共查询到19条相似文献,搜索用时 218 毫秒
1.
利用荧光原位杂交技术分析了两个小麦-外源种杂种花粉母细胞中1BL/1RS 小麦-黑麦易位染色体和外源染色体包括中间偃麦草(Thinopyrum intermedium (Host) Barkworth & DR Dewey)、簇毛麦(Haynaldia villosa (L.) Schur)染色体的减数分裂行为. 我们首次发现:在减数分裂后期, 1BL/1RS 小麦-黑麦易位染色体发生错分裂,形成两个易位染色单体. 这种错分裂导致易位染色单体在末期Ⅰ分配到两个正在形成的细胞核内,错分裂的易位染色单体进一步形成微核,并在四分体期观察到黑麦的微核出现.从贵农22×遗4095 的F2代植株中检测到一个2n=41的植株,其含有一对1BL/1RS 小麦-黑麦易位染色体,核型分析表明,其中一条黑麦染色体臂比另一条的黑麦染色体臂短1/3左右.在遗4212×遗4095的F2代中检测到一个具有中间偃麦草染色体小片段易位到小麦染色体端粒部分的小麦-中间偃麦草易位植株.这可能是由于在减数分裂过程中发生非均等分裂导致小麦-黑麦1BL/1RS易位染色体的黑麦染色体段臂缺失1/3及小麦-中间偃麦草非罗伯逊易位.在两个杂种F2植株中,中间偃麦草染色体分布频率为39.6%, 簇毛麦染色体分布频率为43.4%, 1BL/1RS 小麦-黑麦易位染色体分布频率分别为51.8%和56.6%.实验结果表明,1BL/1RS 小麦-黑麦易位染色体与外源染色体包括中间偃麦草、簇毛麦染色体在减数分裂过程中没有相互作用.小麦-黑麦1BL/1RS易位染色体在减数分裂过程中可以发生错分裂,并导致杂种后代黑麦染色体臂发生缺失.这对于培育以小麦为背景含有不同长度的黑麦1R染色体短臂的种质及小麦-外源染色体非罗伯逊易位的小片段易位系具有指导意义. 相似文献
2.
小麦异源易位系的高效诱导和分子细胞遗传学鉴定 总被引:7,自引:0,他引:7
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。 相似文献
3.
单体异附加系花药培养创制小麦- 中间偃麦草纯合易位系 总被引:2,自引:2,他引:0
利用单体异附加系花药培养细胞工程途径,诱导小麦与中间偃麦草发生染色体易位,通过细胞学分析、荧光原位杂交(F ISH)和SSR鉴定出纯合易位系.研究结果表明,经单体异附加系花药培养创制出1个小麦-中间偃麦草纯合易位系99-803;其花粉母细胞(PM C s)减数分裂中期I染色体构型为18.42个环状二价体 2.57个棒状二价体 0.01个单价体;中间偃麦草的7A i-1染色体与小麦7A或7B染色体发生了非罗伯逊易位,且中间偃麦草易位片段较小;通过该途径获得纯合易位系的频率约为2%.以上结果表明,单体异附加系花药培养是一条向小麦转移异源染色体小片段(基因)的快速高效途径. 相似文献
4.
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。 相似文献
5.
利用电离辐射处理整臂易位系成熟雌配子诱导外源染色体小片段易位 总被引:5,自引:0,他引:5
簇毛麦(Haynaldia villosa)是小麦(Triticum aestivum)改良的重要遗传资源.培育小片段易位,特别是中间插入易位,有助于更好地利用外源有益基因.已报道的小麦-簇毛麦易位系大多数属于整臂易位或大片段易位.本研究以60Co-γ谢线(剂量率:1.6Gy/min,三种剂量:16.0,19.2和22.4Gy)处理整臂易位系的成熟雌配子,随后选取适龄穗子去雄套袋,2~3天后再用普通小麦品种“中国春”的新鲜成熟花粉授粉.通过M1植株根尖细胞有丝分裂中期染色体基因组原位杂交(genomic in situ hybridization,GISH),从534株M1材料中检测到97株涉及6V染色体短臂(6VS)的小片段结构变异,包括小片段中间插入易位染色体80条、末端易位染色体57条和6VS缺失55条.在22.4Gy处理中这三种结构变异的诱变频率分别为21.02%,14.01%和14.65%,远远高于已报道的结果.获得了涉及146条6VS小片段结构变异的74株M1材料的回交种子.M1植株中的小片段结构变异可通过回交传递给后代.利用电离辐射处理整臂易位系成熟雌配子是一种高效诱导染色体小片段结构变异、特别是中间插入易位的新方法. 相似文献
6.
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. 相似文献
7.
小麦-黑麦代换系5A/5R与6A/6R杂交诱导同祖染色体配对与易位的研究 总被引:5,自引:0,他引:5
利用两个小麦-黑麦异源双代换系DS 5A/5R与DS 6A/6R杂交,探讨同祖染色体配对的可能性与创制小麦黑麦异源易位系.在方法上对杂种F1的减数分裂行为进行研究,观察5R与5A、6R与6A配对频率,探讨同祖染色体配对规律.实验结果看到杂交F1减数分裂中有22.91%的花粉母细胞有小麦染色体(ABD组)与黑麦染色体(R组)发生同祖配对.在F2及以后世代,通过染色体C分带、原位杂交检测,选择小麦-黑麦易位系.在F2代的45株中检测到9株有易位,易位频率为20%,是目前小麦-黑麦染色体易位频率最高的.染色体易位有的来源于同祖配对的交换,有的来源于单价体错分裂或断裂的重建. 相似文献
8.
普通小麦-大赖草易位系NAU601和NAU618的选育及双端二体测交分析 总被引:2,自引:0,他引:2
利用根尖体细胞有丝分裂中期染色体Giemsa C-分带和荧光原位杂交从普通小麦-大赖草Lr.2、Ir.7异附加系辐射后代中选育出2个纯合易位系:(1)易位系NAU618(MS142-3),2n=44,易位染色体由大赖草Lr.7染色体的大部分(约5/6,包括着丝粒)及小麦染色体1A短臂的一部分(近端1/3)组成,外源染色体片段的长度约占易位染色体总长度的4/5;(2)易位系MAU601(MS101-4),2n=42,易位染色体由小麦染色体4B的整个短臂和4B长臂近着丝粒部分(1/3)及大赖草Lr.2短臂的绝大部分组成,外源染色体片段占易位染色体长臂的1/2。对易位系进行的双端二体侧交分析证交易位所涉及的小麦染色体分别为1A和4B。连续3年单花滴注法进行的田间赤霉病抗性接种鉴定结果表明,普通小麦-大赖草异源异位系MAU618(MS142-3)对赤霉病的抗性与抗病对照品种苏麦3号相仿,易位系MAU601(MS101-4)对赤霉病抗性低于苏麦3号,但明显高于感病亲本中国春。 相似文献
9.
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。 相似文献
10.
含有抗白粉病基因的黑麦染色体小片段向小麦的转移 总被引:7,自引:0,他引:7
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。 相似文献
11.
Y. B. Wang H. Hu J. W. Snape 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1996,92(7):811-816
Six doubled-haploid (DH) lines, derived by anther culture from octoploid triticale x wheat hybrids, were characterized using cytological, biochemical and molecular techniques. Lines varied in their wheat and rye genome composition, and were either wheat-rye chromosome multiple addition lines or had spontaneous substitutions and/or wheat-rye translocations. Most of the lines contained a pair of 4R chromosomes, whereas 1R or 7R were present in others. The results are similar to those previously obtained with hexaploid triticale x wheat crosses and indicate that it is possible to produce alien (wheat/rye) addition, substitution, and translocation lines directly from the anther culture of intergeneric hybrids. 相似文献
12.
黑麦6R抗白粉病基因向小麦的渗进与鉴定 总被引:2,自引:0,他引:2
为了将黑麦6R染色体上抗小麦白粉病的基因导入小麦,选用了一个6R/6D代换系M24为亲本之一,分别与小麦栽培品种和第6部分同源群缺体系杂交,杂种出现6R或/或6A,6B,6D单,双或三单体等各种情况,取其花药进行培养,共获得241个再生植株,对其中32个抗白粉病的花粉植株经染色体计数,C-分带,基因组原位杂交,同工酶等电聚焦电泳和或/RFLP分子标记检测,发现有6株仍保持为6R/6D代换系,有10 相似文献
13.
小麦遗传背景对黑麦抗叶锈基因Lr26的抗性表达的影响 总被引:9,自引:2,他引:7
利用1套从小麦纯系和黑麦自交系培育出的1R附加系、代换系和易位系,研究了1RS上的抗叶锈基因Lr26在小麦中的表达。结果发现,1R二体附加系和纯合1RS/1BL易位系高抗小麦叶锈病;而其小麦亲本、1R(1B)代换系和1BS/1RL易位系重感叶锈病。这一结果指出了黑麦染色体臂1RS上的抗小麦叶锈病基因Lr26在小麦中的表达受小麦染色体臂1BL上的基因的强烈影响,指出了外源基因在小麦中的表达可受染色体臂或基因水平上的相互作用的制约。文中讨论了外源基因与小麦遗传背景相互作用在小麦育种中的意义。 相似文献
14.
Z. Miao J. Zhuang Hu Han 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1988,75(3):485-491
Summary Studies of the chromosomal composition of pollen plants regenerated from the F1 of hybrids produced from Triticum-Agropyron intermediate type and common wheat demonstrated that various gametic types of the F1 could be fully expressed at the whole plant level via anther culture. The observed frequency of each of the eight types of pollen plants (based on their chromosome numbers) was in good agreement with the theoretical probabilities as shown by X2 analysis. Comparative studies of the chromosome composition of somatic cells and pollen mother cells (PMC's) of selected pollen plants permitted classification of the plants into four distinct classes. The majority of these regenerated pollen plants had identical chromosome numbers in both root tip cells and PMC's. An alien disomic addition line, which was cytologically stable for two generations, was obtained directly from anther culture. Moreover, the addition line exhibits resistance to stripe rust disease, a trait which is conferred by the Agropyron chromosome. We suggest that anther culture techniques provide a unique and expeditious route for the introduction of alien genes or chromosomes into wheat cultivars. 相似文献
15.
S. Agache B. Bachelier J. de Buyser Y. Henry J. Snape 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1989,77(1):7-11
Summary Marked effects of genotype on wheat anther culture response have been observed. Genetic factors have been recognised to be one of the major contributors to in vitro responses of cultured wheat tissues. In wheat anther culture, embryo induction, plant regeneration and albina/green ratio have been determined to be heritable traits. Using Chinese Spring (CS) monosomic 1D, single chromosome substitution lines of chromosome 5B or chromosome arm 5BL from Chinese Spring into six varieties, and F1 hybrids heterozygous for the 1B chromosome structure (1BL-1BS/1BL-1RS), the anther culture response was studied: genes on CS1D chromosome and 5BL chromosome arm increases the embryo frequency; gene(s) involved in regeneration ability are located on the 1RS chromosome arm; a gene increasing albina frequency is located on Chinese Spring 5B chromosome. Our results support the fact that without gametic selection, a differential development occurred from the particular classes of microspores carrying genes for higher regeneration ability. Moreover, in some crosses, a few genes with major effects were involved in determination of anther culture response. 相似文献
16.
N. S. Badaev E. D. Badaeva N. L. Bolsheva N. G. Maximov A. V. Zelenin 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1985,70(5):536-541
Summary Hexaploid triticales were crossed with common wheats, and the resultant froms were selected for either triticale (AD 213/5-80) or common wheat (lines 381/80, 391/80, 393/80). The cytogenetic analysis showed that all forms differ in their chromosome composition. Triticale AD 213/5-80 and wheat line 381/80 were stable forms with 2n = 6x = 42. Lines 391/80 and 393/80 were cytologically unstable. In triticale AD 213/5-80, a 2R (2D) chromosome substitution was found. Each of the three wheat lines had a chromosome formed by the translocation of the short arm of IR into the long arm of the IB chromosome. In line 381/80, this chromosome seems to be inherited from the Kavkaz wheat variety. In lines 391/80 and 393/80, this chromosome apparently formed de novo since the parent forms did not have it. The karyotype of line 381/80 was found to contain rye chromosomes 4R/7R, 5R and 7R/4R. About 15% of the cells in line 391/80 contained an isochromosome for the 5R short arm and also a chromosome which arose from the translocation of the long arms of the 5D and 5R chromosomes. About one-third of the cells in the common wheat line 393/80 contained the 5R chromosome. This chromosome was normal or rearranged. Practical applications of the C-banding technique in the breeding of triticale is discussed. 相似文献
17.
N. L. V. Lapitan R. G. Sears B. S. Gill 《TAG. Theoretical and applied genetics. Theoretische und angewandte Genetik》1984,68(6):547-554
Summary The spontaneous occurrence of chromosome breaks, deletions, and translocations in plant tissue cultures is well documented. This study investigated the usefulness of tissue culture as a method of introgressing alien genes into wheat. Wheat X rye hybrids were regenerated from embryo scutellar calli maintained in culture for 222 days. The regenerated seedlings then were treated with colchicine to produce amphidiploids (AABBDDRR). The karyotypes of ten amphidiploids were analyzed by C-banding to determine chromosome structural changes that occurred during tissue culture. Three wheat/rye and one wheat/wheat chromosome translocations, seven deletions, and five amplifications of heterochromatin bands of rye chromosomes were identified. One amphidiploid contained a reciprocal translocation between wheat chromosome 4D and rye chromosome 1R. Non-reciprocal translocations between 2B and 3R, and between an unidentified wheat chromosome and 2R, were found independently in two amphidiploids. An additional plant had a translocation between wheat chromosomes 6B and 5A. All deletions involving rye chromosomes were noted in all 10 amphidiploids. Twelve of the 13 breakpoints in chromosomes involved in translocations and deletions occurred in heterochromatin. Amplification of heterochromatin bands on 2RL and 7RL chromosome arms also was observed in five plants. These results indicate a high degree of chromosome structural change induced by tissue culture. Therefore, tissue culture may be a useful tool in alien gene introgression and manipulation of heterochromatin in triticale improvement.Contribution No. 84-188-J, Kansas Agricultural Experiment Station, Kansas State University. Research was supported by the Science and Education Administration of the U.S. Department of Agriculture under Grant No. 59-2201-1-1-639-0 from Competitive Research Grants Office to R.G.S. 相似文献
18.
小麦-冰草附加系Ⅱ-21-2的细胞遗传学与分子标记分析 总被引:1,自引:0,他引:1
在本研究室获得的一套小麦-冰草附加系材料中,附加了冰草(1.4)重组P染色体的附加系Ⅱ-21-2出现了较高频率的多价体。对小麦-冰草附加系Ⅱ-21-2的10个不同株系花粉母细胞减数分裂进行观察与统计,结果表明,不同株系均存在低频率的单价体,染色体异常联会主要表现为出现六价体和四价体,其中株系1-7-3出现六价体频率较高,出现六价体的花粉母细胞为41%,而株系1-7-7有13%的花粉母细胞出现四价体。小麦SSR标记分析表明,不同株系存在小麦基因组或P基因组的多态性。小麦-冰草附加系Ⅱ-21-2染色体异常联会可能与附加的P染色体有关,而其分子水平的多态性和重组可能对于遗传改良具有潜在的意义。 相似文献
19.
黑麦碱基因(Sec–1)表达缺失的1RS/1BL易位系的鉴定 总被引:5,自引:0,他引:5
用改良的Giemsa C-带技术、DNA原位杂交和酸性聚丙烯酰胺凝胶电泳(A-PAGE)对来源于小麦品种绵阳11与不同黑麦自交系远缘杂交获得的高代株系(BC1F7)的染色体结构和醇溶蛋白进行了研究。结果发现,在鉴定的200个株系中,有45个株系经C-带和A-PAGE检测均一致地发现它们含有一对1RS /1BL易位染色体,而一个株系843-1-1,C-带鉴定、原位杂交结果均证明它含有一对1RS/1BL易位染色体,但A-PAGE醇溶蛋白图谱却不具有黑麦1RS染色体臂的黑麦碱特征带,而表达出既不同于黑麦碱又不同于亲本绵阳11的醇溶蛋白带型。这一结果表明,利用不同的黑麦亲本资源,可以获得黑麦碱基因Sec-1表达缺失的新的1RS/1BL易位系。这种新的1RS/1BL易位系缺失了影响小麦品质的黑麦碱蛋白,因此是进一步研究1RS/1BL 易位对小麦品质影响的珍贵材料。研究指出,在利用外源基因的植物育种中,外源种供体材料的遗传多样性是值得重视的基因资源。 相似文献