低温光抑制恢复过程中黄瓜叶片PSⅡ活性及其电子传递对PSⅠ的影响

以“津春4号”黄瓜为试材,通过测定黄瓜叶片叶绿素荧光快速诱导动力学曲线和对820 nm光的吸收曲线,结合叶绿素荧光淬灭分析,研究低温光胁迫(4℃,200 μmol·m-2·s-1)6 h后,黄瓜叶片在常温(25℃)不同光强(0、15、200μmol·m-2·s-1)下PS Ⅰ和PS Ⅱ活性的恢复,以及恢复过程中PS Ⅰ与PS Ⅱ的相互作用.结果表明:低温光胁迫6h后,PS Ⅰ和PS Ⅱ发生不同程度的光抑制.在常温恢复阶段,PS Ⅱ活性快速恢复且对光强不敏感;PS Ⅰ活性在弱光下(15 μmol·m-2·s-1)快速恢复,在较强光(200 μmol·m-2·s-1)下恢复较慢.在低温光抑制恢复过程中,常温下PS Ⅱ活性恢复较快可能导致PS Ⅱ向PS Ⅰ的线性电子传递过快,进而抑制PS Ⅰ的活性恢复.因此,在进行黄瓜抗冷性育种时,不应该仅追求较高的PS Ⅱ抗性和较快的PS Ⅱ恢复速度,还应该注意两个光系统活性的协调.在生产中,应当在低温逆境发生及其之后较长一段时间内采取措施降低叶表面光照强度,以利于对植株光合机构的保护和光合活性的恢复.     

三种常绿阔叶树光系统Ⅱ在低温胁迫下的光抑制及恢复

冬季低温胁迫对亚热带常绿阔叶树光合活性的主要影响之一,体现在光合机构的低温光抑制。为了阐明冬季低温胁迫下常绿阔叶树光系统Ⅱ的光抑制程度及光保护机制,该文研究了冬季自然低温胁迫(零下低温冻害和零上低温寒害)对红叶石楠、枇杷和猴樟三种亚热带常绿阔叶树光合机构光系统Ⅱ(PSⅡ)光抑制的影响以及春季气温回暖后的恢复情况。结果表明:冻害和寒害低温胁迫使猴樟的PSⅡ活性显著降低,PSⅡ受到较严重的光抑制,低温胁迫解除后PSⅡ活性未能完全恢复。红叶石楠PSⅡ活性下降程度和光抑制程度最轻,春季PSⅡ活性显著上升,光抑制显著下降。枇杷PSⅡ活性和光抑制程度介于猴樟和红叶石楠之间。低温胁迫下红叶石楠的非光化学猝灭(NPQ)接近常温水平; 枇杷的NPQ略有降低,春季恢复正常; 猴樟NPQ最低,春季低温解除后仍不能完全恢复。此外,三种常绿阔叶树在冬季低温胁迫和春季恢复时期的NPQ与PSⅡ的光抑制程度存在显著的负相关关系。综合以上结果分析表明,冬季低温对红叶石楠PSⅡ影响不大,对枇杷有一定影响但春季气温回暖后可以及时恢复,对猴樟PSⅡ有显著的光抑制且恢复过程较慢,同时NPQ对保护常绿阔叶树PSⅡ免受冬季低温光抑制有重要的贡献。     

平板式光生物反应器中紫球藻培养条件的优化

研究了平板式光生物反应器中紫球藻(Porphyridium cruentumNaegeli)的培养条件,运用均匀设计法对光照强度、通气速率、装液量、接种密度以及pH等影响紫球藻生长的因素进行优化,获得了在平板式光生物反应器中培养紫球藻的最佳条件:光照强度10 000 lx、通气速率350 L.h-1、装液量6 L、藻细胞接种密度1.1×106mL-1、pH9.0。在最佳条件下藻体的生物量产率和生物量产量分别达到0.431 g.L-1.d-1和3.240 g.L-1,最大生长速率达0.652 g.L-1.d-1,胞外多糖含量高达0.665 g.L-1。另外,在培养过程中隔天补充培养液有利于紫球藻生物量的增加和胞外多糖的产生。     

在盐胁迫下光抑制及其恢复进程对冬小麦光合功能的影响(英文)

研究了盐和强光双重胁迫以及在弱光下恢复对冬小麦 (TriticumaestivumL .)光合功能的影响。结果表明 ,单纯用低浓度盐 (2 0 0mmol/LNaCl)胁迫时 ,对反映PSⅡ光合功能的Fv/Fo、Fv/Fm和qP等参数没有什么影响 ,但已十分明显地抑制光合碳同化能力 ,而高盐 (4 0 0mmol/LNaCl)胁迫损伤PSⅡ功能 ,从而加剧对碳同化功能的抑制 ,说明光合作用对不同盐浓度的响应不同。研究结果还表明 ,盐胁迫能加剧强光对光合功能的损伤 ,使之受到更加严重的光抑制。在低盐浓度下 ,光抑制初期形成的QB_非还原性PSⅡ反应中心 ,在随后的光抑制进程和弱光下恢复期间 ,能有效的被用来合成有活性的PSⅡ和修复可逆性失活的PSⅡ反应中心。而高盐和强光双重胁迫使PSⅡ遭受严重破坏 ,QB_非还原性PSⅡ反应中心只有在光抑制初期可部分地用于修复可逆性失活的PSⅡ ,随着光抑制的进程 ,它们不能用于合成有活性PSⅡ和修复受严重破坏的PSⅡ ,结果导致它们的含量在弱光下恢复时继续增加     

在盐胁迫下光抑制及其恢复进程对冬小科光合功能的影响

研究了盐和强光双重胁迫以及在弱光下恢复对冬小麦（Triticum aestivum L.）光合功能的影响。结果表明,单纯用低浓度盐（200mmol/L NaCl）胁迫时,对反向PSⅡ光合功能的Fv/Fo、Fv/Fm和qP等参数没有什么影响,但巳十分明显地抑制光合碳同化能力,而高盐（400mmol/L NaCl）胁迫损伤PSⅡ功能,从而加剧对碳同化功能的抑制,说明光合作用对不同盐浓度的响应不同。研究结果还表明,盐胁迫能加剧强光对光合功能的损伤,使之受到更加严重的光抑制。在低盐浓度下,光抑制初期形成形成QB-非还原性PSⅡ反应中心,在随后的光抑制进程和弱光下恢复期间,能有效的被用来合成有活性的PSⅡ和修复可逆性失活的PSⅡ反应中心。而高盐和强光双重胁迫使PSⅡ遭受严重破坏,QB-非还原性PSⅡ反应中心只有在光抑制初期可部分地用于修复可逆性失活的PSⅡ,随着光抑制的进程,它们不能用于合成有活性PSⅡ和修复受严重破坏的PSⅡ,结果导致它们的含量在弱光下恢复时继续增加。     

夜间低温对不同光强下生长的两种沟谷雨林树苗荧光参数的影响

 于雾凉季测定了叶片叶绿素荧光参数,探讨了4～6 ℃夜间低温对4种相对光强下生长的两种西双版纳沟谷雨林树苗光系统Ⅱ（PSⅡ）活性的影响及雾对植物的可能保护机制。随夜间低温处理时间延长,不同光强下生长的团花树（Anthocephalus chinensis）和玉蕊（Barringtonia macrostachya）叶片日间和长期光抑制,以及PSⅡ反应中心的可逆失活或破坏加剧,生长环境光越强夜间低温的效应越明显,弱光下其效应不显著。间接表明雾使光强减弱利于缓解自然夜温降低对本区热带植物的影响。中光强下玉蕊对照植株发生了胁迫诱导的光抑制;相同处理条件下玉蕊的光抑制程度均比团花树重,表明玉蕊对夜间低温引起的光抑制更敏感。夜间低温处理后,中等和低光强下团花树的热耗散多于玉蕊,表明其光保护作用较强。夜间低温处理期间两种植物的光抑制与热耗散增多和PSⅡ反应中心的可逆失活或破坏的加剧有关。     

NaCl胁迫加重强光胁迫下超大甜椒叶片的光系统Ⅱ和光系统Ⅰ的光抑制

快速叶绿素荧光动力学可以在无损情况下探知叶片光合机构的损伤程度,快速叶绿素荧光测定和分析技术(JIP-test)将测量值转化为多种具有生物学意义的参数,因而被广泛应用于植物光合机构对环境的响应机制研究.该文研究了超大甜椒(Capsicum annuum)幼苗在强光及不同NaCl浓度胁迫下的荧光响应情况.与单纯强光胁迫相比,NaCl胁迫引起了叶绿素荧光诱导曲线的明显改变,光系统Ⅱ(PSⅡ)光抑制加重,同时PSⅡ反应中心和受体侧受到明显影响,而且高NaCl浓度胁迫下PSⅡ供体侧受伤害明显,同时PSⅠ反应中心活性(P700+)在盐胁迫下明显降低.这些结果表明,NaCl胁迫会增强强光对超大甜椒光系统的光抑制,并且浓度越高抑制越明显,但对PSⅠ的抑制作用低于PSⅡ.高NaCl浓度胁迫易对PSⅡ供体侧造成破坏,且PSⅠ光抑制严重.     

脱落酸对紫球藻（Porphyridiu sp.）生长代谢的影响

为优化培养条件和提高紫球藻(Porphyridiu sp.)生物量及代谢产物产量,研究了7种浓度的脱落酸(ABA)在三种氮素营养水平下对紫球藻生长的影响,结果表明,ABA浓度在0.01～1.0 mg·L-1范围内,外源ABA浓度的升高有利于紫球藻增殖,对紫球藻的干重、叶绿素a含量、蛋白质含量、胞外多糖含量、藻红素含量都有一定的促进作用;但在ABA浓度在10 mg·L-1时,则呈递抑制趋势.其中中氮水平下外源ABA浓度1.0 mg·L-1是紫球藻生长的最佳浓度,最有利于紫球藻生物量及代谢产物的积累,此时紫球藻的生物量为3.463 mg·mL-1,胞外多糖含量最高,占藻体干重的34.31%.在高氦营养水平下还能体现ABA对紫球藻生长所起的作用,而低氮下生长的紫球藻对ABA的作用不敏感.     

盐胁迫下菊芋根系脱落酸对钠离子转运和光系统Ⅱ的影响

通过根系施加脱落酸(ABA)合成抑制剂钨酸钠,研究盐胁迫(150 mmol·L^-1 NaCl)下菊芋根系ABA信号对根系Na⁺转运、叶片Na⁺积累和光系统Ⅱ(PSⅡ)的影响。结果表明:钨酸钠抑制盐胁迫下根系ABA合成,降低根系Na⁺外排,提高根系Na⁺向叶片的转运系数。盐胁迫增加叶片Na⁺含量,没有影响叶片膜脂过氧化、PSⅡ反应中心蛋白合成和PSⅡ最大光化学效率(F_v/F_m)。根系ABA合成受抑制,显著增加盐胁迫下叶片Na⁺积累,加剧叶片膜脂过氧化,损伤PSⅡ反应中心蛋白,显著降低F_v/F_m,诱发PSⅡ光抑制。总之,盐胁迫下菊芋根系ABA信号诱导根系Na⁺外排,抑制Na⁺向地上部转运,有利于减少叶片Na⁺积累,防御PSⅡ氧化损伤。     

低温弱光胁迫对野生大豆和大豆栽培种光系统功能的影响

以野生大豆和栽培大豆为材料,通过同时测定大豆叶片的叶绿素荧光快速诱导动力学曲线和对820nm光的吸收曲线,以及测定超氧化物歧化酶（SOD）和抗坏血酸过氧化物酶（APX）的活性,分析了低温弱光胁迫及常温弱光恢复下这2种大豆光系统Ⅱ（PSⅡ）和光系统Ⅰ（PSI）功能的变化。结果表明,低温弱光胁迫对这2种大豆的PSI和PSⅡ的功能都造成伤害;在低温弱光胁迫下,维持较高的SOD和APX活性和维持PSI和PSⅡ的协调性是野生大豆比栽培大豆耐低温的一个重要原因。     

低温胁迫下不同甘蔗品种(系)光合特性的变化及其与耐寒性的关系

以广西农科院甘蔗研究所自育的7个新材料和2个生产上的主栽品种为研究对象,在甘蔗苗期进行低温胁迫处理,研究了各品种(系)甘蔗形态特征的冷害指数、叶绿素含量及光合特性相关指标的变化及其光合特性相关指标与甘蔗抗寒性间的相关性。结果表明:随着低温胁迫处理时间的延长,冷害指数不断增大,但变化的大小与快慢因品种(系)不同表现不一样。各甘蔗品种(系)叶片叶绿素含量均随时间延长而降低。叶片净光合速率、气孔导度在低温处理与常温处理间具有显著差异。低温胁迫处理显著降低了各甘蔗品种(系)最大光化学效率(Fv/Fm)、PSⅡ实际光能转化效率ΦPSⅡ、光适应下PSⅡ反应中心的最大光能转化效率Fv′/Fm′、光化学猝灭系数qP、电子传递速率ETR,而显著提高了初始荧光Fo、稳态荧光Fs、非光化学猝灭系数qNP。相关性分析表明整个测定时期各指标间相关显著,Fv/Fm、Fv′/Fm′、ΦPSⅡ与冷害指数I之间的相关系数在0.800以上,Fv/Fm、Fv′/Fm′、ΦPSⅡ可以作为甘蔗品种(系)抗寒性鉴定的重要参考指标。     

外源Ca2+对高温强光胁迫下小麦叶绿体D1蛋白磷酸化及光系统Ⅱ功能的影响

用10 mmol·L^-1 CaCl₂溶液预处理灌浆期小麦叶片,以水预处理为对照,然后将预处理植株进行高温强光（35 ℃,1600 μmol·m^-2·s^-1）胁迫,测定胁迫处理过程中小麦旗叶光合电子传递速率、净光合速率、叶绿素荧光参数及D₁蛋白的变化,以研究外源Ca²⁺对高温强光胁迫下小麦叶片类囊体膜D₁蛋白磷酸化和PSⅡ功能的影响.结果表明：CaCl₂溶液预处理使小麦叶片在高温强光逆境下PSⅡ反应中心发生可逆失活,有效抑制了高温强光下D₁蛋白的净降解,保持了较高的D₁蛋白磷酸化水平,暗恢复后PSⅡ反应中心活性迅速恢复,全链电子传递速率和PSⅡ电子传递速率恢复至对照水平,维持了较高的PSⅡ原初光化学效率（F_v/F_m）、实际光化学效率(Ф_PSⅡ)、光化学猝灭系数（q_P）和净光合速率（P_n）.表明外源Ca²⁺通过调节小麦叶绿体D₁蛋白的周转,促进了PSⅡ的正常运转,减轻了高温强光胁迫对叶片光合机构的损伤.     

The Effects of Chilling Temperature on Photosystem II of Cucumber

Chilling (1 ℃ or 5℃, 16 h) treatment inhibited PSⅡ but not PSⅠ of photosynthesis in cucumber, a chilling sensitive plant. Oxygen evolution, variable fluorescence, and DCIP photoreduction were inhibited significantly, and the latter two could be recovered to the control level by adding artificial electron donors. These results suggest that chilling temperature damages PSⅡ of cucumber only on the oxidizing side and does not affect its reaction center.     

水杨酸对高温强光胁迫下小麦叶绿体D1蛋白磷酸化及光系统Ⅱ功能的影响

为了研究水杨酸（SA）对高温强光胁迫下小麦叶片类囊体膜D₁蛋白磷酸化和PSⅡ功能的影响,用0.5 mmol·L^-1 SA溶液预处理灌浆期小麦叶片,以水预处理为对照,然后将预处理植株进行高温强光（35 ℃,1 600 μmol·m^-2·s^-1）处理,测定胁迫处理过程中小麦旗叶光合电子传递速率、净光合速率、叶绿素荧光参数及D₁蛋白的变化.结果表明：SA预处理有效抑制了高温强光下D₁蛋白的净降解,保持了较高的D₁蛋白磷酸化水平、全链电子传递速率和PSⅡ电子传递速率,维持了较高的PSⅡ原初光化学效率（F_v/F_m）、实际光化学效率(Ф_PSⅡ)、光化学淬灭系数（q_P）和净光合速率（P_n）.表明外源SA通过调节小麦叶绿体D₁蛋白的周转,减轻了高温强光胁迫对叶片光合机构的损伤,有利于PSⅡ的正常运转.     

夜间高温胁迫对水稻叶片光合机构的影响

The net photosynthetic rate (Pn), the apparent quantum yield (AQY), the photochemical efficiency of PSⅡ(Fv/Fm), the quantum yield of PSⅡ electron transport (Ф PSⅡ) and the coefficient of photochemical quenching (qp) were decreased in rice (Oryza sativa L.) leaves under high nocturnal temperature (42±1) ℃ stress, but the relative reduction state of PSⅡ (1-qp) was increased. With the increment of stress time, the chlorophyll content and the binding degree of chlorophyll-protein complex declined gradually, the O2(superoxide radical) production rate and H2O2 content in leaves elevated. The activities of superoxide dismutase (SOD), peroxidase (POD) and catalase (CAT) increased for 2-3 days under high temperature stress yet decreased afterwards. The results showed that the photosynthetic efficiency declined in rice leaves under high nocturnal temperature stress with concurrent emergence of the symptom of oxidative damage. The gradual increase of the SOD, POD and CAT activities, as well as that of the ratio of Pr (photo-respiration rate) to Pr+Pn and non-photochemical quenching of chlorophyll fluorescence (NPQ) indicates that those mechanisms related to the changes of these parameters may play an important role in protecting rice leaves from oxidative damage under high nocturnal temperature stress.     

Photochemical Efficiency of PSⅡand Membrane Lipid Peroxidation in Leaves of indica and japonica Rice (Oryza sativa) Under Chilling Temperature and Strong Light Stress Conditions

Relationships between fluorescence parameters and membrane lipid peroxidation in leaves of indica and japonica rice (Oryza sativa L.) during later growth stage were studied under chilling temperature and strong light stress conditions. Results showed that D1 protein contents of PSⅡ in photosynthetic app aratus dropped, the generation of antheraxanthin (A) and zeaxanthin (Z)of xanthophyll cycle were inhibited partly, PSⅡ photochemical efficiency （Fv/Fm）and non photochemical quenching (qN) were also decreased obviously. In addition, endogenous active oxygen scavenger—superoxide dismutase (SOD) reduced, superoxide anion radical (O[SX(B-*3)-[]·[SX]]2) and malondialdehyde (MDA) accumulated, as a result, photooxidation of leaves occurred under chilling temperature and strong light stress conditions. Obvious differences in the changes of the above mentioned physiological parameters between indica and japonica rice were observed. Experiments in leaves treated with inhibitors under chilling temperature and strong light conditions showed that indica rice was more sensitive to chilling temperature with strong light and subjected to photooxidation more than japonica rice. Notable positive correlation between D1 protein contents and Fv/Fm or (A+Z)/(A+Z+V), and a marked negative correlation between Fv/Fm and MDA contents were obtained by regression analysis in indica and japonica rice during chilling temperature and strong light conditions. According to the facts mentioned above, it was inferred that PSⅡ photochemical efficiency（Fv/Fm） was the key index to forecast for the prediction of photooxidation under stress circumstances and the physiological basis were the synthetic capacity of D1 protein and the protection of xanthophyll cycle.     

Photoinhibition and Photooxidation in Leaves of indica and  japonica Rice Under Different Temperatures and Light Intensities

Physiological indices related to the efficiency （ Fv/Fm ） of light energy conversion in PSⅡ and the peroxidation of membrane lipid were measured in leaves of Oryza sativa L. sp. indica rice cv. “Shanyou 63” and sp. japonica rice cv. “9516” under different temperatures and light intensities for 4 days. No changes in Fv/Fm and membrane lipid peroxidation product (MDA) were observed, so neither photoinhibition nor photooxidation happened in both rice cultivars under moderate temperature and medium light intensity. However, Fv/Fm dropped obviously with no change in MDA contents, and photoinhibition appeared in indica rice cv. “Shanyou 63” under medium temperature and strong light intensity. Furthermore, both photoinhibition and photooxidation were observed in two rice cultivars under chilling temperature and strong light intensity. Experiments with inhibitors under chilling temperature and strong light intensity showed that indica rice had a decrease in D1 protein content and SOD activity, and the extent of inhibition of xanthophyll cycle and nonphotochemical quenching ( qN ) was larger, and a higher level of MDA was observed. The photoinhibition and photooxidation in indica rice were more distinct as compared with japonica rice. The authors suggested that PSⅡ light energy conversion efficiency ( Fv/Fm ) and membrane lipid peroxidation were the key indices for the detection of photooxidation.     

水杨酸对高温强光胁迫下小麦叶绿体D1蛋白磷酸化及光系统Ⅱ功能的影响

为了研究水杨酸（SA）对高温强光胁迫下小麦叶片类囊体膜D₁蛋白磷酸化和PSⅡ功能的影响,用0.5 mmol·L^-1 SA溶液预处理灌浆期小麦叶片,以水预处理为对照,然后将预处理植株进行高温强光（35 ℃,1 600 μmol·m^-2·s^-1）处理,测定胁迫处理过程中小麦旗叶光合电子传递速率、净光合速率、叶绿素荧光参数及D₁蛋白的变化.结果表明：SA预处理有效抑制了高温强光下D₁蛋白的净降解,保持了较高的D₁蛋白磷酸化水平、全链电子传递速率和PSⅡ电子传递速率,维持了较高的PSⅡ原初光化学效率（F_v/F_m）、实际光化学效率(Ф_PSⅡ)、光化学淬灭系数（q_P）和净光合速率（P_n）.表明外源SA通过调节小麦叶绿体D₁蛋白的周转,减轻了高温强光胁迫对叶片光合机构的损伤,有利于PSⅡ的正常运转.     

水杨酸和油菜素内酯对低温胁迫下黄瓜幼苗光合作用的影响

为了探明外源水杨酸(SA)和2,4-表油菜素内酯(EBR)对低温胁迫下黄瓜幼苗光合作用的调控机理,以‘优博1-5’黄瓜为试材,用1 mmol·L^-1SA和0.1 μmol·L^-1EBR喷施预处理幼苗,每天喷1次,连喷2 d后置于低温下[10 ℃/5 ℃,光强(PFD)80 μmol·m^-2·s^-1]处理.结果表明: 低温胁迫下黄瓜幼苗生长量及净光合速率(P_n)下降;喷施SA和BER显著提高了P_n、光系统Ⅱ最大光化学效率(F_v/F_m)、光系统Ⅱ实际光化学效率(Φ_PSⅡ)和光化学猝灭系数(q_P),减缓了非光化学猝灭系数(NPQ)增加的幅度,同时核酮糖-1,5-二磷酸羧化/加氧酶(Rubisco)、景天庚酮糖-1,7-二磷酸酯酶(SBPase)、转酮醇酶(TK)和果糖-1,6-二磷酸醛缩酶(FBA)活性明显升高.说明SA和EBR可以通过调节光合关键酶的活性,缓解低温对黄瓜幼苗光合作用的影响,增强其对低温的适应性.     

Stable chloroplast transformation of the unicellular red alga Porphyridium species

Red algae are extremely attractive for biotechnology because they synthesize accessory photosynthetic pigments (phycobilins and carotenoids), unsaturated fatty acids, and unique cell wall sulfated polysaccharides. We report a high-efficiency chloroplast transformation system for the unicellular red microalga Porphyridium sp. This is the first genetic transformation system for Rhodophytes and is based on use of a mutant form of the gene encoding acetohydroxyacid synthase [AHAS(W492S)] as a dominant selectable marker. AHAS is the target enzyme of the herbicide sulfometuron methyl, which effectively inhibits growth of bacteria, fungi, plants, and algae. Biolistic transformation of synchronized Porphyridium sp. cells with the mutant AHAS(W492S) gene that confers herbicide resistance gave a high frequency of sulfomethuron methyl-resistant colonies. The mutant AHAS gene integrated into the chloroplast genome by homologous recombination. This system paves the way for expression of foreign genes in red algae and has important biotechnological implications.