缺氮胁迫下雨生红球藻虾青素积累过程中的基因组MSAP分析

虾青素具有多种生物学活性,雨生红球藻为天然虾青素的最佳来源,缺氮胁迫会导致雨生红球藻积累虾青素。为了解缺氮条件下雨生红球藻虾青素积累的分子机制,该研究通过对雨生红球藻进行缺氮胁迫,结合MSAP法,研究了雨生红球藻在缺氮胁迫下虾青素积累过程中基因组甲基化水平的变化,结果表明:缺氮胁迫0~72 h期间,雨生红球藻生长速度减慢,而虾青素积累主要发生在缺氮处理12~24 h期间,随后积累速度减慢。同时,对缺氮胁迫0、24、72 h的雨生红球藻基因组DNA进行甲基化敏感扩增多态性分析,共得到了291个甲基化多态性位点,其中发生甲基化变化的位点在0~24 h和24~72 h分别占总位点的29.90%和53.95%。在缺氮胁迫24 h处DNA半甲基化率最大(为12.71%),全甲基化率最低(为26.80%);缺氮胁迫72 h处DNA全甲基化率最高(为28.52%),半甲基化率最低(为1.72%)。这表明DNA甲基化调节方式的改变是虾青素积累过程中的一种重要调控模式。     

叶锈菌胁迫下的小麦基因组MSAP分析

内源DNA甲基化是真核生物表观遗传调控的重要组成部分, 在真核生物的基因表达调控中具有重要的作用。生物胁迫为植物提供一种内在的表观遗传进化动力。研究生物胁迫下DNA甲基化的变异模式, 有助于全面理解DNA甲基化的表观调控生物学功能。小麦近等基因系TcLr19、TcLr41及其感病亲本Thatcher在苗期对叶锈菌生理小种THTT、TKTJ分别表现为小种特异性抗病反应和感病反应。文章利用甲基化敏感扩增多态性(Methylation-sensitive amplified polymorphism, MSAP)技术分析了小麦的甲基化水平, 同时比较了苗期在生物胁迫前后基因组DNA胞嘧啶甲基化模式。用60对MSAP引物对接种前后的小麦DNA进行全基因组筛选, 没有直接分离得到接菌前后的甲基化模式的差异, 结果初步表明, 叶锈菌并没有诱导稳定且特异的植物基因组DNA胞嘧啶位点的甲基化模式变化, 但发现TcLr41及其感病亲本Thatcher之间存在表观遗传学差异。     

复幼促进核桃不定根发生的DNA甲基化机制探讨

该研究以核桃的复幼和成龄插穗为材料,通过甲基化修饰依赖性内切酶测序技术(MethylRAD-Seq),在全基因组水平上检测成龄与复幼插穗中DNA甲基化位点分布特征,进一步对复幼处理前后插穗中差异甲基化位点相关基因的表达情况进行分析。结果显示:(1)复幼处理可显著降低核桃插穗的DNA甲基化水平。(2)功能富集分析结果显示,差异甲基化位点相关基因主要参与油菜素内酯信号转导、次级代谢产物生物合成和木质素生物合成等功能,参与光合作用、MAPK(mitogen-activated protein kinase, MAPK)信号通路、果糖和甘露糖代谢、cAMP(cyclic AMP, CAMP)信号途径和苯丙烷生物合成等代谢通路。(3)qRT-PCR分析结果显示,复幼处理前后,不定根发生的关键调控基因NAC1、ARF5、ARF6和WRKY22在复幼和成龄材料中具有不同的表达模式。研究认为,复幼处理降低了核桃插穗中基因组DNA的甲基化水平,进而影响不定根发生过程关键功能基因的表达,可能是复幼调控核桃不定根发生能力的重要途径。     

DNA甲基化在动植物遗传育种中的研究进展

DNA甲基化是真核生物表观遗传学重要的机制之一,对基因转录水平的表达具有重要的调控作用。近年来,DNA甲基化在动植物遗传育种领域的研究引起了人们广泛的关注。我们从DNA甲基化与基因的表达调控、动植物基因组的甲基化状态、甲基敏感扩增片段多态性方法、DNA甲基化与杂种优势,以及DNA甲基化与分子标记等方面,简要综述了国内外有关DNA甲基化在动植物遗传育种研究中的进展,着重于全基因组DNA甲基化模式在动植物遗传育种中的相关研究和应用。     

逆境胁迫对水稻DNA甲基化水平的影响

植物在逆境胁迫下发生复杂的表现遗传变化,包括DNA甲基化、组蛋白修饰和RNA介导的基因沉默等.其中DNA甲基化是表现遗传学中的重要组成部分,主要通过甲基化、去甲基化来参与逆境胁迫下基因表达的调控,进而增强植物体的抗逆性,调节植物体的生长发育.就非生物与生物胁迫对水稻DNA甲基化水平的影响进行综述,为从表观遗传水平研究水稻抗逆性的机制提供理论参考.     

基因组DNA甲基化及组蛋白甲基化

在真核生物中,DNA甲基化是一种非常重要的表观遗传学标记,能影响染色质的结构和基因的表达。随着全基因组甲基化测序的发展,全基因组范围内的DNA甲基化水平得以了解。文章概述了基因组中启动子、基因本体、增强子、沉默子和转座子等不同元件的DNA甲基化的研究进展,以及DNA甲基化与基因表达调控间的关系。启动子的DNA甲基化对基因的表达有抑制作用,而基因本体的DNA甲基化与基因的表达关系因物种或细胞类型不同而异。增强子的DNA甲基化状态与基因活性呈反比关系,沉默子则相反呈正相关。转座子的DNA高度甲基化抑制其转座活性,从而维持基因组的稳定性。文章还探讨了DNA甲基化与组蛋白甲基化间的相互作用及其对基因表达、可变剪切、转录的调控作用,以及本领域的未来研究方向。     

逆境诱导水稻谷胱甘肽合成酶基因的表达研究

用RACE方法获得了全长的水稻谷胱甘肽合成酶(GS)基因的cDNA,并命名为OsGS(GeneBankaccession No.:AY453405)。该cDNA全长1 892 bp,编码一个由540个氨基酸组成的多肽,预测其氨基端(N端)含有一段定位叶绿体的信号肽。比较水稻基因组定位结果表明OsGS基因位于水稻12号染色体短臂上,转录区全长6 321 bp,由12个外显子和11个内含子组成。通过RT-PCR对OsGS在水稻正常生长条件和逆境条件下的表达进行了研究。结果表明,在正常生长条件下,OsGS在水稻幼苗的根和叶以及抽穗期水稻的根中表达;但不在抽穗期水稻的叶、茎和幼穗中表达,这显示OsGS在水稻中的表达具有发育和组织特异性。利用抽穗期水稻的叶片为材料,经高温、干旱和重金属逆境处理后,OsGS在抽穗期叶片中的转录被诱导表达;而在盐、低温、伤害逆境下则不被诱导。在轻度和中度干旱胁迫4 h后OsGS基因可被诱导表达。外源ABA处理也能够提高OsGS的转录水平,这显示OsGS可能是依赖ABA信号途径的环境胁迫诱导基因。     

DNA甲基化与植物抗逆性研究进展

DNA甲基化是真核细胞基因组重要修饰方式之一.DNA甲基化通过与转录因子相互作用或通过改变染色质结构来影响基因的表达,从表观遗传水平对生物遗传信息进行调节,在生长发育过程中起着重要的作用,而且植物DNA甲基化还参与了环境胁迫下的基因表达调控过程.本文对植物DNA甲基化的产生机制、功能,以及DNA甲基化在植物应对逆境胁迫中的作用进行综述,以更好地理解植物DNA甲基化及其对环境胁迫的响应,为植物抗逆性研究及作物遗传改良提供理论参照.     

氮胁迫下高羊茅基因组DNA甲基化的MSAP分析

高羊茅是一种重要的禾本科牧草,尽管其具有良好的耐寒耐热性,但其生长发育过程受外界氮素浓度的直接影响。DNA甲基化作为一种表观遗传调控方式在植物抵御逆境胁迫中起到至关重要的作用。本研究以高羊茅为试验材料,经无氮胁迫15 d后,以未经氮胁迫为对照,对基因组DNA甲基化的变化进行甲基化敏感扩增多态性(MSAP)分析。结果表明:无氮处理15 d后,植株生长受到强烈地抑制,且叶片大面积发黄;MSAP分析选用12对选扩引物,共检测到725个基因位点,其中发生甲基化和去甲基化的位点占16.4%;对照组和氮胁迫组总甲基化水平分别是65.56%和65.47%,显示氮胁迫15 d高羊茅基因组DNA总的甲基化水平未发生显著变化。对15条标记带进行克隆并测序,成功获得14条不同变化类型的序列,这些序列与禾本科植物具有较高的同源性,推测氮胁迫下的高羊茅基因组甲基化可能发生在编码区域。综上,高羊茅对环境的适应性调节可能与氮胁迫诱导的甲基化的变化有关。     

外源NO对转基因白桦外源基因表达及DNA甲基化的影响

为探讨外源NO诱导转基因白桦外源基因表达与基因组DNA甲基化之间的关系,本研究分析了NO供体硝普钠（sodium nitroprusside,SNP）对转基因白桦愈伤组织中外源基因BGT转录的影响,并对此过程中基因组DNA甲基化水平、甲基转移酶基因DRM、MET表达量及生理生化指标进行研究。结果表明：2 mmol·L^-1SNP处理后,转基因白桦防御酶活性、丙二醛（MDA）含量显著升高,表明高浓度NO对白桦细胞正常生命活动产生了伤害;甲基转移酶DRM和MET基因上调表达,基因组DNA甲基化水平由10.6%增加到16.5%,外源基因BGT表达量在6 h时显著增加,3 d时仅为对照的0.46倍,说明转基因白桦外源BGT基因的表达对高浓度NO响应明显且受基因组甲基化水平的影响。本研究揭示了转基因白桦外源BGT基因和甲基转移酶MET、DRM基因对高浓度NO的响应模式,分析了基因组甲基化水平及生理生化特征的变化,为转基因植物生长发育的表观遗传调控和外源基因表达影响机制的研究奠定基础。     

Cytosine methylation at CG and CNG sites is differential during the development of triploid black poplar

It has been widely shown that polyploidization can result in changes in cytosine methylation. However, little is known regarding how cytosine methylation changes in polyploids development, especially in polyploid trees. In this study, we investigated drifting changes of DNA methylation status at 5′-CCGG sites in the apical bud, young and mature leaf tissues of triploid black poplar (Populus. euramericana) with methylation-sensitive amplification polymorphism (MSAP) and assessed the expression of multiple DNA methyltransferases (MTases) and DNA demethylase during different developmental stages. MSAP analysis detected methylation levels at CG and CNG sites of diploid tissues reduced during development from bud to leaves, while for the triploid, methylation at CNG sites increased during development, but levels of methylation at CG sites first decreased in young leaves before increasing in mature leaves. MTase genes related to CG or CNG methylation were respectively preferential in different triploid tissues with high CG or CNG methylation levels. High expression of DNA demethylase was observed in tissue with high demethylation trends. These finding suggest CG and CNG methylation and their related enzymes are involved with different biological functions and networks of gene regulation in different developmental stages of triploid.     

DNA Methylation Alterations and Their Association with High Temperature Tolerance in Rice Anthesis

DNA methylation is an important epigenetic mechanism involved in gene regulation under environmental stresses in plants. However, little information is available regarding its responses to high temperature (HT) and association with HT tolerance in rice. In this study, fourteen rice genotypes were classified into the susceptible, moderate, and tolerant groups by the high temperature susceptibility index (HTSI) after HT treatment. The changes of DNA methylation in rice anthesis under normal and HT30 conditions were investigated using methylation-sensitive amplified polymorphism31 (MSAP). The MSAP results showed that the DNA methylation level significantly increased in the susceptible rice group and decreased in the tolerant rice group under HT treatment, while no significant difference was observed in the moderate rice group. More hypomethylation events were detected in the tolerant rice group, while more hypermethylation was detected in the susceptible rice group. Forty-four differentially methylated epiloci (DME) were generated under both control and HT conditions, which can clearly distinguish the susceptible, moderate, and tolerant genotypes via PCoA analysis. Approximately 43.18% of DMEs were determined to be tolerance-associated epiloci (TAEs). 63.15% TAEs were sequenced and annotated into 12 genes. Quantitative RT-PCR analysis showed that 12 TAE genes were mainly upregulated in 14 rice genotypes, and their expression levels were related to the HT tolerance of rice. Here, DEGs, generated from a number of genotypes, indicate higher probabilities for association with stress tolerance. Overall, these results suggest that DNA methylation regulation might play a key role in adaptation to HT stress in rice.

     

Dynamics of phytohormone and DNA methylation patterns changes during dormancy induction in strawberry (Fragaria?×?ananassa Duch.)

Changes in endogenous phytohormone levels, DNA methylation patterns, and expression levels of related genes during induction of dormancy in two strawberry cultivars, Darselect and All Star, were studied under controlled environmental conditions. At 12°C, regardless of day length, potted, runner-derived plants of both cultivars gradually exhibited morphological traits typical of dormancy after treatment for 8 weeks. These morphological changes were accompanied by a synchronous significant decline in indole-3-acetic acid (IAA) level and increases in abscisic acid (ABA) content and global genomic DNA methylation in young leaves. Exposed at 15°C and a short-day photoperiod, the changes in morphology, phytohormone levels and DNA methylation of both cultivars were similar to those observed at 12°C. Slight but non-significant changes in IAA and ABA levels and genomic DNA methylation occurred in young leaves at both 15°C with long days and 18°C with short days. These results indicated that temperature alone was sufficient to induce strawberry to enter the typical dormant phase, and day length had no impact at 12°C. The higher temperature permissible for dormancy induction in strawberry was 15°C, but at this temperature dormancy induction was modified by day length. The expression patterns of FaPIN1, FaNCED1, FaDRM and FaROS1 were coincident with the changes in phytohormone levels and DNA methylation. Although the two tested cultivars have different temporal responses with the different degree of cold tolerance and depth of dormancy, both the endogenous phytohormone and DNA methylation were changed when induced by external environmental factors.