Subchloroplast localization of polypeptides synthesized by chloroplasts during senescence

To study the localization of polypeptides synthesized by isolated senescent chloroplasts we have fractionated the chloroplasts into stroma, envelope and thylakoid components. The validity of the fractionation procedure was tested by assaying both chlorophyll and enzyme markers, as well as the polypeptide composition of each fraction. Plastids in the transition of etioplast to chloroplast, senescent chloroplasts and kinetin-treated chloroplasts produced acceptable fractions, although their polypeptide compositions varied considerably during the ontogeny, particularly those of the envelope. Most of the polypeptides synthesized by isolated senescent chloroplasts were incorporated into the thylakoids except for a 58 kDa polypeptide localized in the stroma and some minor polypeptides present in both stroma and envelope. Although most of the polypeptides synthesized by isolated chloroplasts from kinetin-treated leaves were incorporated into the thylakoid membrane, several polypeptides were found in the stroma (90, 80, 65 and 54 kDa) and in the envelope (100, 75, 48 and 28–30 kDa). The results indicate that early in senescence, the polypeptides of the envelope change but, that probably, most of the new polypeptides are synthesized in the cytoplasm.     

Light/dark labeling differences in chloroplast membrane polypeptides associated with chloroplast coupling factor 0

The fluorogenic reagent fluorescamine has been used to determine the labeling patterns of Type C spinach chloroplast membrane polypeptides. Membrane polypeptides labeled with fluorescamine were detected by scanning high resolution sodium dodecyl sulfate polyacrylamide gradient slab gels for fluorescence emission.Three membrane polypeptides show a decrease in the extent of labeling when chloroplast membranes are labeled in the light compared to when they are labeled in the dark. These polypeptides have apparent molecular weights of 32 000, 23 000 and 15 000.The decrease in labeling observed in the light is abolished or reduced by treatments which inactivate the light-generated transmembrane pH gradient. CF₁-depleted chloroplasts show neither a light-activated pH gradient nor a light/dark difference in labeling of these three polypeptides. Both a light-activated pH gradient and light/dark differences in labeling are observed in CF₁-depleted chloroplasts which have been treated with N,N′-dicyclohexylcarbodiimide.The same ammonium sulfate fractions of a 2% sodium cholate extract, which are believed to be enriched in the membrane-bound sector of the chloroplast ATPase (CF_o) are also found to be enriched in the 32 000, 23 000 and 15 000 molecular weight polypeptides. The three polypeptides are believed to be components of CF_o, and the light/dark labeling differences may indicate conformational changes within CF_o. Such conformational changes may reflect a mechanism which couples light-generated proton gradients to ATP synthesis.     

The effects of 2, 4-dichIorophenoxyacetk acid altered chloroplast development on photosynthesis

We studied the changes in function and physical properties of isolated radish ( Raphonus sativus L. cv. Sparkler) lamellar membranes 48 h after chloroplast development was altered by 2, 4-(dichlorophenoxy)acet, tc acid. The number of chlorophyll molecules attendant to each electron transport chain was approximately 25% less in the chloroplasts from 2, 4-(dichlorophenoxy)acetic acid-treated plants than in chloroplasts from untreated plants. The maximal turnover rate of Photosystem I] in the treated chloroplasts was slightly less than half the turnover rate in normal chloroplasts. The efficiency of coupling between electron flux and ATP formation was not significantly different in the two chloroplast types. This hight efficiency of photophosphorylation in addition to normal membrane conductance to hydrogen ions indicates that the herbicide has not brought about a general deterioration of the membrane. A dramatic increase in the proton binding capacity of the lamellar membrane was observed in the treated chloroplasts. This increase in hydrogen ion buffering groups was largely accounted for by extrinsic membrane proteins bound to the exterior surface of the lamellar membrane. Although the addition of 2, 4-(dichloro-phenoxy) acetic acid to chloroplasts isolated from untreated plants caused concurrent uncoupling of ATP formation and inhibition of electron transport, our data show that these direct effects of the compound have little to do with its herbicidal action.     

Comparative ultrastructural properties of pallisade tissue and spongy tissue chloroplasts from normal and mutant leaves of Pisum sativum L.*

Abstract. The ultrastructure of chloroplasts from palisade and spongy tissue was studied in order to analyse the adaptation of chloroplasts to the light gradient within the bifacial leaves of pea. Chloroplasts of two nuclear gene mutants of Pisum sativum (chlorotica-29 and chlorophyll b-less 130A), grown under normal light conditions, were compared with the wild type (WT) garden-pea cv. ‘Dippes Gelbe Viktoria’. The differentiation of the thylakoid membrane system of plastids from normal pea leaves exhibited nearly the same degree of grana formation in palisade and in spongy tissue. Using morphometrical measurements, only a slight increase in grana stacking capacity was found in chloroplasts of spongy tissue. In contrast, chloroplasts of mutant leaves differed in grana development in palisade and spongy tissue, respectively. Their thylakoid systems appeared to be disorganized and not developed as much as in chloroplasts from normal pea leaves. Grana contained fewer lamellae per granum, the number of grana per chloroplast section was reduced and the length of appressed thylakoid regions was decreased. Nevertheless, chloroplasts of the mutants were always differentiated into grana and stroma thylakoids. The structural changes observed and the reduction of the total chlorophyll content correlated with alterations in the polypeptide composition of thylakoid membrane preparations from mutant chloroplasts. In sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS-PAGE), polypeptide bands with a relative molecular mass of 27 and 26 kilodalton (kD) were markedly reduced in mutant chloroplasts. These two polypeptides represented the major apoproteins of the light harvesting chlorophyll a/b complex from photosystem II (LHC-II) as inferred from a comparison with the electrophoretic mobility of polypeptides isolated from the LHC-II.     

Effect of Salts and Electron Transport on the Conformation of Isolated Chloroplasts. II. Electron Microscopy

Spinach chloroplasts isolated in media containing salts and the rare chloroplasts which are still within their envelopes alike retain grana similar to those seen in chloroplasts in situ.

Chloroplasts isolated in low-salt media lose their grana without losing any chlorophyll. These grana-free chloroplasts are considerably swollen and consist almost entirely of continuous sheets of paired-membrane structures. These double structures, the lamellae, are only loosely held together, primarily at the edges, by tenuous material which does not react with permanganate.

Addition of salts (methylamine hydrochloride, NaCl, MgCl₂) to the grana-free low-salt chloroplasts provide strong interlamellar attractions. These attractions result in a stacking of the lamellae which is sometimes almost random but sometimes results in regular structures indistinguishable from the original grana.

The phosphorylation-uncoupler atebrin causes further swelling of the chloroplasts in the absence of electron transport by increasing the space between the paired membranes of the lamellae.

The rapid electron transport (Hill reaction) made possible by atebrin-uncoupling is associated with a great decrease in chloroplast volume. This decrease results from a collapsing together of the widely separated lamellar membrane pairs. The pairs approach each other so closely that they usually appear as a single membrane when viewed with the electron microscope. The much slower electron transport which occurs in the absence of uncouplers is associated with a similar but smaller decrease in the space between the lamellar membrane pairs.

Chloroplasts swell during the rapid electron transport made possible by the phosphorylation-uncoupler methylamine. This swelling is accompanied by a degree of membrane distortion which precludes an interpretation of the mechanism. As with atebrin-faciliated electron transport, obviously paired membranes disappear but it is not yet clear whether this is by association or dissociation of the pairs.

     

The molecular anatomy and function of thylakoid proteins

Abstract. The structure of chloroplast membrane proteins and their organization into photosynthetically-active multimeric complexes is described. Extensive use has been made of information derived from gene sequencing and other biochemical studies to predict likely protein conformations. These predictions have been assimilated into structural models of the various thylakoid complexes. The enzymatic activities of the complexes have also been described and where possible related to individual polypeptides.     

Membrane polypeptides of some higher plant chloroplasts

Sodium dodecylsulfate-polyacrylamide gel electrophoresis of membrane polypeptides of the mesophyll cell chloroplasts of barley, pea, and maize show similar profiles, with the polypeptides falling into two major groups: those associated with a membrane fraction enriched in Photosystem I (called Group I polypeptides) and those associated with a membrane fraction enriched in Photosystem II (called Group II polypeptides a, b, and c). In contrast to these profiles, the polypeptides from the extensively unstacked membranes of chloroplasts from the chlorophyll-deficient mutant strains of barley and pea as well as those obtained from the agranal bundle sheath cell chloroplasts of maize are deficient in the Group II polypeptides b and c. It is proposed that these polypeptides are required for membrane stacking in higher plant chloroplasts.These Group II polypeptides b and c are not required for Photosystem II activity since both the barley and pea mutant chloroplasts and the maize bundle sheath chloroplasts possess Photosystem II activities.     

Investigations of the role of the main light-harvesting chlorophyll- protein complex in thylakoid membranes. Reconstitution of depleted membranes from intermittent-light-grown plants with the isolated complex

The functions of the light-harvesting complex of photosystem II (LHC- II) have been studied using thylakoids from intermittent-light-grown (IML) plants, which are deficient in this complex. These chloroplasts have no grana stacks and only limited lamellar appression in situ. In vitro the thylakoids showed limited but significant Mg2+-induced membrane appression and a clear segregation of membrane particles into such regions. This observation, together with the immunological detection of small quantities of LHC-II apoproteins, suggests that the molecular mechanism of appression may be similar to the more extensive thylakoid stacking seen in normal chloroplasts and involve LHC-II polypeptides directly. To study LHC-II function directly, a sonication- freeze-thaw procedure was developed for controlled insertion of purified LHC-II into IML membranes. Incorporation was demonstrated by density gradient centrifugation, antibody agglutination tests, and freeze-fracture electron microscopy. The reconstituted membranes, unlike the parent IML membranes, exhibited both extensive membrane appression and increased room temperature fluorescence in the presence of cations, and a decreased photosystem I activity at low light intensity. These membranes thus mimic normal chloroplasts in this regard, suggesting that the incorporated LHC-II interacts with photosystem II centers in IML membranes and exerts a direct role in the regulation of excitation energy distribution between the two photosystems.     

定位于类囊体膜的PPF1在转基因拟南芥中的表达影响叶绿体的发育

PPF1是一个与植物营养生长相关的基因。它编码的产物可能是一个膜蛋白并与拟南芥叶绿体中的类囊体蛋白ALB3有很高的同源性。免疫电镜分析表明PPF1蛋白同样主要定位于类囊体膜 ,而且在短日照G2豌豆开花两周后仍发育良好的叶绿体中有很高的表达 ,在长日照豌豆同时期非正常叶绿体中丰度非常低。对转基因拟南芥和野生型植株的叶片衰老进程比较发现 ,PPF1在拟南芥中的过量表达可以延缓叶片的衰老 ,而用PPF1反义mRNA抑制拟南芥中的同源基因ALB3则明显加快叶片衰老速度。对转基因拟南芥的超微结构分析显示 ,PPF1在拟南芥中过量表达时 ,转基因植株的叶绿体比野生型植株的叶绿体大并含有更多的基粒和基质类囊体膜 ;相反 ,反义PPF1表达抑制其在拟南芥中的同源物时 ,转基因植株的叶绿体比野生型植株的叶绿体小并含有较少的基粒和发育较差的类囊体膜系统。这些数据表明叶绿体的发育状况与PPF1或拟南芥同源物ALB3的表达水平呈正相关。我们的结果提示PPF1基因可能通过控制叶绿体的发育状况来调节植物的发育。     

The effects of continuous illumination on the function and structure of Micrasterias torreyi Bail. (Conjugatophyceae)

Abstract. The division rate of Micrasterias torreyi cells grown under continuous illumination first accelerated but soon slowed down, and the cells lost their ability to divide after about 1 month. During the treatment the cells became pale green, the pyrenoids became fewer in number and defects appeared in the chloroplasts. After 1 month, the cells also soon died, even when subjected to intermittent illumination. The most striking structural alterations were found in the chloroplasts: the starch granules lost their typical structure, the lamellae were damaged and numerous electron dense precipitates appeared in the chloroplasts. The precipitates were similar to those formed in cells treated with supraoptimal external calcium concentrations and X-ray microanalysis showed that the precipitates were rich in calcium in both cases. The results suggest that light controls and activates the Ca²⁺ uptake in the plasma membrane as well as in the chloroplast envelope, that the large sized chloroplasts of Micrasterias are effective in regulation of cytoplasmic Ca²⁺ concentration, and that the injuries caused by continuous illumination may be largely due to the accumulation of Ca²⁺ in the chloroplasts.     

A modifiedEscherichia coli chaperonin (groEL) polypeptide synthesized in tobacco and targeted to the chloroplasts

The coding region for theEscherichia coli groEL (chaperonin-60) polypeptide was fused downstream of a pea rubisco small subunit transit peptide coding sequence under the control of a tandem 35S CaMV promoter. Transgenic tobacco plants (Nicotiana tabacum cv. Xanthi) containing this modifiedgroEL gene were produced. The modified groEL polypeptide was correctly imported into chloroplasts and accumulated to high or low levels in different plants. The majority of the modified groEL polypeptide was processed correctly to the mature form within the chloroplasts. Approximately 20% of the imported polypeptides retained a portion of the N-terminal transit peptide (TPgroEL). Both groEL and TPgroEL polypeptides assembled into tetradecameric species in the chloroplasts. In plants accumulating high levels of these products, the majority of the plant chaperonin-60 polypeptides in the chloroplast were present in novel hybrid tetradecameric species containing both bacterial and plant chaperonin-60 polypeptides. In plants accumulating low levels of groEL, the predominant species present appeared to be authentic plant cpn60₁₄ and authentic bacterial groEL₁₄. The growth and development of transgenic and control tobacco plants were indistinguishable.Abbreviations cpn60 chaperonin-60 - cpn10 chaperonin-10 - hsp heat shock protein - rubisco ribulose-1,5-bisphosphate carboxylase-oxygenase - ssu small subunit - spp stromal processing peptidase - SDS sodium dodecyl sulfate - PAGE polyacrylamide gel electrophoresis     

Formation,d'inositol par les chloroplastes isolés de pois

It was possible to synthesize d-inositol-1-phosphate from glucose-6-phosphate with extracts of chloroplasts isolated from pea-leaves. (U-¹⁴C)Inositol produced by alkaline phosphatase hydrolysis was studied under various conditions. The enzyme d-glucose-6-phosphate cyclase was isolated from the chloroplast preparation. The results showed the role of chloroplasts in the synthesis of their endogenous inositol.     

The case for chloroplast thylakoid carbonic anhydrase

Washed thylakoid membranes and photosystem II-enriched membrane fragments from cyanobacteria, green algae, and chloroplasts from both C₃ and C₄ plants possess the ability to reversibly hydrate CO₂. That is, the membranes have an intrinsic carbonic anhydrase activity. The present review outlines the discovery of thylakoid carbonic anhydrase and presents the evidence that it is a unique isozyme, distinct from other cellular carbonic anhydrases. It appears that at least some thylakoid carbonic anhydrase is closely associated with photosystem II and may be required for electron transport. This would explain why all inhibitors of carbonic anhydrase also inhibit photosystem II. Several speculative functions of thylakoid carbonic anhydrase are discussed. These include a possible role in carbon metabolism, in the protonation of plastoquinone, and/or in oxygen evolution.     

蚕豆萎蔫病毒2号分离物侵染对蚕豆叶片光合活性和叶绿体超微结构的影响

研究了受蚕豆萎蔫病毒2号（Broad bean wilt virus 2,BBWV2）中国分离物B935和欧洲分离物PV131侵染的蚕豆（Vicica faba）叶片光合特性、叶绿素荧光诱导动力学参数和叶绿体超微结构变化。感病蚕豆叶绿素含量减少,叶绿素a／b比逐步降低;光合气体交换参数Pn值和Gs值降低,Ci值升高;叶绿素荧光诱导动力学参数Fv/Fm、FV＇/Fm＇、ΦPSII、qP值均有不同程度降低,NPQ值升高;光合器结构遭到不同程度的破坏,B935侵染后叶绿体发育不良,片层结构疏松,PVl31侵染后叶绿体肿胀变圆,片层结构疏松瓦解。与B935相比,PV131侵染对以上各参数的变化有更大影响,且对叶绿体的破坏更为严重。实验结果表明BBWV2不同分离物对光系统II（PSII）的抑制作用与光合器受损程度相关。     

Extremely fast photoelectric signals from suspensions of broken chloroplasts and of isolated chromatophores

This paper concerns transient photoelectric signals that are observed when a suspension of photosynthetic vesicles is illuminated with flashing light of nonsaturating energy using a pair of electrodes positioned at different depths along the path of the exciting light. With chloroplasts we observed two different types of signals. One rose extremely fast, the rise time (10–90%) was less than 200 ps under excitation with a single pulse from a mode-locked ruby laser, while the other rose more slowly (typically 10 μs). These signals displayed several different properties such as their polarity, kinetics, apparent source impedance, and sensitivity to structural integrity of the chloroplast lamellar system. Experimentally, signal ‘Fast’ could only be induced by very short light pulses (shorter than approx. 60 ns), whereas signal ‘Slow’ appeared only under longer excitation. The detection of signal Fast required special instrumentation, particularly fast preamplifiers with low input capacitance. Our results support the more recent idea that signal Slow did not reflect the primary transmembrane charge separation, as postulated in the earlier literature, but rather lateral movement of charge carriers along the intact lamellar system of chloroplasts. On the other hand, signal Fast may reflect the primary outwardly directed electron transfer across the thylakoid membrane. Its polarity, however, was opposite to that previously postulated to appear in response to this event. For comparison we also studied photoelectric effects in a suspension of structurally more homogeneous chromatophores from Rhodopseudomonas sphaeroides. These vesicles displayed only a signal of the same polarity and similar kinetics as signal Fast from chloroplasts. When the secondary quinone electron acceptor (Q) was chemically reduced, the decay time was shortened from approx. 30 ns to approx. 10 ns. The acceleration to approx. 10 ns is known for the rapid, supposedly transmembrane back-reaction of the primary charge separation. Therefore, we conclude that the electrodes monitor the primary charge separation. There is still the unresolved problem with the polarity of the electric signal which we attribute to an as yet unidentified property of the pick-up system. Because its signal-to-noise ratio under extremely high time resolution is superior to that obtained in flash spectroscopy, signal Fast represents a very good means to measure the spatial separation between the very primary electron carriers in the photosynthetic reaction center.     

Na2CO3胁迫对星星草叶肉细胞超微结构的影响

利用透射电镜技术对Na2CO3胁迫下星星草叶肉细胞超微结构进行了观察。结果表明：未胁迫的叶肉细胞排列疏松,各种细胞器结构完整,叶绿体含少量淀粉粒和脂质球。轻度盐胁迫（2g/L,4g／LNa2CO3）对叶肉细胞超微结构影响较小。中度盐胁迫（6g／L,8g／L Na2CO3）引起叶肉细胞超微结构的变化,叶绿体类囊体肿胀,基粒紊乱,不含淀粉粒,脂质球数量增加,叶绿体由原来的梭形或椭球形变成圆球状;部分线粒体嵴消失,出现晶体结构;中央大液泡破裂;核逐渐降解。高度盐胁迫（10g／L,12g／LNa2CO3）下,叶绿体片层结构消失,脂质球数量增加,体积变大,被大量的膜片层所包围,叶绿体内、外膜消失,叶肉细胞中看不到叶绿体的存在;膜片层包围线粒体;叶肉细胞中可见大量的泡状结构和膜片层,叶肉细胞死亡。上述结果表明,细胞器特别是叶绿体膜结构的破坏与盐胁迫叶肉细胞最终死亡密切相关。     

Membrane proteins synthesized but not processed by isolated maize chloroplasts

One-dimensional maps of proteolytic fragments generated by digestion with Staphylococcus aureus protease in sodium dodecyl sulfate (SDS) were used to identify three polypeptides synthesized by isolated Zea mays chloroplasts. This technique does not depend upon proper incorporation of the newly synthesized polypeptides into a more complex structure for their identification. The only preliminary purification required is electrophoretic separation on SDS-polyacrylamide gels. The pattern of radioactive fragments from labeled proteins which co-migrate with the alpha and beta subunits of chloroplast coupling factor (CF1) corresponds precisely to the pattern of stainable fragments derived from subunits of the purified enzyme. A 34,500-dalton protein is the major membrane-associated product of protein synthesis by isolated maize chloroplasts. From the similarity in the fragments formed by digestion with S. aureus protease, it appears that this radioactive protein is probably a precursor of a 32,000-dalton protein which is a component of the thylakoid. The alpha and beta subunits of CF1 newly synthesized by isolated chloroplasts are not fully extractable by procedures which normally solubilize the enzyme from membranes. The 34,500-dalton protein is not processed to the 32,000-dalton form in any great amount by isolated chloroplasts. A 19,000-dalton fragment of the 32,000-dalton protein is protected from digestion when thylakoids are treated with proteases, while the newly synthesized 34,500-dalton protein is fully susceptible. The isolated chloroplast does not appear to be able to fully integrate these newly made proteins into the membrane structure.     

Temperature-sensitivity of D1 protein metabolism in isolated Zea mays chloroplasts

The effects of low temperature on the synthesis and stability of the 32 kDa D1 protein of photosystem II were investigated in chloroplasts isolated from maize (Zea mays cv. LG11) leaves. The synthesis of D1 by intact chloroplasts in vitro was strongly dependent on temperature; the Q₁₀ for the initial rate of incorporation of [³⁵S]-methionine into D1 was ca. 2.6 over the range 13–25°C. The synthesis of other thylakoid polypeptides exhibited a similar temperature dependence, whilst synthesis of stromal proteins was considerably less temperature-dependent, with the exception of two polypeptides of ca. 56 and 59.5 kDa. The stability of newly-synthesized D1 in the thylakoid membranes was dependent both on the temperature at which the plants were grown and on the temperature during the pulse-labelling period when the protein was synthesized. In chloroplasts isolated from maize leaves grown at 25°C, D1 that was synthesized and assembled at 25 °C in vitro was rapidly degraded during the chase period. At lower chase temperatures the protein was more stable. When chloroplasts from 25°C-grown leaves were pulse-labelled at 13°C, the stability of D1 was markedly enhanced at all temperatures during the chase period. This effect was even more pronounced in chloroplasts isolated from plants grown at 14°C. The implications of these results are discussed with regard to the ability of maize to recover from photoinhibitory damage at low temperatures.     

Photosynthetic activities of cadmium-treated tomato plants

Tomato plants (Lycopersicum esculentum Mill. cv. Moneymaker) grown on nutrient medium containing cadmium exhibit reduced net photosynthesis and reduced contents of chlorophyll and accessory pigments. In chloroplasts isolated from cadmiumtreated plants photosystem II activity, as measured by 2,6-dichlorophenolindophenol photoreduction, and photosystem II + I activity (H₂O → methyl viologen) were both inhibited to about 60%. When 1,5-diphenylcarbazide was used as artificial electron donor, no significant cadmium effect was observed. Photosystem I activity was not affected by cadmium. The fine structure of chloroplasts in cadmium-treated plants was degenerated, similarly to senescence response. The principal symptom of cadmium action was the occurrence of large plastoglobules and a disorganization of the lamellar structure, mainly grana stacks. Transfer of cadmium-treated plants into a medium with increased manganese level caused grana stacking and restoration of photosystem II activity.