普通小麦-华山新麦草异代换系的分子细胞遗传学研究

利用荧光原位杂交和染色体C-分带技术对普通小麦-一华山新麦草的异代换系进行了研究。荧光原位杂交结果显示：异代换系H921—6—12和H924—3—4均含有2条华山新麦草的染色体。对这2个材料和华山新麦草进行染色体C-分带带型比较,结果认为：H921—6—12可能是普通小麦-华山新麦草的5A／N5^b代换系,H924—3—4可能是3D／N4^b代换系。     

小麦—黑麦异代换及小麦种内易位系的分子细胞遗传学检测

研究应用基因组原位杂交、染色体C-分带和RAPD技术,对八倍体小黑麦×普通小麦杂种F2经电离辐射处理后的高代材料98-60进行了检测。基因组原位杂交结果表明,该材料为小麦-黑麦异代换系。进一步通过C-分带分析表明,该品系为5R代换系,并且还包含有5AS/6AS小麦种内的染色体易位。通过RAPD分析,在该品系中找到了来源于八倍体小黑麦亲本"新麦73"的黑麦染色体特异扩增产物OPA-01350和与两个亲本不同的特异重组产物OPF-14800、OPF-14920,进一步验证了基因组原位杂交和C-分带的鉴定结果。     

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。     

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。     

巨穗小麦种质中外源遗传物质的细胞遗传学和分子生物学鉴定

利用C分带、基因组原位杂交并结合分子生物学手段,对12份巨穗小麦种质材料中的外源遗传物质进行了检测.结果表明,12份材料染色体数均为42,其中5份材料均具有一对小麦-黑麦(Triticum aestivum-Secalecereal)1BL/1RS易位染色体和一对中间偃麦草(Agropyron intermedium Garten)染色体、3份材料只具有一对中间偃麦草染色体、3份材料只具一对1BL/1RS染色体、1份材料无1BL/1RS和中间偃麦草染色体.进一步细胞学分析表明,此中间偃麦草染色体代换了普通小麦(Triticum aestivum L.)中的2D染色体,因其良好的同源补偿性,表示为2Ai.同时对2Ai在巨穗小麦种质中存在的遗传学意义及小麦遗传改良中的应用进行了讨论.     

用顺序GISH-FISH 技术鉴定小麦-中间偃麦草小片段易位系

利用顺序基因组-重复序列原位杂交技术对1个来自中3不育系和普通小麦恢75杂种后代稳定株系H96276-2的染色体组成进行了分析。以中间偃麦草（Agropyronintermedium）基因组DNA为探针的荧光原位杂交结果表明,H96276-2的体细胞中有42条染色体,包括20对小麦染色体和1对小麦-中间偃麦草易位染色体,中间偃麦草染色体的易位片段位于1对小麦染色体的端部。进而用重复序列探针pSc119进行第2次荧光原位杂交,证明H96276-2中的中间偃麦草染色体易位片段位于小麦2B染色体的短臂上。     

小偃6号背景下黑麦遗传物质的荧光原位杂交分析

利用普通小麦(Triticum aesttvum L.)"小偃6号"与黑麦(Secale cereale L.)品种"德国白粒"杂交,选育出"小偃6号"类型带有黑麦性状的种质材料.应用总基因组原位杂交(GISH)进行检测,在8份材料中探测到黑麦染色质的存在,其中附加系3个,代换系1个,易位系4个;进一步用荧光绿标记探针pScll9.2及荧光红标记探针pAsl的双色荧光原位杂交(FISH)技术,对其中部分品系的染色体组成进行分析鉴定,结果表明:易位系BCll6-1是1RS/1BL小麦/黑麦易位系,BCl52-l是涉及一条lB染色体的1RS/1BL易位系,代换系BC97-2是2R(2D)二体代换系;附加系BCl22-3附加了一条6R黑麦染色体,一条6B染色体的长臂缺失.同时,对连续的总基因组原位杂交和双色荧光原位杂交技术在小麦育种中的应用进行了讨论.     

小麦异源易位系的高效诱导和分子细胞遗传学鉴定

利用杀配子染色体(gametocidal chromosome)和低剂量(10Gy)γ-射线辐射花粉两种方法诱导小麦(Triticum aestixum L)-滨麦(Leymus mollis Trin)和小麦-中间偃麦草[Thinopyrum intermedium(Host)Barkwarth]的易位系。通过基因组原位杂交(GISH)分析,在59个小滨麦代换系M8724-8-13与离果山羊草(Aegilops trincialis L)3C染色体附加系的杂交后代中获得了3株小麦-滨麦易位系,易位频率达到5．08％。其中1个易位系经C-分带证明是小麦的7D染色体与1条滨麦的染色体发生了整臂易位。同时还获得了3个滨麦染色体的缺失系。滨麦染色体发生结构变异的总频率为8．47％。除了滨麦染色体以外,在一些植株中还观察到小麦的染色体也发生了缺失。在69个普通小麦与小麦-中间偃麦草附加系TAI-14辐射花粉的杂交后代中,得到2株小麦-中间偃麦草的易位系,易位频率为2．90％。两个易位系都是小片段易位,经C-分带证明两个易位系所涉及的小麦染色体分别是3A和4A。利用杀配子染色体和低剂量γ射线辐射花粉诱导小麦异源易位系都是行之有效的方法,但这两种方法各有优缺点,在实际工作中应根据不同的目的选用不同的实验体系。     

小偃6号背景下黑麦遗传物质的荧光原位杂交分析

利用普通小麦(Triticum aestivum L.)“小偃6号”与黑麦(Secale cereale L.)品种“德国白粒”杂交,选育出“小偃6号”类型带有黑麦性状的种质材料。应用总基因组原位杂交(GISH)进行检测,在8份材料中探测到黑麦染色质的存在,其中附加系3个,代换系1个,易位系4个;进一步用荧光绿标记探针pSc119.2及荧光红标记探针pAs1的双色荧光原位杂交(FISH)技术,对其中部分品系的染色体组成进行分析鉴定,结果表明:易位系BC116-1是1RS/1BL小麦/黑麦易位系,BC152-1是涉及一条1B染色体的1RS/1BL易位系, 代换系BC97-2是2R(2D)二体代换系;附加系BC122-3附加了一条6R黑麦染色体,一条6B染色体的长臂缺失。同时,对连续的总基因组原位杂交和双色荧光原位杂交技术在小麦育种中的应用进行了讨论。     

普通小麦-簇毛麦6V代换系45S rDNA和5S rDNA位点的FISH分析

采用顺序基因组原位杂交和双色荧光原位杂交技术,对普通小麦-簇毛麦6v代换系K0736的45S rDNA和5S rDNA基因位点进行了分析.结果表明,该代换系2n=42,有1对簇毛麦6V染色体,为6V/6A代换系,45S rDNA位点有8对,位于7对染色体上.5S rDNA位点有6对,分别位于6对染色体上.在1AS、1BS、5DS的端部同时存在458 rDNA和5S rDNA位点,并在物理位置上紧密相邻.同时讨论了rDNA位点的数目和分布位置存在变异的可能因素.     

Characterisation of mildew resistant wheat-rye substitution lines and identification of an inverted chromosome by fluorescent in situ hybridisation

Seven different mildew resistant wheat lines derived from crosses between triticale and bread wheat were examined by molecular cytogenetics and chromosome C-banding in order to determine their chromosomal composition. Genomic in situ hybridisation (GISH) showed the presence of rye germplasm in all the lines and identified three substitution lines, three double substitution lines and one addition-substitution line. C-banding identified rye chromosomes 1R and 4R in the addition-substitution line, rye chromosomes 1R and 6R in two substitution lines and 1R and 2R in the third line, and rye chromosome 1R in the three substitution lines. Two of the latter lines (7-102 and 7-169) contained a modified form of the chromosome; fluorescent in situ hybridisation (FISH) using five different repetitive DNA-probes showed a pericentric inversion of 1R in both lines. The breakpoints of the 1R inversion were between (1) the 5S rDNA site and the NOR-region on the satellite of the short arm, and (2) between two AAC(5) sites close to the centromere on the long arm. The role of the rye chromosomes in the mildew resistance, the utilisation of the inverted 1R and the significance of the lines in wheat breeding are discussed.     

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     

小麦新种质4844中外源P染色质的GISH与SSR分析

采用基因组原位杂交(GISH)检测和染色体组成分析方法,对大穗多花小麦新种质4844后代的15个株系进行遗传分析。结果发现,4844-12是1个稳定的异附加系,4844-2和4844-8是稳定的异代换系;对异代换系进行SSR分析表明,代换系中小麦的6D染色体被1对P染色体代换,说明这对冰草染色体与小麦6D染色体有部分同源关系,由此确定4844中的冰草染色体为6P;同时筛选出冰草6P染色体的4个SSR标记。     

Standard karyotype of Triticum longissimum and its cytogenetic relationship with T. aestivum.

C-banding polymorphism was analyzed in 17 accessions of Triticum longissimum from Israel and Jordan, and a generalized idiogram of this species was established. C-banding analysis was further used to identify two sets of disomic T. aestivum - T. longissimum chromosome addition lines and 13 ditelosomic addition lines and one monotelosomic (6S1L) addition line. C-banding was also used to identify T. aestivum - T. longissimum chromosome substitution and translocation lines. Two major nucleolus organizing regions (NORs) on 5S1 and 6S1 and one minor NOR on 1S1 were detected by in situ hybridization using a 18S-26S rDNA probe. Sporophytic and gametophytic compensation tests were used to determine the homoeologous relationships of T. longissimum chromosomes. The T. longissimum chromosomes compensate rather well and fertility was restored even in substitution lines involving wheat chromosomes 2A, 4B, and 6B that contain major fertility genes. Except for the deleterious gametocidal genes, T. longissimum can be considered as a suitable donor of useful genes for wheat improvement.     

Molecular Cytogenetic Identification of Triticum aestivum-Secale cereale Substitution and Addition Lines

Two substitution lines, designated as 930498 and 930483, and one addition line, designated as 930029, via Fo immature embryo culture of Triticum aestivum x octoploid triticale ( x Triti-cosecale Wittmack) were identified. Fluorescence in situ hybridization (FISH) using total genomic DNA of rye ( Secale cereale L. ) as probe corroborated the existence of rye chromosomes, further confirmed through chromosome paring at meiotic metaphase 1, C-banding and glutenin SDS- PAGE. The results demonstrated that the two substitution lines are ID/IR, and the addition line is also IR addition. Rye chromosomes that are distinct to the red-colored wheat chromosomes appear yellow-green at mitotic metaphase after FISH.     

Production of wheat-rye substitution lines and identification of chromosome composition of karyotypes using C-banding, GISH, and SSR markers

Based on the cross (Triticum aestivum L. x Secale cereale L.) x T. aestivum L., wheat-rye substitution lines (2n = 42) were produced with karyotypes containing, instead of a pair of homologous wheat chromosomes, a homeologous pair of rye chromosomes. The chromosome composition of these lines was described by GISH and C-banding methods, and SSR analysis. The results of genomic in situ hybridization demonstrated that karyotype of these lines included one pair of rye chromosomes each and lacked wheat--rye translocations. C-banding and SSR markers were used to identify rye chromosomes and determine the wheat chromosomes at which the substitution occurred. The lines were designated 1R(1D), 2R(2D)2, 2R(2D)3, 3R(3B), 6R(6A)2. The chromosome composition of lines IR(1A), 2R(W)1, 5R(W), 5R(5A), and 6R(W)1, which were earlier obtained according to the same scheme for crossing, was characterized using methods of telocentric analysis, GISH, C-banding, and SSR analysis. These lines were identified as 1R(1A), 2R(2D)1, 5R(5D), 5R(5A), and 6R(6A)1, C-banding of chromosomes belonging to line 1R(1A) revealed the presence of two translocated chromosomes (3DS.3DL-del. and 4AL.W) during simultaneous amplification of SSR markers located on 3DL and 4AS arms. The "combined" long arm of the newly derived chromosome 4A is assumed to be formed from the long arm of chromosome 4AS itself and a deleted segment 3DL. All examined lines are cytologically stable, except for 3R(3B), which does not affect the stability of rye 3R chromosome transfer. Chromosome identification and classification of the lines will permit them to be models for genetic studies that can be used thereafter as promising "secondary gene pools" for the purpose of plant breeding.     

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.     

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.     

三个小黑麦花粉株系的染色体组成分析与抗白粉病鉴定

对来自小黑麦与小麦杂种的３个花粉株系,ＤＨ２２０－４,ＤＨ２２０－５和ＤＨ２２０－１４进行了形态性状观察,染色体组成分析和抗白粉病鉴定。经过染色体形态和数目观察、原位杂交、Ｃ－分带、同工酶等电聚焦和贮藏蛋白的ＳＤＳ－聚丙烯酰胺凝胶电泳分析,证明其中两个株系,ＤＨ２２０－４和ＤＨ２２０－５是６Ｒ／６Ｄ代换系,另一个株系ＤＨ２２０－１４是１Ｒ／１Ｄ代换系。经人工接种鉴定,两个６Ｒ／６Ｄ代换系高抗白粉病。从而进一步证明黑麦的６Ｒ染色体上存在抗白粉病的基因。同时还对小麦遗传背景下异源染色体的识别及６Ｒ染色体的利用价值等问题进行了讨论。