可育与雄性不育万寿菊雌雄配子体发育的比较研究

对可育系和雄性不育系万寿菊的大、小孢子发生及雌、雄配子体发育过程进行了系统地比较观察。结果表明：可育系和不育系万寿菊雌蕊的发育基本相同,二者的雌蕊为二心皮一室,每室1胚珠,单珠被,薄珠心,倒生型胚珠。大孢子母细胞经减数分裂形成线形排列的4个大孢子,合点端为功能大孢子。胚囊发育类型为蓼型。可育系小孢子母细胞经过减数分裂形成四面体形的四分体,成熟花粉是二细胞型,表面有刺。其花药为四室,药壁发育属双子叶型,腺质绒毡层。雄性不育系万寿菊特化小花在花芽分化时即没有产生雄蕊原基,因而不具雄蕊结构,为结构型雄性不育。     

显性核不育亚麻可育、不育花蕾mRNA差异表达研究及差异片段分析

利用mRNA差异显示技术,以显性雄性核不育亚麻不育系分离出的可育株和不育株为材料,对可育、不育花蕾中基因差异性表达进行了研究.对回收的差异片段进行反向Northern杂交验证,获得了7个阳性差异表达基因片段,并对它们进行测序和BLAST分析,最后确定了3个候选基因片段G-E07-100、G-E07-830和G-E07-330.序列分析结果表明:G-E07-100与蓖麻(Ricinus communis)的GTP-结合蛋白基因部分序列高度(90%)同源;G-E07-830与梨(Pyrus pyrifolia)的β-木糖苷酶基因高度同源(80%),并且还包含1个糖基水解酶家族C-末端的保守结构域;G-E07-330与亚麻(Linum usitatissimum)LuP12025D10 cDNA高度(89%)同源.进一步的Northern杂交结果表明3个候选基因均在不育花蕾中表达.     

Identification of Differentially Expressed Genes in the Pheromone Glands of Mated and Virgin Bombyx mori by Digital Gene Expression Profiling

Background

Mating decreases female receptivity and terminates sex pheromone production in moths. Although significant progress has been made in elucidating the mating-regulated inactivation of pheromone biosynthesis-activating neuropeptide (PBAN) secretion, little is known about the mating induced gene expression profiles in pheromone glands (PGs). In this study, the associated genes involved in Bombyx mori mating were identified through digital gene expression (DGE) profiling and subsequent RNA interference (RNAi) to elucidate the molecular mechanisms underlying the mating-regulated gene expression in PGs.

Results

Eight DGE libraries were constructed from the PGs of mated and virgin females: 1 h mating (M1)/virgin (V1) PGs, 3 h mating (M3)/virgin (V3) PGs, 24 h mating (M24)/virgin (V24) PGs and 48 h mating (M48)/virgin (V48) PGs (M48 and V48). These libraries were used to investigate the gene expression profiles affected by mating. DGE profiling revealed a series of genes showing differential expression in each set of mated and virgin female samples, including immune-associated genes, sex pheromone synthesis-associated genes, juvenile hormone (JH) signal-associated genes, etc. Most interestingly, JH signal was found to be activated by mating. Application of the JH mimics, methoprene to the newly-emerged virgin females leaded to the significant reduction of sex pheromone production. RNAi-mediated knockdown of putative JH receptor gene, Methoprene tolerant 1 (Met1), in female pupa resulted in a significant decrease in sex pheromone production in mature females, suggesting the importance of JH in sex pheromone synthesis.

Conclusion

A series of differentially expressed genes in PGs in response to mating was identified. This study improves our understanding of the role of JH signaling on the mating-elicited termination of sex pheromone production.     

苜蓿雄性不育系MS-4 SSH文库构建及基因表达分析

以苜蓿雄性不育系MS-4与可育系花蕾为材料,利用抑制性消减杂交(SSH)技术,分别构建了不育条件下和可育条件下基因差异表达消减cDNA文库,在2个库中分别随机挑选阳性克隆进行测序,经序列比对分析,共获得功能已知的EST序列190条。后经GO功能分类,对推定出的6个相关基因进行荧光定量PCR分析。结果表明:6个基因在苜蓿雄性不育系花蕾不同发育时期中均出现差异表达,推测这6个基因可能与苜蓿雄性育性相关,并且在其育性转换中具有重要作用。     

Identification of Differentially Expressed Genes During Anther Abortion of Taigu Genic Male Sterile Wheat by Combining Suppression Subtractive Hybridization and cDNA Array

Talgu Genlc Male Sterile Wheat （TGMSW; Trltlcum aestlvum L.）, a dominant genic male sterile germplasm, is of considerable value in the genetic Improvement of wheat because of Its stable Inherence, complete male abortion, and high cross-fertilization rate. To Identify specially transcribed genes In sterile anther, a suppression subtractlve hybridization （aSH） library was constructed with sterile anther as the tester and fertile anther as the driver. A total of 2 304 SSH Inserts amplified by polymerase chain reaction were arrayed using robotic printing. The cDNA arrays were hybridized with 32P-labeled probes prepared from the RNA of forward- and reverse-subtracted anthers. Ninety-six clones were scored as upregulated in sterile anthers compared with the corresponding fertile anthers and some clones were selected for sequencing and analysis In GenBank. Based on their putative functions, 87 non-redundant clones were classified Into the following groups： （i） eight genes Involved In metabolic processes; （11） four material transportation genes; （iii） three signal transductlon-assoclated genes; （iv） four stress response and senescence-associated protein genes; （v） seven other functional protein genes; （vi） five genes with no known function; and （vii） another 56 genes with no match to the databases. To test the hybridization efficiency, eight genes were selected and analyzed by Northern blot. The results of the present study provide a comprehensive overview of the genes and gene products Involved In anther abortion In TGMSW.     

Profiling Expression Patterns and Isolating Differentially Expressed Genes by cDNA Microarray System with Colorimetry Detection

A high-density cDNA microarray with colorimetry detection system to simultaneously monitor the expression of many genes on nylon membrane is described and characterized. To quantify the expression of genes and to isolate differentially expressed genes, the southern hybridization process on filter membranes was employed. The levels of gene expression were represented by color intensities generated by colorimetric reactions in place of hazardous radioisotopes or costly laser-induced fluorescence detection. The gene expression patterns on nylon membranes were digitized by devices such as an economical flatbed scanner or a digital camera. The quantitative information of gene expression was retrieved by image analysis software. Quantitative comparison of the northern dot-blotting method with the microarray system is described. Applications employing single-color detection as well as dual-color detection to isolate differentially expressed genes among thousands of genes are demonstrated.     

A Comparison of Anther Tissue Development in Male Sterile Aloe vera and Male Fertile Aloe ciliaris

Cytological differences between the anther development of amale sterile and a male fertile Aloe species are used to explaininteractions between anther tissues. Some deviations in thelayers of the locule wall and the microspores of the male sterileanther are related to each other and their biological functionsare discussed. The cytological development of the male sterility,which can be observed shortly after meiosis, seems to be restrictedto the locular cavity. The tapetal development and breakdownare normal, apart from the size of some orbicules. However,the pollenkitt is not transported to the pollengrains, whichstrongly supports our theory that this process is mechanicallypollen-controlled. The development of the epidermal and endothecialcells is normal, except in a part of the anthers where thesecells do not expand, after which dehiscence is incomplete. Thelatter process is discussed in relation to the deviations insidethe locular cavity. Aloe vera (L.) Burm. fil., Aloe ciliaris Haw., Liliaceae, male sterility, tapetum, pollenkitt, endothecium, anther dehiscence     

棉花细胞核雄性不育两用系差异表达基因分析

应用cDNA-AFLP对棉花ms5ms6双隐性核雄性不育两用系的不育株和可育株花粉发育的3个时期—造孢细胞时期、花粉母细胞时期和花粉粒时期进行对比分析,共得到17个差异表达片段,它们分别属于11种表达模式,其中14个片段可以在NCBI数据库中找到同源序列,功能分析表明这些片段所编码的基因可能参与了信号转导、转录、能量代谢、细胞壁发育等相关过程。Northern杂交结果证明检测片段的表达模式与cDNA-AFLP结果吻合。同时还在可育花药中发现了与玉米T型细胞质雄性不育恢复因子RF2基因高度同源的育性恢复因子类基因。     

肝细胞癌相关差异基因的生物信息学及预后分析

肝细胞癌是全球癌症相关死亡的主要原因,目前对肝细胞癌的发病机制研究尚不完善,探索肝细胞癌发生、发展相关的分子标志物及其预后具有重要意义。从GEO数据库获得肝细胞癌组织和非癌组织的基因表达阵列数据GSE84402,利用GEO2R筛选差异表达基因;采用DAVID数据库对差异基因进行GO富集分析和KEGG通路分析;通过STRING数据库和Cytoscape软件构建差异表达基因对应的蛋白质相互作用网络,并从网络中筛选出核心基因(hub genes);结合KM plotter数据库的临床信息对hub genes进行预后分析。结果显示:共得到1 307个差异表达基因,其中上调基因741个,下调基因566个,这些差异表达基因主要涉及细胞分裂、细胞周期、DNA复制及物质代谢等生物学过程及生物通路。通过GO、KEGG及蛋白质相互作用网络筛选出BUB1、BUB1B、CCNA2、CCNB1、CCNB2、CDC20、CDK1、MAD2L1、PLK1等9个hub genes,进一步分析发现hub genes均与细胞周期的调控相关,表明细胞周期的调控失常在肝细胞癌的发生、发展过程中具有重要作用。生存分析显示9个hub genes在肝细胞癌患者中均为表达上调的基因,且与患者预后不良相关,这为寻找肝细胞癌患者预后相关生物标志物的研究提供了线索。     

萍乡显性核不育水稻育性相关基因的定位和遗传分析

萍乡显性核不育水稻(Pingxiang Dominant Genic Male Sterile Rice,PDGMSR)是在水稻中首次发现的显性核不育材料,其育性由两对显性基因互作控制,一对是萍乡显性核不育基因Ms-p,另一对是显性上位恢复基因(dominant epistatic fertility restorer gene,Rfe)。两者共同存在时显性上位恢复基因能抑制不育基因的表达,从而使育性表现可育。本实验用一个对萍乡显性核不育水稻有恢复能力的水稻品种E823与萍乡显性核不育水稻配制杂交组合,将(萍乡核不育水稻/E823)F2作为定位群体,根据F3株系的育性分离,选择育性分离株系对应F2单株(基因型为Ms-pMs-pRefrfe和Ms-pms-pRferfe)构建可育池,用对应F2株系中的不育单株(基因型为Ms-pMs-prferfe或Ms-pms-prferfe)构建不育池,将显性上位恢复基因Rfe定位在水稻10染色体RM311和RM3152一侧,遗传距离分别为7.9cM和3.6cM。根据已有的Ms-p的定位结果,合成10染色体部分微卫星引物,对不育单株进行分析,发现RM171和RM6745位于Ms-p的两侧,距离分别为0.3cM和3.0cM。根据10染色体的测序结果,将Ms-p界定在约730kb的范围内,并构建了Ms-p的电子重叠群。植物显性核不育的育性恢复机理存在“复等位基因”和“显性上位互作”两种假说,贺浩华等用经典的遗传学方法证明了萍乡显性核不育水稻育性恢复的遗传机理属于“显性上位互作”。理论上认为,确定其遗传机理最为有效的方法是基因定位,如果不育基因和恢复基因位于同一位点,则其遗传机理属于“复等位基因”,否则为“显性上位互作”。本实验将不育基因和恢复基因定位在水稻10染色体不同的位点,用基因定位的方法证实了萍乡显性核不育水稻育性恢复的遗传机理属于“显性上位互作”。     

白菜核雄性不育系可育和不育花药中Ca2+的分布

研究了白菜(Brassica campestris L. ssp.chinensis Makino)细胞核雄性不育系花药中Ca2 的分布特征.在可育花药发育过程中,减数分裂后花药壁细胞中钙颗粒明显增加.早期小孢子开始积累钙颗粒并特异性地附在小液泡膜上.小孢子分裂后,大液泡消失过程中又伴随着许多钙颗粒附在小液泡膜上,显示出Ca2 与花粉中液泡的形成和分解有关.在不育花药中,最早出现的钙颗粒异常分布是在小孢子母细胞的胼胝质壁中积累了较多的钙颗粒.然而,在小孢子细胞质中钙颗粒一直很少,也不形成大液泡,最后通过细胞质收缩的方式败育.这是首次发现Ca2 参与调控花药发育过程,其异常分布与花粉败育密切相关.