寡糖素对红花及三七培养细胞的生理作用

三种寡糖素,即来自人参(Panax ginseng)培养细胞的人参寡糖素、红花(Carthamus tinctorius)培养细胞的红花寡糖素、黑节草(Dendrobium candidum)植物的黑节草寡糖素对红花及三七 (Panax notoginseng)的培养细胞的生长及代谢产物的含量均有显著的促进作用。寡糖素可耐高温高压(121℃、1.2bs／cm2)灭菌15分钟而不失活,其对植物培养细胞的影响与利用过滤方法灭菌的效果相似。红花寡糖素对红花悬浮培养细胞作用的适宜浓度是5-10mg/L,而在愈伤组织中为15mg/L,在三七培养细胞进入生长旺盛(培养至22天)时加入黑节草寡糖素,再培养2天后其生长即提高。黑节草寡糖素均能缩短红花及三七培养细胞生长的延缓期,提前进入对数生长期及指数生长期。并且使红花培养细胞中a-生育酚在细胞生长最活跃的指数生长期大量积累,最终增加了培养细胞及代谢产物的产率。     

诱导子人参寡糖对红花培养细胞的生理效应

从人参(Panax ginseng)培养细胞中分离纯化出不同寡糖。这些寡糖能促进红花(Car-thamus tinctorius)培养细胞的生长及提高细胞中α-生育酚的含量。其中以Ⅶ、Ⅷ、Ⅵ等三种寡糖的效果较为显著。这三种寡糖的最适浓度在愈伤组织培养(5—8 mg/L)中要比在细胞悬浮培养(1—2mg/L)中高。对Ⅶ、Ⅷ两种寡糖不同时期加入的效应进行了试验,结果发现,加入寡糖后1—3天,α-生育酚的含量即提高。在红花细胞悬浮培养过程中同时加入2mg/L 的寡糖Ⅵ和寡糖Ⅶ及1mg/L 的寡糖Ⅷ,可使红花细胞生长速率提高18.11%,α-生育酚含量比对照提高3.5倍,其产率比对照提高4.3倍。     

人参寡糖素M对红花培养细胞生长与α-生育酚形成的影响

人参寡糖素M能提高红花(Carthamus tinctorius)培养细胞的生长速率和培养细胞中代谢产物α-生育酚的含量。其最适作用浓度在愈伤组织培养中为5mg/L。在红花细胞悬浮培养加入人参寡糖素M1d后,培养细胞中α-生育酚的含量即提高,但由于累积效应,因而于细胞接种当天同时加入人参寡糖素M对细胞生长和α-生育酚含量的提高效果较好。加入人参寡糖素M可缩短红花悬浮培养细胞生长的延缓期,并于指数生长期作用最明显;另外可使细胞生长及α-生育酚积累同时提前达到最高值,因而缩短了细胞收获时间。     

高产人参寡糖素培养细胞克隆系的筛选

人参（ＰａｎａｘｇｉｎｓｅｎｇＣ．Ａ．Ｍｅｙ．）培养细胞经细胞平板克隆,获得近３００个克隆系。克隆系在细胞生长速率和寡糖素含量及产率上均存在显著差异,且寡糖素产率和细胞生长之间有明显的相关性。经１１代连续继代培养观察及过氧化物酶同工酶谱特征分析,筛选到一株寡糖素产率高且稳定的克隆系ＰＧ－１８０,其平均生长速率是０．４９５ｇ于重／Ｌ·天,为原始株系的１．３９倍,平均寡糖素含量为１４．６９％干重,是亲本的１．６５倍,平均寡糖素产率是２．１８３ｇ／Ｌ,为原始株系的２．３２倍。比较克隆系ＰＧ－１８０和原始株系细胞悬浮培养时间进程发现,由人参培养细胞生产寡糖素的最佳细胞收获期为３周左右。     

寡糖素对红花及三七培养细胞的生理作用

三种寡糖素,即来自人参（Ｐａｎａｘ ｇｉｎｓｅｎｇ）培养细胞的人参寡糖素、红花（Ｃａｒｔｈａｍｕｓ ｔｉｎｃｔｏｒｉｕｓ）培养细胞的红花寡糖素、黑节草（Ｄｅｎｄｒｏｂｉｕｍ ｃａｎｄｉｄｕｍ）植物的黑节草寡糖素对红花及三七（Ｐａｎａｘ ｎｏｔｏｇｉｎｓｅｎｇ）的培养细胞的生长及代谢产物的含量均有显著的促进作用。寡糖素可耐高温高压（１２１℃、．ｂｓ／ｃｍ＾２）灭菌１５分钟而不失活,其对植物培养细胞的     

细胞培养生产人参寡糖素降低成本的途径

在人参（Ｐａｎａｘｇｉｎｓｅｎｇ）细胞悬浮培养中,以无离子水代替重蒸馏水,细胞生长速率和寡糖素产率分别降低２．３％和２．９％。用白糖代替蔗糖,细胞生长速率和寡糖素产生率分别降低１．７４％和１．２３％。综合上述两方面结果,以无离子水和白糖分别替代原培养基中的重蒸馏水和蔗糖组成替代培养基,用替代培养基培养人参培养细胞,其生长速率可达０．５０９ｇＤＷ／Ｌ．ｄ．寡糖素产率可达１．４４３ｇ／Ｌ,和原培养基相     

高产人参寡糖素培养细胞变异克隆系的筛选

用２ｍｍｏｌ／Ｌ的ＭＮＮＧ处理经过滤的人参悬浮培养细胞１小时后,细胞存活率下降显著,细胞克隆植板率只是对照组的１０．１２％。经细胞平板克隆共获得克降系１５１株,其中很多克隆系转移培养中生长缓慢,甚至不生长而死亡,经分析可供测定的克隆系生长的寡糖素含量的差异,对１１株寡糖素含量较高克隆系经连续１０代继代培养观察,选出一株稳定高产人参寡糖素优良克隆系ＰＧＭＢ－３７,其平均生长速率是０．５５８ｇＤＷＬ＾     

不同营养因子对新疆紫草悬浮培养细胞生长及紫草宁衍生物形成的影响

报道了不同碳源、维生素、氨基酸、钙盐及肌醇对新疆紫草悬浮培养细胞生长及紫草宁衍生物形成的影响。蔗糖是最适碳源、最佳浓度为３％。Ｂ族维生素对细胞生长及紫草宁衍生物形成的促进效果不大。酪氨酸以及甘氨酸会抑制产物的形成;而１０－５ｍｏｌ／ｌ的Ｌ－苯丙氨酸以及１０－７—１０－６ｍｏｌ／ｌ维生素Ｃ可明显提高紫草宁衍生物的含量及产量。肌醇对细胞生长的影响不大,但２００ｍｇ／ｌ肌醇可促进产物的形成。适于细胞生长及紫草宁衍生物形成的钙源分别为３３２ｍｇ／ｌＣａＣｌ２·２Ｈ２Ｏ和１４００ｍｇ／ｌＣａ（Ｎｏ３）２·４Ｈ２Ｏ。文末列出了改良的生长培养基及其配方。     

三七.人参和西洋参细胞悬浮培养的比较研究

用薄层层析对三七、人参和西洋参愈伤组织进行的初步鉴定表明,三种愈伤组织都含有皂甙和主要皂甙成分Rb_1、Rg_1,三七愈伤组织还含有一种抗癌皂甙Rh_1。对愈伤组织的生长,三七低于人参高于西洋参;对愈伤组织中总皂甙含量,三七均高于人参和西洋参。三种植物细胞悬浮培养结果类似于他们的愈伤组织培养,但生长又进一步提高。三七细胞悬浮培养中皂甙产生的时间进程几乎与生长平行,合适的收获期为培养30天。寡糖素不仅增强三七培养细胞的皂甙形成而且促进细胞生长,较合适的浓度为1.25 ppm。通过以上研究,使三七悬浮培养细胞的生长(干重增加178毫克)为最初培养愈伤组织的4倍以上,总皂甙产率高达20.6毫克,为最初培养愈伤组织的8.5倍。     

高产人参寡糖素培养细胞克隆系的诱变筛选

紫外辐射能显著地降低人参培养细胞单细胞克隆的植板率。当紫外辐射悬浮细胞３０ｓ后,细胞克隆的植林率是对照组的２１．４３％。细胞克隆平板培养６０ｄ,挑取克隆连续转移培养３次,共获得克隆系１２２株。对所有克隆系进行变异分析并经１０代连续继代培养,从中筛选到一株稳定的高产寡糖素克隆系ＰＧＵＡ－０８,而且它的过氧化物酶同工酶谱特征也保持稳定。克隆系ＰＧＵＡ－０８的生长速率为０．５３７ｇＤＷＬ－１ｄ－１,是亲本的１．４６倍,寡糖素含量为１７．１６％ＤＷ,是亲本的１．８１倍,寡糖素产率为２．７６４ｇ／Ｌ,是亲本的２．６２倍。     

Kinetics of photoautotrophic growth of Marchantia polymorpha cells in suspension culture

Chlorophyllous, cultured cells of Marchantia polymorpha L. (HYA-2 cell line) grow actively under photoautotrophic (lithotrophic) conditions. The maximum specific growth rate (μ_cell) was 0.64 day⁻¹ and the doubling time was 1.08 days under optimum conditions (165 μmol m⁻² s⁻¹, 1% carbon dioxide enriched atmosphere, 25^°C). The photosynthetic activity was 1.30 μmol CO₂-fixed (10⁶ cells)⁻¹ h⁻¹ [66 μmol (mg chlorophyll)⁻¹ h⁻¹] in the exponential phase. The growth course has two distinct phases, an exponential and a linear one. The exponential phase is observed as long as the population density is sufficiently low (less than 7.9 × 10⁶ cells ml⁻¹), so that practically all individual cells directly receive the full incident light. The effect of light on the specific growth rate is a linear function of photon flux density. Linear growth occurs after the population density is so high that the incident light is almost completely absorbed by the cell suspension. The growth rate is a logarithmic function of photon flux density, in contrast to the specific growth rate, and saturates at high photon flux densities. The conditions of maximum growth, however, are not wellbalanced between cell mass production and cell division. Therefore, the maximum growth does not continue for a long time.     

The Physiological Effects of Elicitor Ginseng-oligosaccharides on oell Culture of Carthamus tinctorius

Different kinds of oligosaccharides were isolated and purified from the culture cells of Panax ginseng. Results showed that these oligosaccharides could increased the cell growth rate and α-tocopherol content of the cell culture of Carthamus tinctorius. Among them, the effects of oligosaccharide Ⅵ, Ⅶ and Ⅷ were more significant than the others. The optimum effective concentrations of oligosaccharide Ⅵ, Ⅶ and Ⅷ were higher in callus culture than in suspension culture. Studies on the time course of addition of oligosaccharide Ⅶ and Ⅷ in different culture. period of Carthamus tinctorius cultures revealed that the α-tocopherol content was increased after addition of oligosaccharides for 1–3 days. The cell growth rate was increased by 18.11%. The α-tocopherol content and yield were increased by 3.5 and 4.3 folds respectively when supplement with 2 mg/L of oligosaccharide Ⅵ and Ⅶ and 1 mg/L of oligosaccharide Ⅷ to the suspension medium at the same time.     

稀土元素对红豆杉细胞悬浮培养及紫杉醇合成的影响

研究了在250mL摇瓶中,不同浓度的硝酸镧、硫酸铈铵、硝酸亚铈3种稀土化合物对细胞生长及紫杉醇分泌和释放的影响。结果表明,在培养初期加入稀土元素。3种不同稀土化合物对细胞生长影响强弱不同,但趋势相似,均使细胞的延迟期缩短。1ppm的Ce^4 促进细胞生长的效果最明显。细胞干重第17d达到10.9g/L。在指数期加入稀土元素。10ppmCe^3 刺激细胞生长的效果最明显,细胞干重最高值达到11.5g/dL,比对照高1.5g/L,而10ppm的La^3 抑制细胞的生长。经稀土元素处理后,细胞胞内和胞外紫杉醇含量都有大幅度的提高,其中以10ppmCe^3 处理,胞外紫杉醇释放率最大,达37.7%。     

High cell density culture of Anabaena variabilis with controlled light intensity and nutrient supply

Controlling the light energy and major nutrients is important for high cell density culture of cyanobacterial cells. The growth phase of Anabaena variabilis can be divided into an exponential growth phase and a deceleration phase. In this study, the cell growth in the deceleration phase showed a linear growth pattern. Both the period of the exponential growth phase and the average cell growth rate in the deceleration phase increased by controlling the light intensity. To control the light intensity, the specific irradiation rate was maintained above 10 micromol/s/g dry cell by increasing the incident light intensity stepwise. The final cell density increased by controlling the nutrient supply. For the control of the nutrient supply, nitrate, phosphate, and sulfate were intermittently added based on the growth yield, along with the combined control of light intensity and nutrient concentration. Under these control conditions, both final cell concentration and cell productivity increased, to 8.2 g/l and 1.9 g/l/day, respectively.     

Cell cycle analysis of Taxus suspension cultures at the single cell level as an indicator of culture heterogeneity

Single cell growth and division was measured via flow cytometry in order to characterize the metabolic variability of Taxus cuspidata suspension cultures, which produce the valuable secondary metabolite Taxol. Good agreement was observed between the cell cycle distribution and biomass accumulation over the batch culture period. Specific growth rates of 0.13 days(-1) by fresh weight and 0.15 days(-1) by dry weight were measured. Elicitation with methyl jasmonate (MJ) significantly decreased both cell cycle progression and biomass accumulation, as the specific growth rate decreased to 0.027 days(-1) by fresh and dry weight. Despite the decrease in biomass accumulation for MJ elicited cultures, sucrose utilization was not significantly different from control cultures. MJ elicitation also increased the accumulation of paclitaxel and other taxanes. The accumulation of upstream taxanes (baccatin III and 10-deactylbaccatin III) increased during exponential growth, reached a maximum around day 12, and then declined throughout the stationary phase. The paclitaxel concentration increased during both exponential growth and stationary phase, reaching a maximum around days 20-25. Throughout the culture period, greater than 70% of the cells were in G(0)/G(1) phase of the cell cycle. Studies using bromodeoxyuridine (BrdU) incorporation showed that approximately 65% of the Taxus cells are noncycling, even during exponential growth. Although the role of these cells is currently unknown, the presence of a large, noncycling subpopulation can have a significant impact on the utilization of plant cell culture technology for the large-scale production of paclitaxel. These results demonstrate that there is a high degree of metabolic heterogeneity in Taxus cuspidata suspension cultures. Understanding this heterogeneity is important for the optimization of plant cell cultures, particularly the reduction of production variability.     

石竹细胞悬浮培养研究

石竹细胞继代周期为 7d时 ,悬浮细胞培养系生长最快 ,生长率最高 ,而且培养物中胚性细胞较多 ,并能保持较快的分裂和生长 ,能促进已形成的大细胞团的生长和分化。转代时接种物与新鲜培养基的体积比以1∶2较好 ,悬浮系细胞生长最快 ,生长率最高 ,以 1∶2和 1∶3的高倍稀释接种有利于胚性细胞的形成及产生小的胚性细胞团 ,对悬浮系添加椰乳和水解乳蛋白的混合物 ,可较大幅度地提高悬浮细胞系的生长速率 ,单独添加上述两种物质的效果均不如二者的综合效应好。在 6种不同激素组合中 ,配方 2 (2 ,4 D 1 .5mg/L +NAA0 .5mg/L +6 BA 0 .5mg/L)最好 ,生长率最高。配方 5 (2 ,4 D 1 .5mg/L +NAA 0 .5mg/L +6 BA 1 .0mg/L)其次 ;配方 1 (2 ,4 D 1 .0mg/L +NAA 0 .5mg/L +6 BA 0 .5mg/L)次之。     

Establishment of callus and cell suspension culture of Scrophularia striata Boiss.: an in vitro approach for acteoside production

In the present study, a protocol was optimized for establishment of callus and cell suspension culture of Scrophularia striata Boiss. as a strategy to obtain an in vitro acteoside producing cell line for the first time. The effects of growth regulators were analyzed to optimize the biomass growth and acteoside production. The stem explant of S. striata was optimum for callus induction. Modified Murashige and Skoog medium supplemented with 0.5 mg/l naphthalene acetic acid + 2.0 mg/l benzyl adenine was the most favorable medium for callus formation with the highest induction rate (100 %), the best callus growth and the highest acteoside content (1.6 μg/g fresh weight). Incompact and rapid growing suspension cells were established in the liquid medium supplemented with 0.5 mg/l naphthalene acetic acid + 2.0 mg/l benzyl adenine. The optimum time of subculture was found to 17–20 days. Acteoside content in the cell suspension was high during exponential growth phase and decreased subsequently at the stationary phase. The maximum content of acteoside (about 14.25 μg/g cell fresh weight) was observed on the 17th day of the cultivation cycle. This study provided an efficient way to further regulation of phenylethanoid glycoside biosynthesis and production of valuable acteoside, a phenylethanoid glycoside, on scale-up in S. striata cell suspension culture.     

红豆杉悬浮细胞放大培养的细胞生长与紫杉醇合成动力学

研究了在Murashige&skoog s(MS)和 6 2号两种不同的培养基中 ,红豆杉细胞悬浮细胞从摇瓶到 1 0L机械通气搅拌式反应器放大培养过程中细胞生长与紫杉醇合成动力学 .结果表明 :尽管在不同的培养条件下 ,细胞生长曲线均呈现“S”型 .紫杉醇在延迟期与指数生长期中基本上没有积累 ,而且随着培养规模的增大 ,紫杉醇的含量逐渐降低 .进一步对各级放大培养的细胞生长 ,比生长率与胞内外紫杉醇合成量进行分析 ,发现MS利于细胞生长但不利于紫杉醇合成 ,而 6 2号则相反 .根据此文的结果 ,提出了红豆杉细胞培养条件的优化和大规模细胞培养生产紫杉醇应采取的策略     

红花单细胞克隆的建立

KT,2,4-D 及 NAA 能提高红花(Cathamus tinctorius)细胞克隆平板培养的植板率。这三种激素对细胞生长的最佳搭配是2,4-D2.0mg/l,KT0.3mg/l,NAA 0.5mg/1。红花细胞悬浮继代培养代数不同,其植板率相差甚远,用悬浮培养第三代的细胞做材料最好,其植板率是第一代悬浮培养细胞做材料的8.5倍。红花细胞克隆的条件培养的植板率是普通平板培养的3.6倍。固-液双层培养的植板率是普通平板培养的4.7倍。对已建立的红花细胞克隆进行生长速率的比较表明,生长最漫的克隆的生长速率为3.08g/g/35天,生长最决的克隆的生长速率高达23.33g/g/35天。