大白菜萝卜细胞质雄性不育系RC7的选育及其特性研究

利用甘蓝型油菜萝卜细胞质雄性不育材料RC97-1为不育源,采用种间杂交,将RC97-1的不育性导入大白菜,再通过连续回交转育和严格经济性状选择育成新的大白菜胞质雄性不育系RC7.RC7表现为:蜜腺正常,雌蕊功能健全,能吸引蜜蜂等昆虫正常采蜜传粉;在不同的生态区和播期条件下不育性稳定,不育株率和不育度均达100%,且自然结实性良好,配合力高;高抗霜霉病,抗病毒病和黑斑病;生长整齐,叶色正常,生育期85 d,株高58.6 cm,株幅45.3 cm,叶球纵径和横径分别为48.5和16.3 cm,球形指数2.98,单球质量3.6 kg左右.RC7的一代杂种金秋70和金秋90抗病性强,适应性广,优质、丰产、稳产.因此,RC7是优良的大白菜萝卜细胞质雄性不育系,具有较高的利用价值.     

大白菜温敏雄性不育系育性转化相关基因的cDNA-AFLP分析

为了分析大白菜温敏雄性不育系TsCMS7311育性转化的相关基因,先对现蕾的TsCMS7311低温处理,然后不同时间连续提取幼蕾(≤1.0 mm,包括顶端分生组织)的RNA,进行cDNA-AFLP表达差异分析.结果表明,用256对引物扩增出连续性差异片段212条,按照时间顺序,划分为4种差异带类型,即无→有→无"、有→无→有"、无→有"、有→无".在175条低温诱导产生的差异带型中,无→有→无"类型165条,占总差异带的78%;无→有"类型10条,占总差异带的5%.对部分差异片段进行回收、克隆、测序,共得到100条序列,其大小为100~700 bp.经BLAST序列比对分析发现,温度调控的育性转化与新陈代谢、能量、防御、细胞构建、蛋白质合成及运输、转录翻译、细胞通信及信号转导等相关蛋白有关.     

大白菜细胞质雄性不育系和其保持系的RAPD分析

利用RAPD技术对大白菜细胞质雄性不育系CMS341-7和其保持系3411-7的基因组DNA进行了比较分析,共使用了269个随机引物,其中有163个引物在两系之间都得到了扩增产物,79个引物扩增结果在两系之间表现出了遗传多态性。找到了不育系和保持系的特异扩增条带CMSOPL01670和MOPB04600。并对这些特异片段的来源及其在细胞质雄性不育中的作用进行了讨论。     

叶用芥菜细胞质雄性不育相关基因orf 220的分子特性

采用榨菜细胞质雄性系为不育源,通过变种间杂交和回交的方法,转育叶用芥菜细胞质雄性不育种质。根据Brassica nap型细胞质雄性不育相关基因off222设计兼并引物,利用特异引物PCR方法,分别在不育源、F1、BC2以及BC3世代中扩增出一条600～700bp大小的特异条带,而在叶用芥菜保持系中无此条带,具细胞质基因遗传特性。进一步序列分析表明,此特异条带大小为663bp,具有起始密码子和终止密码子,编码220个氨基酸,定名为off220。同时,off220推导的氨基酸序列存在两个跨膜区,氨基端与Oenothera berteriana中的COXⅢ(线粒体细胞色素氧化酶复合体亚基)、萝卜中的ATP8(线粒体ATP酶复合体亚基)以及向日葵中的ORFB(ATP酶复合体α亚基相关)蛋白氨基端高度同源。RT-PCR方法分析表明,off220基因的表达为组成性表达,无器官特异性。     

大白菜新型细胞质雄性不育系6w-9605A的育性鉴定和花药败育的细胞学观察

采用石蜡切片技术,研究了大白菜(Brassica campestris L.ssp.pekinensis)细胞质雄性不育系6w-9605A及其保持系6w-9605B的花药发育过程的细胞形态学特征,确定不育系花药败育时期及方式,并对不育系6w-9605A进行花器官观察和育性鉴定.结果表明:保持系6w-9605B花药发育正常;不育系6w-9605A花药发育受阻于孢原分化时期,占总败育花药的66.7％,不形成花粉囊和花粉粒,属于无花粉囊型败育;另外33.3％的败育花药可形成花粉囊,小孢子均受阻于单核靠边期或者二胞期,败育特点为绒毡层细胞异常肥大,挤压小孢子,导致小孢子和绒毡层解体;6w-9605A的不育性稳定、彻底,不育株率和不育度均为100％.     

利用RNA指纹技术分析大白菜胞质雄性不育相关基因的差异表达

采用改进的RNA指纹技术(RAP-PCR)对两套大白菜胞质雄性不育材料及其杂种F1花蕾的总RNA进行了分析, 通过对186条随机引物的筛选, 获得4个重复性较好的差异片段S47-412, S93-622, S176-343, S199-904, 并对其克隆、测序。根据各差异条带的测序结果合成长引物进行验证, S47, S93所对应的差异消失, 而S176, S199长引物验证的结果与RAP-PCR相似, 序列分析表明: S176-343, S199-904两差异片段均和油菜Polima不育胞质线粒体基因组orf224/atp6位点有着极高的同源性, 两差异片段序列部分重叠, 这说明两差异片段可能和大白菜胞质雄性不育有很高的相关性。     

大白菜雄性不育系的组织培养和快速繁殖技术研究

以大白菜雄性不育系Bm5-3为材料,研究其组培快繁技术的结果表明:腋芽以组培快繁技术保存、扩繁大白菜雄性不育系是可行的。适合其腋芽增殖的培养基是MS+2mg·L-16-BA+0.1mg·L-1NAA,增殖系数为4.58,一般通过4￣5次继代即可脱分化;适合其生根的培养基是B5+0.1mg·L-1IBA,平均每株生根数为8.5条,平均根长8.18cm,这一培养基上生长的根较粗壮。具有4~5片叶子且根系发达的试管苗,移栽成活率高达95%。田间栽培的试管苗与供体植株的外部形态与生理特性完全一致。     

大白菜胞质雄性不育系RC7及其保持系的细胞学和蕾期基因表达差异分析

以大白菜雄性不育材料RC7及其保持系B7为材料,通过对两材料花药发育过程进行细胞学观察,并利用cDNA-AFLP技术分析两材料花蕾的基因表达差异,以明确RC7发生雄性败育的时期和方式,为大白菜CMS的分子机理研究提供依据。结果显示:(1)细胞学观察发现,大白菜雄性不育材料RC7及其保持系B7的小孢子母细胞减数分裂属同时型,小孢子在四分体中的排列属四面体型,保持系B7花药的绒毡层属于腺质型;不育材料RC7在四分体时期绒毡层细胞内出现大的液泡,呈现败育征兆,单核期绒毡层解体,中层退化,小孢子核开始解体、败育,属于单核花粉败育型。(2)对两材料蕾期基因的cDNA-AFLP差显比较分析表明,共获得了23条阳性差异片段,其中在不育系RC7花蕾中特异表达的有8条,在保持系B7花蕾中特异表达有10条,两系中共有条带5条。(3)对不育系中特异表达的8条谱带进行Blast搜索发现,H1与拟南芥光合反应蛋白基因有较高的一致性,H26与拟南芥钙调磷酸酶类磷酸酯酶家族蛋白质的部分序列存在90%的一致性,属于细胞信号转导基因;对来自保持系的10条谱带的差异片段功能以及一致性进行比对分类发现,它们包括糖代谢基因、蛋白质的合成与运输基因、乙烯诱导基因、电子传递和能量途径基因、未知或假定蛋白等。研究表明,大白菜雄性不育材料RC7可能是由于绒毡层细胞液泡化和径向肥大,小孢子受挤压后破裂降解,不能形成正常的成熟花粉粒而败育;乙烯诱导基因(H29)在保持系中特异表达,在不育系中沉默,表明不育系中缺乏乙烯相关基因。     

大白菜细胞质雄性不育系RAPD特异扩增片段的克隆及其序列分析

利用RAPD技术从大白菜细胞质雄性不育系CMS3411-7的DNA中得到1个特异扩增片段CMSO-PL01670,进一步以该片段为探针进行Dot和Southern杂交证实了该片段为不育系所特有。回收该特异扩增片段并将其克隆到pGEM-T Easy载体上进行序列测定。测序结果表明该片段全长673bp,其碱基组成为A T=67.16％。通过与GenBank EMBL DDBJ PDB中的455 972个序列进行比较,同源性均小于30％,表明该片段为一新发现序列。并且该序列的 4 - 216的区域内含有1个可编码70个氨基酸的开放阅读框架。上述结果为今后从分子水平进一步研究大白菜细胞质雄性不育打下了坚实的基础。     

大白菜细胞质雄性不育保持系3411-7--RAPD特异扩增片段的克隆测序

利用RAPD技术从大白菜细胞质雄性不育保持系3411-7的DNA中得到一个特异扩增片段MOPB04600。回收该特异扩增片段并将其克隆到pGEM-TEasy载体上进行序列测定。结果表明该片段全长600bp,其碱基组成为A+T=72.33%。通过与GenBank+EMBL+DDBJ+PDB中的455,972个序列进行同源性比较,同源性均小于30%,表明该片段为一新发现的序列。并对该特异片段的来源及其可能的作用进行探讨。     

大白菜细胞质雄性不育的分子生物学研究

细胞质雄性不育(cytoplasmic male sterility,CMS)是作物杂种优势利用的一 条重要途径。对其机制的研究不仅具有重要的理论意义,而且具有重要的应用价值。对大白菜而言,利用CMS最关键的环节是要育成不育系和其相应的保持系。利用不育系和其它材料杂交产生F1代种子;用不育系和保持系杂交来繁殖不育系;保持系自交繁殖种子。但采用常规的方法来选 育不育系和其相应的保持系周期长、见效慢,远不能满足生产发展的需要。现代生物技术为创造新的不育系和保持系提供了便利。本论文对大白菜细胞质雄性不育的分子机理和 RAPD分析的有关问题进行了研究。     

三分体形成是大白菜2n雄配子发生的主要途径

用能自然产生２ｎ配子的二倍体大白菜ＢＰ０５８为材料,研究了２ｎ雄配子发生的细胞学机制。结果表明,大白菜２ｎ雄配子的形成主要是由于减数分裂过程中,中期Ⅱ两个纺锤体的定向发生改变所致,即由正常的相互垂直定向改变为八字形和平行形定向。     

大白菜部分形态性状的QTL定位与分析

应用352个标记位点的大白菜AFLP和RAPD图谱和一套栽培品种间杂交获得的重组自交系群体,采用复合区间作图的方法对大白菜9个形态性状进行QTL定位及遗传效应研究。在14个连锁群上检测到50个QTL:其中控制株型的QTL有5个;控制株高的QTL有6个;控制开展度的QTL有5个;控制最大叶长的QTL有7个;控制最大叶宽的QTL有4个;控制叶形指数的QTL有6个;控制中肋长的QTL有7个;控制中肋宽的QTL有4个;控制抽苔的QTL有6个。另外,估算了单个QTL的遗传贡献率和加性效应。这将为大白菜品种改良中形态性状的分子标记辅助选择提供理论依据。     

不结球白菜种质资源形态性状多样性分析

分析了125份不结球白菜的形态多样性.结果表明,我国不结球白菜具有丰富的形态多样性,以江苏的平均多样指数最高,达0.972,性状中以叶柄长的变异系数最大,达59.77%.通过多变量的主成分分析,第一主成分和第二主成分代表了不结球白菜形态多样性的48.4%.通过系统聚类,把125份不结球白菜种质资源聚成6类,普通白菜不同程度地分别与塌菜、菜心、分蘖菜和薹菜聚在一起,说明普通白菜与其它种类间存在一定的亲缘关系.     

Cloning and Characterization of the Microspore Development-Related Gene BcMF2 in Chinese Cabbage Pak-Choi (Brassica campestris L. ssp. chinensis Makino)

For the sake of providing some important information relevant to the study of the molecular mechanism of genic male sterility in plants, gene differential expression in flower buds at different developmental stages, as well as in rosette leaves, florescence leaves, and scapes was analyzed using cDNA amplified fragment length polymorphism (cDNA-AFLP) in the genic male sterile A and fertile B line of Chinese cabbage pak-choi. Following amplification of 125 pairs of primer combinations, 11 differential fragments were obtained, of which eight were from the B line and the other three were from the A line. Of 11 differential fragments, four were verified by Northern hybridization that were expressed preferentially in fertile flower buds. Results of GenBank BLAST showed that one fragment was with unknown function,whereas the other fragments have strong nucleotide sequence similarities with the polygalacturonase (PG)gene, the pectinesterase (PE) gene, and the polygalacturonase inhibitory protein (PGIP4) gene. Only fulllength cDNA from the differential fragment BcMF-A18T16-1 was amplified by rapid amplification of cDNA ends (RACE) and Northern analysis showed that this fragment was expressed only in medium and largesized flower buds of the B line. The full-length cDNA, designated as BcMF2 (Brassica campestris Male Fertile 2), was 1 485 bp long and was composed of a 1 263-bp open reading frame, which had 83% nucleotide similarity to a PG gene from Arabidopsis encoding polygalacturonase. Analysis of the basic structure of the protein revealed that it had one polygalacturonase active site (RVTCGPGHGLSVGS) at 256th site of amino acids and was classified as being a member of family 28 of the glycosyl hydrolases. The role of the BcMF2 gene on microspore development is discussed in the present paper.     

Cloning and Characterization of the Microspore Development-Related Gene BcMF2 in Chinese Cabbage Pak-Choi （Brassica campestris L. ssp. chinensis Makino）

For the sake of providing some important information relevant to the study of the molecular mechanism of genic male sterility in plants, gene differential expression in flower buds at different developmental stages, as well as in rosette leaves, florescence leaves, and scapes was analyzed using cDNA amplified fragment length polymorphism (cDNA-AFLP) in the genic male sterile A and fertile B line of Chinese cabbage pak-choi. Following amplification of 125 pairs of primer combinations, 11 differential fragments were obtained, of which eight were from the B line and the other three were from the A line. Of 11 differential fragments, four were verified by Northern hybridization that were expressed preferentially in fertile flower buds. Results of GenBank BLAST showed that one fragment was with unknown function, whereas the other fragments have strong nucleotide sequence similarities with the polygalacturonase (PG) gene, the pectinesterase (PE) gene, and the polygalacturonase inhibitory protein (PGIP4) gene. Only fulllength cDNA from the differential fragment BcMF-A 18T 16-1 was amplified by rapid amplification of cDNA ends (RACE) and Northern analysis showed that this fragment was expressed only in medium and largesized flower buds of the B line. The full-length cDNA, designated as BcMF2 (Brassica campestris Male Fertile 2), was 1 485 bp long and was composed ofa 1 263-bp open reading frame, which had 83% nucleotide similarity to a PG gene from Arabidopsis encoding polygalacturonase. Analysis of the basic structure of the protein revealed that it had one polygalacturonase active site (RVTCGPGHGLSVGS) at 256th site of amino acids and was classified as being a member of family 28 of the glycosyl hydrolases. The role of the BcMF2gene on microspore development is discussed in the present paper.     

Agrobacterium-mediated transformation of cotyledonary explants of Chinese cabbage (Brassica campestris L. ssp. pekinensis)

 A procedure for producing transgenic Chinese cabbage plants by inoculating cotyledonary explants with Agrobacterium tumefaciens strain EHA101 carrying a binary vector pIG121Hm, which contains kanamycin-resistance and hygromycin-resistance genes and the GUS reporter gene, is described. Infection was most effective (highest infection frequency) when explants were infected with Agrobacterium for 15 min and co-cultivated for 3 days in co-cultivation medium at pH 5.2 supplemented with 10 mg/l acetosyringone. Transgenic plants of all three cultivars used were obtained with frequencies of 1.6–2.7% when the explants were regenerated in shoot regeneration medium solidified with 1.6% agar. A histochemical GUS assay and PCR and Southern blot analyses confirmed that transformation had occurred. Genetic analysis of T1 progeny showed that the transgenes were inherited in a Mendelian fashion. Received: 15 December 1998 / Revision received: 2 July 1999 · Accepted: 8 July 1999