盐胁迫对甜樱桃砧木生理特性及光合荧光参数的影响

以1年生甜樱桃砧木‘吉塞拉6号’和‘考特’幼苗为材料,采用盆栽试验,研究不同浓度NaCl(0、50、100、150 mmol·L^(-1))处理对其主要渗透调节物质、抗氧化酶活性、光合特性以及叶绿素荧光参数的影响,探究甜樱桃砧木对盐胁迫响应的生理机制。结果表明:(1)NaCl处理促进了甜樱桃砧木叶片中可溶性糖、可溶性蛋白和脯氨酸等渗透调节物质的积累。(2)随着NaCl处理浓度的升高,甜樱桃砧木叶片中SOD活性呈现升高趋势,而POD活性表现出先升高后降低趋势。(3)随着NaCl处理浓度的升高,甜樱桃砧木叶片的净光合速率(P_(n))、气孔导度(G_(s))逐渐降低,而胞间CO_(2)浓度(C i)逐渐升高,非气孔限制为甜樱桃砧木叶片P_(n)下降的主要因素。(4)NaCl处理抑制了甜樱桃砧木叶片的最大光化学效率(F_(v)/F_(m))、光化学淬灭系数(q P)和电子传递效率(ETR),增加了非光化学淬灭系数(NPQ)。研究发现,盐胁迫破坏了甜樱桃砧木的光合机构,抑制了电子传递速率和光化学量子效率,降低了对光能的利用率,导致光合速率降低;甜樱桃砧木在盐胁迫条件下主要通过增加渗透调节物质含量和提高抗氧化酶活性来缓解渗透胁迫并降低氧化损伤,从而提高对盐胁迫的适应能力;‘吉塞拉6号’在盐胁迫条件下表现出更强的适应能力,其耐盐性更强;甜樱桃砧木在高于100 mmol·L^(-1)NaCl处理时表现出明显受害症状。     

荔枝新品种‘贵妃红’和‘草莓荔’嫁接亲和性试验

以荔枝新品种‘贵妃红’和‘草莓荔’与10种砧木为试材,对各砧穗组合的嫁接成活率及嫁接苗田间生长指标进行测定及比较。结果表明,不同砧穗组合间嫁接成活率以及嫁接苗田间生长势存在明显差别,‘贵妃红’以钦州红荔、黑叶、禾荔为砧木的嫁接成活率分别达80.0%、78.0%和74.0%,‘草莓荔’以禾荔为砧木的嫁接成活率最高,达82.0%。综合其成活率及嫁接苗生长状况等指标,‘贵妃红’宜以黑叶、禾荔、钦州红荔、白腊为砧木进行嫁接,而‘草莓荔’宜以黑叶、禾荔、钦州红荔、镇奉为砧木进行嫁接。     

复合茶树接穗与接穗母本的代谢物差异分析

以两个通过群体选育获得的云南普洱茶优良品种‘云瑰’和‘福云6号’为接穗,均以茶树品种‘短节白毫’为砧木所形成的嫁接复合茶树为研究对象,通过代谢组学技术,对两个品种的接穗与接穗母本的代谢物进行分析,考察嫁接前后茶树品种‘云瑰’和‘福云6号’的差异代谢物和共同代谢物的种类、数量变化特征。结果发现：(1)两品种茶树嫁接后比嫁接前的农艺性状均有所改善,嫁接优势明显。(2)相对于‘云瑰’,‘福云6号’的接穗与接穗母本茶叶中差异代谢物的数量与种类都比较少,说明‘福云6号’嫁接在‘短节白毫’上时,接穗能最大程度地保留母本的特点。(3)‘云瑰’的接穗和接穗母本茶叶中检测和定量了115个差异代谢物,且含量表现上调的代谢物数量低于下调的数量;‘福云6号’的接穗和接穗母本茶叶中共检测和定量了47个差异代谢物,且含量表现上调的代谢物数量高于下调的数量。(4)‘云瑰’的接穗和接穗母本茶叶中差异代谢物在38条KEGG通路中富集,大多数已经鉴定的差异代谢物存在于苯丙氨酸代谢等相关途径中;‘福云6号’的接穗和接穗母本茶叶中差异代谢物在21条KEGG通路中富集,大多数已经鉴定的差异代谢物存在于与嘌呤代谢等相关途径中。该研究结果对充分发挥茶树嫁接技术在茶叶生产中的作用提供了理论依据。     

蜜柚不同砧穗组合苗期嫁接亲和性评价

为评价蜜柚砧穗的嫁接亲和性,以红绵蜜柚(Citrus grandis‘Hongmianmiyou’)、三红蜜柚(‘Sanhongmiyou’)、红肉蜜柚(‘Hongroumiyou’)、黄金蜜柚(‘Huangjinmiyou’)和琯溪蜜柚(‘Guanximiyou’)作接穗,枳(Poncirus trifoliata)、香橙(Citrus junos)、酸柚(Citrus grandis)作砧木,田间调查15个砧穗组合苗期生长指标,测定嫁接愈合期叶片多酚氧化酶(PPO)和过氧化物酶(POD)活性、可溶性蛋白和可溶性糖含量,采用主成分分析和聚类分析方法对蜜柚砧穗组合嫁接亲和性进行评价。结果表明,以柚作砧木的砧穗组合保存率高、生长势旺盛、抽梢能力强,以枳和香橙作砧木的砧穗组合部分指标存在差异,其中红绵蜜柚和黄金蜜柚以枳作砧木时表现出不亲和现象。不同砧穗组合嫁接愈合时期PPO、POD、可溶性蛋白和可溶性糖变化趋势基本一致。主成分分析结果表明,4个主成分基本反映了15个指标91.33%的数据信息。聚类分析将15个砧穗组合分为4类,与主成分分析结果基本一致。因此,琯溪蜜柚、红肉蜜柚和三红蜜柚嫁接可采用枳和柚作砧木,红绵蜜柚和黄金蜜柚嫁接可采用柚作砧木,红绵蜜柚和黄金蜜柚嫁接不可采用枳作砧木。     

中国樱桃与甜樱桃花粉原位萌发及花粉管生长的差异

以‘垂丝’、‘东塘’(中国樱桃)和‘莫利’、‘拉宾斯’(甜樱桃)为试材,分别于自花、异花授粉后不同时间切取花柱,用FAA固定,荧光染色后压片观察。结果显示,中国樱桃和甜樱桃的自花、异花花粉均能在柱头萌发,且其花粉管在花柱中表现为“极快—慢—快—稳定”的动态变化过程。但甜樱桃花粉萌发率高于中国樱桃,异花高于自花。中国樱桃自花、异花都有花粉管到达花柱基部;甜樱桃‘莫利’ב拉宾斯’和‘拉宾斯’自交有花粉管到达花柱基部,而‘莫利’自交的花粉管在花柱中上部已停止生长。结果表明,中国樱桃表现自交亲和性,而甜樱桃除人工诱变导致自交亲和的‘拉宾斯’等品种外,表现典型的植物配子体自交不亲和性。     

不同苹果砧穗组合的生长及光合特性

以‘垂丝海棠’（Malus halliana）和‘平邑甜茶’（Malus hupehensis）为基砧,分别嫁接品种‘烟富6号’和‘长富2号’接穗,测定4种砧穗组合的嫁接亲和性、接穗生长量、光合与荧光参数及叶绿素含量（SPAD）,并用主成分分析法综合评价砧穗组合的优劣,探讨不同苹果砧穗组合嫁接苗的生长及光合特性,为西北盐碱地选择适宜的苹果砧木提供理论依据。结果表明：（1）4种砧穗组合中‘垂丝海棠/烟富6号’的上下口粗度比最接近1,嫁接亲和性最好。（2）整个生长期内,以‘垂丝海棠’为基砧的2个组合嫁接苗的生长量、净光合速率（P_n）、最大荧光（F_m）、PSⅡ最大光能转化率（F_v/F_m）均显著大于‘平邑甜茶’为基砧的组合,但其胞间CO₂浓度（C_i）及初始荧光（F₀）显著低于‘平邑甜茶’为基砧的组合;光化学猝灭系数（qP）在4种砧穗组合中无显著差异。（3）在8月份光照强度较高时,‘垂丝海棠/烟富6号’ 嫁接苗的气孔导度（G_s）高于其他砧穗组合;以‘垂丝海棠’为基砧的2个组合嫁接苗叶片的蒸腾速率（T_r）和相对叶绿素含量（SPAD）显著高于‘平邑甜茶’ 基砧组合。（4）根据主成分分析对各项指标进行综合评价,按照4个砧穗组合的综合得分由高到低依次为：‘垂丝海棠/烟富6号’、‘垂丝海棠/长富2号’、‘平邑甜茶/长富2号’、‘平邑甜茶/烟富6号’。研究发现,基砧‘垂丝海棠’的适应性优于‘平邑甜茶’,且‘垂丝海棠/烟富6号’砧穗组合的嫁接亲和性高,长势强,光合能力优,为甘肃中部地区适宜的砧穗组合。     

甜樱桃品种及其砧木的RAPD分析

利用RAPD技术,从130个随机引物中筛选出46个引物,对欧洲甜樱桃、欧洲酸樱桃、马哈利樱桃和野生中国樱桃4个类型樱桃种,以及欧洲甜樱桃与中国樱桃的种间杂交种共15个品种的基因组遗传变异进行分析。结果表明,46个随机引物均得到了稳定可重复的RAPD图谱,扩增出的DNA条带大小在100~2625bp之间,多态性位点数517个,多态性位点百分率为98.85%,每个随机引物扩增出的多态性DNA条带数在4~23条。品种间Nei遗传距离在0.166~0.479之间,平均遗传距离0.329;甜樱桃新品种‘秦樱1号’与‘秦岭玛瑙’、‘CDR-1’等10个樱桃砧木之间的遗传距离在0.248~0.376,并且根据遗传距离可以相互区分,所分析的15个樱桃品种均扩增出了特有的DNA条带,每个樱桃特有标记带在2~17个之间,共扩增出149个特有标记,据此可以进行樱桃品种及砧木的RAPD鉴定。研究认为利用RAPD技术可以在分子水平上对甜樱桃品种及其砧木进行快速鉴定。     

砧木对梨叶芽休眠的影响及其与多胺代谢的关系

以分别嫁接在杜梨和豆梨上的砂梨品种‘丰水’为试材,研究了2008和2009年11～12月气温变化和不同砧木对‘丰水’梨叶芽休眠进程的影响,分析叶芽中游离态和束缚态内源多胺种类和含量的变化,结果表明：嫁接在豆梨上的‘丰水’叶芽自然休眠结束的时间要比嫁接在杜梨上的‘丰水’叶芽早10d左右,且游离态和束缚态腐胺（Put）、戊二胺（Cad）、己二胺（Hex）、亚精胺（Spd）和精胺（Spm）5种内源多胺含量开始升高的时间与供试材料叶芽自然休眠结束的时间一致,表明梨叶芽的休眠进程与砧木种类和多胺代谢有密切关系,尤其是与束缚态多胺含量变化的关系更为密切。     

叶面喷施矮壮素对番茄嫁接愈合的调节作用

该研究选用番茄接穗品种‘硬粉8号’和砧木品种‘砧爱1号’为试材,分别在嫁接前6 d和12 d叶面喷施100 mg·L^-1生长抑制剂矮壮素(CCC),测定番茄幼苗生长指标和嫁接接合部植物激素含量,监测CCC处理对嫁接愈合进程的影响。结果显示：(1)‘硬粉8号’和‘砧爱1号’幼苗生长受到CCC显著抑制,株高分别显著降低33.30%和33.96%,两幼苗地上部鲜重及‘砧爱1号’幼苗干重也均显著降低。(2)嫁接后12 h和48 h, CCC处理显著降低了嫁接接合部GA₁₅和GA₈含量,嫁接后48 h和72 h显著提高了嫁接接合部GA₃₄和GA₃含量;嫁接后12、48和72 h, CCC处理显著提高了嫁接接合部L-色氨酸、吲哚-3-乙酸甲酯、色胺、吲哚-3-乙酸、反式-玉米素-9-Β葡萄糖苷和异戊烯腺嘌呤-9-葡萄糖苷含量。(3)嫁接后48～168 h, CCC处理显著提高了嫁接接合部维管束品红吸收含量和平均荧光强度;嫁接后72 h, CCC处理的嫁接接合部已可见木质部导管分子连接;嫁接...     

黄瓜贴接苗砧木子叶淀粉代谢的动态变化特征

该研究以黄瓜品种‘中农18号’、南瓜砧木品种‘京欣砧5号’为试验材料,以南瓜自根苗(P)和去除1片子叶及生长点的南瓜苗( /P)为对照,采用单子叶贴接法进行黄瓜/南瓜异体嫁接(C/P)和南瓜/南瓜自体嫁接(P/P),测定嫁接后砧木子叶形态指标和淀粉代谢的动态变化,分析嫁接后去除砧木子叶对嫁接苗生长发育的影响,以揭示砧木子叶淀粉代谢在黄瓜嫁接苗生长中的作用,为黄瓜嫁接苗的壮苗培育提供理论依据。结果显示：(1)贴接后,C/P、P/P和 /P砧木子叶鲜质量和面积显著增大,且增加量依次递减,表现为 /P > C/P > P/P > P。(2)贴接后,C/P和P/P砧木子叶中淀粉含量在嫁接后0~3 d时降低,之后迅速升高,至嫁接后13 d再次逐渐降低,且C/P砧木子叶淀粉含量及其淀粉分支酶(SBE)和水解酶(β AL)活性均显著高于P/P。(3)在嫁接后0~10 d 去除砧木子叶可显著抑制C/P嫁接苗接穗和根系生长,减弱根系活力,同时降低根系可溶性糖含量及其CWIN、HXK基因表达水平,并以嫁接后0 d 去除砧木子叶的抑制效果最显著。研究表明,黄瓜C/P单子叶贴接苗中,砧木子叶作为贮存器官,在幼苗生长早期以淀粉形式储存光合产物,之后淀粉水解成单糖为嫁接苗接穗和根系快速生长提供物质和能量。     

剥鳞和激素处理对大樱桃花芽休眠解除及内源激素变化的影响

采用高效液相色谱法(HPLC)分析了剥鳞与激素处理对大樱桃花芽休眠解除及内源生长素(IAA)、赤霉素(GAD、玉米素(ZT)和脱落酸(ABA)变化的影响。结果表明,花芽中的ABA主要分布于鳞片内,鳞片中的GA3和ZT含量远低于去鳞芽,也低于完整芽。剥鳞能明显增加休眠花芽中内源GA2和ZT的含量,降低ABA的含量,对IAA含量的影响不大。剥鳞降低了ABA／GA3、ABA／ZT的比值,使花芽向促进生长、抑制休眠的方向转化。同时,休眠前、后期剥鳞均能明显提高萌芽率,中期剥鳞效果不明显。剥鳞后施用外源激素随休眠时期不同而有不同的破眠效果,早期剥鳞GA3的效果最好,6-BA次之,IAA最差;中期破眠效果不如早期,GA。和6-BA没有明显差别;后期以6-BA效果最好,其次是GA3和IAA;3次处理中ABA均明显抑制花芽萌发。     

Changes in polyamine pattern mediates sex differentiation and unisexual flower development in monoecious cucumber (Cucumis sativus L.)

Changes in the levels of polyamines are associated with fundamental physiological processes such as embryogenesis, induction of flowering, fruit development and ripening, senescence, and responses to environmental stresses, but the role of polyamines in sex differentiation and unisexual flower development has not been deeply studied. To extend the knowledge on the regulatory mechanisms of flowering in monoecious plant (producing unisexual flowers), we investigated the morphogenesis and free polyamine levels in Cucumis sativus during sex differentiation and unisexual flower development in vitro using histocytological and biochemical methods. As shown in our study, floral development in vitro was undisturbed and flowers of both sexes were produced. Sex differentiation relied on preventing the development of generative organs of the opposite sex, as we observed carpel repression in male flowers and stamen repression in female flowers. Pollen viability was negatively correlated with female flower development on the same node. Biochemical analysis revealed increased accumulation of aliphatic amines (tri, tetra‐amines) in generative (flower buds and flowers) compare to vegetative (axillary buds and leaves) organs. Undifferentiated floral buds contained elevated levels of agmatine, cadaverine, spermidine and spermine. Sex differentiation was associated with significantly decreased levels of agmatine and cadaverine. Our results showed that female flowers contained higher levels of total polyamine than male flowers. The increased level of cadaverine was associated with macrogametogenesis and female flower maturation. Putrescine was important for male flower development. Such results support the hypothesis that aliphatic amines are involved in unisexual flower development.     

Polyamine metabolism,floral initiation and floral development in Chrysanthemum (Chrysanthemum morifolium Ramat.)

In the short-day plant Chrysanthemum (Chrysanthemum morifolium Ramat. variety Pavo) putrescine and spermidine conjugates appeared in the apical bud before the first observable transformation of the meristem into floral structures. These compounds accumulated on floral initiation and well before floral evocation. Spermidine conjugates were predominant during floral initiation whereas free amines did not accumulate to any significant extent. Different associations of amides were observed during floral initiation as compared with the reproductive phase. 3,4-Dimethoxyphenethylamine conjugates (water-insoluble compounds) were the predominant amine conjugates observed during flower development. These compounds decreased drastically after fertilization. In vegetative buds from plants grown in long days polyamine conjugates were very low and appeared as plants aged. We present evidence that ornithine decarboxylase (ODC) regulates putrescine biosynthesis during floral initiation and floral development. When ODC action was blocked by DFMO (-DL-difluoromethylornithine, a specific, irreversible inhibitor of ODC), flowering was inhibited, and free and conjugated polyamines were not detected. This treatment led to a slight enhancement of ADC activity. When putrescine was added, polyamine titers and flowering were restored. A similar treatment with DFMA (-DL difluoromethylarginine, a specific, irreversible inhibitor of ADC) did not affect flowering and the polyamine titers. The results suggest that ODC and polyamine conjugates are involved in regulating floral initiation in Chrysanthemum.Abbreviations ADC arginine decarboxylase - ODC ornithine decarboxylase - DFMA -DL-difluoromethylarginine - DFMO -DL-difluoromethylornithine     

Rhizophagus irregularis MUCL 41,833 Association with Green Cuttings of Prunus sp. Rootstocks

Journal of Plant Growth Regulation - Sour cherry ‘Latvijas Zemais’ (Prunus cerasus) is a promising dwarfing rootstock for sweet cherries in Latvia, but low growing rate of newly...     

Mapping of Candidate Genes Involved in Bud Dormancy and Flowering Time in Sweet Cherry (Prunus avium)

The timing of flowering in perennial plants is crucial for their survival in temperate climates and is regulated by the duration of bud dormancy. Bud dormancy release and bud break depend on the perception of cumulative chilling during endodormancy and heat during the bud development. The objectives of this work were to identify candidate genes involved in dormancy and flowering processes in sweet cherry, their mapping in two mapping progenies ‘Regina’ × ‘Garnet’ and ‘Regina’ × ‘Lapins’, and to select those candidate genes which co-localized with quantitative trait loci (QTLs) associated with temperature requirements for bud dormancy release and flowering. Based on available data on flowering processes in various species, a list of 79 candidate genes was established. The peach and sweet cherry orthologs were identified and primers were designed to amplify sweet cherry candidate gene fragments. Based on the amplified sequences of the three parents of the mapping progenies, SNPs segregations in the progenies were identified. Thirty five candidate genes were genetically mapped in at least one of the two progenies and all were in silico mapped. Co-localization between candidate genes and QTLs associated with temperature requirements and flowering date were identified for the first time in sweet cherry. The allelic composition of the candidate genes located in the major QTL for heat requirements and flowering date located on linkage group 4 have a significant effect on these two traits indicating their potential use for breeding programs in sweet cherry to select new varieties adapted to putative future climatic conditions.     

Polyamines and Flower Development in the Male Sterile Stamenless-2 Mutant of Tomato (Lycopersicon esculentum Mill.) : II. Effects of Polyamines and Their Biosynthetic Inhibitors on the Development of Normal and Mutant Floral Buds Cultured in Vitro

The floral organs of the male sterile stamenless-2 (sl-2/sl-2) mutant of tomato (Lycopersicon esculentum Mill.) contain significantly higher level of polyamines than those of the normal (R Rastogi, VK Sawhney [1990] Plant Physiol 93: 439-445). The effects of putrescine, spermidine and spermine, and three different inhibitors of polyamine biosynthesis on the in vitro development of floral buds of the normal and sl-2/sl-2 mutant were studied. The polyamines were inhibitory to the in vitro growth and development of both the normal and mutant floral buds and they induced abnormal stamen development in normal flowers. The inhibitors of polyamine biosynthesis also inhibited the growth and development of floral organs of the two genotypes, but the normal flowers showed greater sensitivity than the mutant. The inhibitors also promoted the formation of normal-looking pollen in stamens of some mutant flowers. The effect of the inhibitors on polyamine levels was not determined. The polyamine-induced abnormal stamen development in the normal, and the inhibitor-induced production of normal-looking pollen in mutant flowers support the suggestion that the elevated polyamine levels contribute to abnormal stamen development in the sl-2/sl-2 mutant of tomato.     

Cold storage to overcome dormancy affects the carbohydrate status and photosynthetic capacity of Rhododendron simsii

Global warming leads to increasing irregular and unexpected warm spells during autumn, and therefore natural chilling requirements to break dormancy are at risk. Controlled cold treatment can provide an answer to this problem. Nevertheless, artificial cold treatment will have consequences for carbon reserves and photosynthesis. In this paper, the effect of dark cold storage at 7 °C to break flower bud dormancy in the evergreen Rhododendron simsii was quantified. Carbohydrate and starch content in leaves and flower buds of an early (‘Nordlicht’), semi‐early (‘M. Marie’) and late (‘Mw. G. Kint’) flowering cultivar showed that carbon loss due to respiration was lowest in ‘M. Marie’, while ‘Mw. G. Kint’ was completely depleted of starch reserves at the end of cold treatment. Gene isolation resulted in a candidate gene for sucrose synthase (SUS) RsSus, which appears to be homologous to AtSus3 and had a clear increase in expression in leaves during cold treatment. Photosynthesis measurements on ‘Nordlicht’ and the late‐flowering cultivar ‘Thesla’ showed that during cold treatment, dark respiration decreased 58% and 63%, respectively. Immediately after cold treatment, dark respiration increased and stabilised after 3 days. The light compensation point followed the same trend as dark respiration. Quantum efficiency showed no significant changes during the first days after cold treatment, but was significantly higher than in plants with dormant flower buds at the start of cold treatment. In conclusion, photosynthesis stabilised 3 days after cold treatment and was improved compared to the level before cold treatment.     

Relation of polyamine biosynthesis to the initiation of sprouting in potato tubers

The polyamines putrescine, spermidine, and spermine and their biosynthetic enzymes arginine decarboxylase, ornithine decarboxylase and S-adenosyl-l-methionine decarboxylase are present in all parts of dormant potato (Solanum tuberosum L.) tubers. They are equally distributed among the buds of apical and lateral regions and in nonbud tissues. However, the breaking of dormancy and initiation of sprouting in the apical bud region are accompanied by a rapid increase in ornithine decarboxylase and S-adenosyl-l-methionine decarboxylase activities, as well as by higher levels of putrescine, spermidine, and spermine in the apical buds. In contrast, the polyamine biosynthetic enzyme activities and titer remain practically unchanged in the dormant lateral buds and in the nonbud tissues. The rapid rise in ornithine decarboxylase, but not arginine decarboxylase activity, with initiation of sprouting suggests that ornithine decarboxylase is the rate-limiting enzyme in polyamine biosynthesis. The low level of polyamine synthesis during dormancy and its dramatic increase in buds in the apical region at break of dormancy suggest that polyamine synthesis is linked to sprouting, perhaps causally.     

Metabolic changes in cherry flower buds associated with breaking of dormancy in early and late blooming cultivars

Changes of metabolic activities during dormancy and breaking of dormancy in the cherry flower buds of early blooming (EB) cultivar ( Prunus avium L. cv. Coeur de Pigeon) and late blooming (LB) cultivar ( Prunus serrulata Lindl. cv. Kwanzan) were determined. The LB buds had higher polyamines, protein and 1-(malonylamino) cyclopropane-1-carboxylic acid (MACC) content than the EB buds. During the dormant state, the DNA, RNA, protein and polyamines in the EB buds were low but increased slowly and steadily, whereas those in the LB buds remained at a consistently higher level. The transition from dormancy to the active state in both cultivars was characterized by a sharp increase in DNA, RNA, protein, polyamines, S-adenosyl-methionine (SAM), 1-aminocyclopropane-1-carboxylic acid (ACC) and MACC. After initial swelling and development of flowers, the levels of all these components decreased. Polyamine and ethylene biosyntheses did not seem to be competing for their common substrate, SAM, during flower bud development.