增强UV-B辐射对柚树苗生长和生理特性效应研究

增强的UV-B辐射明显降低柚树苗的株高,叶面积,比叶面积,增加叶片厚度和叶肉密度.柚树苗叶片叶绿素,可溶性蛋白含量和硝酸还原酶活性降低,可溶性糖含量上升.不同品种柚苗对UV-B辐射反应存在差异,酸柚抗性较强.经UV-B增强处理后,叶片Pn值下降,Rd先上升后恢复原有水平.Fv/Fm,ΦPSⅡ,qP均有不同程度的降低,而qN和KD升高,表明增强UV-B导致PSⅡ失活,PSⅡ原初光化学效率、开放PSⅡ中心数目和非环式电子传递效率下降.部分激发能通过非光化学荧光猝灭形式耗散.UV-B辐射使叶片膜脂过氧化产物MDA含量大幅度上升.SOD和APX活性在处理初期提高,随后下降,初步推测:增强UV-B辐射诱导膜脂过氧化作用,攻击光合作用中心靶点并导致PSⅡ失活,进而降低植物光合能力和物质代谢强度,最终导致柚树苗生长受到抑制.     

不同混合速率下阳光UV辐射对假微型海链藻PSⅡ功能的影响

以浮游硅藻假微型海链藻(Thalassiosira pseudonana(Hustedt)Hasle et Heimdal CCMP 1335)为材料,研究不同混合速率下,随辐射水平增加,UV辐射和可见光PAR对其光系统Ⅱ功能的影响。结果显示,混合速率慢时,随着PAR及UV辐射水平的增加,假微型海链藻PSⅡ的光化学效率(F_v/F_m)持续受到抑制,光合效率α和相对最大电子传递速率rETR_(max)下降。尤其是UV辐射存在时,PSⅡ反应中心D1蛋白含量下降,有活性的PSⅡ反应中心数量减少,单位反应中心吸收(ABS/RC)和耗散(DI_0/RC)的能量增加。混合速率快时,PAR辐射下PSⅡ光化学活性相比混合速率慢时升高,D1蛋白含量增加;而UV辐射存在下各光合参数表现出与混合速率慢时类似的变化趋势。研究结果表明水体混合速率的加快可缓解高水平可见光导致的光抑制,而对UV辐射的抑制效应并未产生显著改变。     

镉离子对菠菜叶绿体光系统Ⅱ的影响

环境污染因子重金属离子镉(Cd~(2 ))对菠菜(Spinacia oleracea L.)叶绿体光合作用有明显的抑制作用,其中对光系统Ⅱ(PSⅡ)的抑制作用显著。5mmol/l Cd~(2 )可抑制 PSⅡ放氧活性53％。Cd~(2 )使叶绿体和 PSⅡ制剂的 DCIP 光还原活性降低;可变荧光也受到抑制。加入 PSⅡ的人工电子供体 DPC 仅使被抑制的 DCIP 光还原活性稍有恢复;加入羟胺对被抑制的可变荧光并无明显影响。因此我们认为 Cd~(2 )除了作用于 PSⅡ氧化侧外,还可能直接损伤了 PSⅡ反应中心。不同浓度的 Cd~(2 )处理后,叶绿体全电子链的电子传递活性比放氧活性的速率降低快。这暗示着 PSⅡ氧化侧不是 Cd~(2 )唯一的作用部位,在 PSⅡ与 PSⅠ之间的电子传递链上还存在有对 Cd~(2 )敏感的部位。     

水分胁迫对长期UV—B辐射下柚树苗生理特性的影响

水分胁迫下,柚[Citrus maxima(Burm.)Merr.]树苗叶片相对含水量（RWC）、水势（ΨW)、净光合速率（Pn)、可溶性蛋白质和叶绿素（Chl)含量下降,丙二醛（MDA）、脯氨酸（Pro)含量和超氧化物歧化酶（SOD）活性升高,过氧化氢酶（CAT）活性先上升后下降,抗坏血酸过氧化物酶（APX）活性、抗坏血酸（AsA)和还原型谷胱甘肽（GSH）含量明显降低。叶绿素荧光参数中光系统Ⅱ光化学原初效率（Fv/Fm)、光系统Ⅱ电子传递量子效率（ΦPSⅡ）和光化学猝灭（qp)下降,非光化学猝灭（qN)和热能耗散系数（KD）升高。显示膜系统和PSⅡ是水分胁迫的主要抑制位点。抗旱性强的品种具有较高的活性氧清除能力。长期紫外线－B（UV－B）增强辐射能缓解水分胁迫下柚树苗叶片RWC、ΨW、APX活性和GSH、AsA含量下降,但对水分胁迫下的Pro含量、Pn和叶绿素荧光特性作用不明显。初步推测：UV－B和水分胁迫对植物有部分相同的作用机制,都导致植株膜脂过氧化程度加剧和PSⅡ的失活,同时存在各自作用方式的特异性。     

远紫外辐射对紫杉幼苗针叶膜脂过氧化及内源保护系统的影响

实验室条件下用远紫外线（ＵＶ－ＢＣ）光源照射紫杉幼苗,随照射时间延长、针叶的离子渗出率、膜脂过氧化水平、组织自动氧化快速率及Ｈ２Ｏ２含量显著增加,可溶性蛋白、抗坏血酸、类胡萝卜素和叶绿素含量下降,叶绿体光系统ＩＩ电子传递活性显著下降,外源活性氧清除剂苯甲酸钠和抗坏血酸对针叶膜脂过氧化有抑制作用;甲基紫精和ＤＤＣ对针叶膜脂过氧化有促进效果,远紫外线引起的紫杉伤害可能和针叶树的越冬光氧化伤害有类似之处     

两种生态型芦苇叶绿体的光合电子传递和抗氧保护体系

分布于甘肃省河西走廊的两种不同生态型芦苇-水生芦苇(水芦,生长在深约1m的水滩里)和沙丘芦苇(沙芦,生长在高约5m的沙丘上)在其离体叶绿体的光化学活性上表现为前者高于后者。其中,沙芦全链电子传递速率及光系统Ⅱ(PSⅡ)电子传递速率明显低于水芦,而光系统Ⅰ(PSⅠ)电子传递速率却与水芦接近。沙芦叶片和叶绿体中抗氧化酶活性及叶片抗坏血酸含量均高于水芦。综合结果表明,喜水植物芦苇登陆后,在自然选择压力下,为适应长期的自然干旱胁迫环境,其抗氧保护系统在保护PSⅠ免受水分胁迫诱导的氧化伤害中可能发挥着重要作用。     

模拟酸雨对龙眼叶片PSⅡ反应中心和自由基代谢的影响

酸雨对植物光合机构的伤害机理一直是生态学研究的热点之一,为了探讨叶面酸化导致的PSⅡ反应中心损伤和光合机构自由基累积之间的内在联系,以1年生龙眼(Dimocarpus longana Lour.)实生小苗为研究对象,采用盆栽试验,研究了模拟酸雨胁迫对龙眼叶片叶绿素荧光参数和自由基代谢的影响.结果表明:酸雨胁迫改变了龙眼叶片的快速叶绿素荧光诱导动力学曲线形状,伤害PSⅡ反应中心;pH2.5酸雨胁迫5d后最大光化学效率(Fv/Fm)、PSⅡ反应中心活性(1/F0-1/FM)、反应中心含量(RC/CSo)急剧下降;有活性反应中心的关闭程度(VJ)、失活反应中心的比例(Non-QA和Non-QB)显著增加,QA迅速还原;放氧复合体(OEC)被破坏;PSⅡ受体侧电子传递体数(Sm)、电子转化效率(ψ0)和电子传递速率((φ)E0)明显降低,叶面酸化导致光系统线性电子传递受损.pH2.5酸雨胁迫5d后叶片超氧阴离子自由基(O2(-))、过氧化氢(H2O2)和丙二醛(MDA)含量显著增加;抗坏血酸(AsA)和谷胱甘肽(GSH)转化为氧化型,还原型减少;超氧化物歧化酶(SOD)、抗坏血酸过氧化物酶(APX)、单脱氢抗坏血酸还原酶(MDAR)、脱氢抗坏血酸还原酶(DHAR)和谷胱甘肽还原酶(GR)活性下降,叶绿体内自由基不能被及时清除,过多的自由基损伤光合器官,导致龙眼叶片PSⅡ受伤害.模拟酸雨胁迫伤害龙眼叶片PSⅡ反应中心供体侧和受体侧的电子传递体,造成同化力不足,清除自由基能力下降,导致叶绿体自由基累积,光合机构受到伤害.     

五节芒不同种群对Cd污染胁迫的光合生理响应

通过盆栽模拟试验,以分别来自粤北大宝山矿区和惠州博罗非矿区的两个五节芒种群为试验材料,比较研究了两个种群在Cd胁迫下的气体交换参数、叶绿素荧光特性、光合色素含量和叶绿体超微结构变化的差异。结果表明:(1)Cd胁迫下五节芒两种群叶片净光合速率(Pn)、蒸腾速率(E)、气孔导度(Gs)、胞间二氧化碳浓度(Ci)、叶绿素含量(Chl)都有不同幅度的下降;叶绿体超微结构遭到破坏。矿区种群随Cd胁迫程度的加深,净光合速率下降较慢,叶绿体的外形及基粒结构受到的影响较小。(2)轻度Cd胁迫下气孔限制是五节芒非矿区种群Pn降低的主要因素,中度和重度Cd胁迫下非气孔限制是Pn降低的主要因素。(3)Cd胁迫下五节芒两种群PSⅡ反应中心最大光化学效率(Fv/Fm)、PSⅡ潜在活性(Fv/Fo)、PSⅡ有效光化学效率Fv′/Fm′均有所下降。总体上矿区种群降幅较小,PSⅡ利用光能的能力及PSⅡ的潜在活性均较强。PSⅡ光化学猝灭系数(qP)、非光化学猝灭系数(NPQ)的变化表现为Cd胁迫下两种群qP值降低、NPQ值升高,总体上抗性强的矿区种群qP降低的幅度低且NPQ升高幅度大。随着Cd胁迫浓度增加,矿区种群实际光化学反应效率(ΦPSⅡ)和电子传递速率(ETR)变化幅度不大,而非矿区种群显著下降,表明矿区种群PSⅡ反应中心电子传递活性受到的影响小,光合机构的损伤程度低。研究表明,五节芒矿区种群对重金属Cd有较强的耐受能力,适合作为金属矿区植被恢复建设的禾本科先锋物种。     

光合作用电子传递的研究——Ⅰ.新鲜和老化叶绿体的光还原作用

叶绿体在老化过程中对DCIP的光还原活性逐渐下降,温热加速了活性的丧失,似与光合膜结构在老化过程中的解体和温热加速光合膜的破损有关。从光合链上PSⅡ氧化侧加入人工电子供体DPC,可显著恢复老化叶绿体对DCIP的光还原,如象DPC对被羟胺和Tris处理新鲜叶绿体后的恢复作用一样。似乎老化叶绿体DCIP光还原活性的下降,主要是由于PSⅡ氧化侧那部分光合膜受损所造成。用切断PSⅡ→PS Ⅰ间电子流的抑制剂水杨醛肟处理新鲜和老化叶绿体,对DCIP和Fecy的光还原都有抑制,并以对新鲜叶绿体的抑制更甚,加入DPC不能使新鲜叶绿体的光还原活性恢复,但可使老化叶绿体的光还原活性有显著促进,尤以对DCIP的光还原促进更大。似乎DCIP和Fecy接受电子的部位随叶绿体状态不同而有改变,即新鲜叶绿体主要在PS Ⅰ还原侧,老化叶绿体则主要在PSⅡ还原侧,推测此与光合膜的完整或破损和人工电子受体同膜亲和的难易程度有关。     

CaCl_2对UV-B辐射下菠菜叶片光合特性的影响

以"丹麦旺盛菠菜"为材料,通过UV-B和CaCl2复合处理,测定光合色素含量、Hill反应活力、叶绿素荧光、MDA含量和抗氧化酶活性等参数,探讨了CaCl2对UV-B辐射下菠菜叶片电子传递链和光合膜酶保护系统的影响。结果表明,UV-B处理下,光合色素含量、chl/car、类囊体膜上PSII潜在活性(Fv/Fo)、光化学淬灭系数(qP)、非光化学淬灭系数(qN)、PSII光量子产量(ΦPSⅡ)、原初光能转化效率(Fv/Fm),以及Hill反应活力等降低,chla/chlb和MDA含量升高;喷洒CaCl2可不同程度缓解UV-B的伤害。不同处理下,POD、SOD和CAT活性的变化呈现补偿效应。UV-B强度与菠菜叶片PSII功能受损程度呈正相关,CaCl2则主要通过提高chlb含量、类囊体膜上的光量子产量和POD活性,以缓解伤害。重度UV-B辐射下,CaCl2使chlb含量显著提高可能是导致PSII捕光效率提高的重要因素。     

Comparative study of the action of ultraviolet-C and ultraviolet- B radiation on photosynthetic electron transport

The effect of ultraviolet-C (UV-C, mainly 254 nm radiation) and ultraviolet-B (UV-B, 290-320 nm) radiation on the photosynthetic electron transport reactions has been investigated. The rates of Hill activity mediated by ferricyanide and dichlorodimethoxy-p-benzoquinone (DCDMQ) were differently sensitive to UV-C but equally inhibited by UV-B. Replacement of water with diphenylcarbazide was ineffective in restoring the activity of dichlorophenol indophenol (DCPIP) Hill reaction in UV-B treated chloroplasts, but had significant effect in UV-C treated chloroplasts.
Photobleaching of carotenoids in the presence of carbonyl cyanide-m-chlorophenyl-hydrazone, an indicator of the photochemical reaction associated with the reaction centre of photosystem II, was suppressed and is paralleled by the changes in Hill activity only in UV-B-treated chloroplasts. Carotenoid photobleaching occurred even in UV-C treated chloroplasts showing no measurable Hill activity. UV-C and UV-B irradiation diminished variable fluorescence. With UV-B treated, but not with UV-C treated chloroplasts, an increase in the fluorescence yield was observed upon the addition of 3-(3,4-dichIorophenyl)-l,l-dimethylurea (DCMU) and/or Na dithionite.
Photosystem I activity was found to be unaffected by both UV-C and UV-B radiation at the fluences tested. Kinetics of P700 photooxidation and dark reversal in UV treated chloroplasts indicate that only the electron flow from photosystem II to photosystem I is impaired. It is concluded that while UV-B radiation inactivates specifically the photosystem II reaction centre, UV-C radiation acts at plastoquinone, the quencher Q, and the water oxidizing enzyme system.     

Studies of the Ndh complex and photosystem II from mesophyll and bundle sheath chloroplasts of the C4-type plant Zea mays

In C(4) plants, granal mesophyll (MS) chloroplasts contain higher photosystem (PS) II and lower PS I activity than agranal bundle sheath (BS) chloroplasts. The maize NAD(P)H dehydrogenase or NAD(P)H-plastoquinone oxidoreductase (also named Ndh complex) from MS and BS chloroplasts, contains at least 11 subunits (NdhA-K) and is homologous to NADH dehydrogenase or Complex I from mitochondria and bacteria. The amount of Ndh complex is higher in BS compared with MS chloroplasts. However, there is little information about the interdependence of the PS II and Ndh complex in chlororespiration and linear and cyclic electron transport in C(4) plants. To characterize the expression of the PS II and Ndh complex in maize plastids, we used cytochrome b559 (cyt b559) antibodies and Ndh immunoglobulins (IgG) to analyze the Ndh complex and PS II in both MS and BS chloroplasts from maize leaves by Western blotting and immunolabeling. In Western blot experiments, it was found that the amount of cyt b559 (a marker for PS II) is 7-8 times higher in MS than BS chloroplasts. Conversely, the NdhH, -J, -K and -E content is 2.5-3 times higher in BS than MS chloroplasts. Similar results were obtained in immunolabeling experiments using Ndh IgGs and cyt b559 antibodies in MS and BS chloroplasts. These data suggest that in BS chloroplasts, ATP could be produced mainly by cyclic electron transport around PS I and Ndh complexes. Conversely, the linear electron transport in BS chloroplasts via PS II could have a lower production of ATP. These results also suggest that the contribution of the Ndh complex in the production of ATP in MS chloroplasts is minimal and that instead, this complex could have a chlororespiratory role.     

Mechanism of inhibition by local anesthetics of electron transport at the donor site of the photosystem II

The mechanism of inhibition by local anaesthetics of the procaine group of electron transport at the donor site of photosystem II (PS II) from pea chloroplasts was investigated. It was found that besides the inactivation of the O2 release system the anaesthetics used at one order of magnitude lesser concentration exert an uncoupling effect. With a rise in pH the inhibiting activity increases; however, this process is not coupled with the protonophore effect but is due to the generation of a neutral form of the amine. The increment of the inhibiting activity of the anaesthetics in the course of deprotonation seems to be regulated by changes in the coefficient of distribution between the membrane and the aqueous phase. The rate of inactivation of the H2O-dissociating complex increases considerably upon illumination. Electron transport through PS II in anaesthetic-treated chloroplasts in restored by diphenylcarbaside, but not by hydroxylamine. It is concluded that the anaesthetics induce the inhibition by interacting with the electron carrier. The role of the Ca2+--calmodulin-like protein in the functioning of the electron transport chain of PS II is discussed.     

Photosynthetic Electron Transport During Senescence of the Primary Leaves of Phaseolus vulgaris L.: II. THE ACTIVITY OF PHOTOSYSTEMS ONE AND TWO, AND A NOTE ON THE SITE OF REDUCTION OF FERRICYANIDE

The activity of photosystems one and two (PS I and PS II) wasmeasured in chloroplasts isolated from the primary leaves ofPhaseolus vulgaris. During foliar senescence, the rates of electrontransport through PS I and PS II declined by approximately 25%and 33% respectively. These losses of activity could not accountfor the decrease of 80% in the rate of coupled, non-cyclic electrontransport during senescence. It is therefore suggested thatan impairment of electron flow between the photosystems limitednon-cyclic electron transport in chloroplasts from older leaves.In this study the activity of PS II was measured using oxidizedp-phenylenediamine as the electron acceptor, and trifluralinas an inhibitor of electron transport between PS II and PS I.In chloroplasts from young leaves the reduction of ferricyanidewas a measure of non-cyclic electron transport, but in preparationsfrom older leaves ferricyanide received a large proportion ofelectrons from PS II.     

叶绿体结构状态与光化学活性的关系

叶绿体被膜阻碍以Fecy为受体的电子传递,而对以DCIP为受体的电子传递无妨。被膜完整度越高则P/O值也越高。类囊体膜结构的完整度高,则电子传递速率和P/O值也比膜结构受到破损时高。类囊体膜结构的完整度对保持PS Ⅱ活性是必要的,随着完整度的降低,PS Ⅱ在电子传递中所占比重相应减少。     

Nano-Anatase Relieves the Inhibition of Electron Transport Caused by Linolenic Acid in Chloroplasts of Spinach

Linolenic acid is an inhibitor of electron transport in chloroplasts of higher plants. It has obvious effects on the structure and function of chloroplasts. In the present paper, we investigated the nano-anatase relieving the inhibition of photoreduction activity and oxygen evolution caused by linolenic acid in spinach chloroplasts. The results showed that linolenic acid in various concentrations could obviously reduce the whole chain electron transport and the photoreduction activity of two photosystems, especially on the oxidative reside and reduce reside of photosystem II (PS II). After adding nano-anatase to chloroplasts treated by linolenic acid, the whole chain electron transport rate, the photoreduction activity of two photosystems, and the oxygen evolution rate were increased significantly, indicating that nano-anatase could obviously decrease the inhibition of linolenic acid on the electron transport, photoreduction activity, and oxygen evolution of spinach chloroplasts.     

Adaptation of photosynthesis under iron deficiency in maize

This paper explores the effects of high light stress on Fe-deficient plants. Maize (Zea mays) plants were grown under conditions of Fe deficiency and complete nutrition. Attached, intact leaves of Fe-deficient and control plants were used for gas exchange experiments under suboptimal, optimal and photoinhibitory illumination. Isolated chloroplasts were used to study photosynthetic electron transport system, compromised by the induction of Fe deficiency. The reaction centers of PS II (measured as reduction of Q, the primary electron acceptor of P 680) and PS I (measured as oxidation of P 700) were estimated from the amplitude of light induced absorbance change at 320 and 700 nm, respectively. Plants were subjected to photoinhibitory treatment for different time periods and isolated chloroplasts from these plants were used for electron transport studies. Carbon dioxide fixation in control as well as in Fe-deficient plants decreased in response to high light intensities. Total chlorophyll, P 700 and Q content in Fe-deficient chloroplasts decreased, while Chl a/b ratio and Q/P 700 ratio increased. However, electron transport through PS II suffered more after photoinhibitory treatment as compared to electron transport through PS I or whole chain. Electron transfer through PS I+PS II, excluding the water oxidation complex showed a decrease in Fe-deficient plants. However, electron transport through this part of the chain did not suffer much as a result of photoinhibition, suggesting a defect in the oxidising side of PS II.     

Structural and functional stability of isolated intact chloroplasts

The effect of in vitro ageing on the ultrastructure, electron transport, thermoluminescence and flash-induced 515 nm absorbance change of isolated intact (type A) chloroplasts compared with non-intact (types B and C) chloroplasts was studied.When stored in the dark for 18 h at 5°C, the structural characteristics of intact and non-intact chloroplasts were only slightly altered. The most conspicuous difference between the two was in the coupling of the electron transport which was tighter and more stable in intact chloroplasts. Under dark-storage the activity of PS 2* decreased and the -20°C peak of thermoluminescence increased at the expense of the emission at +25°C. These changes were less pronounced in the intact chloroplasts. PS 1 activity and the flash-induced 515 nm absorbance change were not affected by dark-storage.When kept in the light (80 W m^-2 (400–700 nm) for 1 h at 5°C), the thylakoid system of chloroplasts rapidly became disorganized. Although the initial activity of electron transport was much higher in intact chloroplasts, after a short period of light-storage the linear electron transport and the electron transport around PS 2 decreased in both types of preparations to the same low level. These changes were accompanied by an overall decrease of the intensity of thermoluminescence. PS 1 was not inhibited by light-storage, while the flash-induced 515 nm absorbance change was virtually abolished both in preparations of intact and non-intact chloroplasts.The data show that in stored chloroplast preparations intactness cannot be estimated reliably either by the FeCy test or by inspection under the electron microscope. These tests should be cross-checked on the level and coupling of the electron transport.     

The coleoptile chloroplast: Distinct distribution of xanthophyll cycle pigments,and enrichment in Photosystem II

Recent studies have shown that coleoptile chloroplasts operate the xanthophyll cycle, and that their zeaxanthin concentration co-varies with their sensitivity to blue light. The present study characterized the distribution of photosynthetic pigments in thylakoid pigment–protein complexes from dark-adapted and light-treated coleoptile and mesophyll chloroplasts, the low temperature fluorescence emission spectra, and the rates of PS I and PS II electron transport in both types of chloroplasts from 5-day-old corn seedlings. Pigments were extracted from isolated PS I holocomplex, LHC IIb trimeric and LHC II monomeric complexes and analyzed by HPLC. Chlorophyll distribution in coleoptile thylakoids showed 31% of the total collected Chl in PS I and 65% in the light harvesting complexes of PS II. In mesophyll thylakoids, the values were 44% and 54%, respectively. Mesophyll and coleoptile PS I holocomplexes differed in their Chl t a/Chl t b ratios (8.1 and 6.1, respectively) and -carotene content. In contrast, mesophyll and coleoptile LHC IIb trimers and LHC II monomers had similar Chl t a/Chl t b ratios and -carotene content. The three analyzed pigment–protein complexes from dark-adapted coleoptile chloroplasts contained zeaxanthin, whereas there was no detectable zeaxanthin in the complexes from dark-adapted mesophyll chloroplasts. In both chloroplast types, zeaxanthin and antheraxanthin increased markedly in the three pigment–protein complexes upon illumination, while violaxanthin decreased. In mesophyll thylakoids, zeaxanthin distribution as a percentage of the xanthophyll cycle pool was: LHC II monomers > LHC IIb trimers > PS I holocomplex, and in coleoptile thylakoids, it was: LHC IIb trimers > LHC II monomers = PS I holocomplex. Low temperature (77 K) fluorescence emission spectra showed that the 686 nm emission of coleoptile chloroplasts was approximately 50% larger than that of mesophyll chloroplasts when normalized at 734 nm. The pigment and fluorescence analysis data suggest that there is relatively more PS II per PS I and more LHC I per CC I in coleoptile chloroplasts than in mesophyll chloroplasts. Measurements of t in vitro uncoupled photosynthetic electron transport showed approximately 60% higher rates of electron flow through PS II in coleoptile chloroplasts than in mesophyll chloroplasts. Electron transport rates through PS I were similar in both chloroplast types. Thus, when compared to mesophyll chloroplasts, coleoptile chloroplasts have a distinct PS I pigment composition, a distinct chlorophyll distribution between PS I and PS II, a distinct zeaxanthin percentage distribution among thylakoid pigment–protein complexes, a higher PS II-related fluorescence emission, and higher PS II electron transport capacity. These characteristics may be associated with a sensory transducing role of coleoptile chloroplasts.     

He-Ne激光对增强UV-B辐射后小麦幼苗光合作用的影响

以"晋麦8号"小麦幼苗为研究材料,分别采用He-Ne激光(辐照剂量为5 mW·mm-2)、增强UV-B(辐射剂量为10.08 kJ·m-2·d-1)以及二者的复合辐照进行处理.循坏处理不同天数(4、5、6、7、8 d)后,利用电导仪、低温荧光测定法检测了小麦叶绿体电子传递速率、膜透性和荧光发射光谱的变化;采用紫外分光光...