D^2型小麦细胞质雄性不育系及其保持系和恢复系线粒体DNA的比较研究

ｍｓＤ２－ＣＡ８０５７是新育成的具有粗厚山羊草（Ａｅ．ｃｒａｓａ,６ｘ）胞质的Ｄ２型小麦细胞质雄性不育系。采用ＲＦＬＰ和ＲＡＰＤ方法对该不育系及其具有普通小麦（Ｔ．ａｅｓｔｉｖｕｍ）胞质的保持系ＣＡ８０５７和恢复系保－７６９－２２－６的线粒体ＤＮＡ进行分析和比较,发现该不育系的线粒体ＤＮＡ组织结构明显不同于其保持系,也不同于其恢复系。Ｓｏｕｔｈｅｒｎ结果表明,该不育系线粒体基因组在ａｔｐＡ、ａｔｐ９、ｃｏｂ和ｃｏｘⅡ基因上或附近具有显著的组织结构差异。ＲＡＰＤ分析证实了这一点。相反,ＲＦＬＰ和ＲＡＰＤ结果都表明保持系与恢复系之间线粒体基因组结构非常相似。这支持了该不育系的胞质遗传特点来源于与普通小麦胞质差异较大的野生型胞质的事实。推测这种胞质差异与育性有关     

小麦胞质突变型雄性不育系85EA与其保持系线粒体DNA的比较研究

８５ＥＡ是通过电子束辐照获得的胞质突变型小麦不育要用ＲＦＬＰ和ＲＡＰＤ技术对８５ＥＡ及春保持系的线粒体ＤＮＡ进行了比较研究。ＲＦＬＰ分析表明８５ＥＡ线粒体基因组中ｃｏｘⅡ基因的位置结构与保持系发生了变化；ＲＡＰＤ分析中引物ＯＰＤ－１５扩增产物在不育系和保持系间有明显差异，不育系的扩增产物比保持系多１条分子量为０．６ｋｂ的特展览 要带，用Ｔ－ｅａｓｙ ｖｅｃｔｏｒ克隆该不育系特异条带并命名为ＯＰＤ－     

普通小麦三种细胞质雄性不育系线粒体DNA的比较研究

对细胞质分别来源于粘果山羊草（Ａｅ．ｋｏｔｓｃｈｙｉ）、偏凸山羊草（Ａｅ．ｖｅｎｔｒｉｃｏｓａ）、提莫菲维（Ｔ．ｔｉｍｏｐｈｅｅｖｉ）的３种普通小麦雄性不育系,其相应保持系和共有的一种恢复系的ｍｔＤＮＡ进行了ＲＦＬＰ比较分析。发现Ｋ型和Ｖ型不育系的ｍｔＤＮＡ在组织结构上不同于Ｔ型,说明Ｋ、Ｖ型不育系是有别于Ｔ型的两种新不育类型。Ｋ型、Ｖ型不育系的ｍｔＤＮＡ与保持系和恢复系显著不同,推测ｍｔＤＮＡ与小麦细胞质雄性不育性有关。实验同时发现Ｔ型不育系与其保持系的ｍｔＤＮＡ非常相似,对这种相似性的原因进行了讨论。     

一个恢复力受单基因控制的水稻CMS育性回复突变体

利用￣（６０）Ｃｏ－γ射线对具有印尼水田谷细胞质的籼稻细胞质雄性不育系Ⅱ－３２Ａ干种子进行诱变处理,获得了一育性回复突变体Ｔ２４。育性基因未纯合的突变体分离出可育株和完全不育株,比例为３∶１;其与Ⅱ－３２Ａ和珍汕９７Ａ测交,Ｆ１代分离出１∶１的可育株和不育株。育性稳定株系与Ⅱ－３２Ａ和珍汕９７Ａ杂交,Ｆ２分离成３∶１的可育株和不育株。表明其育性回复是由一对基因显性突变所致。这一突变体对不育系的育性恢复机制不同于明恢６３、２０９６４等恢复系,后者表现为两对显性恢复基因作用。未观察到Ｔ２４与亲本Ⅱ－３２Ａ除育性以外的其他性状的差异,因而两者构成育性恢复基因的近等基因系。本文还对不育系育性回复类型和Ｔ２４的理论意义与育种价值进行了讨论。     

叶绿体基因组的翻译产物与细胞质雄性不育性

本实验通过对叶绿体基因组翻译产物的分析,发现高粱3197 A不育系及其核代换系白马丁A和遗3 A不育系均比保持系(3197 B)多1个52,000道尔顿的变异多肽。而细胞质来源不同的粒息A不育系除52,000道尔顿多肽外还有1个特有的80,000道尔顿变异多肽。小麦T型不育系具有1个54,000道尔顿的变异多肽。甜菜不育系与保持系无差异。这说明某些作物的细胞质雄性不育性与叶绿体遗传系统有关。在高粱恢复系和F_1叶绿体蛋白质中发现三种特有的多肽。它们是由核基因编码的,这可能是恢复基因的产物。由于恢复基因的作用,在F_1恢复育性的同时其叶绿体变异多肽的合成也受到了强烈的抑制。这进一步证明了不育性与叶绿体的联系。     

水稻离体育性变异研究

对野败型不育系珍汕９７Ａ、保持系珍汕９７Ｂ、恢复系ＩＲ２４、ＩＲ２６、泰引１号、明恢６３、红莲型不育系红源Ａ、包台型不育系包源Ａ、光敏核不育系农垦５８ｓ、温敏核不育系Ｗ６１５４ｓ等１０个水稻材料的幼穗在不同的培养基上培养、再生植株及对其后代进行育性鉴定,探讨了体细胞无性系变异中雄性不育突变发生的机率以及影响离体筛选雄性不育变异体因素。因素表明：在５个材料（珍汕９７Ｂ、红源Ａ、包源Ａ、Ｗ６１５４ｓ和     

小麦D^2型与K型,V型,T型细胞质雄性不育系线粒体DNA的RAPD比较分析

采用ＲＡＰＤ方法比较新育成的小麦（ＴｒｉｔｉｃｕｍａｅｓｔｉｖｕｍＬ．）Ｄ２型不育系ｍｓＤ２ＣＡ８０５７与Ｋ型、Ｖ型和Ｔ型细胞质雄性不育系的线粒体ＤＮＡ（ｍｔＤＮＡ）。结果表明,ｍｓＤ２ＣＡ８０５７的ｍｔＤＮＡ不同于其它３种类型不育系,而其它类型不育系的ｍｔＤＮＡ彼此也各不相同。这一结果从分子水平上为鉴定该Ｄ２不育系的不育类型提供了证据。实验还发现在胞质来源相同而核背景不同的Ｔ型不育系间存在线粒体基因组多态性,这是关于小麦中Ｔ型不育系ｍｔＤＮＡ在常规回交转育过程中发生变异的直接证据。这种变异在很大程度上可能是受不同核背景影响的结果。     

3种小麦细胞质雄性不育系及其杂种线粒体DNA的RFLP分析

对细胞质分别来源于提莫菲维（Ｔ．ｔｉｍｏｔｈｅｅｖｉｉ）,粘果山羊草（Ａｅ．ｋｏｔｓｃｈｙｉ）,偏凸山羊草（Ａｅ．ｖｅｎｙｒｉｃｏｓａ）的３种普通小麦的雄性不育系,相应保持系和恢复系及其上的ｍｔＤＮＡ用１２个线粒体基因探针进行了ＲＦＬＰ分析,结果为：⑴Ｔ、Ｋ、Ｖ型不育系的ｍｔＤＮＡ在组织结构上存在显著差异;⑵Ｔ、Ｋ、Ｖ不育系的ｍｔＤＮＡ与共同的保持系间显著不同,失测ｍｔＤＮＡ与小麦ｃｍｓ有关;⑶在     

红莲型杂交稻(红莲2号)及其骨干亲本的RAPD分析与鉴定

利用RAPD技术,从248个随机寡核苷酸引物（10－mer）中筛出18个引物对红莲型杂交稻组合红莲2号及其亲本（T－07A、T－07B、YD6－05）,另6个红莲型胞质不育系的骨干恢复和汕优63及其亲本共14份水稻材料进行分析。共检测到173个多态性标记。聚类分析结果表明：不育系与保持系间因核背景相似,遗传差异很小;杂种（F1）的基因型更倾向于恢复系;恢复系与保持系间遗传距离的相对较大,但各恢复系之间的遗传距离较小。利用这些标记能有效地地区交组合中不育系,保持系、恢复系和杂种（F1）。     

水稻体细胞无性系R_1、R_2代中的雄性育性变异观察

通过水稻幼穗培养,１９９１－１９９２两年间,在５个品种（珍汕９７Ｂ、红源Ａ、包源Ａ、Ｗ６１５４ｓ,和南广占）中共获得了５０株雄性不育变异株,其中Ｒ_１代有４８株,Ｒ_２代有２株。在Ｒ１代,共获得５２６８株再生植株,雄性不育变异的平均频率为０．９１％（０．８３－１．０８％）;在Ｒ_２代（珍汕９７Ｂ）发生雄性不育变异的频率为２％。本文报道了多种花粉败育类型之间可以相互转变现象,此外不育和可育之间亦可以相互转变。对离体培养产生的雄性不育变异株用一批现有ＣＭＳ（Ｃｙｔｏｐｌａｓｍｉｃｍａｌｅｓｔｅｒｉｌｅ）不育系的典型保持系、恢复系进行测交,结果表明,Ｗ６１５４ｓ产生的雄性育性变异株仍保持核不育的特性;红源Ａ产生的雄性育性变异株有的可能是嵌合体,有的其败育花粉类型虽发生了变化,但其恢保关系并没有改变,有的则可能已转成类似ＷＡ型的不育材料;南广占产生的典败变异株,其恢保关系类似ＷＡ型,可能属核不育转成ＣＭＳ的首例发现。     

Testing cms-P-linked AFLPs for selection of rye hybrid components

Application of AFLPs linked to pollen fertility restoration and non-performing genes evaluated in the C394-F2 hybrid was studied using a set of male sterile lines in the sterilising Pampa cytoplasm, several restorers and maintainer lines and, finally, two inbred lines backcrossed into cms-P, cms-R, cms-S and cms-C cytoplasms each. The set of male sterile lines based on the Pampa cytoplasm exhibited gradual variation in their ability to restore pollen fertility (starting from low and closing with high) in crosses with three unrelated restorers. Variations in the AFLPs between the analysed materials were observed, however, no clustering of the lines according to their sterile and fertile phenotypes was observed. The same markers, when applied to the population restorer (cv. Walet) that formed the C394-F2 cross permitted identification of plants with genotypes that could be recognized as restorers.     

Linkage analysis of a fertility restoring mutant generated from CMS rice

 DNA polymorphism between a cytoplasmic male-sterile rice line II-32A, the male-fertile maintainer counterpart II-32B, a fertile revertant (T24), as well as two commercial indica restorers, was analyzed with randomly amplified polymorphic DNA (RAPD). A very low degree of polymorphism was found between the revertant T24 and II-32A compared with that of indica rice varieties. This result, together with agronomic and genetic evidence, suggests the revertant to be a product of a nuclear mutation. An analysis of polymorphism between II-32A and the revertant T24 with 510 RAPD decamer primers identified the co-segregating markers OPB07₆₄₀ and OPB18₁₀₀₀ to be linked to a sterile allele of the restoring locus in the revertant T24, at a distance of 5.3 cM. RAPD analysis of a mapping population of Tesanai2/CB with primer OPB07 revealed linkage of OPB07₆₄₀ with RG374 (10.8 cM) and RG394 (8.8 cM) on chromosome 1. Thus the restorer gene, designated Rf ₅, was tentatively localized between RG374 and RG394 on chromosome 1 and appears to be independent of other mapped restorer genes in rice. Received: 11 November 1997 / Accepted: 17 December 1997     

A comparative cytogenetic study of the rice (<Emphasis Type="Italic">Oryza sativa</Emphasis> L.) autotetraploid restorers and hybrids

We studied pollen fertility, seed set and cytogenetic characteristics of restorer lines and F1 hybrids of autotetraploid rice. T4002, T4063, T461A × T4002 and T461A × T4063 showed significantly higher pollen fertility and seed set than T4132 and T461A × T4132. Meiotic pairing configurations of T4002, T4063, T4132, T461A × T4002, T461A × T4063 and T461A × T4132 were 0.05 I + 19.96 II (9.89 rod + 10.07 ring) + 0.01 III + 2.00 IV, 0.11 I + 19.17 II (8.90 rod + 10.37 ring) + 0.09 III + 2.26 IV + 0.01 VI, 1.34 I + 9.46 II (4.50 rod + 4.96 ring) + 0.80 III + 6.02 IV + 0.09 VI + 0.09 VIII, 0.02 I + 14.36 II (6.44 rod + 7.91 ring) + 0.01 III + 4.80 IV + 0.01 VIII, 0.06 I + 17.67 II (11.01 rod + 6.67 ring) + 0.06 III + 3.10 IV + 0.01 VI and 1.11 I + 11.31 II (5.80 rod + 5.51 ring) + 0.41 III + 5.63 IV + 0.03 VI + 0.03 VIII, respectively. Configuration 16 II + 4 IV and 12 II + 6 IV occurred in the highest frequency among the autotetraploid restorers and hybrids. Meiotic chromosome behaviors were less abnormal in the tetraploids with high seed set than those with low seed set. The hybrids had fewer frequencies of bivalents, univalents, trivalents and multivalents than the restorers, but higher frequency of quatrivalents than the restorers at MI. The frequency of univalents at MI had the most impact on pollen fertility and seed set, i.e., pollen fertility decreased with the increase of univalents. The secondary impact factors were trivalents and multivalents, and bivalents and quatrivalents had no effect on pollen fertility and seed set. The correlative relationship between pollen fertility and cytogenetic behaviors could be utilized to improve seed set in autotetraploidy breeding.     

Marker-assisted identification of restorer gene(s) in iso-cytoplasmic restorer lines of WA cytoplasm in rice and assessment of their fertility restoration potential across environments

Iso-cytoplasmic restorers possess the same male sterile cytoplasm as the cytoplasmic male sterile (CMS) lines, thereby minimizing the potential cyto-nuclear conflict in the hybrids. Restoration of fertility of the wild abortive CMS is governed by two major genes namely, Rf3 and Rf4. Therefore, assessing the allelic status of these restorer genes in the iso-cytoplasmic restorers using molecular markers will not only help in estimating the efficiency of these genes either alone or in combination, in fertility restoration in the hybrids in different environments, but will also be useful in determining the efficacy of these markers. In the present study, the efficiency of molecular markers in identifying genotypes carrying restorer allele of the gene(s) Rf3 and Rf4, restoring male fertility of WA cytoplasm in rice was assessed in a set of 100 iso-cytoplasmic rice restorers using gene linked as well as candidate gene based markers. In order to validate the efficacy of markers in identifying the restorers, a sub-set of selected 25 iso-cytoplasmic rice restorers were crossed with four different cytoplasmic male sterile lines namely, IR 79156A, IR 58025A, Pusa 6A and RTN 12A, and the pollen and spikelet fertility of the F₁s were evaluated at three different locations. Marker analysis showed that Rf4 was the predominant fertility restorer gene in the iso-cytoplasmic restorers and Rf3 had a synergistic effect on fertility restoration. The efficiency of gene based markers, DRCG-RF4-14 and DRRM-RF3-10 for Rf4 (87%) and Rf3 (84%) genes was higher than respective gene-linked SSR markers RM6100 (80%) and RM3873 (82%). It is concluded that the gene based markers can be effectively used in identifying fertility restorer lines obviating the need for making crosses and evaluating the F₁s. Though gene based markers are more efficient, there is a need to identify functional polymorphisms which can provide 100% efficiency. Three iso-cytoplasmic restorers namely, PRR 300, PRR 363 and PRR 396 possessing both Rf4 and Rf3 genes and good fertility restoration have been identified which could be used further in hybrid rice breeding.     

Cytoplasmic male sterility of rice with boro II cytoplasm is caused by a cytotoxic peptide and is restored by two related PPR motif genes via distinct modes of mRNA silencing

Cytoplasmic male sterility (CMS) and nucleus-controlled fertility restoration are widespread plant reproductive features that provide useful tools to exploit heterosis in crops. However, the molecular mechanism underlying this kind of cytoplasmic-nuclear interaction remains unclear. Here, we show in rice (Oryza sativa) with Boro II cytoplasm that an abnormal mitochondrial open reading frame, orf79, is cotranscribed with a duplicated atp6 (B-atp6) gene and encodes a cytotoxic peptide. Expression of orf79 in CMS lines and transgenic rice plants caused gametophytic male sterility. Immunoblot analysis showed that the ORF79 protein accumulates specifically in microspores. Two fertility restorer genes, Rf1a and Rf1b, were identified at the classical locus Rf-1 as members of a multigene cluster that encode pentatricopeptide repeat proteins. RF1A and RF1B are both targeted to mitochondria and can restore male fertility by blocking ORF79 production via endonucleolytic cleavage (RF1A) or degradation (RF1B) of dicistronic B-atp6/orf79 mRNA. In the presence of both restorers, RF1A was epistatic over RF1B in the mRNA processing. We have also shown that RF1A plays an additional role in promoting the editing of atp6 mRNAs, independent of its cleavage function.     

Mitochondrial DNA rearrangements in Pennisetum associated with reversion from cytoplasmic male sterility to fertility

Endonuclease restriction fragment patterns of Pennisetum americanum L. mitochondrial DNAs (mtDNAs) from a cytoplasmic male-sterile (CMS-A1), fertile revertants and a normal fertile cytoplasm were variable, while chloroplast DNA from those lines lacked variation. Comparisons between mtDNAs of CMS-A1 (parental) and fertile revertant lines revealed the presence of a unique 4.7 kbp PstI fragment in the sterile line that was not detected in any of the revertant lines. A 9.7 kbp PstI fragment was found in all of the revertants, but not in the CMS-A1. Neither of those fragments was found in the normal cytoplasm mtDNA. Hybridization studies revealed two sets of multiple homologies: 1) the 4.7 kbp fragment had homology with a 10.9 kbp and a 13.6 kbp fragment; and 2) the 9.7 kbp fragment was homologous with the 13.6 kbp fragment. The presence of those two repeated mitochondrial sequences on the altered fragments suggests that they may be involved in the recombinational associated events with reversion from CMS to fertility in P. americanum.Florida Agricultural Experiment Station Journal Series No.7797.     

Nuclear-cytoplasmic interactions in restoration of male fertility in the ‘9E’ and A4 CMS-inducing cytoplasms of sorghum

 The genetics of male-fertility restoration in sorghum in the “9E” and A4 CMS-inducing cytoplasms, was studied by crossing a number of fertility restorer lines of A1 cytoplasm to CMS lines [9E]T×398 and [A4]T×398 and the line [9E]Milo-10, which was obtained by backcrossing Milo-10 to [9E]T×398. It was revealed that both A4 and “9E” cytoplasms are characterized by a sporophytic mode of restoration of male fertility. Depending on the nuclear background of the male parents, fertility restoration was controlled by one or two dominant genes. Fertility-restorer genes of one of the tester lines, KVV-114, were effective in [9E]T×398 but could not restore [9E]Milo-10. A fertile line obtained from the fertile hybrid [9E]T×398/KVV-112, with “9E” cytoplasm, also failed to restore [9E]Milo-10. In a number of hybrid combinations with both A4 and “9E” cytoplasms a novel and unusual phenomenon of gradual restoration of male fertility in subsequent backcross generations was observed. Pollen from the fertile revertants did not transmit fertility restoration in progeny from crosses with the original CMS line and was poorly transmitted in sib-crosses. The appearance of fertile revertants and the different reactions of different CMS lines with the same cytoplasm in test-crosses may be caused by the action of recessive nuclear genes of the recurrent male parents that were accumulated during backcrossing; these may induce changes in cytoplasmic genes controlling CMS. Received: 5 March 1998 / Accepted: 7 April 1998     

Genetic and cytological analyses of the male sterility mutation induced in a sorghum tissue culture with streptomycin

Treatment of sorghum callus cultures with 500–1000 mg/l streptomycin led to a high regeneration frequency of plants with complete or partial male sterility (MS), up to 100% of all green regenerants. The induced MS mutation (ms-str) was preserved in the F₁ and BC₁ progenies and was genetically unstable: many families produced semisterile and fertile revertants, whose progenies again contained semisterile and sterile mutants. The ms-str mutation was maintained through eight generations via selection and self-pollination of semisterile plants. The mutation was inherited as a recessive nuclear mutation in test crosses of sterile plants segregated in the progenies of fertile and semisterile revertants and was expressed only in single cases in a test cross for ms-str transfer through pollen of hybrids with restored male fertility. Recessive nuclear mutations determining a low plant height (dwarfness) and the lack of waxy bloom on the stem and leaves (bloomless) were found in male-sterile plants with the ms-str mutation. Cytological analysis of sterile plants reveal multiple abnormalities at various pollen development stages and in tapetal cells: cytomyxis, defects of chromosome conjugation, distorted cytokinesis in meiotic division II, a lack of tetrad separation, a defective formation of the microspore coat, generation of microspores with two to four nuclei, and the formation of micronuclei and large vacuoles in tapetal cells. A possible transfer of the induced cytoplasmic MS mutation into the nuclear genome and the causes of the high genetic instability are discussed.     

应用RFLP研究水稻基因突变的特性

选用覆盖整个水稻遗传图谱的１２９和１０６个ＤＮＡ探针,分别分析了灿稻品系ＩＲ５４、５４６０、５４６０Ｓ之间和粳稻品系农垦５８、农垦５８Ｓ及其育性回复突变系之间的ＲＥＬＰ。在ＩＲ５４／５４６０、５４６０／５４６０Ｓ和ＩＲ５４／５４６０Ｓ检测到ＲＦＬＰ的探数分别为４３、１４和３２。而且,５４６０／５４６０Ｓ的多态性探针均能在ＩＲ５４和５４６０之间检测到差异性,其中１１个（７８．６％）在５４６０Ｓ与ＩＲ     

空间搭载诱导水稻种子突变的分子标记多态性分析

以卫星空间搭载广东水稻品种特籼占13干种子,返地种植后经5代选择、培育,获得一批形态及育性变异的突变体及品系（种）,如株高变矮,稻穗变大,雄性不育等。为了探索空间诱变的本质,对选出的6个突变体及2个优良品系,选用了130个10－mer随机扩增多态性DNA（RAPD经物和17对扩增片段长度多态性（AFLP）引物组合,分别对其基因组DNA进行多态性位点扫描分析,两种方法的结果均显示：不同的突变体与原种DNA之间存在不同程度的多态性差异,且由两法得到的结果较接近,为6％－12％。此结果从分子水平上进一步证明了空间环境确实对植物种子存在诱变作用。