6V异代换系）幼胚培养SC2后代中,用原位杂交方法鉴定出T240－6为6VS端体异代换系。以此为材料,采用微细玻璃针切割法及“单管反应”技术体系,对6VS进行切割分离及LA（Linker adaptor)-PCR扩增。扩增带在100－3000bp之间,大部分集中在600－1500bp。利用^32P标记的簇毛麦基因组为探针进行Southern杂交,证实扩增产物来源于簇毛麦。扩增产物纯化后,连续到pGEM-T载体上,构建了6VS DNA质粒库。对库的分析表明,库大约有17000个白色克隆;插入片段分布在100－1500bp,平均600bp。点杂交结果表明,37％克隆有中度到强烈的杂交信号,证明含有中度或高度重复序列;63％克隆有较弱的信号或没有信号,证明为单／低拷贝序列克隆。从库中获得8个簇毛麦特异克隆,对其中两个克隆pHVMK22和pHVMK134进行了RFLP分析和序列分析,并利用该探针对小麦抗白粉病基因Pm21进行了检测。RFLP结果表明,两个克隆一个为低拷贝序列克隆（pHVMK22),另一个为高度重复序列克隆,均为簇毛麦专化DNA序列。以pHVMK22为探针对抗、感病小麦（Triticum aestivum L.)品系的Southern杂交发现抗病品系有一条2kb的特征带,该探针可能作为检测抗病基因Pm21的探针。     

利用phlb突变体创造普通小麦—簇毛麦６ＶＳ端二体代换系

用中国春phlb突变体（C.S.phlbphlb)与普通小麦－簇毛麦６Ｖ（６Ａ）异代换系（Ｓub.6V)杂交,再用phlb突变体与Ｆ１回交,在高配对植株中筛选出一个６Ｖ染色体发生变化的植株,编号为ＬＶ０２,用染色体Ｃ－分带和荧光原位杂交技术,对ＬＶ０２株系的后代进一步鉴定,在ＢＣ１Ｆ２中筛选鉴定出１株编号为ＬＶ０２－０１的植株,该株含有４０条普通小麦染色体,１条簇毛麦６Ｖ染色体和１条６Ｖ短臂端着丝粒染色体,在ＬＶ０２－０１的分离后代中用同样技术鉴定出８株普通小麦－族毛麦６ＶＳ端二体代换系。     

用基因组原位杂交与RFLP标记鉴定小麦——簇毛麦抗白粉病代换系

用荧光素标记的簇毛麦(Haynaldia villosa)基因组总DNA作探针,以普通小麦基因组总DNA作封阻,与花粉母细胞减数分裂中期Ⅰ制片的染色体进行原位杂交。结果表明,抗白粉病小麦品系GN22是普通小麦-簇毛麦二体代换系;用已定位在小麦第6部分同源群上的RFLP探针psr113、psr371进行Southern分析,进一步证明,小麦品系GN21、GN22是普通小麦-簇毛麦6A(6V)代换系;结合同工酶等电聚焦电泳分析,首次把簇毛麦编码的α-淀粉酶-1生化位点定位在簇毛麦6V染色体长臂上,暂命名为α-Amy-Ⅴ1。研究结果表明,原位杂交与RFLP技术相结合是全面、准确鉴定小麦外源染色体及其与小麦染色体部分同源关系的有效方法。     

幼胚培养创造抗白粉病簇毛麦6VS端体

通过白粉病抗性鉴定、生化标记及分子原位杂交相结合的方法,从小麦(Triticum aestivum L.)幼胚培养组合T240 (普通小麦×小麦-簇毛麦(Haynaldia villosa Lam.) 6D/6V异代换系)的32个SC2代株系中,筛选出T240-6株系,其所有的抗白粉病单株均缺失簇毛麦6V染色体长臂上的谷草转氨酶位点GOT-V2,而具有短臂上的醇溶蛋白位点Gli-V2.细胞学染色体观察表明,该株系的所有抗病单株均具有1～2个端体,这些端体不能与小麦染色体配对,双端体之间可以配对.经原位杂交分析,端体杂交呈阳性,表明它们均为簇毛麦6V染色体短臂(6VS).     

利用phlb突变体创造普通小麦-簇毛麦6VS端二体代换系

用中国春phlb突变体（C.Sphlbphlb)与普通小麦柎-簇毛麦6V（6A）异代换系（Sub.6V)杂交,再用phlb突变体与F     

Identification, mapping, and application of polymorphic DNA associated with resistance gene Pm21 of wheat.

A new powdery mildew resistance gene designated Pm21, from Haynaldia villosa, a relative of wheat, has been identified and incorporated into wheat through an alien translocation line. Cytogenetic and biochemical analyses showed that chromosome arms 6VS and 6AL were involved in this translocation. Random amplified polymorphic DNA (RAPD) analysis was performed on recipient wheat cultivar Yangmai 5, the translocation line, and H. villosa with 180 random primers. Eight of the 180 primers amplified polymorphic DNA in the translocation line, and the same results were obtained in four replications. Furthermore, RAPD analysis was reported for substitution line 6V, seven addition lines (1V-7V), and the F1, as well as F2 plants of (translocation line x 'Yangmai 5'), using two of the eight random primers. One RAPD marker, specific to chromosome arm 6VS, OPH17-1900, could be used as a molecular marker for the detection of gene Pm21 in breeding materials with powdery mildew resistance introduced from H. villosa. Key words : RAPD analysis, 6VS-specific marker, Pm21, Erysiphe graminis f.sp. tritici, Triticum aestivum - Haynaldia villosa translocation.     

节节麦和硬粒小麦-簇毛麦双二倍体间杂种的产生及其细胞遗传学研究

通过胚培养产生了节节麦和硬粒小麦-簇毛麦双二倍体间的杂种。结果表明节节麦和硬粒小麦-簇毛麦双二倍体杂交以节节麦作母本较易结实,3个组合的结实率分别为59.18%、67.72%和60.22%,胚培成苗率分别为39.13%、38.10%和50%。杂种F_1生活力旺盛,形态像父本硬粒小麦-簇毛麦双二倍体。杂种自交可孕,3个组合自交结实率平均为7.63%。杂种F_1(ABVD)的减数分裂平均构型为25.36个单价体,1.21个二价体和0.06个三价体,平均每个细胞交叉结频率为1.38,高于“中国春”单倍体的配对频率,推测V组和A、B、D组染色体间有部分同源关系。节节麦和硬粒小麦-簇毛麦双二倍体杂交可能是产生八倍体(AABBDDVV)的又一途径。     

Isolation of a chromosomally engineered durum wheat line carrying the Aegilops ventricosa pchl gene for resistance to eyespot.

The chromosome 7Dv of Aegilops ventricosa (syn. Triticum ventricosum, 2n = 4x = 28, genome DvDvMvMv) carries the gene Pch1 for resistance to eyespot. This gene has previously been transferred to chromosome 7D of bread wheat, T. aestivum (2n = 6x = 42, genome AABBDD). To (1) enhance the level of resistance of bread wheat by increasing the copy number of Pch1, and (2) create eyespot-resistant triticales, meiotically stable Pch1-carrying durum lines were selected from the backcross progenies of a cross between Ae. ventricosa and T. durum cv. Creso ph1c (2n = 4x = 28, genome AABB). The Pch1 transfer, likely resulting from homoeologous recombination, was located at the distal position on the long arm of chromosome 7A. The 7A microsatellite marker Xgwm 698 was found closely linked in repulsion to the introgression in the resistant recombination lines, and the endopeptidase allele located on chromosome 7A of cv. Creso ph1c was lost.     

Cytogenetics of Triticum x Dasypyrum hybrids and derived lines

Genomic in situ hybridization was used to study Triticum x Dasypyrum wide hybrids and derived lines. A cytogenetic investigation was carried out in progenies of (i) amphiploids derived from T. turgidum var. durum (T. durum; 2n = 14; genomes AABB) x D. villosum (2n = 14; genome VV), (ii) three-parental hybrids (T. durum x D. villosum) x T. aestivum (2n = 42, genomes A'A'B'B'D'D'), and (iii) T. aestivum aneuploid lines carrying D. villosum chromosomes or chromatin. The amphiploids derived from T. durum x D. villosum showed a stable chromosomal constitution, made up of 14 V chromosomes, 14 chromosomes carrying the wheat A genome and 14 chromosomes carrying the B genome. High karyological instability was observed in the progenies of three-parental hybrids ([T. durum x D. villosum] x T. aestivum). Plants having the expected 14 A chromosomes, 14 B chromosomes, 7 D chromosomes, and 7 V chromosomes were rather rare (4.5%). Many progeny plants (45.5%) had the hexaploid wheat genome with 42 chromosomes and lacked any detectable D. villosum chromatin. Other plants (50%) had 14 A chromosomes and 14 B chromosomes, plus variable numbers of D and V chromosomes, the former being better retained than the latter in most cases. Some T. aestivum lines carrying D. villosum chromosomes or chromatin, as the result of addition, substitution, or recombination events or even a combination of these karyological events, were found to be stable. Other lines were unstable, and these lines carried 1V, 3V, or 5V chromosomes or their portions. Substitution or recombination events where 1V chromosomes were involved could concern the homeologous counterparts in both the A and B and D genomes of wheat. No line could be recovered where the shorter arm of 3V chromosomes was present. Changes in the morphology and banding pattern of V chromosomes were observed in hybrids that did not carry the entire D. villosum complement. By comparing the results of our cytogenetic analyses with certain phenotypic characteristics of the lines studied, genes for discrete traits could be assigned to specific V chromosomes or V chromosome arms. From the frequency of V chromosomes that were involved in chromatin exchanges with or substituted for one of their homeologous counterparts in the A, B, and D wheat genomes, it was inferred that D. villosum belongs to the same phyletic lineage as T. urartu (donor of the A genome of wheat) and Aegilops speltoides (B genome), and that Ae. squarrosa (D genome) diverged earlier from D. villosum.     

Standard karyotype of Triticum umbellulatum and the characterization of derived chromosome addition and translocation lines in common wheat

A standard karyotype and a generalized idiogram of Triticum umbellulatum (syn. Aegilops umbellulata, 2n = 2x = 14) was established based on C-banding analysis of ten accessions of different geographic origin and individual T. umbellulatum chromosomes in T. aestivum — T. umbellulatum chromosome addition lines. Monosomic (MA) and disomic (DA) T. aestivum — T. umbellulatum chromosome addition lines (DA1U = B, DA2U = D, MA4U = F, DA5U = C, DA6U = A, DA7U = E = G) and telosomic addition lines (DA1US, DA1UL, DA2US, DA2UL, DA4UL, MA5US, (+ iso 5US), DA5UL, DA7US, DA7UL) were analyzed. Line H was established as a disomic addition line for the translocated wheat — T. umbellulatum chromosome T2DS·4US. Radiation-induced wheat — T. umbellulatum translocation lines resistant to leaf rust (Lr9) were identified as T40 = T6BL·6BS-6UL, T41 = T4BL·4BS-6UL, T44 = T2DS·2DL-6UL, T47 = Transfer = T6BS·6BL-6UL and T52 = T7BL·7BS-6UL. Breakpoints and sizes of the transferred T. umbellulatum segments in these translocations were determined by in situ hybridization analysis using total genomic T. umbellulatum DNA as a probeContribution no. 94-349-J from the Kansas Agricultural Experiment Station, Kansas State University, Manhattan, KS 66506-5502, USA     

Development of Wheat-alien Lines with Added Leymus racemosus Chromosomes and 6VS/6AL Translocation Chromosomes

By chromosome C-banding and bi-color fluorescence in situ hybridization (FISH) using digoxigenin-labelled total genomic DNA of Leymus racemosus (Lam.) Tzvel. and biotinylated total genomic DNA of Haynaldia villosa (L.) Schur as probes, three wheat-alien lines with L. racemosus Lr.7 addition and H.　villosa 6VS/6AL translocated chromosomes, and eight lines with L.　racemosus Lr.14 addition and H.villosa 6VS/6AL translocated chromosomes were respectively identified from DALr.7×T6VS/6AL (93G51-4×P64) and DALr.14×T6VS/6AL （94G15×P64）F2 or F3 hybrids. Fluorescein-isothiocyanate-conjugated avidin and rhodamine-conjugated sheep anti-digoxigenin Fab fragment were used in bi-color FISH detection. The chromosomes of L.racemosus and 6VS fragment of H.　villosa were simultaneously detected by their red and green fluorescence. Powdery mildew and scab resistance were also evaluated. The result showed that the obtained plants had high resistance to these two diseases. The potential usage of bi-color FISH in identifying chromatin of L.racemosus and H.villosa was discussed.