拟南芥AtR8 lncRNA对盐胁迫响应及其对种子萌发的调节作用

长链非编码RNA (lncRNA)是一类长度大于200个核苷酸且不编码蛋白质的非编码RNA, 主要由RNA聚合酶II转录生成, 大量存在于生物体内并具有多种生物学功能。AtR8 lncRNA是拟南芥(Arabidopsis thaliana)中RNA聚合酶III转录的长链非编码RNA。前期研究发现, 水杨酸(SA)处理诱导萌发种子中AtR8 lncRNA的表达, AtR8 lncRNA缺失抑制SA胁迫下的种子萌发。进一步研究发现, AtR8 lncRNA转录区域内存在保守的盐胁迫响应元件(TCTTCTTCTTTA); NaCl处理抑制萌发种子中AtR8 lncRNA的表达; 与野生型相比, 高浓度NaCl处理明显抑制了atr8 (AtR8 lncRNA部分缺失型拟南芥)种子萌发。研究结果表明, AtR8 lncRNA在拟南芥种子萌发期的盐胁迫中起重要作用。     

NaCI胁迫对盐芥和拟南芥光合作用的影响

本研究检测了与盐芥(Ghellungiella halophila)和拟南芥(Arabidopsis thaliana)光合作用相关的叶绿素、净光合速率(photosynthetic rate,Pn)、气孔导度(stomatal conductance,Gs)、胞间隙CO2浓度以及叶绿素荧光参数等指标,观察到随着NaCl浓度逐渐增加,盐芥的叶绿素a／b值(Chl a／Chl b)、类胡萝卜素／总叶绿素值(Car／Chl)显著高于拟南芥,且二比值变化幅度较小并保持较高水平。盐胁迫下拟南芥净光合速率下降、气孔导度下降和胞间CO2浓度减小。气孔因素是引起拟南芥光合能力下降的主要因素。叶绿素荧光参数的变化表明,50-200 mmol·L-1NaCl降低拟南芥叶绿体对光能的吸收能力,而且降低叶绿体的光化学活性,使电子传递速率和光能转化效率大幅度下降,造成光能转化为化学能的过程受阻,进一步加剧了光合放氧和碳同化能力的降低。而50-200 mmol·L-1NaCl胁迫没有使盐芥的光合作用受到不良影响。     

NaCl 胁迫对盐芥和拟南芥光合作用的影响

本研究检测了与盐芥(Ghellungiella halophila)和拟南芥(Arabidopsis thaliana)光合作用相关的叶绿素、净光合速率(photosynthetic rate, Pn)、气孔导度(stomatal conductance, Gs)、胞间隙CO2浓度以及叶绿素荧光参数等指标, 观察到随着NaCl浓度逐渐增加, 盐芥的叶绿素a/b值(Chl a/Chl b)、类胡萝卜素/总叶绿素值(Car/Chl)显著高于拟南芥, 且二比值变化幅度较小并保持较高水平。盐胁迫下拟南芥净光合速率下降、气孔导度下降和胞间CO2浓度减小。气孔因素是引起拟南芥光合能力下降的主要因素。叶绿素荧光参数的变化表明, 50-200 mmol.L-1 NaCl降低拟南芥叶绿体对光能的吸收能力, 而且降低叶绿体的光化学活性, 使电子传递速率和光能转化效率大幅度下降,造成光能转化为化学能的过程受阻,进一步加剧了光合放氧和碳同化能力的降低。而50-200 mmol.L-1 NaCl 胁迫没有使盐芥的光合作用受到不良影响。     

乙烯调控植物耐盐性的研究进展

乙烯具有复杂的生物学功能,它调节着植物生长发育和许多的生理生化过程。乙烯也被认为是一种胁迫应答激素,直到近几年关于乙烯生物合成及信号转导途径与植物盐胁迫的关系才逐渐被挖掘出来。乙烯在不同水平、层次参与盐胁迫反应,包括乙烯合成关键酶(ACS)和乙烯受体,细胞质中CTR1和EIN2以及细胞核中EIN3传导、响应盐信号。但是乙烯合成和信号转导途径在植物盐胁迫响应过程中仍然存在许多未解决的问题。主要介绍乙烯合成及信号转导途径的各组分与盐胁迫关系的最新研究进展,并讨论其存在的主要问题。     

谷胱甘肽转移酶基因过量表达能加速盐胁迫下转基因拟南芥的生长

盐地碱蓬谷胱甘肽转移酶基因(glutathione s-transferase gene,GST)克隆到植物表达载体pROKⅡ35s启动子的下游,通过农杆菌介导,利用花絮浸泡法转化拟南芥.转化子在含有卡那霉素的培养基上经过筛选以后,将初步验证为阳性的转基因植株通过PCR-Southem进一步证实.经过选育,筛选并分离到卡那霉素的抗性并且遗传稳定的T3代纯合子转基因拟南芥品系.通过Northern杂交证实外源基因在转基因拟南芥中表达.在盐胁迫条件下,通过测量转基因植株(GT)和野生型植株(wY)的生物量和谷胱甘肽(氧化型:GSSG;还原型:GsH)发现:转基因植株的生物量较野生型有一定程度的提高;GssG含量在转基因品系中比野生型的含量明显高.因此,过量表达GsT能够提高转基因植株在盐胁迫条件下的生长,而且这很可能是由于还原型谷胱甘肽被氧化的结果.     

氯盐胁迫下氮素对西瓜根系生长的调控作用

为揭示氯盐胁迫下氮素对西瓜根系的调节机制和提供西瓜氯毒害调控理论依据,以西瓜为供试作物,采用土培试验,研究不同施氮量(0,0.1,0.15,0.2,0.25 g/kg)对氯盐胁迫下西瓜根系的影响,并应用主成分分析法对各施氮量下根系生长情况进行综合评价。结果表明,(1)与不施氮相比,施氮0.15 g/kg处理可使西瓜根系生物量、干物质累积量、脯氨酸含量、可溶性糖含量、根系活力分别显著提高58.83%、20.83%、98.33%、70.37%和29.44%,丙二醛含量显著降低40.30%,同时使总根长、总根表面积、根尖数、分枝数分别显著增加103.42%、46.41%、64.44%、87.80%,总根体积和总根系直径分别减少23.05%和40.15%。(2)在本试验氯盐胁迫条件下,施氮0.14~0.17 g/kg时西瓜具有较理想的根系构型和较高的根系活力。(3)根系分枝数、根系活力、总根体积、根尖数可作为氯盐胁迫下氮素对西瓜根系生长影响的综合评价指标,各施氮水平对氯盐胁迫的缓解效果表现为0.15 g/kg>0.20 g/kg>0.10 g/kg>0.25 g/kg。可见,在氯盐胁迫下,适量施氮有助于西瓜建立良好的根系构型,提高根系渗透物质含量,降低细胞渗透势,减少根系丙二醛含量,维持较强的根系活力,增加根系生物量和干物质,缓解高浓度氯盐对西瓜生长的抑制作用。     

拟南芥ANAC055基因突变体对高盐和渗透胁迫的响应

高盐和渗透等非生物胁迫是影响农作物产量和品质的重要因素,非生物胁迫发生时,植物通过体内各类转录因子启动胁迫应答反应,进而降低非生物胁迫对植物的损伤。本研究筛选出植物特异性转录因子ANAC055编码基因的纯合T-DNA插入突变体SALK_152738,测序分析发现T-DNA插在ANAC055基因的3'UTR区域。实时荧光定量PCR结果表明叶中ANAC055基因表达量最高;与野生型相比,突变体叶、茎和花中ANAC055基因表达量分别下降了40%、50%和70%。高盐胁迫后,野生型和突变体叶中ANAC055基因表达量分别比对照上升了320%和55.4%;而渗透胁迫时,该基因叶中的表达量分别比对照下降了47.7%和56.3%;电子表达谱分析发现该基因根中的表达可受高盐和渗透等多种非生物胁迫的诱导表达。高盐和渗透胁迫时野生型和突变体幼根的生长均受到明显抑制,但高盐胁迫对突变体根生长的抑制作用比对野生型根生长的抑制作用更大。上述分析表明拟南芥ANAC055基因可受高盐和渗透等非生物胁迫的诱导表达,并且其在拟南芥幼根的生长发育过程中具有一定的作用,本研究有助于进一步明确其在非生物胁迫过程中的作用。     

Ca2+在植物盐胁迫响应机制中的调控作用

对植物而言,Ca2+不仅作为一种必须的营养元素,更重要的是作为耦联胞外信号与胞内生理反应的第二信使,当植物受到外界的环境刺激时,细胞中Ca2+会出现变化,引起一系列保护性生理反应,从而减轻环境胁迫对植物体的伤害.我国盐碱地面积广阔,极大地限制了作物种植和农业生产.大量研究表明,Ca2+可以提高植物对盐胁迫的抗性,针对盐胁迫对植物的伤害机制,重点讨论了盐胁迫条件下Ca2+参与的植物体内有关响应途径及作用机制.     

Response to Salinity in Legume Species: An Insight on the Effects of Salt Stress during Seed Germination and Seedling Growth

The process of soil salinization and the preponderance of saline water sources all over the world represent one of the most harmful abiotic stress to plant growth. This pointed to the importance of obtaining plants which are tolerant or resistant to salt, considering that projection of climate change for the coming years indicate an increase in temperature and rain scarcity. In the current study, the effect of NaCl was investigated on germinating seeds of Lathyrus sativus L., Vicia sativa L., Vigna radiata L. R.Wilczek and Vigna unguiculata L. Walp., by combining physiological, biochemical, biostatistical and ultrastructural analyses. Our results revealed that germination was not influenced by high NaCl concentrations, while seedling growth was affected even at low NaCl concentrations, probably due to an alteration in water uptake and in organic matter biosynthesis. Nevertheless, the synthesis of antioxidant enzymes, phenolic acids and flavonoids was registered in all species, which tended to cope with the increasing salt stress, allowing a response mechanism such as cytoplasm detoxification and cellular turgor maintenance. Besides, the ultrastructural analysis evidenced plasmolyzed cells close to cells with a normal ultrastructure with no appreciable differences among the species. This research deeply investigates the mechanism of salt-stress response focusing on species never tested before for their possible tolerance to salinity.     

Rapid Response of the Yield Threshold and Turgor Regulation during Adjustment of Root Growth to Water Stress in Zea mays

Responses of cortical cell turgor (P) following rapid changes in osmotic pressure ([pi]m) were measured throughout the elongation zone of maize (Zea mays L.) roots using a cell pressure probe and compared with simultaneously measured root elongation to evaluate: yield threshold (Y) (minimum P for growth), wall extensibility, growth-zone radial hydraulic conductivity (K), and turgor recovery rate. Small increases in [pi]m (0.1 MPa) temporarily decreased P and growth, which recovered fully in 5 to 10 min. Under stronger [pi]m (up to 0.6 MPa), elongation stopped for up to 30 min and then resumed at lower rates. Recoveries in P through solute accumulation and lowering of Y enabled growth under water stress. P recovery was as much as 0.3 MPa at [pi]m = 0.6 MPa, but recovery rate declined as water stress increased, suggesting turgor-sensitive solute transport into the growth zone. Under strong [pi]m, P did not recover in the basal part of the growth zone, in conjunction with a 30% shortening of the growth zone. Time courses showed Y beginning to decrease within several minutes after stress imposition, from about 0.65 MPa to a minimum of about 0.3 MPa in about 15 min. The data concerning Y were not confounded significantly by elastic shrinkage. K was high (1.3 x 10-10 m2 s-1 MPa-1), suggesting very small growth-induced water potential gradients.     

Single-Molecule Imaging of mRNA Localization and Regulation during the Integrated Stress Response

1. Download high-res image (201KB)
2. Download full-size image