萌发中花生胚轴的耐干性与热稳定蛋的

成熟花生种子吸胀１８ｈ发芽率达１００％,在这１８ｈ的范围内,胚轴即使经干燥处理,萌发生长率仍保持１００％,而热稳定蛋白含量变化很小。吸胀２４ｈ后,经干燥的花生胚完全丧失蓝发生长能力。ＳＤＳ－ＰＡＧＥ和和双向电泳表明,花生胚轴的热稳定蛋白主要是贮藏蛋白,该蛋白中的花生球蛋白大亚基,伴花生球蛋白Ｉ和２５蛋白的降解与胚轴的耐干性丧失有关。     

豌豆种子吸胀过程中脱水耐性变化的时间模式

研究了豌豆种子吸胀过程中脱水耐性的变化模式。种子在吸胀初期迅速吸收水分,然后缓慢吸收直到平台期。电解质渗漏速率在吸胀初期增加直到11h,然后随着吸胀下降。在吸胀过程中,种子的萌发率逐渐增加,种子和胚轴的脱水耐性逐渐丧失,10％和50％的种子和胚轴被脱水致死的含水量明显增加。赤霉素和脱落酸处理改变豌豆种子的萌发特性,提高胚轴的脱水耐性。研究结果表明,吸胀的豌豆种子脱水耐性的丧失是一种数量性状,正常性种子吸胀后脱水耐性的变化能够作为种子顽拗性研究的模式系统。     

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。     

不同品种花生种子蛋白质的电泳分析

对中国花生（ＡｒａｃｈｉｓｈｙｐｏｇａｅａＬ．）５种不同类型的４６个栽培品种的种子蛋白质进行电泳分析。ＳＤＳＰＡＧＥ和ＩＥＦＳＤＳＰＡＧＥ（双向电泳）的结果显示,不同品种的花生种子蛋白多肽组成存在４种类型。与初步纯化的花生球蛋白及伴花生球蛋白的ＳＤＳＰＡＧＥ结果比较,花生种子蛋白组成的主要差异在于花生球蛋白亚基组成的不同,其中类型Ⅰ花生球蛋白主要含有４１ｋＤ、３８５ｋＤ和２个１８ｋＤ亚基,类型Ⅱ主要含４１ｋＤ、３８５ｋＤ、３７５ｋＤ和３个１８ｋＤ亚基,类型Ⅲ主要含４１ｋＤ、３８．５ｋＤ、３６．５ｋＤ和３个１８ｋＤ亚基,类型Ⅳ主要含４１ｋＤ、３８．５ｋＤ、３７５ｋＤ、３６．５ｋＤ和３个１８ｋＤ亚基。不同品种的伴花生球蛋白多肽组成基本一致。对不同类型８个品种种子蛋白的氨基酸组成进行测定,发现类型Ⅰ的含硫氨基酸含量较高。     

花生种子发育和萌发过程中贮藏蛋白的合成和降解

以花生品种汕油5 2 3种子为材料,分离纯化花生球蛋白的41 kD和38.5 kD两种主要亚基及伴花生球蛋白的6 0.5 KD亚基并制备抗体.We stern blot分析表明,3种亚基在花生胚组织分化期的胚轴和子叶中就开始合成,其中60.5 kD亚基是最先在胚轴和子叶中大量合成和积累的贮藏蛋白,41 kD和38.5 kD亚基在随后的发育中积累量不断增加;种子萌发时这3种亚基的降解进程不一样,胚轴和子叶中41 kD和38.5kD亚基的降解均先于60.5 kD亚基.     

去胚轴对花生子叶肽链内切酶和贮藏蛋白质降解的影响

从离体子叶与连体子叶在水中培养一段时间后的比较,看到它们之间在肽链内切酶活性和盐溶蛋白及花生球蛋白降解上的差异并不大,这表明去除胚轴对子叶肽链内切酶活性和贮藏蛋白降解的影响很轻微。亚胺环己酮(蛋白质合成抑制剂)不能完全抑制离体子叶肽链内切酶活性的提高,子叶的大部分大分子贮藏蛋白同样被降解。这表明,在花生种子萌发过程中降解大部分贮藏蛋白的子叶肽链内切酶并非全部是在种子萌发时新合成的,子叶贮藏蛋白降解和肽链内切酶活性基本不受胚轴调控,子叶与胚轴之间在调控关系上可能是一种新的调节类型。     

脱落酸和抑制剂对萌发花生子叶肽链内切酶和花生球蛋白降解的影响

脱落酸（Ａｂｓｃｉｓｉｃａｃｉｄ,ＡＢＡ）抑制花生种子萌发的作用与核酸和蛋白质合成抑制剂的作用不同．ＡＢＡ（１００μｍｏｌ／Ｌ）在萌发零时施用,明显抑制肽链内切酶活性和同工酶表现以及花生球蛋白降解,萌发４８ｈ施用ＡＢＡ（１００μｍｏｌ／Ｌ）只降低肽链内切酶活性．ＡＢＡ的抑制作用不依赖于核酸和蛋白质合成．核酸合成抑制剂（３＇－脱氧腺苷,放线菌素Ｄ,５－氟尿嘧啶）和蛋白质合成抑制剂（亚胺环己酮）只能部分降低肽链内切酶活性,对肽链内切酶同工酶表现和花生球蛋白降解无明显影响．实验结果表明花生子叶肽链内酶不是在种子萌发过程中重新（ｄｅｎｏｖｏ）合成,文中讨论了肽链内切酶活性调节和花生贮藏蛋白降解的起始模式．     

预吸胀对绿豆种子脱水耐性的影响

绿豆 (Vignaradiata)种子的吸水曲线未出现明显的“平稳期”。种子萌发 5 0 %的时间和热时间分别为 11h和 11 5度天。在吸胀初期 ,种子的相对电导率迅速增加 ,然后下降。随着脱水时间的延长 ,预吸胀不同时间的绿豆种子的含水量和存活率、由存活种子产生的幼苗鲜重、胚根和下胚轴长度明显下降 ;而且随着预吸胀时间的增加 ,种子对脱水的敏感性显著加强 ;预吸胀种子的相对渗漏率在脱水初期缓慢增加 ,然后迅速增加 ,且预吸胀时间愈长 ,相对渗漏率增加的幅度愈大。结果表明预吸胀的绿豆种子的脱水耐性是逐渐丧失的 ;吸胀的能萌发的正常性种子的脱水敏感性可以作为研究种子顽拗性的一种模式系统     

去胚轴对花生子叶肽链内切酶和贮藏蛋白质降解的影响

从离体子叶与连体子叶在水中培养一段时间后的比较,看到它们之间在肽链内切酶活性和盐溶蛋白及花生球蛋白降解上的差异并不大,这表明去除胚轴对子叶肽链内切酶活性和贮藏蛋白降解的影响很轻微。亚胺环己酮（蛋白质合成抑制剂）不能完全抑制离体子叶肽链内切酶活性的提高,子叶的大部分大分子贮藏蛋白同样被降解。这表明,在花生种子萌发过程中降解大部分贮藏蛋白的子叶肽链内切酶并非人全部是在种子萌发是新合成的。子叶贮藏蛋白降     

不同活力玉米种子胚萌发过程中蛋白质的变化

从不同人工老化处理中筛选出３组分别代表不同活力的玉米种子。萌发期间,中、低活力种子胚蛋白的降解比高活力对照种子慢,萌发前期胚蛋白合成能力也较低。吸胀２４ｈ,不同活力胚的蛋白合成能力差异显著,可以作为衡量种子活力的指标。     

Patterns of protein synthesis during the germination of pea axes,and the effects of an interrupting desiccation period

As germination of axes of Pisum sativum L. seeds progressed, profound quantitative and qualitative changes occurred in the patterns of protein synthesis. This was shown by fluorography of gels following two-dimensional polyacrylamide gel electrophoresis separation of [³⁵S]methioninelabelled proteins. The effects of desiccation during germination on these in-vivo protein-synthesis patterns were followed. Desiccation differentially affected the synthesis of proteins. Usually, however, upon rehydration following desiccation the types of proteins being synthesized were recognizable as those synthesized earlier during imbibition of control, once-imbibed axes: seeds imbibed for 8 h, and then dried, did not recommence synthesis of proteins typical of 8-h-imbibed control seeds, but rather of 4-h-imbibed control seeds. Seeds imbibed for 12 h, and then dried and rehydrated, synthesized proteins typical of 4-h-and 8-h-control seeds. Thus drying of germinating pea axes caused the proteinsynthesizing mechanism to revert to producing proteins typical of earlier stages of imbibition. Drying during germination never caused the seed to revert to the metabolic status of the initial mature dry state, however.Abbreviation DR dried and rehydrated     

花生种子萌发过程中胚轴多胺氧化酶的活性变化

研究花生(Arachis hypogaea)种子萌发过程中胚轴多胺氧化酶(PAO)的活性变化及其与种子萌发的关系表明：胚轴中的PAO活性是在种子萌发过程中逐渐形成的,而黑暗条件更有利于该酶的活性形成;放线菌素D(10mg／L)、环己酰亚胺(10mg／L)处理对种子萌发的抑制率分别为26.3％和87.3％,对胚轴PAO活性的抑制率分别为41.1％和94.0％,显示胚轴中的PAO很可能参与花生种子的萌发过程,且其mRNA在种子发育过程中已合成并贮存于种子中,萌发时PAO活性的出现主要是由于这些mRNA转译合成了PAO。     

Maturation proteins associated with desiccation tolerance in soybean

A set of proteins that accumulates late in embryogenesis (Lea proteins) has been hypothesized to have a role in protecting the mature seed against desiccation damage. A possible correlation between their presence and the desiccation tolerant state in soybean seeds (Glycine max L. Chippewa) was tested. Proteins that showed the same temporal pattern of expression as that reported for Lea proteins were identified in the axes of soybean. They were distinct from the known storage proteins and were resistant to heat coagulation. The level of these “maturation” proteins was closely correlated with desiccation tolerance both in the naturally developing and in the germinating seed: increasing at 44 days after flowering, when desiccation tolerance was achieved, and decreasing after 18 hours of imbibition, when desiccation tolerance was lost. During imbibition, 100 micromolar abscisic acid or Polyethylene glycol-6000 (−0.6 megapascals) delayed disappearance of the maturation proteins, loss of desiccation tolerance, and germination. During maturation, desiccation tolerance was prematurely induced when excised seeds were dried slowly but not when seeds were held for an equivalent time at high relative humidity. In contrast, maturation proteins were induced under both conditions. We conclude that maturation proteins may contribute to desiccation tolerance of soybean seeds, though they may not be sufficient to induce tolerance by themselves.     

Changing desiccation tolerance of pea embryo protoplasts during germination

Protoplasts were isolated from pea (Pisum sativum L. cv. Alaska) embryonic axes during and after germination to determine whether the loss of desiccation tolerance in the embryos also occurs in the protoplasts. At all times studied, protoplast survival decreased as water content decreased; however, the sensitivity to dehydration was less when the protoplasts were isolated from embryos that were still desiccation-tolerant (12 h and 18 h of imbibition) than when protoplasts were derived from axes that were sensitive (24 h and 36 h of imbibition). The water content at which 50% of the population was killed (WC50) increased throughout germination and early seedling growth for both the intact tissue and the protoplasts derived from them. Prior to radicle emergence, protoplasts were less desiccation-tolerant than the intact axes; however, protoplasts isolated from radicles shortly after emergence had lower WC50s than the intact radicles. A comparison of protoplast survival after isolation and dehydration in either 500 mM sucrose/raffinose or 700 mM sucrose revealed no difference in tolerance except at 24 h of imbibition, when protoplasts treated in the more concentrated solution had improved tolerance of dehydration. Although intact epicotyls are generally more desiccation-tolerant than radicles, protoplasts isolated separately from epicotyls and radicles did not differ in tolerance. Collectively, these data suggest that protoplasts gradually lose desiccation tolerance during germination, as do the orthodox embryos from which they were derived. However, even prior to radicle emergence, protoplasts display a sensitivity to progressive dehydration that is similar to that shown by recalcitrant and ageing embryos.     

Ascorbic acid metabolism in ageing recalcitrant sal (Shorea robusta Gaertn. f.) seeds

Changes in ascorbate content and its enzymatic utilization pattern were studied in embryonic axes and cotyledons of sal seeds undergoing rapid loss of viability, at ambient conditions. Ascorbate levels were significantly higher initially in the embryonic axes (0.32 mg/g fresh weight) and cotyledons (0.21 mg/g fresh weight) of freshly mature, relatively hydrated (42.2% moisture content) and 100% viable sal seeds. It declined sharply as the tissues; embryonic axes and cotyledons, desiccated with absolutely no detectable amount in non-viable seeds (21% moisture content). Significantly strong correlation was obtained between desiccation of embryonic axes (r = 0.96) and cotyledon (r = 0.97) with loss of ascorbate levels and loss of germinability. Higher rates of ascorbic acid utilization (AAU) recorded in the embryonic axes of 100% viable seed declined sharply as the seed viability reduced due to desiccation below 36.8% moisture content. AAU was not detected in the cotyledons.     

Proteomic analysis of rice (Oryza sativa) seeds during germination

Although seed germination is a major subject in plant physiological research, there is still a long way to go to elucidate the mechanism of seed germination. Recently, functional genomic strategies have been applied to study the germination of plant seeds. Here, we conducted a proteomic analysis of seed germination in rice (Oryza sativa indica cv. 9311) - a model monocot. Comparison of 2-DE maps showed that there were 148 proteins displayed differently in the germination process of rice seeds. Among the changed proteins, 63 were down-regulated, 69 were up-regulated (including 20 induced proteins). The down-regulated proteins were mainly storage proteins, such as globulin and glutelin, and proteins associated with seed maturation, such as "early embryogenesis protein" and "late embryogenesis abundant protein", and proteins related to desiccation, such as "abscisic acid-induced protein" and "cold-regulated protein". The degradation of storage proteins mainly happened at the late stage of germination phase II (48 h imbibition), while that of seed maturation and desiccation associated proteins occurred at the early stage of phase II (24 h imbibition). In addition to alpha-amylase, the up-regulated proteins were mainly those involved in glycolysis such as UDP-glucose dehydrogenase, fructokinase, phosphoglucomutase, and pyruvate decarboxylase. The results reflected the possible biochemical and physiological processes of germination of rice seeds.     

Protein Patterns, Characterized by Computer Image Analysis, of Lentil Embryo Axes Germinating Under Salt Stress

Following 16, 40 and 64 h exposure to 0.33 M NaCl given after 8 h water imbibition, lentil seeds showed a gradual decrease of germination upon their transfer to water. These salt related changes were accompanied by modifications in the protein patterns of embryo axes as revealed by two-dimensional electrophoresis separation and by the computer image analysis of protein spots. In comparison with 8 h water imbibed seeds, prominent proteins comprised between the 5.1 – 7.6 pH isoelectric point in the first dimension and 75 – 50 kDa molecular mass in the second dimension showed a significant increase in their abundance as salt exposure increased. On transfer to water to complete germination, the content of many of these proteins decreased at 24h in 2 – 3 cm length embryo axes in comparison with the corresponding embryo axes of seeds continuously imbibed in water for 24 h. Some groups of proteins ranging between 15.5 – 17.3 kDa, already present after 8 h water imbibition, were not detectable after 24 h but were expressed in seeds exposed to NaCl and transferred to water for 24 h. Up- and down-regulated proteins in lentil embryo axes, imbibed under non-lethal salt stress conditions, have been tentatively identified by comparison with the protein map of germinating seeds of the model plant Arabidopsis. This revised version was published online in July 2006 with corrections to the Cover Date.     

渗调物质和fluridone对离体花生胚蛋白质合成的调节

离休花生胚发育过程中,渗透调节（简称渗调）物质提高了胚内源ＡＢＡ含量,促进了贮藏蛋白质花生球蛋白和伴花生球蛋白Ⅱ两个组分的合成,诱导和促进ＬＥＡ蛋白的合成,内源ＡＢＡ合成抑制剂ｆｌｕｒｉｄｏｎｅ抑制了渗调物质的作用。