饲养层细胞对绵羊胚胎干细胞体外培养的影响

家畜胚胎干细胞(embryonic stem cell,ES细胞)的研究进展缓慢,绵羊ES细胞的研究虽早有报道,但仍未建立可稳定传代的细胞系。在已建立的绵羊体外受精发育体系的基础上,摸索了饲养层(Feeder)细胞对绵羊ES细胞生长的影响,包括在一定的丝裂霉素浓度下处理Feeder的时间、细胞种类、代数、接种密度及新鲜制备和冷冻复苏后的Feeder细胞,通过试验比较研究,目的在于筛选合适的饲养层细胞,为建立绵羊ES细胞体外培养体系奠定基础。结果表明,10μg/ml丝裂霉素C处理2~2.5h获得的1~5代的SEF和1~3代的MEF及两者的1∶1混合细胞都能较好地支持绵羊ES细胞的生长。     

植物苯丙氨酸解氨酶(PAL)在细胞分化中的作用

烟草、丹参和甜叶菊愈伤组织在分化过程中一般都出现两个PAL活性高峰。第一高峰在培养第一、二、三天中出现;第二高峰在第十一天前后出现。前者在分化或不分化培养基中都存在,似与组织分化无关,后者只在分化条件下才有,似可作为组织启动分化的指示酶。分化程度不同的组织,PAL活性有很大差异,即将或刚分化的组织活性最高,随着分化的进程活性趋于降低,老化的组织甚至丧失活性。PAL活性、木质素合成和管状份子形成之间有着紧密的相关性。     

小麦—天兰偃麦草—黑麦三属杂种花粉植株诱导条件的研究

研究表明,三属杂种处于单核中晚期阶段的花粉最适于诱导形成愈伤组织。低温预处理对促进三属杂种花粉愈伤组织的诱导有一定的作用。利用以马铃薯提取物为基础物质的马铃薯-Ⅱ培养基作诱导培养基,其愈伤组织诱导与分化的频率比目前两个较好的合成培养基要高。同一个三属杂种F_1春、秋播种植株之间在形成愈伤组织的能力上有较大的差异,秋播材料形成愈伤组织的能力明显高于春播材料。F_(?)杂种植株诱导愈伤组织和分化植株的频率均比F_1杂种明显提高。     

细毛樟愈伤组织培养

从富含香叶醇的细毛樟（ＣｉｎｎａｍｏｍｕｍｔｅｎｕｉｐｉｌｕｍＫｏｓｔｅｒｍ）叶片外植体诱导出愈伤组织。愈伤组织生长较合适的培养基为ｐＨ５．８附加ＩＡＡ２ｍｇ／Ｌ和ＫＴ０１ｍｇ／Ｌ的ＭＳ培养基,在２５℃下暗培养。愈伤组织无性系继代培养到第６代后芳香成分初步分析结果表明主成分仍为香叶醇。     

Rhododendrol biosynthesis and metabolism in Acer nikoense callus

Cell suspensions derived from Acer nikoense callus, not containing (S)-rhododendrol, converted 4-(p-hydroxyphenyl)-2- butanone into (R)-, (S)-rhododendrol and their glycosides. (R)- and (S)-rhododendrol formed was only detected in the culture medium and their glycosides only in the cells. The former compound disappeared within a short time and the latter one also tended to decrease during prolonged culture. Quantitative analysis of rhododendrol glycosides in the callus showed that most of them were (S)-rhododendrol 2-O--D-glucopyranoside and its content was much lower than that of the original plants. © Rapid Science Ltd. 1998     

Improved Culture Media for Embryogenic Callus Generation in Sorghum [<i>Sorghum bicolor</i> (L.) Moench]

Many attempts on optimization of sorghum [Sorghum bicolor (L.) Moench] tissue culture induction media have been made, but the culture system remains with some bottlenecks compared to that of other crops. This study aimed at assessing the suitability of various induction media to produce embryogenic callus (yellow and friable) with high induction rates and reduced phenolic exudation. The six culture medium modifications: 3 based on Murashige and Skoog (MS) medium and one each based on Chu N6, Gamborg B5 and 190-2 media respectively were applied in the culture of mature embryos from 10 sorghum genotypes. Although there was a genotype influence on the attainment of a yellow callus, friability of the callus was determined to be dependent on the culture medium and not the genotype. Half strength MS medium with 0.2 mg/l 2,4-D with 2.8 g/l Gelrite® as the gelling agent modified with 1.0 g/l KH₂PO₄, 1.0 g/l L-proline, 1.0 g/l L-asparagine and 0.16 mg/l CuSO₄·5H₂O (type E) was found to be the most effective resulting in about 60% yellow coloured callus induction with 25% friability. Addition of CuSO₄·5H₂O, KH₂PO₄, L-proline and L-asparagine significantly reduced the phenolic production. Half strength MS medium was observed to contribute to quality callus production when compared to full strength MS media modified with the compounds. The half strength MS medium was also observed to suppress phenolic production. Medium 190-2 produced the highest regeneration frequency (40%) among the 3-regeneration media tested. The results provide information on a suitable sorghum callus induction medium necessary for embryogenesis.     

亚麻胚性细胞悬浮培养体系的建立和影响因素

亚麻品种‘双亚五号’的胚性愈伤组织诱导最佳培养基为MB（MS无机盐加B5维生素）＋1.0mg·L^-12,4-D;细胞初始悬浮培养的最佳培养基为MB＋0.2mg·L-16-BA;细胞继代悬浮培养的最佳培养基为改良的MB（NH4NO3减半,KNO3加倍）＋0.02mg·L^-12,4-D＋0.2mg·L^-16-BA;适宜的蔗糖量为50g·L^-1;适宜的继代接种量为1.0～1.5g·（25mL）^-1;继代间隔为5～7d。     

Rationally optimized cryopreservation of multiple mouse embryonic stem cell lines: I—Comparative fundamental cryobiology of multiple mouse embryonic stem cell lines and the implications for embryonic stem cell cryopreservation protocols

The post-thaw recovery of mouse embryonic stem cells (mESCs) is often assumed to be adequate with current methods. However as this publication will show, this recovery of viable cells actually varies significantly by genetic background. Therefore there is a need to improve the efficiency and reduce the variability of current mESC cryopreservation methods. To address this need, we employed the principles of fundamental cryobiology to improve the cryopreservation protocol of four mESC lines from different genetic backgrounds (BALB/c, CBA, FVB, and 129R1 mESCs) through a comparative study characterizing the membrane permeability characteristics and membrane integrity osmotic tolerance limits of each cell line. In the companion paper, these values were used to predict optimal cryoprotectants, cooling rates, warming rates, and plunge temperatures, and then these predicted optimal protocols were validated against standard freezing protocols.