盐地碱蓬叶片液泡膜H^＋—ATPase B亚基的克隆及盐胁迫下表达分析

植物液泡膜H^ -ATPase在建立跨液泡膜质子梯度、促进液泡Na^ 区域化、提高植物耐盐性方面发挥着重要作用。本实验从盐生植物盐地碱蓬(Suaeda salsa L.)cDNA文库分离到碱蓬叶片液泡膜H^ -ATPase B亚基cDNA克隆。测序表明该基因长达1974bp,开放阅读框有1470bp编码489个氨基酸,含有一个保守的ATP结合位点,其蛋白分子量约为54．29kD。Northern及Western印迹表明盐地碱蓬液泡膜H^ -ATPase B亚基表达明显受NaCl胁迫诱导,并且在NaCl胁迫下,B亚基在转录及翻译水平上与液泡膜H^ -ATPase c亚基存在协同作用。盐胁迫下,盐地碱蓬液泡H^ -ATPase B亚基与c亚基的协同表达增加了液泡H^ -ATPase的数量,从而提高了液泡H^ -ATPase活性,为碱蓬叶片液泡Na^ 区域化提供了动力,最终提高了碱蓬植株的耐盐性。     

盐胁迫下盐地碱蓬叶片液泡膜H+-ATPase H 亚基的克隆与表达分析

利用EST随机挑取克隆测序的方法从盐地碱蓬叶片cDNA文库中分离得到了盐地碱蓬V-H -ATPase H亚基cDNA序列,并进行了H、c亚基基因表达及V-H -ATPase活性分析.结果表明,H亚基基因全长1 969 bp,包括100 bp的5′-非编码区和471 bp的3′-非编码区.开放阅读框为1 398 bp,编码465个氨基酸残基,分子量约52.8 kD.N orthern杂交分析表明盐胁迫明显诱导了H亚基表达,而且盐胁迫下H、c亚基及V-H -ATPase活性存在协同作用.这些结果表明盐胁迫下H和c亚基基因上调及V-H -ATPase活性的增加为N a 区隔化到液泡中提供了质子驱动力.     

K+营养对NaCl胁迫下盐地碱蓬生长及叶片液泡膜V-H+-ATPase和V-H+-PPase活性的影响

对溶液培养的盐地碱蓬(Suaeda salsa L.)幼苗进行不同浓度NaCl胁迫并改变培养液中K+浓度,以了解K+营养对NaCl胁迫下盐地碱蓬幼苗生长及叶片液泡膜V-H+-ATPase、V-H+-PPase活性的影响.提高培养液K+浓度可明显增加盐胁迫下碱蓬植株的鲜重、干重,促进盐地碱蓬叶片及根部组织K+积累.盐地碱蓬叶片液泡膜V-H+-ATPase至少由A、B、C、D、E及c亚基组成,其表达量在缺K+处理(12 μmol/L K+)下随盐胁迫浓度的增加而减小,而在正常K+(6 mmol/L)培养下则随盐胁迫浓度的增加而增加;盐地碱蓬叶片液泡膜V-H+-PPase分子量为72 kD,在缺K+和正常K+供应情况下,V-H+-PPase均有较高表达.V-H+-ATPase及V-H+-PPase活性变化与其亚基表达量变化基本成正相关.结果表明: K+对盐生植物碱蓬的耐盐性有重要作用,盐胁迫下,K+可能参与了V-H+-ATPase和V-H+-PPase活性调控.     

K^＋营养对NaCl胁迫下盐地碱蓬生长及叶片液泡膜V—H^＋—ATP和V—H^＋—PPase活性的影响

对溶液培养的盐地碱蓬（Suaeda salsa L.)幼苗进行不同浓度NaCl胁迫并改变培养液中K^ 浓度,以了解K^ 营养对NaCl胁迫下盐地碱蓬幼苗生长及叶片液泡膜V－H^ -ATPase、V－H^ -PPase活性的影响。提高培养液K^ 浓度可明显增加盐胁迫下碱蓬植株的鲜重、干重,促进盐地碱蓬叶片及根部组织K^ 积累。盐地碱蓬叶片液泡膜V－H^ -ATPase至少由A、B、C、D、E及c亚基组成,其表达量在缺K^ 处理（12μmol/L K^ )下随盐胁迫浓度的增加而减小,而在正常K^ （6mmol/L)培养下则随盐胁迫浓度的增加而增加;盐地碱蓬叶片液泡膜V－H^ -PPase分子量为72kD,在缺K^ 和正常K^ 供应情况下,V－H^ -PPase均有较高表达。V－H^ -ATPase及V－H^ -PPase活性变化与其亚基表达量变化基本成正相关。结果表明：K^ 对盐生植物碱蓬的耐盐性有重要作用,盐胁迫下,K^ 可能参与了V－H^ -ATPase和V－H^ -PPase活性调控。     

K~ 营养对NaCl胁迫下盐地碱蓬生长及叶片液泡膜V-H~ -ATPase和V-H~ -PPase活性的影响(英文)

对溶液培养的盐地碱蓬 (SuaedasalsaL .)幼苗进行不同浓度NaCl胁迫并改变培养液中K 浓度 ,以了解K 营养对NaCl胁迫下盐地碱蓬幼苗生长及叶片液泡膜V_H _ATPase、V_H _PPase活性的影响。提高培养液K 浓度可明显增加盐胁迫下碱蓬植株的鲜重、干重 ,促进盐地碱蓬叶片及根部组织K 积累。盐地碱蓬叶片液泡膜V_H _ATPase至少由A、B、C、D、E及c亚基组成 ,其表达量在缺K 处理 (12 μmol/LK )下随盐胁迫浓度的增加而减小 ,而在正常K (6mmol/L)培养下则随盐胁迫浓度的增加而增加 ;盐地碱蓬叶片液泡膜V_H _PPase分子量为 72kD ,在缺K 和正常K 供应情况下 ,V_H _PPase均有较高表达。V_H _ATPase及V_H _PPase活性变化与其亚基表达量变化基本成正相关。结果表明 :K 对盐生植物碱蓬的耐盐性有重要作用 ,盐胁迫下 ,K 可能参与了V_H _ATPase和V_H _PPase活性调控     

NaCl胁迫对盐芥质膜和液泡膜ATPase活性的影响

以盐生植物盐芥和中生植物拟南芥幼苗为材料,研究了盐胁迫对它们叶片和根质膜、液泡膜H+-ATPase、Ca2+-ATPases和K+-ATPase活性以及H+-ATPase、Na+/H+ 逆向转运蛋白表达的影响.结果显示:在NaCl胁迫下,盐芥叶片和根质膜的H+-ATPase活性分别比对照显著升高41%～212%和35%～53%,液泡膜的H+-ATPase分别显著升高281%～373%和4%～38%,而拟南芥却比相应对照都显著降低;相同盐浓度胁迫下,盐芥叶片的H+-ATPase活性比根部高4～8倍,盐芥根也远高于拟南芥.在NaCl胁迫下,盐芥叶片和根的液泡膜H+-ATPase蛋白质β亚基含量变化与其酶活性变化趋势一致,质膜Na+/H+ 逆向转运蛋白的表达量与Na+含量变化趋势一致.盐胁迫下盐芥根中Ca2+-ATPases和K+-ATPase活性的增加与根中Ca2+和K+含量呈显著正相关.研究发现,在盐胁迫条件下,盐芥能有效增强H+-ATPase蛋白和Na+/H+逆向转运蛋白表达,显著提高其根系与叶片质膜和液泡膜的H+-ATPase、Ca2+-ATPase和K+-ATPase活性,维持细胞质中较高的Ca2+和K+水平,从而缓解盐胁迫的伤害,增强耐盐性.     

NaCl和Na2CO3对盐地碱蓬胁迫效应的比较

在相同的Na 浓度(如100 mmol/L)下,NaCl处理促进碱蓬植株干重增加,提高根系活力,而Na2CO3处理导致植株干重减少,根系活力降低;与NaCl胁迫相比,Na2CO3胁迫下叶片内Na 含量上升和K 含量下降幅度更大,叶肉细胞质Na 含量和叶内脯氨酸含量增加幅度更大,而V-H -ATPase(液泡膜H -ATPase)和V-H -PPase (液泡膜H -PPase)增加幅度较少;与NaCl胁迫不同,Na2CO3胁迫下SOD(超氧化物歧化酶)活性不是增加,而是降低,与此相一致,MDA(丙二醛)含量大幅度增加.上述结果表明,碱蓬对Na2CO3胁迫的抗性低于对NaCl的抗性,这可能与Na2CO3胁迫引起的Na 、K 离子严重失衡、活性氧清除能力降低有关.     

NaCl胁迫对高粱根、叶鞘和叶片液泡膜ATP酶和焦磷酸酶活性的影响

NaCl胁迫初期 ,Na 主要在根和叶鞘中积累。相应地 ,根和叶鞘液泡膜ATP酶和焦磷酸酶水解活性、依赖ATP和PPi的质子泵活性及Na /H 逆向转运活性均明显增加 ,根和叶鞘的生长没有受到抑制。NaCl胁迫后期 ,Na 开始向地上部分运输并在叶片中积累。此时 ,叶片液泡膜质子泵和Na /H 逆向转运活性开始增加 ,根和叶鞘的Na/K比增加 ,其液泡膜ATP酶和焦磷酸酶水解活性、质子泵活性和Na /H 逆向转运活性下降。相应地 ,根和叶鞘的生长也下降。当保温介质中Na/K比超过 1时 ,液泡膜微囊ATP酶和焦磷酸酶活性均随Na/K比的增加而下降。表明非盐生植物液泡膜质子泵在盐胁迫的初期对Na 在液泡内的积累及其耐盐性起重要作用     

NaCl胁迫对宁夏枸杞幼苗根系质膜和液泡膜H+-ATPase活性的影响

以宁夏枸杞为材料,研究NaCl胁迫下枸杞幼苗组织含水量、干物质重量、无机离子分布、质膜透性、丙二醛 (MDA)含量及幼根质膜、液泡膜H -ATPase活性和耐盐性之间的关系。结果表明,在0．3％NaCl胁迫下,干物质重量、质膜透性、MDA含量略有增加,组织含水量略有下降;随着NaCl胁迫强度的增加,Na 、Cl-含量逐渐增加, K 含量则呈现下降的趋势;质膜透性增大与MDA含量升高呈显著正相关;质膜和液泡膜H -ATPase活性逐渐增加,且液泡膜H -ATPase活性显著高于质膜H -ATPase活性,表明枸杞具有较强的抗盐性。     

盐胁迫对豌豆根液泡膜H^＋—ATPase活性及含量的影响

为了阐明液泡膜H^ -ATPase在盐胁迫下的作用和适应性调节机制,对豌豆（Pisum sativum L.）植株进行不同盐浓度和不同盐胁迫时间（1－3d）的处理后,分别测定液泡膜H^ -ATPase的H^ 转运活性、水解性和蛋白含量（A亚基）的变化。结果表明,100mmol/L和200mmol/L NaCl 处理1dH^ -ATPase的水解活性没有变化,而250mmol/L NaCl处理1d引起水解活性降低约25％。100mmol/L NaCl处理2d内水解活性没有变化,而第3天活性下降约20％。但是上述盐胁迫均能提高液泡膜H^ -ATPase的质子转运活性,说明盐胁迫后H^ -ATPase的水解活性和质子转运活性的变化不成比例,盐胁迫可能导致偶联比率的改变。Western blot研究发现,上述盐胁迫对液泡膜H^ -ATPase（A亚基）的含量基本无影响,仅100mmol/L NaCl处理3d后A亚基的量略有下降,这些结果证明,盐胁迫能刺激提高豌豆根液泡膜H^ -ATPase的H^ 泵效率,且泵效率的提高是源于偶联比率的改变,而不是由于ATP水解活性的提高和蛋白含量的增加。     

一氧化氮调节盐胁迫下小麦幼苗根部质膜H+-ATPase和焦磷酸酶活性提高耐盐性

采用外源一氧化氮(NO)供体硝普钠(SNP)研究了NO对盐胁迫下小麦(Triticum aestivum L.)幼苗耐盐性的影响.结果表明,0.1 mmol/L SNP处理显著缓解了1 50 mmol/L NaCl胁迫对小麦幼苗生长的抑制效应,包括水分丧失以及叶绿素降解,从而提高了小麦幼苗的耐盐性.进一步结合1 mg/mL血红蛋白处理则显著逆转了SNP诱导的上述效应;利用亚硝酸钠和铁氰化钾作为对照也证实了NO对小麦幼苗耐盐性的专一性调节作用,并可能与NO对小麦幼苗根部质膜H -ATPase和焦磷酸酶活性诱导有关.此外,尽管NO显著提高了盐胁迫下小麦幼苗根部细胞质膜H -ATPase和焦磷酸酶的ATP水解活性,但是对跨膜H 转运则没有明显影响.应用外源CaSO4和EGTA处理也证实,Ca2 可能在NO诱导的质膜H -ATPase和焦磷酸酶活性的提高过程中起信号作用.另外,分析盐胁迫下小麦幼苗根部Na 和K 含量的变化也发现,NO对Na 含量没有明显影响,但是却显著提高了K 水平和K /Na 比,这可能也是NO提高小麦幼苗耐盐性的原因之一.     

NaCl-induced accumulation of tonoplast and plasma membrane H+-ATPase message in tomato

NaCl-induced changes in the accumulation of message for the 70 kDa subunit of the tonoplast H⁺-ATPase and plasma membrane H⁺-ATPase were studied in hydroponically grown plants of Lycopersicon esculentum Mill. cv. Large Cherry Red. There was increased accumulation of message for the 70 kDa (catalytic) subunit of the tonoplast H⁺-ATPase in expanded leaves of tomato plants 24 h after final NaCl concentrations were attained. This was a tissue-specific response; levels of this message were not elevated in roots or in young, unexpanded leaves. The NaCl-induced accumulation of this message was transient in the expanded leaves and returned to control levels within 7 days. The temporal and spatial patterns of NaCl-induced accumulation of message for the plasma membrane H⁺-ATPase differed from the patterns associated with the 70 kDa subunit of the tonoplast H⁺-ATPase. NaCl-induced accumulation of the plasma membrane H⁺-ATPase message occurred in both roots and expanded leaves. Initially accumulation of the plasma membrane H⁺-ATPase message was greater in root tissue than in expanded leaves, but increased to higher levels in expanded leaves after 7 days. These results suggest that increased expression of the tonoplast H⁺-ATPase is an early response to salinity stress and may be associated with survival mechanisms, rather than with long-term adaptive processes.     

Two Na^＋ and Cl^- Hyperaccumulators of the Chenopodiaceae

The authors found five sodium (Na^ ) and chloride (Cl^-) hyperaccumulating halophytes in the Temperate Desert of Xinjiang, China and studied two of them (Suaeda salsa (L.) Pall. and Kalidium folium (Pall.) Moq.). K. folium and S. salsa had a NaCl content of 32.1% and 29.8%, respectively, on a dry weight basis. X-ray microanalysis of the Na in the vacuole, apoplasts and cytoplasm of the two plants indicated a ratio of 7.3:5.6:1.0 in K. folium and 7.3:6.6:1.0 in S. salsa. These data show that K. folium and S. salsa both have a high Na and Cl^- accumulating capacity, which is related to high activity of tonoplast H^ -ATPase and H^ -PPase.     

盐度和CO2倍增环境下碱蓬幼苗呼吸酶活性的变化

研究了生长在正常大气CO₂和CO₂倍增环境中的盐生植物碱蓬(Suaedasalsa)幼苗呼吸酶活性对KCl和NaCl的反应。结果表明,在CO₂倍增(700μl·L^-1)和正常大气CO₂(350μl·L^-1)下,300mmol·L^-1KCl和NaCl均能抑制琥珀酸脱氢酶(SDH)和苹果酸脱氢酶(MDH)活性,而异柠檬酸脱氢酶(IDH)活性为NaCl抑制、KCl促进; NaCl和KCl明显抑制细胞色素氧化酶(CO)和光呼吸中乙醇酸氧化酶(GO)、羟基丙酮酸还原酶(HPR)活性; 并指出在KCl胁迫下,CO₂使三羧酸循环(TCAC)的运行变慢,NaCl胁迫下使其加快,TCAC运行限速步骤与MDH无关,CO为盐对呼吸代谢影响的重要位点。另外,K⁺、Na⁺对蛋白表达的影响有差异,CO₂可使盐胁迫下的碱蓬幼苗蛋白表达降低。     

Phosphorylation-dephosphorylation of membrane proteins controls the microsomal H-ATPase activity of corn roots

The Mg²⁺-dependent H⁺-ATPase activity of a sealed microsomal vesicle fraction isolated from corn (Zea mays L.) roots appears to be controlled by a phosphorylation-dephosphorylation cycle. Phosphorylation of the microsomal fraction is carried out by a Ca²⁺/calmodulin (CaM)-stimulated process. The H⁺-ATPase activity decreases with increasing phosphorylation of the membranes and becomes only slightly uncoupled by ionophores and less inhibited by dicyclohexylcarbodiimide (DCCD), diethylstilbestrol (DES), NO₃⁻ and vanadate. The inhibitory effect of phosphorylation is greater on the NO₃⁻-sensitive H⁺-ATPase activity than on the vanadate-sensitive activity. Restoration of H⁺-ATPase activity is achieved by allowing the phosphorylated membranes to dephosphorylate either in the absence or presence of exogenous alkaline phosphatase. Moreover, the presence of fluphenazine during the Ca²⁺/CaM-stimulated treatment inhibits membrane phosphorylation and protects the H⁺-ATPase activity from inhibition.     

磷饥饿对番茄幼苗H+分泌及Pi吸收的影响

磷饥饿条件下番茄幼苗的H⁺分泌速率明显提高。质膜质子泵专一性抑制剂钒酸盐能显著抑制番茄幼苗的H⁺分泌,也能显著抑制其Pi吸收。此结果表明,磷饥饿时番茄幼苗Pi吸收速率的变化与H⁺分泌速率的变化之间可能具有一定的相关性,并进一步暗示质膜H⁺-ATPase可能参与其中。本文结果还表明,Pi/H⁺的准量关系约为1:1。     

Specific regulation of SOD isoforms by NaCl and osmotic stress in leaves of the C3 halophyte Suaeda salsa L

The halophyte Suaeda salsa L., exposed to different NaCl concentrations (100 and 400 mmol/L) and polyethylene glycol (isoosomotic to 100 mmol/L NaCl) containing nutrient solutions under normal or K+-deficient conditions for 7 days, was used to study effects of NaCl salinity and osmotic stress on chlorophyll content, chlorophyll fluorescence characteristics, malonedialdehyde (MDA) content, and superoxide dismutase (SOD) isoform activities. Photosynthetic capacity was not decreased by NaCl treatment, indicating that S. salsa possesses an effective antioxidative response system for avoiding oxidative damage. Seven SOD activity bands were detected in S. salsa leaf extracts, including an Mn-SOD and several isoforms of Fe-SOD and CuZn-SOD. It turned out that NaCl salinity and osmotic stress lead to a differential regulation of distinct SOD isoenzymes. This differential regulation is suggested to play a major role in stress tolerance of S. salsa.     

Influence of ATPase activity on PPi dependent H-transport in tonoplast vesicles of Acer pseudoplatanus

Tonoplast H⁺-ATPase and H⁺-pyrophosphatase (H⁺-PPase) were previously characterized in Acer pseudoplatanus cells (A. Pugin et al., Plant Sci., 73 (1991) 23–34; A. Fraichard et al., Plant Physiol. Biochem., 31 (1993) 349–359). The present study concerns the relationships between these two enzymes in vitro. ATP and PPi hydrolysis were additive and the inhibition of one did not affect the activity of the second one. ATP and PPi H⁺-transports were also additive. The H⁺ -PPase inhibition did not change ATP-dependent H⁺-transport but H⁺-ATPase inhibition inhibited the PPi dependent H⁺-transport. Because H⁺-PPase was reported to transport H⁺ and K⁺ into the vacuole (Davies et al., Proc. Natl. Acad. Sci. USA, 89 (1992) 11701–11705), these results led us to suggest that the inhibition of the H⁺-ATPase activity could modify the H⁺/K⁺ stoichiometry for the benefit of K⁺-transport.