The Small, Methionine-Rich Chloroplast Heat-Shock Protein Protects Photosystem II Electron Transport during Heat Stress1

Evidence suggests that the small chloroplast heat-shock protein (Hsp) is involved in plant thermotolerance but its site of action is unknown. Functional disruption of this Hsp using anti-Hsp antibodies or addition of purified Hsp to chloroplasts indicated that (a) this Hsp protects thermolabile photosystem II and, consequently, whole-chain electron transport during heat stress; and (b) this Hsp completely accounted for heat acclimation of electron transport in pre-heat-stressed plants. Therefore, this Hsp is a major adaptation to acute heat stress in plants.

Excited-state dynamics in photosystem II: Insights from the x-ray crystal structure

The heart of oxygenic photosynthesis is photosystem II (PSII), a multisubunit protein complex that uses solar energy to drive the splitting of water and production of molecular oxygen. The effectiveness of the photochemical reaction center of PSII depends on the efficient transfer of excitation energy from the surrounding antenna chlorophylls. A kinetic model for PSII, based on the x-ray crystal structure coordinates of 37 antenna and reaction center pigment molecules, allows us to map the major energy transfer routes from the antenna chlorophylls to the reaction center chromophores. The model shows that energy transfer to the reaction center is slow compared with the rate of primary electron transport and depends on a few bridging chlorophyll molecules. This unexpected energetic isolation of the reaction center in PSII is similar to that found in the bacterial photosystem, conflicts with the established view of the photophysics of PSII, and may be a functional requirement for primary photochemistry in photosynthesis. In addition, the model predicts a value for the intrinsic photochemical rate constant that is 4 times that found in bacterial reaction centers.

Quenching of chlorophyll fluorescence in the major light-harvesting complex of photosystem II: a systematic study of the effect of carotenoid structure.

The role of carotenoids in quenching of chlorophyll fluorescence in the major light-harvesting complex of photosystem II has been studied with a view to understanding the molecular basis of the control of photoprotective nonradiative energy dissipation by the xanthophyll cycle in vivo. The control of chlorophyll fluorescence quenching in the isolated complex has been investigated in terms of the number of the conjugated double bonds for a series of carotenoids ranging from n = 5-19, giving an estimated first excited singlet state energy from 20,700 cm-1 to 10,120 cm-1. At pH 7.8 the addition of exogenous carotenoids with >=10 conjugated double bonds (including zeaxanthin) stimulated fluorescence quenching relative to the control with no added carotenoid, whereas those with n photosystem II was induced by a lowering of pH to 5.5, carotenoids with n photosystem II could only be reversed by violaxanthin. These results are discussed in terms of the two theories developed to explain the role of zeaxanthin and violaxanthin in nonphotochemical quenching of chlorophyll fluorescence.

Destruction of a single chlorophyll is correlated with the photoinhibition of photosystem II with a transiently inactive donor side.

Pigments destroyed during photoinhibition of water-splitting photosystem II core complexes from the green alga Chlamydomonas reinhardtii were studied. Under conditions of a transiently inactivated donor side, illumination leads to an irreversible inhibition of the electron transfer at the donor side that is paralleled by the destruction of chlorophylls a absorbing maximally around 674 and 682 nm. The observed stochiometry of 1 +/- 0.1 destroyed chlorophyll per inhibited photosystem II suggests that chlorophyll destruction could be the primary photodamage causing the inhibition of photosystem II under these conditions.

Proximity of the manganese cluster of photosystem II to the redox-active tyrosine YZ.

Electron spin echo electron-nuclear double resonance (ESE-ENDOR) experiments performed on a broad radical electron paramagnetic resonance (EPR) signal observed in photosystem II particles depleted of Ca2+ indicate that this signal arises from the redox-active tyrosine YZ. The tyrosine EPR signal width is increased relative to that observed in a manganese-depleted preparation due to a magnetic interaction between the photosystem II manganese cluster and the tyrosine radical. The manganese cluster is located asymmetrically with respect to the symmetry-related tyrosines YZ and YD. The distance between the YZ tyrosine and the manganese cluster is estimated to be approximately 4.5 A. Due to this close proximity of the Mn cluster and the redox-active tyrosine YZ, we propose that this tyrosine abstracts protons from substrate water bound to the Mn cluster.

Molecular characterization of PsbW, a nuclear-encoded component of the photosystem II reaction center complex in spinach.

We describe the isolation and characterization of cDNAs encoding the precursor polypeptide of the 6.1-kDa polypeptide associated with the reaction center core of the photosystem II complex from spinach. PsbW, the gene encoding this polypeptide, is present in a single copy per haploid genome. The mature polypeptide with 54 amino acid residues is characterized by a hydrophobic transmembrane segment, and, although an intrinsic membrane protein, it carries a bipartite transit peptide of 83 amino acid residues which directs the N terminus of the mature protein into the chloroplast lumen. Thylakoid integration of this polypeptide does not require a delta pH across the membrane, nor is it azide-sensitive, suggesting that the polypeptide chain inserts spontaneously in an as yet unknown way. The PsbW mRNA levels are light regulated. Similar to cytochrome b559 and PsbS, but different from the chlorophyll-complexing polypeptides D1, D2, CP43, and CP47 of photosystem II, PsbW is present in etiolated spinach seedlings.

A multimer model for P680, the primary electron donor of photosystem II.

We consider a model of the photosystem II (PS II) reaction center in which its spectral properties result from weak (approximately 100 cm-1) excitonic interactions between the majority of reaction center chlorins. Such a model is consistent with a structure similar to that of the reaction center of purple bacteria but with a reduced coupling of the chlorophyll special pair. We find that this model is consistent with many experimental studies of PS II. The similarity in magnitude of the exciton coupling and energetic disorder in PS II results in the exciton states being structurally highly heterogeneous. This model suggests that P680, the primary electron donor of PS II, should not be considered a dimer but a multimer of several weakly coupled pigments, including the pheophytin electron acceptor. We thus conclude that even if the reaction center of PS II is structurally similar to that of purple bacteria, its spectroscopy and primary photochemistry may be very different.

Detection of one slowly exchanging substrate water molecule in the S3 state of photosystem II.

The exchangeability of the substrate water molecules at the catalytic site of water oxidation in photosystem II has been probed by isotope-exchange measurements using mass spectrometric detection of flash-induced oxygen evolution. A stirred sample chamber was constructed to reduce the lag time between injection of H2(18)O and the detecting flash by a factor of more than 1000 compared to the original experiments by R. Radmer and O. Ollinger [(1986) FEBS Lett. 195, 285-289]. Our data show that there is a slow (t1/2 approximately 500 ms, 10 degrees C) and a fast (t1/2 <25 ms, 10 degrees C) exchanging substrate water molecule in the S3 state of photosystem II. The slow exchange is coupled with an activation energy of about 75 kJ/mol and is discussed in terms of a terminal manganese oxo ligand, while the faster exchanging substrate molecule may represent a water molecule not directly bound to the manganese center.

Phototoxicity of photosystem II (PSII) herbicides to coral

Recent reports of contamination of the Great Barrier Reef Marine Park by herbicides used in antifouling paints and in agriculture have caused concern over the possible effects on corals in nearshore areas. Pulse-Amplitude Modulated (PAM) chlorophyll fluorescence techniques were used to examine changes in the maximum effective quantum yield (ΔF/Fm′) of symbiotic dinoflagellates within the host tissues (in hospite) of the coral Seriatopora hystrix exposed to a number of Photosystem II (PSII) inhibiting herbicides in short-term toxicity tests. The concentration of herbicide required to reduce ΔF/Fm′ by 50% (median effective concentration [EC50]) differed by over 2 orders of magnitude: Irgarol 1051 (0.7 μg l-1) > ametryn (1.7 μg l-1) > diuron (2.3 μg l-1) > hexazinone (8.8 μg l -1) > atrazine (45 μg l-1) > simazine (150 μg l-1) > tebuthiuron (175 μg l-1) > ionynil (> 1 mg l-1). Similar absolute and relative toxicities were observed with colonies of the coral Acropora formosa (Irgarol 1051 EC50: 1.3 μg l-1, diuron EC50: 2.8 μg l-1), Time-course experiments indicated that ΔF/Fm′ was rapidly reduced (i.e. within minutes) in S. hystrix exposed to Irgarol 1051 and diuron. On return to fresh running seawater, ΔF/Fm′ recovered quickly in diuron-exposed corals (i.e. in minutes to hours), but slowly in corals exposed to Irgarol 1051 (i.e. hours to days). Time-course experiments indicated that the effects of diuron (3 μg l-1) on S. hystrix were inversely related to temperature over the range 20 to 30 °C, although initially the effects were less at the lower temperatures. Repeated exposure to pulses of Irgarol 1051 (daily 2 h exposure to 30 μg l -1 over 4 d) resulted in a 30% decrease in the density of symbiotic dinoflagellates in the tissues of S. hystrix.

Effects of Photosystem II inhibiting herbicides on mangroves - preliminary toxicology trials

Mangroves are sensitive to the root application of Photosystem II inhibiting herbicides and Avicennia marina is more sensitive than other mangroves tested. Seedlings of four mangrove species, including two salt-excreting species (A. marina and Aegiceras corniculatum) and two salt-excluding species (Rhizophora stylosa and Ceriops australis) were treated with a range of concentrations of the herbicides diuron, ametryn and atrazine. Assessment of responses required the separation of seedlings into two groups: those that had only their roots exposed to the herbicides through the water (A. marina and R. stylosa) and those that had both roots and leaves exposed to herbicides through the water (A. corniculatum and C australis). Salt-excreting species in each group were more susceptible to all herbicide treatments than salt-excluding species, indicating that root physiology was a major factor in the uptake of toxic pollutants in mangroves. Submergence of leaves appeared to facilitate herbicide uptake, having serious implications for seedling recruitment in the field. Each herbicide was ranked by its toxicity to mangrove seedlings from most damaging to least effective, with diuron > ametryn > atrazine. The relative sensitivity of A. marina found in these pot trials was consistent with the observed sensitivity of this species in the field, notably where severe dieback had specifically affected A. marina in the Mackay region, north eastern Australia. (c) 2004 Elsevier Ltd. All rights reserved.

光系统II反应中心吸能和转能的分子机理研究

全文分两部分，(1)．PsⅡ反应中心色素分子光破坏的分子机理研究;(2)．PSⅡ反应中心原初反应的动力学机理研究。 在第一部分中，在分离纯化的光系统Ⅱ反应中心Dl/D2/Cyt b559复合物中，采用高效液相色谱技术，首次发现PSⅡ反应中心去镁叶绿素分子的光照破坏，研究了去镁叶绿素的光破坏机理，观察到PsⅡ反应中心内部存在一个与光化学活性无关的去镁叶绿素分子，从而提供了PSⅡ反应中心存在两条电子传递链的第一个实验证据，提出了去镁叶绿素对PsⅡ反应中心的光保护假说和光合作用反应中心第二条电子传递支路的光保护假说。用高效液相色谱技术还观察到PSⅡ反应中心的6个叶绿素a分子，有三种不同的存在状态，认为PSl反应中心的最小色素组成为每个反应中心含有4个叶绿素a和2个去镁叶绿素。用光破坏的方法证明PsⅡ原初电子供体P680是由两个叶绿素n分子组成，认为P680是以一个二聚体形式存在，首次发现P680的光破坏过程包含失去中心镁原子的反应。 在第二部分中，用皮秒和飞秒时间分辨光谱技术，在PsⅡ颗粒、PsⅡ核心复合物和PSⅡ反应中心三个层次上，研究了PsⅡ原初反应的动力学性质，着重研究电荷分离和PsⅡ反应中心内部的能量传递过程。结果表明，B-胡萝卜素和P680之间的能量传递时间常数为350p8左右，去镁叶绿素a与P680之间的能量传递时间为lOOp8左右，提出了可能的动力学模型。 在目前分歧最大的原初电荷分离时间常数测定这一焦点问题上，得到的初步结果表明PsⅡ反应中心电荷分离时间为3-3.5pa左右，这一结论与文献上报道的21pa不同，丽倾向于支持国际上3p8的观点。

光系统II反应中心复合物组成性质与光仰制分子机理研究

由于光系统Ⅱ反应中心Dl/D2/Cyt b559色素蛋白复合物(PSII-RC)的红 区吸收光谱严重重叠，给其组成特性研究及光抑制分子机理研究造成 了困难，因此我们运用多种光谱分析技术配合计算机数据处理技术对 PSII-RC复合物的组成特性进行了研究，并用自己建立的方法对PSII-RC 的色素和多肽的化学计量进行了进一步确定，另外还重点研究了单线 态氧在PSII-RC光破坏中的作用，据此提出新的PSD[-RC光抑制分子机 理。主要结果如下： 1．用反相HPLC外标法测定我们制备的色谱纯PSR-RC样品的色素化 学计量结果为Chl:Pheo:Car= 6:2:2。我们发现，当PSII-RC中存在微量CP47 时，Chl: Pheo的比例与CP47的含量呈正相关关系，说明较高的Chl比例 可能表示样品中有CP47污染。结果还表明PSII-RC中Car: Pheo的比例也与 CP47含量有关，说明CP47可影响Car在PSII-RC上的结合，这暗示CP47可 能结合Car，或者CP47对PSII-RC上Car的结合位点有影响，这一推测对阐 明CP47的功能有一定启发作用。 2．建立了一种估算PSII-RC多肽化学计量的理论计算方法，即利用计 算机统计PSII-RC中各多肽组分的不同氨基酸残基数量，以确定不同多 肽化学计量时的理论氨基酸残基组成，并与PSlI-RC的实测氨基酸残基 组成进行比较，得到所用PSII-RC样品的多肽化学计量值为D1+D2:Cyt b559-o+邮：I=2:1:1. 3．对PSII-RC的红区吸收光谱进行了高斯解析，发现680 nm附近含有 峰高和半高宽明显不同的两个高斯组分，它们对光抑制处理的响应具 有明显差别，分别表现了P680和Pheo的特征。由此可知，在680nm处除了 有P680的信号外，PSII-RC中的Pheo在这个区域也有跃迁组分。这个结果 表明光抑制进程中PSII-RC红区吸收光谱信号的下降除了P680的破坏 外，还与Pheo的破坏有关。 4．用Ste)anov关系式分析了PSII-RC色素激发态分布的平衡状态，发现 经过暗适应的PSII-RC的激发态可达到充分的平衡，光抑制处理可导致 PSIL-RC激发态平衡受到破坏。 5．用荧光发射光谱观察到PSII-RC在光抑制进程中有弱光破坏和强光 破坏两个破坏过程，前者是与色素间能量传递的色素结合状态与 取向的破坏，后者与色素本身化学结构的破坏有关。通过研究不同激发波长下的发射光谱发现Car的弱光破坏过程比Chl快，暗示Car可能的保护作用，而Pheo的破坏程度比Chl小。从发射光谱组分的光破坏时间 进程推断强光破坏过程导致的色素破坏是多步反应，验证我们小组原 先报导的PSII-RC的多步反应特性。 6．首次将磁圆二色光谱( MCD)技术应用于PSII-RC研究，发现MCD明显表现出比吸收光谱要丰富得多的光谱精细结构，同时还具有较高的灵敏度和分辨率，不经过任何解析就可直接观察到680 nm组分及其它色素组分的变化，而且PSⅡ-RC中的Car没有明显MCD信号，使PSII-RC谱 图简化，便于进一步分析。用MCD技术还观察到光抑制初期Chl从PSII- RC复合物上脱离及Pheo的光破坏现象。 7．分别用HPLC法、吸收光谱高斯解析法、荧光发射光谱分析法和MCD法共四种方法证明了PSII-RC中Pheo的光破坏，充分证实我们小组关于Pheo光破坏的报导，同时还证明Pheo的光破坏是单线态氧作用的结果。 8．给出了单线态氧参与PSII-RC色素和蛋白光破坏的直接实验证 据，即发现光抑制过程中色素和蛋白的破坏受到单线态氧的特异性清除剂的保护，用化学方法在暗中产生的单线态氧同样造成与光抑制相 似的PSII-RC各组分的损伤，由此说明单线态氧是PSII-RC光抑制过程中 的直接破坏因子。 9．提出了PSII-RC中Hiis残基光破坏的一种新的分子机理。用组氨酸残基的特异性化学修饰剂证实以前我们实验室发现的PSI[-RC组氨酸残基的光破坏，根据比较蛋白变性前后的测定结果，初步证明PSIl-RC中 受光破坏的His残基位于P680附近。我们还观察到光抑制处理后，PSII- RC表现与组氨酸残基被修饰后的样品相似的紫外吸收特征，由此提出 PSII-RC中His残基光破坏的一种分子机理，即His残基的眯唑环上的两个氮原子与其它多肽上的游离氨基在单线态氧的作用下发生反应形成酰 胺键而导致PsII-RC多肽间的共价交联，推测PSII-RC中His残基的光破坏与其蛋白的光致交联和降解有直接的因果联系。

光系统II复合物的光仰制特征及其内源保护机理

本文以菠菜PSⅡ颗粒PSⅡ核心复合物和PSⅡ反应中心复合物为材料通过比较光抑制处理和单线态氧处理对上述制剂色素、蛋白和光谱特性的影响，．以及光抑制对细胞色素b559 (Cyt b559)和放氧的影响，研究了PSⅡ光抑制及其内源保护机理得到如下的结果: 1)光抑制处理和外源单线态氧处理对PSⅡ具有相似的破坏特性,同时，加入单线态氧的特异性清除剂组氨酸(His)可明显遏制光抑制处理对PSⅡ各组分的破坏这些结果说明单线态氧参与了PSⅡ的光破坏过程. 2) PSⅡ蛋白组分不仅受到强光的破坏，而且在照光后暗放置过程中还继续受到破坏 这种暗放置破坏过程具有温度敏感性因此推测在光照后暗放置过程中的PSⅡ蛋白降解是酶促反应这些结果证明，PSⅡ蛋白的光破坏具有活性氧损伤和酶促水解两种可能的破坏机理． 3)首次观察到PSⅡ中Cyt b559的高电势态(qt b559 HP)的百分含量在光抑制初期上升，随后下降的现象且这种变化受到外加强His的遏制。表明光抑制产生的单线态氧参与了Cytb559 HP百分含量的改变,同时还观察到这种变化的时间进程与PSⅡ蛋白二级结构在光抑制中变化的时间进程相似后者也表现出双相变化进程这说明光抑制产生的单线态氧引起了蛋白构象的变化后者导致了Cytb559 HP百分含量的改变. 4)在不同的处理条件下，PSⅡ放氧活性的变化与Cyt b559 HP百分含量的变化具有明显的相关性它们的变化可能具有相同的原因，即PSⅡ蛋白构象的改变． 5)无氧条件下照光时’PSⅡ反应中心复合物中的Cytb559的低电势态(Cytb559 LP)可从Pheo得到电子而被还原具有较高反应活性的Pheo被清除这体现了Cytb559 LP的一种光保护功能. 综合上述结果及参考已有的文献我们提出了一种以Cytb559为中心的PSⅡ光抑制快速内源保护机理的调控模型。光抑制通过影响PSⅡ蛋白构象而使Cytb559 HP和Cytb559 LP发生相互转换。Cytb559 HP具有清除活性氧的功能，而Cytb559 LP态则具有从Pheo或QA吸收电子的作甩因此它们可受PSⅡ不同状态的调节进行相互转换以淬灭活性自由基达到保护PSⅡ功能的目的。

磷脂对光系统II光合放氧的影响及其作用机理的研究

以类囊体膜中唯一的阴离子型磷脂一磷脂酰甘油(PG)为研究对象，应用放氧测定和富立叶红外光谱等实验方法和技术手段，对PG与光系统II (PSII)之间的相互作用进行了研究。 研究表明，PG对PSII的放氧活性产生显著影响，具有明显的浓度效应。在低浓度(2～22 mg PG／mg Chl)时对PSII的放氧活性有明显的促进作用，而在高浓度(24～40 mg PG／mg Chl)下则表现出显著的抑制作用。 PG对PSII放氧活性的影响与其引起蛋白结构的改变密切相关。结果显示，PG的作用导致PSII颗粒中蛋白质二级结构的改变，主要表现为α-螺旋、β-折叠的增加和无规卷曲的减少。 不仅如此，红外光谱的分析还表明，PG还使蛋白酪氨酸残基中的酚基构象及其周围的微极性发生改变，即在红外光谱的1620—1500 cm-1，之间芳香环骨架的伸缩振动带向高频方向变化，其吸收强度也相应增加;在3500～3100 cm. -1间出现新的氢键吸收峰。 PG除能促进PSII的放氧活性以外，还对PSII表现出新的作用，即PG可以使PSII颗粒因缺钙而受抑制的放氧活性得到恢复;外加Ca2+可使PG表现出对缺钙PSII颗粒(dc。PSII)放氧活性的更大促进作用，且随Ca2+浓度的增加，促进作用也越显著。 PG的作用也使dc。PSII蛋白的结构发生了改变，导致蛋白二级结构中a-螺旋、p_折叠结构的增加和转角、无规卷曲成分的减少，即可使PSII颗粒因缺钙而改变的蛋白结构基本得到恢复。PG还能与Ca2+形成离子对似的配合物，而这种配合物的形成可以优化缺钙PSII颗粒的功能如放氧活性等。

高等植物光系统II捕光天线结构与功能的研究

高等植物光系统II的捕光天线蛋白（LHC II）在光能的吸收、传递和调节激发能在两个光系统之间的分配以及维持类囊体膜的垛叠等方面都起着重要的作用，因而得到了广泛的研究。目前普遍认为LHC II在植物体内是以三聚体的形式存在并行使功能的，但也有研究者发现了单体和寡聚体等多种形式的LHC II。本论文以菠菜为研究对象，采用改进的方法从类囊体膜中提取纯化了LHC II三聚体，对膜脂和色素在三聚体形成和蛋白空间结构中的影响，以及不同聚集态LHC II组成、结构和功能的差异进行了较系统的研究。此外，还将Lhcb2基因反向插入到烟草中，利用转基因植物来研究其生理功能。获得了如下结果： 1，采用改进的方法从菠菜类囊体膜中分离纯化了LHC II。与改进前比，其流程可以缩短2小时且产率也有明显的提高。SDS变性电泳和Triton X-100非变性电泳的检测结果表明，此样品纯度较高，是由三条分子量分别为29KD、28KD和26KD的多肽组成的异质三聚体。同时样品的吸收光谱和荧光光谱分析结果也与前人的报道一致。 2，分析了LHC II三聚体中的膜脂和脂肪酸组成及含量。与PSII相比，LHC II含有相同的四种膜脂：MGDG、DGDG、PG和SQDG。但LHC II中PG的含量是PSII的两倍，说明PSII中的PG主要富集在外周天线区域。同时PG中含有特异的反式十六碳一烯酸，且含量很高。用专一消化PG上Sn-2位脂肪酸链的磷脂酶A2（PLA2）处理LHC II三聚体，然后再加入PG重组的方法证明了含十六碳一烯酸的PG在三聚体结构的维持中起着至关重要的作用。去掉PG后， LHC II三聚体的结构受到了影响，部分解聚成了单体，同时其光谱特性也发生了变化，表现为叶绿素b分子的吸收峰及其激发的荧光发射峰都明显下降。回加PG则可使解聚的单体又重新聚集成三聚体。 3，分别用电洗脱和蔗糖密度梯度离心两种方法分离了LHC II三聚体、二聚体和单体。两者比较，电洗脱对样品的破坏较大，而蔗糖密度梯度离心更加温和，对蛋白上结合的色素影响不大。系统研究了不同聚集态LHC II的组成和光谱特性后发现，三种聚集态的LHC II有相同的多肽组成，并且都结合着5种色素，但是色素的含量差异较大。二聚体和单体中，叶绿素b和类胡萝卜素分子的含量比三聚体的低很多，此外，单体叶绿素a分子的含量也明显减少。对三种聚集态LHC II的各种光谱特性进行分析的结果表明，由于叶绿素b和类胡萝卜素分子含量较少，二聚体和单体中叶绿素b和类胡萝卜素的吸收均有所下降，而且从类胡萝卜素到叶绿素b以及从叶绿素b到叶绿素a的能量传递效率都低于LHC II三聚体，总体表现为三聚体 > 二聚体 > 单体。此外，不同单体之间叶绿素a到叶绿素a的能量传递也被破坏。推测三种聚集态LHC II在吸能、传能和结构上的差异，可能是植物适应不同外界环境的一种调控机制。 4，模拟体内过程，在体外将大肠杆菌中表达的Lhcb2蛋白和色素进行重组，以此来研究色素与蛋白组装过程中蛋白二级结构和色素结合状态的变化。结果表明色素在脱辅基蛋白的体外重折叠中至关重要。在与色素重组的过程中，蛋白二级结构中-螺旋含量逐渐上升并最终接近天然水平，而无规卷曲逐渐减少。从光谱的变化可以看出，色素分子与蛋白的结合经历了一个由无序到有序的过程，色素蛋白复合物的光谱信号由弱变强，重组得到的样品与天然LHC II十分相似。 5，为了更好地研究LHC II异质三聚体中单体可能具有的独特生理功能，建立了Lhcb2基因的反义抑制植物表达载体pBI-antiLhcb2，用根癌农杆菌介导法转化烟草，获得了转基因植株。酶切和PCR鉴定证明，Lhcb2基因已经成功地插入到烟草里。进一步的分子鉴定和生理生化功能分析还在进行中。