Cell Suspension and Callus Culture from Somatic Tissue of Maize

Cell suspension and callus cultures from somatic tissue of inbred lines of maize (Zea mays L.) were cultured on media that were defined via modification of a Linsmaier and Skoog preparation. Germlings incubated on the primary medium originally employed required long-term incubation for callus induction. Modification of the primary medium with high levels of iron and (ethylene dinitrillo)tetraacetic acid (EDTA), B vitamin amendments and vitamin E, shortened incubation by 75% and nearly doubled the percentage of germlings which produced callus. Callus did not remain viable in subcultures to the secondary medium originally employed, whereas a preparation, developed via modification of the original secondary medium, enabled perpetuation of callus through repeated subculture. Modification with high levels of iron and EDTA, plug B vitamins and vitamin E, with decreased concentrations of five inorganic salts, suppressed aberrant organogenesis and stabilized culture growth as viable callus. Similar modification, with the exception that EDTA was omitted, was employed for the development of a liquid medium. Tonicity of the medium was adjusted with a lowered level of sucrose, with the liquid further modified by addition of acetate. Upon development of this liquid, maize became the sixth monocot species for which somatic cells remain viable through repeated subculture in liquid suspensions.     

若干因子对鸡冠花悬浮培养中花色素苷积累的影响

本文研究几种植物生长调节剂和蔗糖浓度对鸡冠花细胞悬浮培养中花色素苷积累的影响。结果表明,细胞分裂素KT使花色素苷积累明显高于6-BA,且KT在2 μmol/L时积累量最高;2,4-D在2 μmol/L时对花色素苷积累效果明显,其它浓度的2,4-D和NAA对花色素苷积累效果不明显。高浓度蔗糖有利于花色素苷积累;MS+2,4-D(2 μmol/L)+KT(2 μmol/L)+蔗糖(292 mmol/L)为鸡冠花悬浮细胞培养生产花色素苷的最佳培养基。研究中还发现,在黑暗条件培养下无花色素苷积累,推断光是诱导花色素苷积累的主要因素。随着继代次数的增加,花色素苷含量明显增高,但到第4代时基本稳定。     

Molecular Architecture of the Cell Wall of Poplar Cells in Suspension Culture, as Revealed by Rapid-Freezing and Deep-Etching Techniques

The architecture of the primary cell wall of poplar cells insuspension culture was observed after application of rapid-freezingand deep-etching techniques both before and after the sequentialextraction of cell wall polysaccharides. The architecture ofthe cell wall was also examined after treatment with pectin-degradingenzymes. The dimensions of interfibrillar spaces or pores increasedafter the extraction of pectins by chemical or enzymatic treatment.The ordered spacing of cellulose microfibrils was only slightlyaltered after treatment with 0.7 M KOH but was dramaticallyaltered after treatment with 4.3 M KOH. These results suggestthat a hemicellulose, perhaps xyloglucan, may have a substantialrole in maintaining the three-dimensional conformation via interfibrillarpolysaccharide linkages in the cell wall of this dicotyledonousspecies. ²Present address: Tobacco Central Laboratory, Japan TobaccoIndustry Co. Ltd., Midoriku, Yokohama, Kanagawa, 227 Japan     

Some Factors Affecting the Anthocyanin Formation by Populus Cells in Suspension Culture

In order to elucidate the mechanism of anthocyanin formation by Populus cells in suspension culture, the favourable conditions for anthocyanin formation were investigated. The influence of some factors affecting the anthocyanin formation, i.e. light, sucrose and riboflavin etc. were also examined. Light irradiation and high sucrose concentrations brought about a marked increase of PAL activity, which increased rapidly at the lag phase preceding the anthocyanin formation. The effect of blue light on anthocyanin formation was markedly superior to other kinds of monochromatic light (green and red) or white light. Riboflavin was effective only under light exposure. It was inferred that light, sucrose, riboflavin and PAL activity etc. were closely related with the anthocyanin formation. Especially, light and sucrose cooperated in the increase of PAL activity which was a key enzyme in the biosynthesis of anthocyanin.     

除虫菊细胞的悬浮培养

除虫菊悬浮细胞从培养后第8天开始迅速生长,14 d达到最大生长量,其最适培养基为:MS 4mg·L-12,4-D 0.1mg·L-1NAA 0.3 mg·L-16-BA 30 g·L-1蔗糖,最适接种量为15 g·L-1,摇瓶装液的体积分数为40%,初始培养的最适pH值为5.8,收获时pH下降为4.6±1,最适培养温度为25℃.     

Isolation and Identification of Camptothecin from Cells of Camptotheca acuminata Suspension Cultures

Ten strains of non-sulfur purple photosynthetic bacteria were isolated from soil and water samples gathered in Bangkok and its surrounding area. The isolated strains from Thailand were divided into two groups, Al to A4 and BI to B6. They were identified as Rhodopseudomonas gelatinosa and Rhodopseudomonas sphaeroides, respectively. All strains grew well either at 30°C or 40°C, but failed to grow at 45°C. Strains belonging to group A had weak activities of nitrogenase (acetylene reduction) and hydrogen production, while strains of group B showed much higher activities than group A. The activities of nitrogenase and hydrogen production of isolates in Thailand were compared with those of isolates in Japan. The activities of isolated strains in Thailand at 40°C were almost equal to those at 30°C or even higher. On the other hand, both hydrogen production and the nitrogenase activity of isolates in Japan decreased significantly at 40°C as compared to the activities at 30°C. These results suggest an intrinsic thermostability in hydrogen production by the non-sulfur purple photosynthetic bacteria of Thailand. Among isolated strains in Thailand, strain B5 was the most active in nitrogenase and hydrogen production, and its activity was significantly higher than strain TN3 at 40°C. TN3 had been selected as the most active strain among isolates in the Sendai area.     

从水稻根部悬浮培养细胞分离原生质体及植株再生

以长香稻(Oryza sativa L．)(糯稻)的幼嫩种子根为材料,在Ms和N6培养基上诱导产生结构松软而分散的愈伤组织,经过AA液体培养基振荡悬浮培养,悬浮培养细胞经酶解后得到了活性较高的原生质体,试验结果表明这是分离原生质体较理想的材料。在附加2,4-D lmg／L(以下单位同)、KT(激动素)0．2、各氨酰胺876、天门冬酰胺266的Ms琼脂糖培养基中,诱导出了大量愈伤组织,在含KT2、NAA(α-萘乙酸)0．2、zT(玉米素)0．2、cH(水解酪蛋白)1000和4％椰子汁的N6培养基中成功地诱导出了由原生质体再生的植株。当代原生质体再生植株能正常开花、结实、产生种子;染色体数均为二倍性(2n＝24),最显著的特点是结实率低,穗粒数减步、生育期延迟。     

草麻黄细胞悬浮培养体系的建立

目的:建立草麻黄悬浮培养体系.方法:采用组织培养的方法探讨了水解酪蛋白(CH)、基本培养基、取材时间、和摇床转速对麻黄愈伤组织悬浮培养的影响.结果:MS基本培养基、300mg/l水解酪蛋白、继代25d的愈伤组织、转速110r/min是愈伤组织悬浮培养的适宜条件,愈伤组织细胞增殖量分别为0.76g、0.80g、0.80g、0.80g.结论:初步选择出草麻黄愈伤组织细胞的悬浮培养条件,为麻黄细胞扩大培养及有效成分提取奠定基础.     

沙枣细胞悬浮培养体系的建立

分别以沙枣幼嫩叶片,茎段为外植体诱导沙枣愈伤组织,选择生长旺盛的松散愈伤组织进行细胞悬浮培养,探讨了培养基种类和激素组合对其产生的影响.结果表明,最适的沙枣愈伤组织诱导培养基为NT(包括0.1 mg·L-1BA和0.1 mg·L-1TDZ);沙枣悬浮细胞在MS,NT,WPM,B5和IS培养基中均可生长,其中在NT培养基中生长状态最好,呈现生长均一的绿色疏松状态.激素组合对沙枣细胞生长影响很大,其中附加BA 0.1 mg·L-1和TDZ 0.1 mg·L-1组合的NT液体培养基可获得大量繁殖速度快、生长均匀一致的悬浮细胞,细胞增长系数达5.73.HPLC测定结果证明沙枣细胞中含有一定量的浓缩鞣质达5.2022 mg/gDW,这为利用沙枣悬浮细胞生产次生代谢产物提供了一条有效途径.     

犬皮肤成纤维细胞的分离、培养及鉴定

目的探索和建立适用于犬皮肤成纤维细胞的体外分离、培养及鉴定的技术方法。方法采用组织贴块培养法和胰蛋白酶、胶原酶Ⅰ联合消化法对犬皮肤成纤维细胞进行体外培养、传代。并对所培养的细胞进行倒置显微镜观察和苏木素-伊红染色,观察成纤维细胞形态,并对培养细胞行波形蛋白免疫荧光染色。结果倒置相差显微镜下可见长梭形细胞生长,苏木素-伊红染色可见细胞呈漩涡状、平行排列,第5代细胞免疫荧光检测波形蛋白(vimentin)表达阳性。结论建立了高效快速分离和稳定培养成纤维细胞的方法,为诱导犬心房纤维化提供了充足的种子细胞。     

成年小鼠心肌细胞的分离培养及鉴定

目的探讨成年小鼠心肌细胞分离培养的方法,评价心肌细胞的存活状况。方法应用改良Langendorff方法进行成年小鼠心脏灌流,分离并培养心肌细胞,评价杆状心肌细胞的比例变化。台盼蓝染色判定心肌细胞活力,应用毒胡萝卜素(thapsigargin)治疗心肌细胞24 h后,WST方法测定细胞生存率。结果在每个成年小鼠心脏分离了40~60万的心肌细胞,台盼蓝染色结果68%为存活心肌细胞。心肌细胞培养1 h2、4 h及48 h后,杆状心肌细胞的比例分别为70%、50%及30%。心肌细胞生存率随着毒胡萝卜素浓度的增加逐渐减低,其中1、5及10μmol/L毒胡萝卜素的生存率明显低于对照组(P<0.05,P<0.01)。结论应用改良Langendorff方法及严格控制心脏灌流培养的条件,可以成功地分离培养成年小鼠心肌细胞,有助于进行细胞分子水平的研究。     

Establishment of Orthosiphon stamineus Cell Suspension Culture for Cell Growth

Callus of Orthosiphon stamineus could be induced successfully from petiole, leaf and stem tissues but not roots when cultured on MS medium containing different concentration of NAA (0–4.0 mg l^–1) and 2,4-D (0–2.0 mg l^–1). Highest fresh weight callus production was obtained from leaf explants and those with best friability were obtained on MS medium plus 1.0 mg l^–1 2,4-D plus 1.0 mg l^–1 NAA. Cell suspension cultures were established from these cultures. The appropriate cell inoculum size for the best cell growth was 0.75 g of cells in 20 ml culture medium. Cell suspension culture using MS medium supplemented with 1.0 mg l^–1 2,4-D promoted the best cell growth with maximum biomass of 8.609 g fresh weight and 0.309 g dry weight 24 days after inoculation. Cells that grew in MS medium supplemented with 1.0 mg l^–1 2,4-D reached the stationary growth phase in 15 days as compared to the cells that grew in MS medium supplemented with 1.0 mg l^–1 2,4-D + 1.0 mg l^–1 NAA reached the stationary phase in 24 days. MS medium supplemented with 1.0 mg l^–1 2,4-D was considered as the maintenance medium for maintaining the optimum cell growth of O. stamineus in the cell suspension cultures with 2-week interval subculture.     

烟草脆散型愈伤组织获取及其细胞悬浮培养(简报)

以烟草叶片为外植体,以2/3MS BA 0.5mg/L NAA 0.1mg/L 为愈伤组织诱导培养基,继代培养3次后,转入添加3332.48mg/L Ca(NO3)2的该培养基上继代,可获得脆散型愈伤组织,并由此建立细胞悬浮培养系统。     

Studies on Cell Suspension Culture and Fermentation Culture in Arnebia euchroma

This paper reports some characteristics of cell suspension and fermentation culture in Arnebia euchroma (Royle) Johnst. The yield of suspension culture reached 22.0g dry wt/L per month when inoculum quantity was 2.50 g dry wt/L. Time-course study showed that cell growith lagged in 0–3 days and enhanced greatly in 3–12 days, and almost ceased after 12 days of culture, pH value changed during the culture period and peaked on the 12th day after inoculation. When cells were cultured in liquid production medium, the contents of shikonin derivatives increased quickly and reached to the maximum about the 25th day. The cell yield of 9.47 and 9.34 g dry wt/L per month was obtained in fermentation culture. Timecourse of cell growth in fermentation culture was similar to that in suspension culture. The total content of shikonin derivatives in fermentation culture was 14.26% dry weight from 10 L bioreactor. The yield of shikonin derivatives was 1.93 g/L.     

葡萄子房胚性细胞悬浮系的建立及其生长特性研究

由葡萄栽培品种“蜜汁”子房诱导的愈伤组织,经不同浓度２,４－Ｄ试验表明,０．５ｍｇ／Ｌ的２,４－Ｄ最有利于形成胚性细胞;该浓度下形成的质地紧密适度的愈伤组织经２个月的悬浮振荡培养,成功地建立了分散性好、生长旺盛的胚性细胞悬浮系;并通过培养过程中生长曲线的测定,确定了细胞悬浮系的生长特性。     

云南红豆杉细胞的悬浮培养

在云南红豆杉细胞悬浮培养中,适宜的培养基为B5,接种量为0．5～0．8g干重细胞／100ml培养基,2,4－D浓度为1．0mg／L;培养细胞的生长周期约30d;培养基中较高浓度的蔗糖（40g／L）可提高紫杉醇含量;添加的椰子汁（CM）、酪蛋白氨基酸（C）和水解乳蛋白（LH）3种有机添加剂均能提高培养细胞中紫杉醇的含量,但只有CM和CA能促进细胞的生长。于B5培养基中添加不同浓度的NH4NO3对培养细胞无明显影响。     

Studies on Cell Suspension Culture of Panax notoginseng

The optimum period of harvesting in cell suspension culture of Panax notoginseng was 30 days. The time course of sap.nih formation proceeded almost in parallel with the cell growth. An appropriate concentration of oligosaccharms from Panax ginseng, precursor fames.l, mannffol and lysozymum which were added into tbe culture broth 10 days before harvesting, all induced saponin biosynthesis significantly. Oligosaecharins at a concentration of 15ppm(it increased 1 fold of saponin yield, and increased 22.7%(of cell growth rate compared with those of the control) and farnesol at 200ppm(it increased 70.5% of sap.nih yield and stimulated cell growth compared with those of the control) were more effective.     

黄连细胞培养物中小檗碱的分离与鉴定

用黄连幼叶切块,接种在含1．0～2．0mg／L 2,4-D和0．1mg／LKT的6．7-v固体培养基上,诱导形成愈伤组织。选择较松散的愈伤组织转入液体悬浮培养,获得游离细胞和细胞聚集体。通过平板培养和细胞株的筛选．选择小檗碱含量较高的细胞株。经35次转代培养后,进行固体、液体培养。收集悬浮培养细胞进行化学提取和分离,获得黄色晶体,经TLc、UV、IR、MS鉴定分析为小檗碱,与天然植物提取分离的小檗碱具有相同的生理活性。