非生物胁迫下植物脱水素的研究进展

脱水素是LEA蛋白中的一类,广泛存在于植物的各个组织器官及植物胚胎发育后期.脱水素是植物在受低温、干旱和高盐等非生物逆境胁迫时合成的一类高亲水性保护蛋白,具有保护核酸、胞内蛋白和膜结构免受损害的功能.许多研究已经证实在非生物胁迫下,植物脱水素的表达与积累和植物抗逆性之间存在着紧密的联系.对脱水素的结构、亚细胞定位、基因表达模式及非生物胁迫下脱水素作用的最新研究成果进行了综述.     

Ca2+、ABA预处理蝴蝶兰类原球茎的脱水保护系统比较及信号传导关系

CaCl2和ABA溶液及两者联合分别预处理蝴蝶兰类原球茎(PLB)后脱水,对比PLB脱水前后的成活率、脱水保护系统指标变化及Ca2+与ABA信号传导关系.结果表明,CaCl2和ABA溶液及两者联合预处理均能明显提高PLB脱水后的成活率.CaCl2和ABA溶液对可溶性糖、蔗糖、还原糖、SOD和总抗氧化能力有相同的效应趋势,对可溶性蛋白、热稳定蛋白含量及POD、CAT活性的作用趋势有所差异.ABA溶液提高PLB耐脱水性的能力被胞质Ca2+ 螯合剂BAPTA/AM 和钙调蛋白拮抗剂氯丙嗪所削弱,Ca2+预处理提高PLB耐脱水能力被ABA合成抑制剂环丙嘧啶醇削弱.在蝴蝶兰PLB的耐脱水性诱导中,Ca2+和ABA具有基本相同的生理生化基础,在信号传递中两者互相关联,CaCl2取代ABA用于提高PLB耐脱水性是可行的.     

低温诱导蛋白及其与植物的耐寒性研究进展

低温诱导蛋白是植物在温度逆境条件下诱导产生的一系列蛋白,以抗冻蛋白、脱水蛋白、热激蛋白和热稳定蛋白较多,而且低温诱导蛋白质一旦在体内形成,植物体就会尽快地适应外界环境,表现出较强的抗逆性.本文对几种主要的低温诱导蛋白——抗冻蛋白、脱水蛋白、热激蛋白和热稳定蛋白的特性及其与植物耐寒性的关系研究进行综述,以期为进一步阐明植物耐寒的分子机制以及提高植物耐寒力研究提供新的思路.     

渗透胁迫下脱水蛋白DHN1在猕猴桃细胞中表达及亚细胞分布的动态变化

以绿色荧光蛋白(GFP)为报告分子, 通过构建DHN1-mGFP4融合蛋白表达载体, 研究了渗透胁迫条件下脱水蛋白DHN1的表达及其亚细胞分布的动态变化. 采用PCR方法在脱水蛋白基因dhn1两端引入XbaⅠ和BamHⅠ限制性内切酶位点, 克隆到质粒pBIN-35S mGFP4, 构建DHN1-mGFP4融合蛋白表达载体, 并采用基因枪转化猕猴桃(A. delicisoa)悬浮细胞. 培养10 h后观察到高效表达的GFP绿色荧光, 绿色荧光只出现在细胞核内. 提高培养介质渗透势后, 可以诱导脱水蛋白向细胞质分布(主要集中在质膜周围), 并且增加介质渗透势可以明显缩短细胞质出现绿色荧光的时间. 蛋白合成抑制剂环己亚胺能够抑制细胞质绿色荧光的出现, 暗示细胞质出现的脱水蛋白是诱导产生的结果. ABA可以明显促进细胞质绿色荧光的出现, 并且随着介质渗透势的升高迅速缩短细胞质绿色荧光的出现时间.     

脱水素在植物低温胁迫响应中的作用

脱水素(dehydrin)是一类胚胎发育后期丰富蛋白(LEA.late embryogenesis abundant proteins),含有富含赖氨酸的K片段,属于具有高度热稳定性的亲水性蛋白,在植物脱水条件下能保护细胞内蛋白质和膜结构免受破坏.低温胁迫下,耐低温植物细胞内部会发生一系列的生理生化反应来抵御低温所造成的伤害.很多研究表明植物脱水素的表达和积累与多种双子叶植物(包括草本和木本植物)以及冬季栽培的禾本科植物品种(特别是小麦和大麦)的耐低温能力密切相关.本文对近年来国内外关于脱水素的结构、功能以及内源ABA(abscisie acid)含量、拟南芥CBF(C-repeat binding factor)同源转录激活因子、春化基因、光周期信号等对脱水素基因的表达调控机制进行综述.     

茶树种子脱水过程差异基因的研究

利用cDNA-AFLP方法在转录水平上对茶树无性系龙井43种子脱水前后基因表达的变化进行分析,探讨脱水差异和生物学中的衰老与死亡的联系,并为茶树等顽拗型种子植物的种质资源保存提供理论依据.结果显示:64对引物组合产生87条差异条带.对其中的6条克隆测序,发现4条与已知功能基因相关,包括植物衰老蛋白、PPR、硫氧还蛋白,翻译控制肿瘤蛋白,其中硫氧还蛋白在茶树种子中首次被发现.     

茶树叶片类脱水素蛋白的Western-blot分析

为了解茶树脱水素种类与功能,采用Western-blot技术,研究了不同季节及越冬过程中茶树叶片脱水素蛋白家族的表达模式。结果显示:(1)茶树叶片总蛋白提取采用酚-甲醇/醋酸铵沉淀法,用时短、蛋白浓度高、SDSPAGE电泳条带清晰,背景干净,满足茶树Western-blot技术要求。(2)在不同季节及越冬期中发现14~95kD共9种不同分子量的茶树类脱水素蛋白,其中95、65、48、37、34和14kD等6种蛋白表达量较为稳定,季节与越冬期变化不明显;58kD脱水素仅在冬季表达,越冬期不断上升,2月份增加到最高,表达丰度高;28kD脱水素蛋白在冬季表达量高,越冬期与茶树抗寒力变化规律一致;21kD脱水素在夏季和越冬期后期有较高的表达。研究表明,这3种脱水素可能在茶树抗逆中起着重要作用。     

油茶脱水素样蛋白的基因克隆与序列分析及其生理功能预测

以油茶EST文库为基础,采用5-′RACE技术,分离克隆了一个脱水素样基因的全长cDNA序列(GenBank接受号EU856537),同源分析表明其编码的208 aa的小分子蛋白(id号ACF72673)属于SK2型脱水素,命名为CoDHN2.CoDHN2的肽链内2个类K-片段间富含苏氨酸,有别于脱水素一般性结构特点,并且同油茶种子中另一类脱水素一样也具有一个十分保守的基序(EDDGQAGRRKK),这可能有利于脱水素的磷酸化和亚细胞定位;采用多种方法预测其二级结构,表明CoDHN2为内在性无规则蛋白,但其中远离C端的一个类K-片段可形成两亲性α-螺旋.CoDHN2含有较多的组氨酸残基以及良好的可溶性,推测它可结合金属离子从而减少活性氧的来源并清除活性氧,并在生理脱水时充当缓冲液.结合其它物种脱水素的研究进展,认为CoDHN2极有可能在油茶油脂合成高峰期同正在发育的脂体结合而保护脂体免受活性氧危害,这为油茶种子细胞的脂体发育研究提出了一个新的方向.     

花生种子耐脱水力的获得与热稳定蛋白的关系

花生（ＡｒａｃｈｉｓｈｙｐｏｇａｅａＬ．）种子的耐脱水能力在果针入土后４５ｄ以后的胚胎发育期逐渐增加,与一组９～１５．５ｋＤ低分子量热稳定蛋白的丰富表达有关。缓慢干燥可以诱导不耐脱水的果针入土后２５ｄ及３５ｄ花生胚获得耐脱水能力并同时诱导胚轴表达这组热稳定蛋白。成熟脱水促进花生胚耐脱水能力的获得,并增加了花生球蛋白的热稳定性。     

小麦类脱水素的表达、纯化及多克隆抗体的制备

脱水素在胚胎发育后期累积,外源脱落酸(ABA)、低温、干旱和其他一些环境条件下能诱导脱水素的产生,尽管植物在脱水条件下脱水素广泛存在于细胞中,但其生化功能仍不清楚.为研究小麦在不同时期脱水素基因的表达情况和生物学功能及抗体制备,以小麦幼芽为材料,经干旱胁迫处理后,提取总RNA,通过RT-PCR得到小麦类脱水素基因片段(WZY1-1),再连接至克隆载体PUCM-T,并成功构建重组表达质粒PET-32a( )-wzy1-1,将阳性重组质粒转化于受体菌BL21(DE3)感受态细胞中,经IPTG诱导表达,进行表达产物的聚丙烯酰胺凝胶电泳(SDS-PAGE)检测.结果表明,表达蛋白位于37ku处,小麦类脱水素基因获得高效表达.表达蛋白经Ni2 琼脂糖凝胶亲和层析和透析袋电洗脱法纯化后,对兔子进行免疫,制备的抗血清通过ELISA检测到较高的多克隆抗体效价.蛋白质印迹结果显示,利用纯化的蛋白质制备的兔抗血清可以很好地和所表达的蛋白质带特异性结合,且郑引1号小麦幼苗进行干旱处理,提取粗蛋白,SDS-PAGE,蛋白质印迹检测显示,在分子质量28ku处出现特异的蛋白质条带,这说明所制备的抗血清可以与小麦叶片所表达的dehydrin蛋白特异性结合,证明其具有良好的免疫原性.     

Pea dehydrins: identification,characterisation and expression

An antiserum raised against dehydrin from maize (Zea mays) recognised several polypeptides in extracts of pea (Pisum sativum) cotyledons. A cDNA expression library was prepared from mRNA of developing cotyledons, screened with the antiserum and positive clones were purified and characterised. The nucleotide sequence of one such clone, pPsB12, contained an open reading frame which would encode a polypeptide with regions of significant amino acid sequence similarity to dehydrins from other plant species.The deduced amino acid sequence of the pea dehydrin encoded by B12 is 197 amino acids in length, has a high glycine content (25.9%), lacks tryptophan and is highly hydrophilic. The polypeptide has an estimated molecular mass of 20.4 kDa and pI=6.4. An in vitro synthesised product from the clone comigrates with one of the in vivo proteins recognised by the antiserum.A comparison of the pea dehydrin sequence with sequences from other species revealed conserved amino acid regions: an N-terminal DEYGNP and a lysine-rich block (KIKEKLPG), both of which are present in two copies. Unexpectedly, pea dehydrin lacks a stretch of serine residues which is conserved in other dehydrins.B12 mRNA and dehydrin proteins accumulated in dehydration-stressed seedlings, associated with elevated levels of endogenous abscisic acid (ABA). Applied ABA induced expression of dehydrins in unstressed seedlings. Dehydrin expression was rapidly reversed when seedlings were removed from the stress or from treatment with ABA and placed in water.During pea cotyledon development, dehydrin mRNA and proteins accumulated in mid to late embryogenesis. Dehydrin proteins were some of the most actively synthesised at about the time of maximum fresh weight and represent about 2% of protein in mature cotyledons.     

A dehydrin cognate protein from pea (Pisum sativum L.) with an atypical pattern of expression

Dehydrins are a family of proteins characterised by conserved amino acid motifs, and induced in plants by dehydration or treatment with ABA. An antiserum was raised against a synthetic oligopeptide based on the most highly conserved dehydrin amino acid motif, the lysine-rich block (core sequence KIKEK-LPG). This antiserum detected a novel M _r 40 000 polypeptide and enabled isolation of a corresponding cDNA clone, pPsB61 (B61). The deduced amino acid sequence contained two lysine-rich blocks, however the remainder of the sequence differed markedly from other pea dehydrins. Surprisingly, the sequence contained a stretch of serine residues, a characteristic common to dehydrins from many plant species but which is missing in pea dehydrin.The expression patterns of B61 mRNA and polypeptide were distinctively different from those of the pea dehydrins during seed development, germination and in young seedlings exposed to dehydration stress or treated with ABA. In particular, dehydration stress led to slightly reduced levels of B61 RNA, and ABA application to young seedlings had no marked effect on its abundance.The M _r 40 000 polypeptide is thus related to pea dehydrin by the presence of the most highly conserved amino acid sequence motifs, but lacks the characteristic expression pattern of dehydrin. By analogy with heat shock cognate proteins we refer to this protein as a dehydrin cognate.     

Development of Desiccation Tolerance during Embryogenesis in Rice (Oryza sativa) and Wild Rice (Zizania palustris) (Dehydrin Expression,Abscisic Acid Content,and Sucrose Accumulation)

The ability of seeds to withstand desiccation develops during embryogenesis and differs considerably among species. Paddy rice (Oryza sativa L.) grains readily survive dehydration to as low as 2% water content, whereas North American wild rice (Zizania palustris var interior [Fasset] Dore) grains are not tolerant of water contents below 6% and are sensitive to drying and imbibition conditions. During embryogenesis, dehydrin proteins, abscisic acid (ABA), and saccharides are synthesized, and all have been implicated in the development of desiccation tolerance. We examined the accumulation patterns of dehydrin protein, ABA, and soluble saccharides (sucrose and oligosaccharides) of rice embryos and wild rice axes in relation to the development of desiccation tolerance during embryogenesis. Dehydrin protein was detected immunologically with an antibody raised against a conserved dehydrin amino acid sequence. Both rice and wild rice embryos accumulated a 21-kD dehydrin protein during development, and an immunologically related 38-kD protein accumulated similarly in rice. Dehydrin protein synthesis was detected before desiccation tolerance had developed in both rice embryos and wild rice axes. However, the major accumulation of dehydrin occurred after most seeds of both species had become desiccation tolerant. ABA accumulated in wild rice axes to about twice the amount present in rice embryos. There were no obvious relationships between ABA and the temporal expression patterns of dehydrin protein in either rice or wild rice. Wild rice axes accumulated about twice as much sucrose as rice embryos. Oligosaccharides were present at only about one-tenth of the maximum sucrose concentrations in both rice and wild rice. We conclude that the desiccation sensitivity displayed by wild rice grains is not due to an inability to synthesize dehydrin proteins, ABA, or soluble carbohydrates.     

Isolation and characterization of a novel dehydrin gene from Capsella bursa-pastoris

A novel dehydrin gene designated as Cbcor29 was cloned from Capsella bursa-pastoris by rapid amplification of cDNA ends (RACE) and genome walker technique. The full-length cDNA of Cbcor29 was 1101 bp long with a 783 bp open reading frame (ORF), encoding a putative protein of 261 amino acids. Like other dehydrin proteins, CbCOR29 contained a high percentage of charged and polar amino acids, in which Cys and Trp amino acids were absent. Besides, predicted CbCOR29 protein possesses three conserved repeats of the characterized Lys-rich domains (K-segments), and a Ser-rich domain (S-segment) prior to the first Lys-rich domain, which presented a typical SK3 structure of dehydrins. Analysis of Cbcor29 genomic DNA revealed that it contained 2 exons and 1 intron, which was a typical character of dehydrin genes. Subsequent bioinformatic analysis also showed that the sequence of CbCOR29 had high homology with other dehydrin proteins, especially with cor47 from Arabidopsis thaliana. Moreover, semi-quantitative RT-PCR revealed that the expression of Cbcor29 could be induced by exposure to drought, low-temperature, NaCl and exogenous ABA treatment respectively. Our study implied that the Cbcor29 gene was a new member of the dehydrin gene family and might exert functions in drought-, cold- and salt- responsiveness in Capsella bursa-pastoris.     

A 25-kDa dehydrin associated with genotype- and age-dependent leaf freezing-tolerance in Rhododendron: a genetic marker for cold hardiness?

Dehydrins are plant proteins that may play a critical role in stabilizing cell functions during freezing and other dehydrative stresses. This study examines whether dehydrin expression in leaves is associated with varying levels of freezing-tolerance among F₂ segregants, species, and cultivars of evergreen Rhododendron. Experiments were also conducted to determine whether physiological and chronological aging affects freezing-tolerance and dehydrin accumulation in Rhododendron leaf tissues. Our results indicate that in cold-acclimated F₂ populations, levels of a 25-kDa dehydrin were closely associated with differences in leaf freezing-tolerance (LFT) among segregants. Studies of wild and cultivated plants indicated that LFT increased with both chronological age and developmental phase-change (juvenile to mature plants) and that this trend was accompanied by increased accumulation of the 25-kDa dehydrin. It is suggested that presence or absence of the 25-kDa dehydrin could serve as a genetic marker to distinguish between super cold-hardy and less cold-hardy rhododendron genotypes. Similarly, the relative level of this protein within a genotype can serve as a physiological indicator of freezing-tolerance status under a range of phenological (acclimation) or developmental (age) conditions. Received: 5 March 1999 / Accepted: 12 May 1999