Production of Biomass and Ginsenosides from Adventitious Roots of Panax ginseng in Bioreactor Cultures

Organic nutrients play a central role during Panax ginseng adventitious root culture in bioreactor systems. To understand how the nutrient elements were uptaken during the adventitious root growth as well as the production of biomass and natural ginsenosides, a biotechnological approach to identifying the nutritional physiology of ginseng in a commercial‐scale bioreactor was necessary. Normal MS medium nutrient in the bioreactor culture of adventitious roots resulted in slow growth, low biomass, and Rg and Rb ginsenoside contents. When the ginsenoside production increased to higher levels, a group of regulatory nutritional elements that have the potential to interact with biomass was identified. The effects of the salt strength of the medium, of macroelements, metal elements, the ammonia/nitrate ratio, sucrose concentration, and osmotic agents on the growth, the formation of biomass and the production of ginsenosides from adventitious roots were investigated. Appropriate conditions allowed for a maximum ginsenoide production of up to 12.42 [mg/g DW] to be obtained after 5 weeks of culture. The results demonstrated that the key organic nutrients can be regulated to improve the biomass and growth, and increase the ginsenoside yield in bioreactor cultures of P. ginseng adventitious roots.     

Dynamics of Predator‐Prey Interactions in Continuous Cultures

This paper studies the behavior of a general unstructured kinetic model for continuous bioreactors involving interactions between predator, prey and a limiting substrate. The analysis carried out in this paper shows how closed analytical conditions for arbitrary growth rates can be derived that describe the conditions for the existence of the interacting species in an oscillatory behavior. It is also demonstrated how practical diagrams in terms of operating and kinetic parameters can be constructed that classify the different behavior predicted by the model. Applications of these general results to a number of experimentally validated models have revealed that the saturation model always predicts hard oscillations for a certain range of dilution rates, for any values of model parameters. Bifurcation diagrams in the operating parameter space permitted the delineation of regions of hard oscillations, regions of static coexistence, regions of predator washout and regions of total washout. The analysis of the double saturation model has proven its ability to predict two Hopf points. Hard oscillations are therefore expected within the dilution rates corresponding to the two Hopf points. Practical diagrams were also constructed to delineate the boundaries separating hard oscillations from static coexistence and washout conditions.     

茉莉酸甲酯诱导下红豆杉细胞产生紫杉烷类物质群代谢轮廓分析

红豆杉细胞培养物经甲醇提取和固相萃取粗分离,进行反相高效液相色谱分析,获得了约含13个与紫杉醇极性相关的化合物色谱图,通过质谱联用和对照品参照,归属了这些化合物组成。进一步利用茉莉酸甲酯（MJ）诱导细胞,比较这些组分在诱导前后的相对色谱峰面积变化,结果表明,所有紫杉烷组分的浓度在诱导后都提高,其中以taxchinin M及其结构类似物提高最显著,紫杉醇,B-Ⅲ和B-Ⅵ等比C14位取代的taxuyunnanine C及其衍生物的浓度增加幅度要大,提示MJ对紫杉醇合成中非有效乙酰化旁路代谢有促进作用,而对C14位取代物生成的旁路促进作用不明显。本文为紫杉醇的生物合成研究提供了新的思路和方法。     

气升式生物反应器在杂交瘤细胞培养中的应用

前述研究工作基础上,设计开发了10L规模的动物细胞培养用气升式生物反应器。应用该生物反应器悬浮培养杂交瘤细胞．通过平行试验,考察了该反应器设计的合理性和可靠性。结果显示该反应器不存在限制细胞生长、代谢和产物生成的因素,而且细胞破损技彻底消除,表明该气升式生物反应器给细胞生长、代谢和产物生成提供了理想的培养环境,其设计是成功的。     

动物细胞培养用生物反应器设计原理

动物细胞培养用生物反应器设计和放大的关键问题是细胞破损与供氧和混合的矛盾,在分析细胞破损机理基础上,提出了动物细胞培养生物反应器的设计原理——设计模型和有关设计条件,从而清楚地确立了细胞死亡速度与培养基组成、反应器设计和操作参数间的定量关系,以及反应器设计应遵循的保证细胞生长和满足传质要求的条件。还对强化传质和抑制细胞破损这一矛盾作了简要分析和讨论。     

Rapid Fibroblast Removal from High Density Human Embryonic Stem Cell Cultures

Mouse embryonic fibroblasts (MEFs) were used to establish human embryonic stem cells (hESCs) cultures after blastocyst isolation¹. This feeder system maintains hESCs from undergoing spontaneous differentiation during cell expansion. However, this co-culture method is labor intensive, requires highly trained personnel, and yields low hESC purity⁴. Many laboratories have attempted to minimize the number of feeder cells in hESC cultures (i.e. incorporating matrix-coated dishes or other feeder cell types^5-8). These modified culture systems have shown some promise, but have not supplanted the standard method for culturing hESCs with mitomycin C-treated mouse embyronic fibroblasts in order to retard unwanted spontaneous differentiation of the hESC cultures. Therefore, the feeder cells used in hESC expansion should be removed during differentiation experiments. Although several techniques are available for purifying the hESC colonies (FACS, MACS, or use of drug resistant vectors) from feeders, these techniques are labor intensive, costly and/or destructive to the hESC. The aim of this project was to invent a method of purification that enables the harvesting of a purer population of hESCs. We have observed that in a confluent hESC culture, the MEF population can be removed using a simple and rapid aspiration of the MEF sheet. This removal is dependent on several factors, including lateral cell-to-cell binding of MEFs that have a lower binding affinity to the styrene culture dish, and the ability of the stem cell colonies to push the fibroblasts outward during the generation of their own "niche". The hESC were then examined for SSEA-4, Oct3/4 and Tra 1-81 expression up to 10 days after MEF removal to ensure maintenance of pluripotency. Moreover, hESC colonies were able to continue growing from into larger formations after MEF removal, providing an additional level of hESC expansion.     

Pretreatment of Parsley (Petroselinum crispum L.) Suspension Cultures with Methyl Jasmonate Enhances Elicitation of Activated Oxygen Species

Suspension-cultured cells of parsley (Petroselinum crispum L.) were used to demonstrate an influence of jasmonic acid methyl ester (JAME) on the elicitation of activated oxygen species. Preincubation of the cell cultures for 1 d with JAME greatly enhanced the subsequent induction by an elicitor preparation from cell walls of Phytophtora megasperma f. sp. glycinea (Pmg elicitor) and by the polycation chitosan. Shorter preincubation times with JAME were less efficient, and the effect was saturated at about 5 [mu]M JAME. Treatment of the crude Pmg elicitor with trypsin abolished induction of activated oxygen species, an effect similar to that seen with elicitation of coumarin secretion. These results suggest that JAME conditioned the parsley suspension cells in a time-dependent manner to become more responsive to elicitation, reminiscent of developmental effects caused by JAME in whole plants. It is interesting that pretreatment of the parsley cultures with 2,6-dichloroisonicotinic and 5-chlorosalicylic acid only slightly enhanced the elicitation of activated oxygen species, whereas these substances greatly enhanced the elicitation of coumarin secretion. Therefore, these presumed inducers of systemic acquired resistance exhibit a specificity different from JAME.     

Photoautotrophic Cell and Tissue Culture in a Tubular Photobioreactor

An externally illuminated tubular photobioreactor was constructed from 3.4 m stainless steel tubes and 22.1 m glass tubes for the cultivation of photoautotrophic organisms. The 30‐L reactor can be equipped with helical static mixers in order to create a uniform radial exchange within the tubes, 40 mm in diameter. A flexible construction of the reactor allows scale‐down experiments to be carried out with axial velocities between 0.3–2.5 m/s, gassing‐in rates of 0–0.5 L/min, k_L a values of 0.002–0.006 s^–1 and six metal halide lamps inducing photon flux densities in the range of 70–300 μE/m²s. Two model organisms, the green microalgae Chlorella vulgaris and the bryophyte Physcomitrella patens, were chosen to characterize cell growth and physiology in submerse cultures. Comparative experiments with Chlorella vulgaris in two configurations of the reactor with inserted helical static mixers and plates resulted in maximum growth rates of 1.6 d^–1. No growth enhancement was obtained in the case of helical static mixers at a mean PFD of 150 μE/m²s and an axial velocity of 0.4 m/s. No homogenous flow could be obtained in the case of inserted plates. Physcomitrella patens was successfully cultivated in the reactor (μ = 0.36 d^–1), whereas average axial velocities of ca. 0.6 m/s guarantee favorable gas transport without contributing to cell damage. This makes tubular photobioreactors a promising production system for the production of glycosylated recombinant proteins derived from moss.     

Effects of Methyl Jasmonate on Shikonin and Dihydroechinofuran Production in Lithospermum Cell Cultures

Methyl jasmonate, when administered to Lithospermum erythrorhizoncell suspension cultures, was found to induce the productionof shikonin derivatives (the red naph-thoquinone pigments ofthe root) and dihydroechinofuran (an abnormal metabolite ofgeranylhydroquinone). Culture experiments showed that methyljasmonate caused a rapid increase in the activities of enzymesinvolved in the biosynthesis of shikonin such as p-hydroxybenzoategeran-yltransferase, which was followed by the rapid accumulationof dihydroechinofuran and the delayed production of shikonin.The induction patterns observed were similar to those elicitedby oligogalacturonides in Lithospermum cells, suggesting thatjasmonic acid or its derivative may act as a signaling moleculein the elicitation of shikonin biosynthesis. Interestingly,however, the copper ion, which is essential for inducing shikoninbiosynthesis by oligogalacturonides, was not required for shikonininduction by methyl jasmonate ¹Present address: Laboratory of Molecular & Cellular Biology,Department of Agricultural Chemistry, Kyoto University, Kitashirakawa,Kyoto, 606-01 Japan     

High Frequency in vitro Multiplication of Centella asiatica: An Important Industrial Medicinal Herb

An efficient protocol was developed for rapid clonal propagation of the important medicinal plant, Centella asiatica (L.) Urban, using shoot tip culture. High frequency bud break (88 %) and multiple shoot formation (16.8 shoots/shoot tip) were induced from a shoot tip segment, which was cultured on MS medium supplemented with 6‐benzylaminopurine (BAP) (17.76 μM) and gibberillic acid (GA₃) (1.44 μM). Half‐strength Murashige and Skoog (MS) medium supplemented with naphthalen acetic acid (NAA) (10.74 μM) induced the maximum (27.66) number of roots. Plantlets with 3–4 fully expanded leaves and well‐developed roots were successfully transferred to potted soil which exhibited a 95 % survival. The protocol enables the harvest of more than 25,000 plantlets within 160 days starting from a single shoot tip explant.     

茉莉酸甲酯与水杨酸对肉苁蓉悬浮细胞中苯乙醇甙合成的影响

向肉苁蓉悬浮细胞培养系中添加茉莉酸甲酯(MJ)和水杨酸(SA) ,分别考察了这两种诱导子的添加浓度及添加时间对肉苁蓉悬浮细胞系中苯乙醇甙含量的影响。研究结果表明:MJ和SA能够促进肉苁蓉悬浮细胞系中苯乙醇甙(PeG)和松果菊甙(Echinacoside)的合成,但两者的适用的浓度范围和最佳添加时间存在差异。与未经诱导子处理的细胞培养结果相比,MJ在对数生长初期(培养14d) ,添加浓度为5 μmol L条件下,可使肉苁蓉悬浮细胞系中PeG含量提高2 5 9倍,Echin含量提高3 82倍;而SA在对数生长后期(培养2 8d) ,添加浓度为5 0 μmol L条件下,可使PeG含量提高2 71倍,Echin含量提高3 16倍。     

Chemical Components of Cell Cultures of Arnebia euchroma

Five naphthaquinones were isolated from the petroleum ether extract of the cell cultures of Arnebia euchroma (Royle) Johnst.. Their structures were identified as deoxyshikonin, β,β-dimethylacrylshikonin, acetylshikonin, teracrylshikonin and β-hydroxyisovalerylshikonin by means of chemical methods, HPLC, IR and 1H-NMR data respectively. There was no shikonin in the cell cultures, which was obtained from the roots of A. euchroma. The contents of each compound in the cell cultures are different from those in the roots of A. euchroma.     

动植物细胞或组织生物反应器悬浮培养过程中的通气方式

通气在动植物细胞或组织生物反应器培养过程中起着至关重要的作用,而同时通气过程所产生的机械损伤力亦可对细胞造成直接的伤害,因此,通气方式是动植物细胞或组织生物反应器培养过程设计与工程放大的关键技术之一。本文综述了动植物细胞或组织生物反应器悬浮培养过程中三种主要通气(异养培养时又称供氧)方式的结构特点,及其对气液传质、生物量、代谢产物量和细胞损伤的影响,以及改进的新型通气方式和几种通气方式的融合并用。     

Induction of a Stress Protein in Developing Cell Cultures of the Rat Cerebellum

Abstract: We examined the ability of developing cere-bellar cell cultures to synthesize a 71,000 MW stress protein (SP71) in response to heat shock and Cd²⁺ treatment. The induction of SP71 synthesis appeared to be dependent on both the age of the culture and the stressor used. Heat shock induced SP71 synthesis in freshly prepared cells and in cell cultures at each age examined, whereas Cd²⁺ was effective only in cultures at 7 days of age and older. These findings are discussed with reference to the development of various cell types in these cultures.     

A Novel Bioreactor for High Density Cultivation of Diverse Microbial Communities

A novel reactor design, coined a high density bioreactor (HDBR), is presented for the cultivation and study of high density microbial communities. Past studies have evaluated the performance of the reactor for the removal of COD¹ and nitrogen species^2-4 by heterotrophic and chemoautotrophic bacteria, respectively. The HDBR design eliminates the requirement for external flocculation/sedimentation processes while still yielding effluent containing low suspended solids. In this study, the HDBR is applied as a photobioreactor (PBR) in order to characterize the nitrogen removal characteristics of an algae-based photosynthetic microbial community. As previously reported for this HDBR design, a stable biomass zone was established with a clear delineation between the biologically active portion of the reactor and the recycling reactor fluid, which resulted in a low suspended solid effluent. The algal community in the HDBR was observed to remove 18.4% of total nitrogen species in the influent. Varying NH₄⁺ and NO₃^- concentrations in the feed did not have an effect on NH₄⁺ removal (n=44, p=0.993 and n=44, p=0.610 respectively) while NH₄⁺ feed concentration was found to be negatively related with NO₃^- removal (n=44, p=0.000) and NO₃^- feed concentration was found to be positively correlated with NO₃^- removal (n=44, p=0.000). Consistent removal of NH₄⁺, combined with the accumulation of oxidized nitrogen species at high NH₄⁺ fluxes indicates the presence of ammonia- and nitrite-oxidizing bacteria within the microbial community.     

双碳源单细胞蛋白高密度培养

单细胞蛋白(SCP)培养具有增殖速度快、原料来源广、蛋白质含量高等优点,正在成为重要的蛋白质来源之一。生产SCP的原料包括烷烃、低碳醇类及碳水化合物。由碳水化合物,尤其是由各种农副产品加工的废料、造纸工业废水及木质纤维素水解产物等,生产SCP属于废弃资源的综合利用,具有重要的经济和社会意义。这类原料中常含有多种碳源,例如,在木质纤维水解液中,有以木糖为主的五碳糖,也有以葡萄糖为主的六碳糖,木糖与葡萄糖之比约为1:2。这样,木糖的利用就成了一个关键问题。葡萄糖对木糖代谢的抑制作用随葡萄糖比例的降低而减轻;Slinger和Bothast研究了用混合糖培养Candida shehetane的过程,当木糖与葡萄糖的比例为3:1及1:1时,葡萄糖的利用速度分别比木糖高1.6倍及3.4倍;在低还原势时,酵母产酒精速率降低而细胞增长速率加快,可以达到较高细胞浓度。     

NO和茉莉酸甲酯对黄芩悬浮细胞生长及黄芩苷合成的影响

以硝普钠(sodium nitroprusside,SNP)为一氧化氮(nitric oxide,NO)的供体,向黄芩(Scutellaria baicalensis)悬浮培养细胞系中添加SNP和茉莉酸甲酯(methyl jasmonate,MJ),考察这两种诱导子在不同的添加时间、添加浓度及混合配比使用对黄芩悬浮细胞系生长和黄芩苷含量的影响。研究结果表明：低浓度的外源NO有利于细胞的生长,但对黄芩苷积累无作用,而MJ有利于黄芩苷的合成,但抑制细胞生长,且两者的适用浓度范围和添加时间存在差异。在细胞培养初期(0天)添加0.05 mmol·L~(-1)SNP,而在细胞生长对数中期(8天)添加10μmol·L~(-1)的MJ,细胞鲜重可达到对照的1.2倍,黄芩苷总量达到对照的2.96倍。