Differential Expression Analysis of Genie Male Sterility A/B Lines in Chinese Cabbage-Pak-Choi (Brassica campestris ssp. chinensis Makino)

To determine differential expression of genie male sterility A/B lines in Chinese cabbage-pak-choi (Brassica campestris ssp. chinensis Makino var. communis Tsen et Lee), we used the RNA fingerprinting technique, cDNA-AFLP analysis, in different developmental stages and different tissues. While no obvious differential expressions were observed in rosette leaves, florescence leaves, and scapes, some differential expressions were found in alabstrums of A/B lines and among leaves, scapes and alabstrums. We analyzed the al-abstrums collected in different developmental stages with 10 primer combinations. We got a unique band between middle size alabstrums and large alabstrums in B line in one of the ten pair primers, and in another one pair, one band reflecting a higher gene-expression level in A line than that in B line was obtained. No unique bands were found with the other primer combinations. The bands reflecting different gene-expression level were confirmed by Northern hybridization. The results indicated that cDNA-AFLP was a suitable tool for studying differential expression of genie male sterility in plants. SDS-polyacrylamide gel electrophoresis patterns of soluble proteins further verified the difference in A/B lines.

Identifying Cytoplasmic Male Sterile Types of Chinese Cabbage(Brassica campestris L.)by Molecular Markers

Different sterile cytoplasm types of nine cabbage cytoplasmic male sterile materials were identified by molecular marker in the study, in order to better use molecular marker to conduct the assisted breeding in the future. Genomic DNA was isolated from Chinese cabbage by CTAB method. The design of two pairs of specific primers was performed on conserved flanking region of orf138 gene in the GenBank. PCR was performed with genomic DNA of the nine Chinese cabbage materials. The bands were sequenced. The homologous comparison was conducted in NCBI, and finally, the type of sterile cytoplasm was determined. The results showed that the bands were amplified only in four Chinese cabbage male sterile materials with two pairs of specific primers PUPIl and PIII/PIV, while the other five materials did not obtain the relative bands. The result was consistent with the field sterility identification. And then four molecular markers of Chinese cabbage Ogura cytoplasmic male sterility （CMS） were obtained. After conducting a homologous comparative analysis with BLAST in GenBank, it was found that the homologous degree was 100% in specific segments of tbe tbree sterility materials （L1-CI, L3-CI and L3- F1 ） and Ogu orf138 gene （GenBank accession No. ： HQ149728） of the reported broccoli Ogu CMS. The homologous degree of L1-F1 was 99% with a variation point. The type of cytoplasmic male sterility of the other five materials needed further research. Four materials of the nine were identified as the radish cytoplasmic male sterility materials and four molecular markers were obtained.

大白菜(Brassica pekinensis L.)对镉富集基因型差异的研究

研究了15种大白菜基因型对镉(Cd)富集的基因型差异,以期筛选出低积累Cd的白菜基因型.盆栽试验结果表明,不同白菜基因型的Cd含量、富集系数(BFs)和转运系数(TFs)差异显著(P<0.05).丰源新3号、现代夏秋和春秋六轮的Cd积累量均小于0.50mg/kg,其富集系数和转运系数都小于1.0,具有一定低积累Cd的潜力.大田试验的结果表明丰源新3号的Cd含量小于0.50mg/kg,富集系数和转运系数均小于1.0,表明其为排斥Cd的白菜基因型.现代夏秋和春秋六轮的富集系数和转运系数均小于1.0,但其地上部Cd含量均高于0.50mg/kg,不属于Cd低积累白菜.值得注意的.北京小杂56在盆栽和大田中的Cd含量、富集系数和转运系数均大于1.0,可用于植物修复污染土壤.

不结球白菜BcCHC1蛋白参与调控TuMV侵染的初步研究

【目的】为增强不结球白菜对芜菁花叶病素养(TuMV)的抗性,研究探讨了不结球白菜中BcCHC1蛋白与TuMV之间的相互作用机制。【方法】首先从不结球白菜中鉴定出重链网格蛋白(CHC)基因家族的成员BcCHCs,随后克隆了1个代表性的CHC1基因,并对其进行了亚细胞定位分析。通过双分子荧光互补实验(BiFC)筛选出与BcCHC1蛋白相互作用的TuMV蛋白,并利用病毒诱导的基因沉默技术(VIGS)来沉默BcCHC1基因,以评估其功能。【结果】(1)成功克隆了不结球白菜的BcCHC1基因,该基因的编码序列长5124碱基对,编码1708个氨基酸。(2)在TuMV感染不结球白菜30 d后,实时荧光定量PCR分析显示,感染TuMV的不结球白菜中BcCHC1基因的表达量显著降低。(3)亚细胞定位研究表明,BcCHC1蛋白主要定位于烟草表皮细胞的细胞膜和细胞核。(4)BiFC实验进一步证实,BcCHC1蛋白能够与TuMV的CI和6K2蛋白发生相互作用,其中与CI的互作主要发生在细胞核内,而与6K2的互作则主要位于细胞膜。(5)通过对BcCHC1基因沉默株系的观察发现,沉默BcCHC1基因会导致植株死亡。【结论】BcCHC1蛋白通过与TuMV的CI和6K2蛋白相互作用,影响网格蛋白依赖的内吞作用途径及病毒复制,从而调控TuMV对不结球白菜的侵染。然而,BcCHC1基因调控TuMV侵染不结球白菜的具体机制仍需进一步研究。

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 full-length 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 large-sized 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.

利用cDNA-AFLP技术分析白菜核雄性不育两用系的表达差异

利用cDNA AFLP技术 ,对白菜核雄性不育两用系可育株群和不育株群分析显示 :花蕾之间基因表达存在差异 ;莲座期叶片之间、开花期叶片之间和花茎之间基因表达无差异 ;叶片、花茎和花蕾之间基因表达存在差异。对开花期的小蕾、中蕾和大蕾分析显示 :10对引物中 ,1对在可育株中蕾和大蕾中扩增出 1条特异带 ,另 1对扩增出 1条在可育株中蕾中表达丰度高于不育株中蕾的条带 ,其余 8对未发现差异条带。对上述表达丰度有差异的基因进行Northern验证 ,结果与之一致 ,表明cDNA AFLP技术可以用于植物雄性不育基因表达差异的研究。

不结球白菜(Brassi cacampestris ssp.chinensis Makino)种质资源SRAP遗传分化分析

利用SRAP分子标记分析了国内外64份不结球白菜种质资源的DNA遗传多样性和遗传分化。21对引物组合共检测出215个位点,其中112个为多态性位点,多态性比率达52.09%,平均每对引物组合产生10.24个位点和5.33个多态性位点。不结球白菜各类型中普通白菜的Nei’s基因多样性指数(0.1410)和遗传丰富度[(190)88.37%]最高;各生态区域中江淮流域不结球白菜的Nei’s基因多样性指数(0.1451)和遗传丰富度[(185)86.05%]最高;国内的Nei’s基因多样性指数(0.1293)和遗传丰富度[(188)87.44%]分别高于国外。遗传变异估算表明,不结球白菜遗传分化系数58.22%,大部分变异存在于种群间;基因流为0.4031,说明群体间基因流动较少,遗传分化程度较高。以遗传相似系数0.872为截值,可把不结球球白菜分为Ⅵ个类群。

菜薹花芽分化及BrcuFLC基因的克隆与表达

通过制作石蜡切片研究了菜薹[Brassi cacampestris L.ssp.chinensis （L.） Makinovar.utilis Tsen et Lee]早熟品种‘油青四九’和晚熟品种‘油青甜菜心80天’的花芽分化过程，结果表明，当展开2-3片真叶时花芽分化开始启动。用已报道的拟南芥Flowering locus C（FLC）基因和FRIGIDA（FRI）基因的保守区域设计引物，通过RT-PCR的方法从两个菜薹品种中均克隆得到了两个决定开花的关键基因，并命名为BrcuFLC（GenBank登录号为EF138603）和BrcuFRI（GenBank登录号为EU700362）。半定量式RT-PCR表达分析表明，BrcuFLC基因在早、晚熟菜薹品种的不同发育时期表达存在差异，表达量随真叶数增加而逐步减少，但在晚熟品种中BrcuFLC表达量降低幅度小；BrcuFRI则在早、晚熟品种的所有阶段表达都较低。BrcuFLC在菜薹不同部位表达的情况不同，在茎、叶中的表达强，花次之，根中表达较弱；而Brcu-FRI在早、晚熟品种根中的表达量明显高于其它3个部位。

白菜核雄性不育两用系AFLP扩增特异片段的克隆及序列分析

利用AFLP技术从白菜核不育两用系"矮脚黄"可育系DNA中得到一个特异扩增片段MF-14.Southern杂交结果证实不育系也存在该片段的同源序列;回收该特异扩增片段并将其克隆到pGEM-TEasy载体进行序列测定.测序结果表明,该片段全长289bp,其碱基组成为A+T=46.02%.与白菜RAPD特异片段S107及其他育性相关基因核苷酸序列比较,同源性均低于50%.表明该片段为一新的序列.

白菜抽薹性状相关基因的cDNA-AFLP分析

先期抽薹严重制约着我国春大白菜及高原或高海拔地区的春夏白菜栽培,给生产造成重大损失,因而研究白菜作物低温春化途径抽薹和开花的相关基因对白菜育种具有重要意义。文章选取极早抽薹株系DH-54和极晚抽薹株系DH-43为材料,利用256对引物组合进行cDNA-AFLP分析,筛选到与抽薹开花相关的差异表达的转录衍生片段(Transcript-derived fragment,TDF)191条,对其中82个TDF进行克隆测序。结果表明:52个TDF与NCBI或TIGR已有序列同源,功能涉及代谢、胁迫及逆境应答、信号转导、转录调控等等;22个TDF在NCBI或TIGR找到同源序列,但功能未知;有8个TDF在NCBI或TIGR找不到同源序列,可能是一些新基因。

白菜春化相关基因BcFLC的克隆及表达研究

运用同源基因克隆法从‘上海青’白菜(Brassica campestris ssp.chinensis var.communis‘Shanghai Qing’)和‘四九’菜薹(var.parachinensis‘Sijiu’)叶片中分离到FLC的同源基因BcFLC的编码序列、启动子以及内含子1序列;序列比对发现,二者编码的核苷酸序列几乎完全一致,而且启动子及内含子1序列也无实质性差异;对‘上海青’进行人工低温春化处理,BcFLC-1基因在‘上海青’茎尖的表达随着低温处理时间的延长逐渐减弱,低温处理20 d时BcFLC-1基因的表达已经非常弱,低温处理30 d时,表达已检测不到,花芽分化石蜡切片也表明,低温处理20 d,茎尖已开始向生殖状态过渡。BcFLC-2基因在‘四九’菜薹未现蕾之前的叶片中有强表达,而现蕾之后叶片中则检测不到。

AFLP分子标记应用于白菜品种鉴定

采用AFLP技术,用混合的模板DNA从数对引物中筛选出6对带型分布均匀、多态性丰富且分辨能力强的引物,对市场上经营的两份大白菜杂交种样品586和587所扩增出的AFLP指纹图谱进行分析,根据数据分析得到了两份大白菜样品与标准样品之间的欧氏距离系数。6对引物对两份大白菜样品和标准样品扩增所得到的指纹图谱分析的结果表明,587与标准样品存在显著的差异,其中多态性位点占总扩增位点的31.7%,欧氏距离系数为3.87,样品587与标准样品不是同一个品种;而样品586与标准样品之间欧氏距离系数近于0,而据此得知此样品与标准样品之间没有明显的差异,判断为同一个品种。本研究采用AFLP技术很好地鉴别了两份样品的不同。这对应用AFLP技术鉴定大白菜品种的真伪,保护品种繁育者、生产者和种子使用者的利益提供了有效技术体系的依据。

不结球白菜同源四倍体Pol CMS及其保持系花药发育的解剖学研究

以秋水仙素人工诱变获得的不结球白菜同源四倍体Pol CMS及其保持系为材料，采用石蜡切片法研究其花药发育过程。结果显示：四倍体Pol CMS与保持系花药发育差异明显，不育系花药发育受阻于孢原细胞分化期，不形成药室，属无花粉囊型。极少数温敏型花药能产生1～2个花粉囊，但四分体时期绒毡层提早退化，导致成熟小孢子数目减少。四倍体保持系花药发育过程与二倍体基本一致，同一时期的可育小孢子四倍体比二倍体大，二倍体花粉粒都为3个萌发孔，而四倍体多为4个萌发孔。四倍体保持系同一花粉囊中花粉粒发育有不同步现象，花粉粒败育频率比二倍体高。研究表明，不结球白菜同源四倍体Pol CMS比其二倍体Pol CMS不育更彻底，更具廊用性。

白菜离体春化相关基因表达的cDNA-AFLP分析

借助cDNA-AFLP技术分离到15个与白菜离体春化反应相关的表达序列标签(EST)。Blast结果表明:低温春化处理抑制性表达的12个EST,多与异化作用相关基因同源性较高;春化诱导表达的3个EST,分别与编码核糖体蛋白的亚基(或与自主开花途径相关的FAC基因连锁的因子),ATPase的亚基,小G-蛋白亚基的基因同源性较高。

大白菜干烧心病性状的QTL定位和分析

在含有105个标记位点的大白菜AFLP连锁图谱上,利用MAPQTL4.0软件采用区间作图方法对控制大白菜干烧心病数量性状基因位点进行QTL定位和遗传效应分析。利用离体叶片扦插方法进行干烧心病的苗期鉴定,共检测到4个与抗干烧心病有关的QTL位点,分布在4个连锁群上。cal-1和cal-2表现为增效加性效应,cal-3和cal-4表现为减效加性效应。4个QTL解释的遗传变异范围在11.0%￣58.9%之间,其中cal-4最大,cal-2次之,而cal-1最小。这为大白菜抗干烧心病分子标记辅助选择提供了依据。

不同倍性不结球白菜Pol CMS及保持系生理生化特性比较

对二、四倍体不结球白菜Pol CMS及其保持系花蕾和薹叶进行生理生化特性比较分析,结果表明:不育系花蕾中可溶性蛋白、可溶性糖、脯氨酸含量均显著低于保持系,且各指标在不育系中四倍体低于二倍体,而在保持系中则四倍体高于二倍体;不育系MDA含量,POD、SOD、CAT活性均高于保持系,不育系中四倍体均高于二倍体,而保持系中四倍体均低于二倍体;薹叶中MDA含量,POD、SOD、CAT活性均为不育系高于保持系,不育系中四倍体高于二倍体;POD、EST同工酶显示不育系与保持系间均具特异酶带,但不同倍性间并无差异。

白菜转录因子BcBHLHogu的克隆及其特征分析

【目的】探明白菜'矮脚黄'OguCMS核质互作的机制。【方法】采用cDNA-AFLP技术分析白菜'矮脚黄'OguCMS及其保持系花蕾基因的表达差异,获得一个在保持系早期花蕾不表达但在OguCMS早、中、晚花蕾中稳定表达的差异片段。利用RACE技术获得其cDNA全长,命名为BcBHLHogu(GenBank登录号:EF127860)。【结果】该基因编码122个氨基酸,具有basic helix-loop-helix(bHLH)结构域;进化分析表明,BcBHLHogu与拟南芥AtBHLH060同源性最高,是冗余基因AtBHLHs060/048的直系同源基因,其功能与BEEs1/2/3(3个油菜素内酯信号的早期应答冗余基因)相似。【结论】BcBHLHogu是白菜bHLH转录因子家族的一个新成员,涉及到花器官发育信号事件,其功能与油菜素内酯应答有关。

不结球白菜BcLRK01基因对芜菁花叶病毒及胁迫诱导的响应

通过cDNA-AFLP技术,从芜菁花叶病毒(TuMV)侵染的不结球白菜幼叶中分离到一条差异表达的基因片段,克隆获得其cDNA全长为2 124bp,编码707个氨基酸的富亮氨酸重复类受体激酶,命名为BcLRK01。利用实时定量PCR研究了该基因在TuMV侵染及高盐、冷胁迫、水杨酸(SA)、茉莉酸(JA)、乙烯(ET)等处理下的表达情况,结果显示,TuMV侵染、高盐、冷胁迫、SA、JA和ET等均能诱导BcLRK01不同程度的表达,说明该基因可能是不结球白菜病毒病的病程相关基因,同时也参与高盐和冷胁迫以及SA、JA、ET等的信号途径。

菜心cDNA-AFLP分析体系的优化与建立

以菜心的顶端分生组织为试材,对影响菜心cDNA-AFLP体系的关键因子进行了探讨,以期建立适于菜心转录组差异表达的cDNA-AFLP分析体系。结果表明:Trizol法适用于菜心总RNA提取;SMART双链cDNA合成法效率较高,其中第二链cDNA合成的最佳循环数为24个;Taq I/Ase I分步各酶切3 h可使双链cDNA酶切完全;预扩增体系以模板稀释20倍,27个循环扩增效果较好,退火温度对扩增结果影响不大,但Mg2+对PCR扩增影响较大,经比较加入2.5μL Mg2+(25 mmoL/L)的预扩及选扩电泳的效果均最佳;预扩产物稀释20倍用于选择性扩增,其PAGE电泳可以获得丰富且重复性好的带型。cDNA-AFLP分析体系的优化与建立为菜心抽薹开花分子机理进一步研究奠定了基础。

大白菜快速碱化因子BrRALF1的克隆与特征分析

利用cDNA-AFLP技术分析大白菜核雄性不育"两用系"AB02可育株(msms)和不育株(Msms)花蕾的基因表达谱,在可育株混合花蕾cDNA中扩增出1条特异表达条带TDF-3,通过RACE和RT-PCR技术克隆了该基因的cDNA全长序列。序列分析表明,该基因编码大白菜快速碱化因子,被命名为BrRALF1;BrRALF1全长cDNA序列为551bp,编码1个包含79个氨基酸残基的前体蛋白;前体蛋白N末端1～28位为信号肽,成熟蛋白含有保守的YIXY结构域、YXRGC结构域和4个半胱氨酸残基;预测BrRALF1蛋白含有5个翻译后修饰性位点。表达模式分析表明,BrRALF1在可育花的花丝、花药、雌蕊、萼片、花瓣中均表达,其中在花药中表达量最高;BrRALF1表达在不育株上受到强烈抑制。