利用RFLP分子标记确定导入小麦的鹅观草(R. kamoji)染色体的部分同源群归属

选用来自小麦族7个部分同源群的26个DNA探针对45个小麦-鹅观草衍生后代株系及鹅观草、中国春和扬麦5号亲本进行RFLP分析,结果表明16个小麦-鹅观草异附加系、异代换系或可能的易位系中所涉及鹅观草染色体分别属于第1、3、5、6、7部分同源群。小麦-鹅观草异染色体系中导入的成对鹅观草染色体能够较稳定地遗传给后代。K139、K141、K214、K218、K219、K224二体附加系所添加的鹅观草染色体属第1部分同源群,但K214和K218所添加的鹅观草染色体与K219、K224的添加的鹅观草染色体分别来自鹅观草不同的染色体组。K147端体添加系涉及鹅观草第1部分同源群染色体长臂,而K139、K141和K147所涉及的鹅观草染色体长臂分别来自鹅观草3个不同的染色体组。鹅观草U染色体与小麦第1部分同源群有同源关系,属第1部分同源群的鹅观草染色体尤其是其长臂与赤霉病抗性有关。鹅观草第1部分同源群与第6部分同源群染色体之间可能涉及重排。K203添加的2条鹅观草染色体分别与第1和6部分同源群同源。K166导入鹅观草染色体涉及第5部分同源群短臂。K177（2n=41,20Ⅱ I）中,所渗入的鹅观草染色质涉及第5（5L）、6（6S）、7（SL）部分同源群。鹅观草S、H和Y3个染色体组间具部分同源性。     

将大赖草种质转移给普通小麦的研究：Ⅶ.一个普通小麦—大赖草等臂？…

通过花粉母细胞减数分裂中期Ｉ染色体配对构型分析ＧｉｅｍｓａＣ－分带,从普通小麦－大赖草第７条染色体二体异附加系自交后代中选育并鉴定出了９３Ｇ５１－９和９３Ｇ５２－８２个等臂染色体异附加系,该异附加系在花粉母细胞减数分裂中期Ｉ,其等臂染色体自身两臂配对频率高,染色体易发生断裂,且又携带有较抗赤霉病的基因,是向小麦转移大赖草赤霉病抗性基因的有用中间材料。     

普通小麦-纤毛鹅观草染色体异附加系的分子标记鉴定

随机选取定位于小麦和大麦7个部分同源群上的135对EST、27对STS和253对SSR引物对24个可能的普通小麦-纤毛鹅观草二体异附加系的基因组DNA进行扩增。结果表明, 55对引物在亲本普通小麦中国春、Inayama Komugi、纤毛鹅观草和Inayama Komugi-纤毛鹅观草双二倍体间有多态性扩增, 其中31对引物可以在异附加系中扩增到纤毛鹅观草特异条带。根据PCR扩增结果, 异附加系07K02、07K06、07K39、07K201、07K202、07K255和07K256所添加的纤毛鹅观草染色体归属小麦第1部分同源群; 07K07、07K08、07K09、07K11、07K14和07K17所添加的纤毛鹅观草染色体归属小麦第2部分同源群; 07K15、07K16、07K21和07K47所添加的纤毛鹅观草染色体归属小麦第6部分同源群。     

将大赖草种质转移给普通小麦的研究——Ⅶ.一个普通小麦-大赖草等臂染色体异附加系的选育与鉴定

通过花粉母细胞减数分裂中期Ⅰ染色体配对构型分析、Giemsa C-分带,从普通小麦-大赖草第7条染色体二体异附加系自交后代中选育并鉴定出了93G51-9和93G52-8 2个等臂染色体异附加系。该异附加系在花粉母细胞减数分裂中期Ⅰ,其等臂染色体自身两臂配对频率高,染色体易发生断裂,且又携带有较抗赤霉病的基因,是向小麦转移大赖草赤霉病抗性基因的有用中间材料。     

VE161小麦促进部分同源染色体配对的遗传

ＶＥ１６１小麦包括具有一对长穗偃麦草染色体的雄性不育代换系、可育附加系和杂育系,杂育系由其代换系×附加系产生。ＶＥ１６１小麦在与其它小麦品系的杂交Ｆ１中,具有促进部分同源染色体配对的作用,但其本身部分同源配对频率较低。研究结果表明,ＶＥ１６１小麦本身部分同源染色体配对水平较低,是因其小麦染色体组中存在有一对纯合隐性上位基因,它能够抑制Ｅ染色体（Ｅｐｈ基因）,促进部分同源染色体配对作用的表达,而一般小麦品系中具有该基因的相对显性基因。同时,在促进小麦部分同源染色体配对作用上,Ｅ染色体（Ｅｐｈ基因）具有剂量效应     

抗白粉病6R(6B)染色体异代换系的选育

以中７９０２（６Ｂ）单体为母本,Ｈｏｌｄｆａｓｔ－ＫｉｎｇⅡ６Ｒ二体异附加系为父本配制杂交组合,经白粉病抗性追踪和细胞学鉴定,选育出抗白粉病６Ｒ（６Ｂ）二体异代换系。其与普通小麦中８６０１以及与“中国春”６Ｂ重双端体的Ｆ１植株,在减数分裂中期Ⅰ染色体构型分别为２０″＋２′和２０″＋１′＋２ｔ′ ,从而,证实６Ｂ染色体被 ６Ｒ染色体代换。同时,对６Ｒ染色体上抗白粉病基因的进一步利用进行了讨论。     

VE161小麦外源染色体的传递特点

VE161小麦包括具有一对长穗偃麦草染色体的雄性不育代换系,可育附加系和杂育系,杂育系由其代换系×附加系产生,其外源染色体（E染色体）具有促进小麦部分同源染色体配对作用。本报道了VE161小麦本身含E染色体配子的传递率为VE161小麦与普通小麦杂交F2,BC1中分离出含E染色体植株的频率,发现VE161小麦本身含E染色体配子的传递率极高,而在F2和BC1代分离群体中保留或消除E染色体都较为容易,这一特点极利于E染色体促进部分同源染色体配对作用在创造易位系上的应用。     

同胞质普通小麦-纤毛鹅观草异附加系D和端体异附加系tBL的选育

用普通小麦－纤毛鹅观草双倍体与普通小麦中国春连续回交两次,然后连续自交,通过形态观察、根尖细胞染色体计数、花粉母细胞减数分裂中期Ｉ染色体配对分析及染色体Ｃ－分带,在ＢＣ２Ｆ２和ＢＣ２Ｆ３群体中,分别筛选到一个端二体异附加系９４Ｋ２２７和一个二体异附加系９４Ｋ２８０,其中Ｃ－分带显示９４Ｋ２２７添加的是纤毛鹅观草染色体Ｂ的一对长臂,９４Ｋ２８０添加的是纤毛鹅观草的一对染色体Ｄ。     

普通小麦—簇毛麦异附加系和异代换系的C—分带鉴定

用改良的C-分带技术鉴定南京农业大学细胞遗传研究室获得的普通小麦的簇毛麦V_2、V_3、V_4、V_6、V_7染色体异附加系和V_2、V_5异代换系,得到与N-分带和染色体配对分析一致的结果,并且由于C-分带可同时鉴别小麦全部21对染色体,鉴定出V_2异代换系中被代换掉的小麦染色体为1A。     

小麦抗赤霉病外源种质的创制和育种利用

小麦赤霉病是危害小麦安全生产的重要病害之一,种植抗病品种是防治赤霉病最经济有效的手段。目前在生产上应用的抗源很少,越来越多的研究者将目光转移到小麦的近缘属种,寻找新的抗源以及寻求新的育种突破。携带抗性基因的外源染色体可以通过染色体工程手段以附加系、代换系和易位系等形式导入小麦。综述了将大赖草等多个小麦近缘种的抗赤霉病基因导入普通小麦、创制抗病外源种质和育种利用的最新研究进展,以期为小麦抗赤霉病育种提供参考信息。     

小麦抗赤霉病利器——他山之石

赤霉病是我国乃至世界小麦(Triticum aestivum)产区的重要病害, 给农业生产和人畜健康造成重大威胁。分离鉴定优质抗病基因、培育抗病品种, 是控制我国麦区赤霉病的重要手段。最近, 山东农业大学孔令让团队完成了二倍体长穗偃麦草(Thinopyrum elongatum)基因组的组装, 并在此基础上通过精细定位和图位克隆分离得到来自长穗偃麦草的抗赤霉病基因Fhb7。他们发现Fhb7编码1个谷胱甘肽转移酶, 对禾谷镰孢菌(Fusarium graminearum)分泌的包括呕吐毒素等在内的多种毒素具有解毒作用, 是1个广谱持久抗病基因。他们还发现Fhb7很可能最初源于内生真菌, 经过基因水平转移进入到偃麦草基因组中。此外, Fhb7不影响其它农艺性状, 且其抗性不受小麦遗传背景影响。这一系列工作揭示了作物抗病演化中的全新机制, 对小麦抗赤霉病育种以及更好地利用长穗偃麦草的丰富基因资源都具有重要意义。     

我国“十三五”育成小麦新品种（系）抗赤霉病进展分析与展望

小麦赤霉病严重威胁我国粮食和食品安全,培育抗赤霉病小麦品种是解决该病害最经济有效的途径。20世纪90年代后,以扬麦158为代表的扬麦、宁麦系列中抗赤霉病品种的育成和大面积推广有效抵御了长江中下游麦区的赤霉病危害,使我国抗赤霉病育种处于国际领先水平。尽管全球明确了7个抗赤霉病基因,为开展抗赤霉病育种提供了重要支撑,但由于赤霉病抗性机制复杂,实现高抗与高产的协调仍极其困难,抗赤霉病仍是当前及未来我国小麦育种的主要目标。对“十三五”期间我国小麦新品系和审定品种的抗性情况以及我国抗赤霉病育种方面取得的进展进行了综述,并提出了重视挖掘和利用扬麦等推广品种中优异抗性基因、将Fhb1导入扬麦等主栽品种的育种技术路线和重视表型精准鉴定等建议,以期为实现我国抗赤霉病育种突破提供借鉴。     

Molecular cytogenetic characterization of alien introgressions with gene Fhb3 for resistance to Fusarium head blight disease of wheat

Fusarium head blight (FHB) resistance was identified in the alien species Leymus racemosus, and wheat-Leymus introgression lines with FHB resistance were reported previously. Detailed molecular cytogenetic analysis of alien introgressions T01, T09, and T14 and the mapping of Fhb3, a new gene for FHB resistance, are reported here. The introgression line T09 had an unknown wheat-Leymus translocation chromosome. A total of 36 RFLP markers selected from the seven homoeologous groups of wheat were used to characterize T09 and determine the homoeologous relationship of the introgressed Leymus chromosome with wheat. Only short arm markers for group 7 detected Leymus-specific fragments in T09, whereas 7AS-specific RFLP fragments were missing. C-banding and genomic in situ hybridization results indicated that T09 has a compensating Robertsonian translocation T7AL·7Lr#1S involving the long arm of wheat chromosome 7A and the short arm of Leymus chromosome 7Lr#1 substituting for chromosome arm 7AS of wheat. Introgression lines T01 (2n = 44) and T14 (2n = 44) each had two pairs of independent translocation chromosomes. T01 had T4BS·4BL-7Lr#1S + T4BL-7Lr#1S·5Lr#1S. T14 had T6BS·6BL-7Lr#1S + T6BL·5Lr#1S. These translocations were recovered in the progeny of the irradiated line Lr#1 (T5Lr#1S·7Lr#1S). The three translocation lines, T01, T09, and T14, and the disomic addition 7Lr#1 were consistently resistant to FHB in greenhouse point-inoculation experiments, whereas the disomic addition 5Lr#1 was susceptible. The data indicated that at least one novel FHB resistance gene from Leymus, designated Fhb3, resides in the distal region of the short arm of chromosome 7Lr#1, because the resistant translocation lines share a common distal segment of 7Lr#1S. Three PCR-based markers, BE586744-STS, BE404728-STS, and BE586111-STS, specific for 7Lr#1S were developed to expedite marker-assisted selection in breeding programs.     

Genomic in situ hybridization (GISH) analyses of Thinopyrum intermedium, its partial amphiploid Zhong 5, and disease-resistant derivatives in wheat

Genomic in situhybridization (GISH) to root-tip cells at mitotic metaphase, using genomic DNA probes from Thinopyrum intermedium and Pseudoroegneria strigosa, was used to examine the genomic constitution of Th. intermedium, the 56-chromosome partial amphiploid to wheat called Zhong 5 and disease-resistant derivatives of Zhong 5, in a wheat background. Evidence from GISH indicated that Th. intermedium contained seven pairs of St, seven J^S and 21 J chromosomes; three pairs of Th. intermedium chromosomes with satellites in their short arms belonging to the St, J, J genomes and homoeologous groups 1, 1, and 5 respectively. GISH results using different materials and different probes showed that seven pairs of added Th. intermedium chromosomes in Zhong 5 included three pairs of St chromosomes, two pairs of J^S chromosomes and two pairs of St-J^S reciprocal tanslocation chromosomes. A pair of chromosomes, which substituted a pair of wheat chromosomes in Yi 4212 and in HG 295 and was added to 21 pairs of wheat chromosomes in the disomic additions Z1, Z2 and Z6, conferred BYDV-resistance and was identical to a pair of St-J^S tanslocation chromosomes (StJ^S) in Zhong 5. The StJ^S chromosome had a special GISH signal pattern and could be easily distinguished from other added chromosomes in Zhong 5; it has not yet been possible to locate the BYDV-resistant gene(s) of this translocated chromosome either in the St chromosome portion belonging to homoeologous group 2 or in the J^S chromosome portion whose homoeologous group relationship is still uncertain. Among 22 chromosome pairs in disomic addition line Z3, the added chromosome pair had satellites and belonged to the St genome and homoeologous group 1. Disomic addition line Z4 carried a pair of added chromosomes which was composed of a group-7 J^S chromosome translocated with a wheat chromosome; this chromosome was different to 7 Ai-1, but was identical to 7 Ai-2. The leaf rust and stem rust resistance genes were located in the distal region of the long arm, whereas the stripe rust resistance gene(s) was located in the short arm or in the proximal region of the long arm of 7 Ai-2. A pair of J^S-wheat translocation chromosomes, which originated from the WJ^S chromosomes in Z4, was added to the disomic addition line Z5; the added chromosomes of Z5 carried leaf and stem rust resistance but not stripe rust resistance; Z5 is a potentially useful source for rust resistance genes in wheat breeding and for cloning these novel rust-resistant genes. GISH analysis using the St genome as a probe has proved advantageous in identifying alien Th. intermedium in wheat. Received: 17 May 1999 / Accepted: 22 June 1999     

Disomic Thinopyrum intermedium addition lines in wheat with barley yellow dwarf virus resistance and with rust resistances.

Zhong 5 is a partial amphiploid (2n = 56) between Triticum aestivum (2n = 42) and Thinopyrum intermedium (2n = 42) carrying all the chromosomes of wheat and seven pairs of chromosomes from Th. intermedium. Following further backcrossing to wheat, six independent stable 2n = 44 lines were obtained representing 4 disomic chromosome addition lines. One chromosome confers barley yellow dwarf virus (BYDV) resistance, whereas two other chromosomes carry leaf and stem rust resistance; one of the latter also confers stripe rust resistance. Using RFLP and isozyme markers we have shown that the extra chromosome in the Zhong 5-derived BYDV resistant disomic addition lines (Z1, Z2, or Z6) belongs to the homoeologous group 2. It therefore carries a different locus to the BYDV resistant group 7 addition, L1, described previously. The leaf, stem, and stripe rust resistant line (Z4) carries an added group 7 chromosome. The line Z3 has neither BYDV nor rust resistance, is not a group 2 or group 7 addition, and is probably a group 1 addition. The line Z5 is leaf and stem rust resistant, is not stripe rust resistant, and its homoeology remains unknown.     

Development of T. aestivum L.eH. californicum Alien Chromosome Lines and Assignment of Homoeologous Groups of Hordeum californicum Chromosomes

Hordeum californicum(2n=2x=14, HH) is resistant to several wheat diseases and tolerant to lower nitrogen. In this study, a molecular karyotype of H. californicum chromosomes in the Triticum aestivum L. cv. Chinese Spring(CS)eH. californicum amphidiploid(2n=6x=56, AABBDDHH) was established. By genomic in situ hybridization(GISH) and multicolor fluorescent in situ hybridization(FISH) using repetitive DNA clones(pTa71, pTa794 and pSc119.2) as probes, the H. californicum chromosomes could be differentiated from each other and from the wheat chromosomes unequivocally. Based on molecular karyotype and marker analyses, 12 wheatealien chromosome lines, including four disomic addition lines(DAH1, DAH3, DAH5 and DAH6), five telosomic addition lines(MtH7L,MtH1 S, MtH1 L, DtH6 S and DtH6L), one multiple addition line involving H. californicum chromosome H2, one disomic substitution line(DSH4) and one translocation line(TH7S/1BL), were identified from the progenies derived from the crosses of CSeH. californicum amphidiploid with common wheat varieties. A total of 482 EST(expressed sequence tag) or SSR(simple sequence repeat) markers specific for individual H. californicum chromosomes were identified, and 47, 50, 45, 49, 21, 51 and 40 markers were assigned to chromosomes H1, H2, H3, H4, H5, H6 and H7, respectively. According to the chromosome allocation of these markers, chromosomes H2,H3, H4, H5, and H7 of H. californicum have relationship with wheat homoeologous groups 5, 2, 6, 3, and 1, and hence could be designated as 5Hc, 2Hc, 6Hc, 3Hcand 1Hc, respectively. The chromosomes H1 and H6 were designated as 7Hcand 4Hc, respectively, by referring to SSR markers located on rye chromosomes.     

DNA marker analysis for pyramided of Fusarium head blight (FHB) resistance QTLs from different germplasm

A pyramided FHB resistance line of wheat (WSY) was previously developed from three FHB resistant cultivars (Sumai 3, Wangshuibai, and Nobeokabouzu) in the Jiangsu Academy of Agricultural Sciences, China. In the present study, we analyzed the genetic relationship between WSY and the three parental cultivars using DNA markers in order to clarify how many and which resistance genes had accumulated in WSY. We analyzed 282 DNA markers from the 21 wheat chromosomes. WSY was found to include different chromosome regions that harbored putative FHB QTLs of the three parental germplasm. Haplotypes of DNA markers on these QTL regions revealed that the 1BL, 2BL, 5AS, and 7AL QTL regions were from Sumai 3, the 2AS, 2DS, 3AS, and 6BS QTL regions were from Wangshuibai, and the 3BS QTL region was from Nobeokabouzu. This study showed that different resistance genes from the different resistant germplasm had indeed accumulated in WSY. WSY is a potential resistant resource for FHB resistance in wheat breeding programs.