小麦族三属杂种F1小孢子发生过程中染色体的行为(简报)

利用八倍体小黑麦劲松49和八倍体小滨麦950059杂交合成了小麦-黑麦-滨麦草三属杂种,对不同基因组染色体在三属杂种F1减数分裂和小孢子发育过程中的行为进行了研究.基因组原位杂交(GISH)结果表明劲松49和小滨950059均包含44条小麦染色体和12条外源染色体,三属杂种F1中含有6条黑麦染色体和6条滨麦草染色体.减数分裂过程中黑麦和滨麦草染色体很少与小麦染色体配对.常以单价体形态存在.小孢子中的微核主要由外源染色体组成.在三属杂种F1的花粉发育过程中还发现了染色体浓缩不同步的现象.     

组织培养诱导的普通小麦─黑麦代换系和附加系分子细胞遗传学检测

通过组织培养从普通小麦（ＴｒｉｔｉｃｕｍａｅｓｔｉｖｕｍＬ．）与八倍体小黑麦（×ＴｒｉｔｉｃｏｓｅｃａｌｅＷｉｔｍａｃｋ）杂种Ｆ０幼胚再生植株后代中获得２个代换系９３０４９８、９３０４８３和１个附加系９３００２９。以黑麦（ＳｅｃａｌｅｃｅｒｅａｌｅＬ．）基因组ＤＮＡ为探针,采用荧光原位杂交（ＦＩＳＨ）证实了黑麦染色体的存在。在有丝分裂中期,经ＦＩＳＨ处理的黑麦染色体为黄绿色,明显区别于红色的小麦染色体。染色体配对、Ｃ分带、麦谷蛋白电泳分析,证明两个代换系为１Ｄ／１Ｒ代换,附加的也是黑麦１Ｒ染色体     

1RS-7DS.7DL小麦-黑麦小片段易位系的鉴定

黑麦(Secale cereale L., RR)是改良普通小麦(Triticum aestivum L., AABBDD)的重要基因资源,将黑麦优异基因转移到普通小麦中,是小麦品种改良的有效途经之一。文章将四川地方品种蓬安白麦子(T. aestivum L., AABBDD) 与秦岭黑麦(S. cereale cv. Qinling, RR)杂交,染色体自动加倍获得八倍体小黑麦CD-13(AABBDDRR);通过顺序FISH和GISH分析,发现该八倍体小黑麦1RS端部与7DS的端部发生相互易位,是一个携带1RS-7DS.7DL小麦-黑麦小片段易位染色体的八倍体小黑麦。利用八倍体小黑麦CD-13与四川推广小麦品种川麦42杂交、连续自交,获得包含60个株系的F₅群体;对F₅群体的58个株系进行GISH和FISH分析发现,其中13个株系含有1RS-7DS.7DL小片段易位染色体。在这13个株系中,株系811染色体数目为2n=6x=42,是稳定的1RS-7DS.7DL小片段易位系;并且1RS特异分子标记和醇溶蛋白分析表明,1RS-7DS.7DL易位染色体1RS小片段的断裂点位于分子标记IB267-IAG95之间,不包含编码黑麦碱蛋白的Sec-1位点;同时1RS-7DS.7DL小片段易位系的千粒重与川麦42相当,远远高于八倍体小黑麦CD-13,对千粒重无负作用。因此,1RS-7DS.7DL小麦-黑麦小片段易位系可作为进一步深入研究1RS小片段上的优异基因及其遗传效应的重要材料。     

小黑麦×小滨麦后代1RS·1BL易位系的选育和鉴定

利用细胞学、染色体C分带和原位杂交方法,对八倍体小黑麦劲松49与八倍体小滨麦杂种后代选育的稳定遗传材料山农030-1进行了鉴定。染色体观察结果表明,山农030-1根尖染色体数目为42,花粉母细胞减数分裂中期I(PMC MI)染色体构型为2ｎ=21Ⅱ。分别以黑麦、滨麦草基因组DNA为探针进行原位杂交,表明山农030-1含有一对黑麦和小麦的整臂易位染色体,不含有来自滨麦草的遗传物质。染色体C分带结果进一步表明此材料为1RS·1BL易位系。接种鉴定表明,山农030-1对白粉病免疫。Abstract: In the progenies of octoploid Triticale Jinsong49 crossed with octoploid Tritileymus, a stable germplasm line named Shannong030-1 was obtained. Its chromosome number was 42, and 21 bivalents could be observed at PMC MI. FISH analysis by using genomic DNAs from S. cereale and genomic DNAs from L. mollis as probes,respectively, showed that Shannong030-1 contained a pair of translocation chromosome between rye and wheat, and had no genetic materials from L. mollis . C-banding analysis showed that it was translocation lines of 1RS·1BL.Resistance identification showed Shannong030-1 was immune to powdery mildew.     

小麦-黑麦染色体代换的研究

本文用八倍体小黑麦,六倍体小黑麦与普通小麦杂交,在杂交后代中选择普通小麦类型带有黑麦性状的品系56个,经C－分带与原位杂交鉴定,选出10个同祖群间的代换系,即1R／1D,1R／1A,5R／5A,6R／6A的代换,这10个代换系表现遗传性稳定,育性正常,具有抗病,抗旱等优良性状,有利于价值。用代换系5R／5A与6R／6A杂交,在杂交后代中获得大量有经济价值的小片段易位系,作者认为可能是同祖染色体间配对与交换产生的。     

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.     

八倍体小黑麦×普通小麦杂种后代群体中的染色体易位

用改良的Giemsa C-带技术以单株为基础分析了八倍体小黑麦×普通小麦的杂种BC_1,F_(?)和F_(?)代植株的核型。在鉴定了C-带核型的1098株杂种后代植株中,发现了78条小麦-黑麦和277条黑麦-黑麦易位染色体。在不同的世代和株系中,小麦-黑麦染色体易位率变化在4.35—14.07%之间,平均7.10%;黑麦-黑麦染色体易位率在0.48—52.78%之间,平均25.23%。鉴定的小麦-黑麦易位染色体涉及了黑麦的14条不同的染色体臂和小麦的A、B和D组染色体。易位的48.57%发生在小麦和黑麦的部分同源染色体之间,51.43%发生在非部分同源染色体之间。不同的黑麦染色体臂参与易位的频率不同。小麦-黑麦染色体易位主要发生在杂种的早期世代,使用适当的选择技术在F_3获得了纯合的易位植株。文中讨论了快速选育易位系的技术和它们在小麦育种中的应用问题。     

异细胞质八倍体小黑麦的获得及其细胞遗传

改变小黑麦细胞质有可能增加减数分裂的稳定性,提高小黑麦的结实率与籽粒饱满度。作者以不同细胞质的“中国春”小麦与黑麦杂交,F_1幼苗用秋水仙素加倍获得双二倍体、或以八倍体小黑麦为父本与F_1杂交,获得异细胞质八倍体小黑麦(Triticale 8x)8个品系。实验结果表明:细胞质不同的“中国春”小麦与黑麦杂交结实率差异显著,出苗率亦不同,F_1株型多为两亲的中间型,花药不开裂,个别组合出现雄蕊雌化现象,有的组合表现生长弱性,减数分裂中期Ⅰ常出现1至数个末端交叉的棒状二价体,其数量在不同组合间差异显著,表明异细胞质对染色体配对有影响。D类细胞质对改进八倍体小黑麦的结实率可能有一定的作用。     

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。     

小麦和黑麦染色体在小黑麦×小麦杂种的不同世代群体中的传递

使用单株植物C-带核型鉴定技术,研究了小麦和黑麦染色体在八倍体小黑麦×普通小麦的F_1,BC_1,F_2和F_3代中的遗传行为。黑麦染色体通过花粉和卵细胞的传递率显著不同,通过卵细胞丢失的染色体较多。黑麦染色体在F_2和F_3的传递率为36.0—38.8%,显著低于通过配子的平均传递率。不同的黑麦染色体通过配子的传递是随机的,而在F_2和F_3中却存在着显著的差异,1R的传递率最高,6R、7R最低。发生上述差异的原因可能是黑麦染色体的丢失不仅发生在配子形成和受精阶段,还受具有不同核型的受精卵在发育过程中夭亡的影响。受黑麦染色体的影响,小麦染色体也有不同程度的丢失。在不同的世代群体中,约有7.3—28.1%的植株丢失了小麦染色体。6R、5R和7R对小麦染色体丢失的作用较大。根据本研究的结果,在使用八倍体小黑麦×小麦的杂交方式利用黑麦遗传物质于小麦育种的工作中,F_2和F_3是有效选择的关键世代。本文建议的单株植物C-带核型鉴定技术是实现这一选择目标的有效方法。     

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.     

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.     

Spontaneous and Divergent Hexaploid Triticales Derived from Common Wheat × Rye by Complete Elimination of D-Genome Chromosomes

Background

Hexaploid triticale could be either synthesized by crossing tetraploid wheat with rye, or developed by crossing hexaploid wheat with a hexaploid triticale or an octoploid triticale.

Methodology/Principal Findings

Here two hexaploid triticales with great morphologic divergence derived from common wheat cultivar M8003 (Triticum aestivum L.) × Austrian rye (Secale cereale L.) were reported, exhibiting high resistance for powdery mildew and stripe rust and potential for wheat improvement. Sequential fluorescence in situ hybridization (FISH) and genomic in situ hybridization (GISH) karyotyping revealed that D-genome chromosomes were completely eliminated and the whole A-genome, B-genome and R-genome chromosomes were retained in both lines. Furthermore, plentiful alterations of wheat chromosomes including 5A and 7B were detected in both triticales and additionally altered 5B, 7A chromosome and restructured chromosome 2A was assayed in N9116H and N9116M, respectively, even after selfing for several decades. Besides, meiotic asynchrony was displayed and a variety of storage protein variations were assayed, especially in the HMW/LMW-GS region and secalins region in both triticales.

Conclusion

This study confirms that whole D-genome chromosomes could be preferentially eliminated in the hybrid of common wheat × rye, “genome shock” was accompanying the allopolyploidization of nascent triticales, and great morphologic divergence might result from the genetic variations. Moreover, new hexaploid triticale lines contributing potential resistance resources for wheat improvement were produced.     

Identification of Haynaldia villosa chromosomes added to wheat using a sequential C-banding and genomic in situ hybridization technique

Genomic in situ hybridization (GISH) offers a convenient and effective method for cytological detection, but can not determine the identity of the chromosomes involved. We integrated C-banding with GISH to identify Haynaldia villosa chromosomes in a wheat background. All chromosomes of H. villosa showed C-bands, either in telomeric regions or in both telomeric and centromeric regions, which allowed unequivocal identification of each H. villosa chromosome. The seven pairs of H. villosa chromosomes were differentiated as 1–7 according to their characteristic C-bands. Using a sequential C-banding and GISH technique, we have analyzed somatic cells of F₃ plants from the amphiploid Triticum aestivum-H. villosa x Yangmai 158 hybrids. Three plants (94009/5-4,94009/5-8 and 94009/5-9) were shown to contain H. villosa chromosome(s). 94009/5-4 (2n = 45) had three H. villosa chromosomes (2, 3 and 4); 94009/5-8 (2n = 45) possessed one chromosome 4 and a pair of chromosome 5, and 94009/5-9 (2n = 43) was found to have one chromosome 6 of H. villosa. The combination of GISH with C-banding described here provides a direct comparison of the cytological and molecular landmarks. Such a technique is particularly useful for identifying and localizing alien chromatin and DNA sequences in plants.     

杀配子染色体特异RAPD 标记及山羊草属与普通小麦间分子多态性的研究

以普通小麦"中国春"、三个"中国春"具杀配子染色体的二体异附加系及作为三个杀配子基因种源的三种山羊草为材料, 用46 个10 nt 随机引物对基因组DNA 进行扩增, 以筛选杀配子染色体特有的RAPD 标记, 并检测普通小麦与三种山羊草之间的RAPD 多态性。结果表明:46 个引物中有35 个扩增出比较稳定的RAPD 产物。其中引物OPF-14 和OPQ-09 分别在普通小麦"中国春"-山羊草附加系间扩增出多态性产物;因而认定OPF-14₁₃₀₀ 与OPQ-09₈₀₀、OPF-14₁₁₆₀ 与OPQ-09₇₇₀、OPF-14₁₂₈₀分别为三个杀配子染色体3C、Gcl 和2C 的特异性RAPD 标记, 可以用于快速跟踪鉴定3C、Gcl、2C 杀配子染色体。对三种山羊草与普通小麦"中国春"进行了基因组DNA多态性分析, 结果表明, 35 个引物在"中国春"中共扩增出162 个产物, 在离果山羊草、拟斯卑尔脱山羊草、柱穗山羊草中分别扩增出140、154 和155 个产物;三种山羊草与"中国春"之间的共有扩增产物分别为69、87、96 个, 占总扩增产物的29.61%、37.70%和43.44%。上述结果, 从分子水平揭示了山羊草属与普通小麦之间存在着较近的亲缘关系。     

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.     

Sequential chromosome banding and in situ hybridization analysis.

Different combinations of chromosome N- or C-banding with in situ hybridization (ISH) or genomic in situ hybridization (GISH) were sequentially performed on metaphase chromosomes of wheat. A modified N-banding-ISH/GISH sequential procedure gave best results. Similarly, a modified C-banding - ISH/GISH procedure also gave satisfactory results. The variation of the hot acid treatment in the standard chromosome N- or C-banding procedures was the major factor affecting the resolution of the subsequent ISH and GISH. By the sequential chromosome banding - ISH/GISH analysis, multicopy DNA sequences and the breakpoints of wheat-alien translocations were directly allocated to specific chromosomes of wheat. The sequential chromosome banding- ISH/GISH technique should be widely applicable in genome mapping, especially in cytogenetic and molecular mapping of heterochromatic and euchromatic regions of plant and animal chromosomes.     

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. × Secale cereale L.) × 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 1R(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.     

Loss of chromosomes 2R and 5RS in octoploid triticale selected for agronomic traits

The advanced lines of octoploid triticale which have been bred for nearly a half century in China show significant improvements in agronomic traits such as plant height, fertility, threshability, maturity and seed plumpness, although no intentional cytological selection had been performed. In this study, eight primary and six advanced lines were analyzed by fluorescence and genomic in situ hybridization to elucidate their chromosome constitutions. In the advanced lines, about 70% of the plants examined had 2n = 56 chromosomes (range: 50 to 58). Almost all advanced lines, however, had lost rye chromosome 2R and the short arm of 5R (5RS). The exceptions were lines Y1005 and Y4683: The former had lost only the 2R chromosome and the latter only 5RS. The reduction of rye chromosomes was compensated by an extra pair of 2D or A-genome (possibly 2A) chromosomes in plants with 2n = 56. This suggests that the loss of 2R and 5RS chromosomes contributes to the improvement of octoploid triticale. Since the plants with chromosome 2R are non-free threshing and chromosome 2D of synthetic wheat is known to carry the Tg (tenacious glumes) gene, it is possible that chromosome 2R carries a gene affecting the threshability, and we carried out selection to remove it. We also discuss the possible relationshipbetween 5RS and the genetic stability of octoploid triticale.