类伸展蛋白OsPEX1对水稻花粉育性的影响

类伸展蛋白(Leucine-Rich Repeats Extensins,LRX)是一类细胞壁嵌合蛋白,其N端包含一个LRR(leucine-rich repeats)结构域,C端含Extensins结构域。研究表明,LRX基因家族在拟南芥(Arabidopsis thaliana)花粉萌发和花粉管生长过程中具有重要作用,而水稻(Oryza sativa L.)LRX基因家族是否在调控花粉发育方面具有保守的生物学功能尚不清楚。本研究首先进行了生物信息学分析,结果显示,水稻LRX基因家族包括8个成员,OsPEX3、OsLRX3、OsLRX5位于水稻第1号染色体;OsLRX1、OsLRX3、OsLRX2、OsPEX1和OsPEX2分别位于第2、第5、第6、第11和第12号染色体,其中OsPEX1基因在花粉中高表达,暗示OsPEX1可能参与了花粉发育调控。为此,本研究采用RNAi技术进一步研究了OsPEX1基因对花粉发育的影响。结果表明,OsPEX1基因的RNAi转基因植株花粉败育,结实率仅为10%-30%。qRT-PCR分析显示,这些RNAi转基因植株OsPEX1基因表达量显著低于野生型,而且其表达量越低花粉育性亦随之降低。上述研究结果表明,水稻OsPEX1基因是水稻花粉发育的重要基因,该基因的克隆和功能分析有助于进一步阐明水稻花粉发育调控的分子遗传学机制。     

水稻OsTB1基因的结构及其表达分析

TCP基因是一类植物中新发现的、可能具有转录因子活性的基因家族,成员包括金鱼草的Cyclodiea (Cyc)、玉米的Teosinte Branched1 (TB1)以及水稻中的PCF1、PCF2等.玉米的TB1基因有维持玉米顶端优势的作用,与分蘖的发生密切相关;水稻和玉米同属禾本科,在发育的过程中都有分蘖的发生.通过筛选水稻的基因组文库,得到了水稻中的一个TB1同源基因Oryza sativa Teosinte Branched1 (OsTB1).该基因不含内含子,基因编码一个长度为388个氨基酸的蛋白,在氨基酸水平上与TB1的同源性为70%,含有保守的TCP区和R区,是属于TCP基因家族的一个成员.RT-PCR和mRNA原位杂交分析结果表明,OsTB1在水稻的侧芽中有很强的表达,在花序中有较弱的表达.以上结果显示该基因可能在水稻侧芽和花序的起始和发育过程中起重要作用.     

拟南芥花药绒毡层细胞中具有基因簇特征的基因进化和功能分析

在植物基因组中, 除了同源基因成簇现象外, 近年来还发现一些具有共表达特性的异源基因也能够以基因簇形式存在, 但这些异源基因簇的进化和生物学功能尚不清楚。花药发育和花粉形成是植物进化出的特有的生殖生物学过程, 同时产生了一些在花药绒毡层中特异表达和特定功能的基因簇基因。该研究通过筛选和分析花药绒毡层中基因簇基因的分子特性、表达调控、基因年龄和基因重复进化等信息, 探讨花药基因簇基因与植物开花功能进化之间的关系。结果表明, 在拟南芥(Arabidopsis thaliana)中共筛选到84个(13个基因簇)花药绒毡层特异高表达的基因簇基因, 它们主要产生于串联重复事件, 76%的基因出现在开花植物分化后的阶段, 主要参与生殖发育、花粉鞘组成和脂代谢等生物学过程。研究初步解析了拟南芥花药绒毡层中基因簇基因的基本特征、生物学功能和基因进化机制, 为深入揭示植物基因簇基因的遗传学功能奠定了基础。     

拟南芥花药绒毡层细胞中具有基因簇特征的基因进化和功能分析

在植物基因组中,除了同源基因成簇现象外,近年来还发现一些具有共表达特性的异源基因也能够以基因簇形式存在,但这些异源基因簇的进化和生物学功能尚不清楚。花药发育和花粉形成是植物进化出的特有的生殖生物学过程,同时产生了一些在花药绒毡层中特异表达和特定功能的基因簇基因。该研究通过筛选和分析花药绒毡层中基因簇基因的分子特性、表达调控、基因年龄和基因重复进化等信息,探讨花药基因簇基因与植物开花功能进化之间的关系。结果表明,在拟南芥(Arabidopsisthaliana)中共筛选到84个(13个基因簇)花药绒毡层特异高表达的基因簇基因,它们主要产生于串联重复事件,76%的基因出现在开花植物分化后的阶段,主要参与生殖发育、花粉鞘组成和脂代谢等生物学过程。研究初步解析了拟南芥花药绒毡层中基因簇基因的基本特征、生物学功能和基因进化机制,为深入揭示植物基因簇基因的遗传学功能奠定了基础。     

玉米花粉特异的非编码RNA基因ZM401 cDNA全长的克隆及其发育表达模式

通过差异筛选法并结合冷噬菌斑筛选,从玉米(Zea mays L.)成熟花粉cDNA文库中克隆到一个玉米花粉特异表达的cDNA片段ZM401(663bp).Northern杂交表明ZM401是一个玉米花粉特异表达的基因.本文采用5'RACE,3'RACE及重叠PCR技术获得了ZM401 cDNA的全长(1 149 bp).采用生物学软件对ZM401 cDNA的序列和结构进行分析,结果表明,该基因缺乏明显的开放阅读框架,序列中最长的开放阅读框架仅有89个氨基酸,但具有poly(A)尾部结构,符合非编码RNA基因的特点.推断ZM401基因是一个非编码基因.RT-PCR及Northern blot分析表明ZM401基因从玉米花粉小孢子四分体时期、单核期、双核期、成熟花粉开始表达,而且表达量依次增强,证明ZM401可能与玉米花粉的晚期发育过程相关.同时,Northern杂交显示ZM401基因在玉米花粉发育中有两种转录本存在.     

玉米花粉特异的非编码RNA基因ZM401 cDNA全长的克隆及其发育表达模式

通过差异筛选法并结合冷噬菌斑筛选,从玉米(Zea mays L．)成熟花粉cDNA文库中克隆到一个玉米花粉特异表达的cDNA片段ZM401(663bp)。Northern杂交表明ZM401是一个玉米花粉特异表达的基因。本文采用5′RACE,3′RACE及重叠PCR技术获得了ZM401 cDNA的全长(1149bp)。采用生物学软件对ZM401 cDNA的序列和结构进行分析,结果表明,该基因缺乏明显的开放阅读框架,序列中最长的开放阅读框架仅有89个氨基酸,但具有poly(A)尾部结构,符合非编码RNA基因的特点。推断ZM401基因是一个非编码基因。RT-PCR及Northern blot分析表明ZM401基因从玉米花粉小孢子四分体时期、单核期、双核期、成熟花粉开始表达,而且表达量依次增强,证明ZM401可能与玉米花粉的晚期发育过程相关。同时,Northern杂交显示ZM401基因在玉米花粉发育中有两种转录本存在。     

一种新型几丁质酶基因LcChi2在转基因水稻中的功能分析

LcChi2是从羊草中克隆获得的一种新型几丁质酶基因,生物信息学分析表明该基因表达一个Ⅱ类几丁质酶,属于19家族。在双子叶模式植物烟草中过表达该基因表现为抗真菌病害的生物学功能提高,然而在单子叶植物中是否具有抗病功能至今未知。以吉林省主栽水稻品种吉粳88为供试材料,构建了含LcChi2基因和除草剂筛选标记Bar基因的双价植物表达载体,利用农杆菌介导的遗传转化方法成功获得LcChi2和Bar基因过表达的转基因水稻。T_1代转基因水稻的PCR、RT-PCR和几丁质酶活性检测结果表明LcChi2基因已成功整合到水稻基因组中,并且表达产物表现出较高的外源几丁质酶活性;稻瘟病活体接种实验结果证明该基因显著提高了水稻的抗病性;抗除草剂鉴定结果表明获得的转基因水稻新材料同时具有除草剂抗性。研究结果证明LcChi2基因可有效提高单子叶植物的抗病性,该基因在利用现代生物技术开展抗病作物遗传改良方面具有重要的应用价值。     

花粉发育的研究进展

近年来,随着现代生物学技术及分子生物学技术在花粉生物学研究领域中广泛的应用,从而使花粉发育过程中一些关键问题及其有关分子机理的研究均获得了重要进展。目前已克隆了许多与花粉发育有关的基因,并鉴定了一些花粉发育的突变体。本文针对花粉发育过程中的细胞质改组;胼胝质壁、淀粉粒和细胞器的动态变化;绒毡层的发育;花粉发育特异基因;以及不对称分裂和细胞命运等几个生物学问题的研究进展作了简要综述,最后还提出了一些研究展望。     

水稻msp1-4突变体的鉴定及其UDT1和GAMYB基因的表达分析

通过对粳稻‘9522’辐射诱变,得到一隐性雄性不育突变体msp1-4（MULTIPLE SPOROCYTE）,用遗传定位方法将该基因座位定位在分子标记WY-4和WY-8之间,相距0．8cM,物理距离247kb。测序分析证明这247kb区间中的MSP1基因的编码区在第758bp到767bp之间发生了10个碱基的缺失。形态学观察结果表明该突变体和已经报告过的msp1突变体的表型基本一致。为分析水稻其它与花药发育相关的基因在msp1-4中的表达变化,用半定量RT-PCR技术检测到影响绒毡层和花粉发育的重要基因UDT1和GAMYB的表达在突变体中比在野生型水稻中低,说明这2个基因可能位于MSP1基因的下游。     

玉米DEAD-box RNA解旋酶基因的克隆及分析

DEAD-box RNA解旋酶参与RNA转录、前体mRNA剪切、核糖体发生、核质运输、蛋白质翻译、RNA降解等重要的生命活动.根据本室在S-Mo17Rf3Rf3cDNA芯片研究中,检测到花粉发育后期RNA解旋酶上调表达的结果,应用RACE技术从S-Mo17Rf3Rf3花粉中克隆得到该RNA解旋酶基因全长cDNA,命名为ZmRH2并在GenBank注册登记 (DQ327709).序列分析表明：该cDNA全长1 652bp,从第163 bp开始到1 386bp含有一个开放阅读框,编码407个氨基酸.其编码的蛋白质具有DEAD-box RNA解旋酶特有的9个保守模体,与水稻、拟南芥和豌豆中的DEAD-box RNA解旋酶的氨基酸序列存在着很高的同源性.RT-PCR分析表明,该基因在近等基因系S-Mo17Rf3Rf3和S-Mo17rf3rf3的叶、根、和雌穗中的表达没有差异,但在花丝和花粉中有明显差异.     

Characterization of a gene family abundantly expressed in Oenothera organensis pollen that shows sequence similarity to polygalacturonase.

We have isolated and characterized cDNA clones of a gene family (P2) expressed in Oenothera organensis pollen. This family contains approximately six to eight family members and is expressed at high levels only in pollen. The predicted protein sequence from a near full-length cDNA clone shows that the protein products of these genes are at least 38,000 daltons. We identified the protein encoded by one of the cDNAs in this family by using antibodies to beta-galactosidase/pollen cDNA fusion proteins. Immunoblot analysis using these antibodies identifies a family of proteins of approximately 40 kilodaltons that is present in mature pollen, indicating that these mRNAs are not stored solely for translation after pollen germination. These proteins accumulate late in pollen development and are not detectable in other parts of the plant. Although not present in unpollinated or self-pollinated styles, the 40-kilodalton to 45-kilodalton antigens are detectable in extracts from cross-pollinated styles, suggesting that the proteins are present in pollen tubes growing through the style during pollination. The proteins are also present in pollen tubes growing in vitro. Both nucleotide and amino acid sequences are similar to the published sequences for cDNAs encoding the enzyme polygalacturonase, which suggests that the P2 gene family may function in depolymerizing pectin during pollen development, germination, and tube growth. Cross-hybridizing RNAs and immunoreactive proteins were detected in pollen from a wide variety of plant species, which indicates that the P2 family of polygalacturonase-like genes are conserved and may be expressed in the pollen from many angiosperms.     

水稻花药发育过程中腺苷三磷酸酶的分布

水稻花粉母细胞中的ATP酶反应颗粒很少,主要分布在细胞核中。组成花药药壁的4层细胞中只有绒毡层细胞核中有较多的ATP酶。减数分裂后,绒毡层细胞质中分化出许多内质网片层,但ATP酶反应颗粒仍很少,其它3层药壁细胞中质膜ATP酶明显增加。在花粉内、外壁中形成了大量的ATP酶反应颗粒,但花粉外壁在小孢子时期形成,ATP酶反应颗粒来自绒毡层细胞的鸟氏体。花粉内壁在二胞花粉时期形成,其中的ATP酶反应颗粒来自花粉营养细胞。二胞花粉的营养细胞比生殖细胞含有更多的ATP酶反应颗粒。     

Identification of a pollen-specific sucrose transporter-like protein NtSUT3 from tobacco.

Pollen cells are symplasmically isolated during maturation and germination. Pollen therefore needs to take up nutrients via membrane carriers. Physiological measurements on pollen indicate sucrose transport in the pollen tube. A cDNA encoding a pollen-specific sucrose transporter-like protein NtSUT3 was isolated from a tobacco pollen cDNA library. NtSUT3 expression is detected only in pollen and is restricted to late pollen development, pollen germination and pollen tube growth. Altogether these data indicate that pollen is supplied not only with glucose, but also with sucrose through a specific sucrose transporter. The respective contribution of each transport pathway may change during pollen tube growth.     

Pollen and Phytolith Evidence for Rice Cultivation and Vegetation Change during the Mid-Late Holocene at the Jiangli Site,Suzhou, East China

Pollen and phytolith analyses were undertaken at the Jiangli site in Suzhou, Jiangsu Province, combined with studies on macrofossils by flotation. The concentration of pollen decreased while the percentage of Poaceae pollen in the profile increased from the late phase of the Majiabang Culture to the Songze Culture suggesting that human impact on the local environment intensified gradually. The discovery of rice paddy implies a relatively advanced rice cultivation in this area during the middle-late Holocene. Other than phytoliths, the high percentage of Oryza-type Poaceae pollen (larger than 40 µm) supplied robust evidence for the existence of rice paddy. Moreover, the fact that the farther from the rice paddy, the lower the concentration and percentage of Poaceae pollen also proves that the dispersal and deposition of pollen is inversely proportional to the distance.     

茶树花粉特异蛋白基因CsPSP1的分离及序列分析

利用cDNA-AFLP技术比较了茶树[Camellia sinensis(L.)O.Kuntze cv.Wulong]花蕾发育早期和晚期的基因表达,结果表明存在明显差异。以E12和M20为引物对在晚期发育花蕾中筛选出一条281 bp特异表达的差异条带TDF53(transcipt-derived-fragment,TDF)。RT-PCR分析表明该片段只在晚期发育花蕾中特异表达。用RACE方法延伸其末端序列,克隆并测序获得全长cDNA序列(GenBank登录号:DQ887753)。该基因全长2079 bp,开放阅读框1701 bp,编码567个氨基酸,其分子量为63 kDa。序列和结构的同源性分析表明:该基因编码的氨基酸序列与烟草、油菜的花粉特异蛋白等同源性较高,由此推定,该基因为编码茶树花粉特异蛋白的基因,并将分离到的花粉特异蛋白基因命名为CsPSP1。     

Isolation and Expression analysis of OsPME1, encoding for a putative Pectin Methyl Esterase from Oryza sativa (subsp. indica)

Pectin Methyl Esterases (PMEs) play an essential role during plant development by affecting the mechanical properties of the plant cell walls. Recent studies indicated that PMEs play important role in pollen tube development. In this study, we isolated a 1.3 kb cDNA clone from rice panicle cDNA library. It contained a 1038 bp of open reading frame (ORF) encoding for a putative pectin methyl esterase of 345 aminoacids with a 20 aminoacid signal peptide and was hence designated as OsPME1 (Oryza sativaPectin Methyl Esterase 1). It contained the structural arrangement GXYXE and GXXDFIF, found in the active groups of all PMEs. OsPME1 gene product shared varying identities, ranging from 52 % to 33 % with PMEs from other plant species belonging to Brassicaceae, Fabaceae, Amaranthaceae and Funariaceae. Southern blot analysis indicated that PME1 exists as a single copy in the rice genome. Expression pattern analysis revealed that OsPME1 is expressed only in pollen grains, during the later stages of their development and was also regulated by various abiotic stress treatments and phytohormones. Functional characterization of this pollen specific PME from rice would enable us to understand its role in pollen development.Key words: Oryza sativa, Pectin Methyl Esterase, Gene Expression, Cell wall and pollen development     

Identification of small RNAs in late developmental stage of rice anthers

Small RNAs including microRNA (miRNA) and small interfering RNA (siRNA) are known as repressors of gene expression. There are many plant proteins involved in small RNA-mediated gene silencing, such as Dicer ribonucleases and RNA-dependent RNA polymerases. However, most of these proteins have been reported to be absent in the late developmental stage of the plant male gamete, pollen. In order to clarify the existence of the small RNAs during maturation of pollen, we cloned and sequenced small RNAs from rice anthers including tricellular pollen. From fifty six candidates of small RNAs, we identified two known miRNAs (miR166 and miR167), eight potential miRNAs, and ten putative heterochromatic siRNAs (hc-siRNAs). RNA gel blot analyses clearly showed that miR166 and miR167 were accumulated in the uninuclear pollen stage of anther development and remained until the tricellular pollen stage. Our cloning and RNA gel blot analyses of small RNAs led us to propose a possible function of small RNA-mediated gene regulation for the development of male gametes in rice.