蝴蝶兰离体培养及其相关生物技术研究进展

对蝴蝶兰(Phalaenopsis)的离体培养、褐化及控制、物理化学诱变、转基因研究进展进行了综述,包括蝴蝶兰离体培养中的外植体选择、体细胞胚胎及类原球茎诱导、培养基及培养条件、培养方式、褐化控制等关键因素,并概括了生物反应器、转基因、诱变育种等相关生物技术研究进展。成体植株的花梗、茎尖和种子以及试管苗的叶片、茎尖、根尖等均可作为外植体;影响外植体褐化的主要因素有培养基的种类、pH值、温度、外植体的生理状况等;蝴蝶兰诱变育种及转基因研究尚处于初步阶段。     

蝴蝶兰叶片外植体褐变过程中PAL基因的表达变化

研究了蝴蝶兰(Phalaenopsis sp.)叶片外植体褐变过程中PAL基因表达的变化。结果表明,在整个褐变过程中,外植体的PAL基因表达出现差异,离体培养第3天的表达明显提高,一直到第8天还维持较高表达水平,以后随着外植体褐变的加重,PAL基因表达水平逐渐降低。与对照相比,在Fe盐浓度加倍为55.6 mg L-1培养基中培养的外植体PAL基因表达水平提高发生的时间比对照早,培养第2天就明显增强,随培养天数的延长,一直维持较高的表达水平;其PAL活性也高于对照,两种培养条件下,外植体总酚含量都随着其褐变加重而增加,说明PAL基因表达与蝴蝶兰外植体褐变过程相关。     

多酚氧化酶抑制剂对蝴蝶兰叶外植体褐变的影响

将多酚氧化酶(PPO)抑制剂添加到酶反应液中,抗坏血酸和半胱氨酸在0.5mmol/L就完全抑制蝴蝶兰PPO活性。300mg/L柠檬酸和100~200mg/L亚硫酸氢钠分别添加到培养基中,可使蝴蝶兰外植体褐变程度降低;采用抑制剂浸泡处理外植体,对外植体褐变抑制效果最好的为50mg/L抗坏血酸,外植体在褐变发生前PPO活性低于对照。     

几种培养基及光照对蝴蝶兰叶片外植体褐变的影响

蝴蝶兰叶片外植体在MS纸桥培养基上培养10 d发生褐变率较低,1/2 MS次之,MS、B₅和N₆培养基外植体褐变率最高。MS培养基中铁盐加倍或微量元素缺乏造成外植体严重褐变,培养基积累很多褐色物质;减少琼脂含量,外植体褐变加重;添加柠檬酸可减轻外植体褐变;而添加活性炭、抗坏血酸或PVP对减轻外植体褐变无显著作用。光照强度增加外植体褐变严重。     

组织培养法快速繁殖川乌头种苗

本研究探讨了川乌头组织培养过程中的外植体诱导建立无菌繁殖系;外植体生长分化和增殖培养基的筛选:生根及驯化移栽等关键技术环节,从而使川乌头通过组培快繁实现大规模育苗成为可能.     

芦荟组织培养研究进展(综述)

从外植体和培养基的选择、植物生长调节剂和添加物的使用、组培条件、褐化和玻璃化的控制等方面,综述近几年芦荟组织培养研究的进展,并对今后工作提出建议。     

百合(Lilium spp)的组培快速繁殖技术研究

用百合的鳞茎和根尖作为外植体进行组培快速繁殖实验:选用MS培养基为基本培养基,添加不同浓度的激素,接种后进行对照试验。结果表明:鳞茎在所有的外植体中愈伤组织的诱导率最高;百合鳞茎愈伤组织的最佳培养基为MS 6-BA 1.0mg/L NAA 0.5 mg/L。     

云南野生稻不同染色体组型和外植体材料的离体培养研究

云南野生稻不同外植体愈伤组织诱导能力差别较大。花粉培养中愈伤组织诱导率差异在0％～11．8％之间,用成熟胚诱导愈伤组织,其诱导率在18．0％～35．2％之间,茎叶培养则在12．0％～25．0％之间。云南野生稻不同外植体诱导的愈伤组织再分化为绿苗的分化率在8．3％～100．0％之间。疣粒稻组培特性最好,东乡普通野生稻和景洪普通野生稻次之,药用稻最难组培。本文建立了疣粒、东乡、景洪普野3种野生稻的离体无性系,为长期保存云南野生稻资源奠定了基础。     

霍山石斛(Dendrobidium huoshanness)的组织培养

霍山石斛(Dendrobidium huoshanness)是重要的药用植物,在组培过程中,其营养器官脱分化困难.本文研究了霍山石斛拟原球茎(PLBs)诱导的适宜条件,发现假鳞茎下段是诱导拟原球茎适宜的外植体,低浓度的NAA和CPPU的诱导效果较好,黑暗培养可缩短诱导时间,提高诱导率.     

霍山石斛(Dendrobidium huoshanness)的组织培养

霍山石斛(Dendrobidium huoshanness)是重要的药用植物,在组培过程中,其营养器官脱分化困难。本文研究了霍山石斛拟原球茎(PLBs)诱导的适宜条件,发现假鳞茎下段是诱导拟原球茎适宜的外植体,低浓度的NAA和CPPU的诱导效果较好,黑暗培养可缩短诱导时间,提高诱导率。     

二十世纪我国植物学家对植物组织培养的贡献

回顾了上一世纪我国植物组织培养的发展。 1934年以来 ,我国的植物组织培养研究一直与国际发展同步进行。我国学者在离体器官发生、茎尖培养、花药培养、子房培养、胚乳培养、原生质体培养和细胞大量培养等分支领域都取得重要进展。本文在引证我国研究者发表的植物组织培养论文的基础上 ,着重评述了那些被国际同行公认的研究成果。此外 ,还介绍了植物组织培养在我国农业和工业上应用的情况     

二十世纪我国植物学家对植物组织培养的贡献

回顾了上一世纪我国植物组织培养的发展.1934年以来,我国的植物组织培养研究一直与国际发展同步进行.我国学者在离体器官发生、茎尖培养、花药培养、子房培养、胚乳培养、原生质体培养和细胞大量培养等分支领域都取得重要进展.本文在引证我国研究者发表的植物组织培养论文的基础上,着重评述了那些被国际同行公认的研究成果.此外,还介绍了植物组织培养在我国农业和工业上应用的情况.     

禾本科植物的组织培养研究及其应用

禾本科植物是粮食作物的主要来源,随着人口的增加和生活水准的提高,人类对粮食的产量、种类和质量的需求也日益迫切。根据国外在1982年对90个发展中国家的统计和预测的结果说明到1990年末,这些国家共缺少72百万吨谷物而到2000年将缺少144百万吨谷物。近十余年以来,随着植物分子生物学的迅猛发展和作为植物生物技术重要组成部分的植物组织培养技术的日臻完善,被公认为非常困难从事的禾本科植物(Gramina-ceae)的组织培养也取得了异常迅速的发展,并且已经在作物改良的生产中取得了成效,显示了越来越大的潜能和威力,为人类从根本上解决食物问题指出了一条切实可行的途径。本文拟在评述近年来禾本利植物组织培养(主要指胚胎培养、器官培养、细胞培养和原生质体培养)的理论性研究和应用性研究的进展,并重点描述和讨沦在应用上较为成熟和有发展前景的几个领域的发展现状以及利用禾本科植物的组织培养技术而进行的基因转移技术的概况。希望能为我国从事植物组织培养的工作者们提供某些参考资料并对于一些问题进行共同的商榷和探讨。     

蕨类植物组织培养研究进展(综述)

蕨类植物组织培养可分为以孢子为外植体的无菌播种和以孢子体为外植体进行的组织培养.本文简要介绍国内外蕨类植物组织培养研究概况,综述培养基成份、培养方式及培养条件对组织培养过程中生长发育的影响,同时介绍蕨类植物组织培养中世代转换的诱导及调控.     

Expression of fetal antigens by normal human skin cells grown in tissue culture.

Normal human sera are capable of causing complement-mediated lysis of normal human skin cells grown in tissue culture. This lytic reactivity can be completely removed by absorption with first trimester fetal tissue. Absorption with a variety of normal adult human tissues including lymphocytes, decidua, skin, and muscle are incapable of absorbing reactivity. Absorption of reactivity by fetal tissue is specific and not due to the introduction of anti-complementary or other nonspecific factors, as evidenced by the inability of simultaneous fetal absorption to remove reactivity from antisera with specificity for HLA antigens. Similarly, absorption of lytic sera with fetal calf serum proteins was incapable of removing reactivity against normal cells in tissue culture. It thus appears that normal human cells in tissue culture express antigens shared by the first trimester human fetus, but not present on a variety of adult human tissues. This "neoantigen" present on normal human cells when grown in tissue culture is a potential source of confusion and must be accounted for in searching for human tumor-specific antigens utilizing tissue culture cells.     

Application of a multiple surface tissue culture propagator for the production of cell monolayers,virus, and biochemicals

A new concept of tissue culture equipment and procedures was developed for the mass-scale growth of several types of animal tissue cells in monolayers on multiple glass surfaces. Continuous, cell lines, primary and diploid cell strains were grown in this equipment. Cells studied include primary bovine kidney, human diploid WI-38, human foreskin, and mouse CCL1 cells. Photomicrographic comparisons of cells grown by these techniques indicate they are morphologically identical to tissue culture cells grown in glass bottles or tubes. The growth of the tissue culture cells in the propagator was monitored by carbohydrate Utilization and acid production. Large-scale production of viruses and biochemicals on cells grown in the multiple-plate tissue culture propagator was accomplished. Virus titers were equal to those obtained from conventional bottle or tube cultures for several strains of influenza, parainfluenza, and respiratory syneytial viruses. High-titred mouse interferon was also produced in this system. In addition to tissue culture cell production, Eaton agent, Mycoplasma pneumoniae was grown on the multiple glass surfaces on a mass scale.     

枣树组织培养研究进展

综述了枣树的器官培养、愈伤组织培养、花药培养、胚与胚乳培养、原生质体培养以及影响枣树组织培养的其他因素。营养器官培养报道的最多,其他外植体的培养相对较少,研究尚处于起步阶段。还针对枣树组织培养存在问题提出了今后的研究方向。     

荔枝生物技术研究进展（综述）

从荔枝的组织培养、花药培养和原生质体培养方面综述荔枝生物技术的研究概况,并提出该领域存在问题及发展方向。     

Possible roles for cell-to-substratum adhesion in neuronal morphogenesis

The role of cell-to-substratum adhesion in the initiation, elongation, and branching of axons from embryonic sensory neurons was investigated. Cells from sensory ganglia of 4–8-day-old chicken embryos were cultured on several substrata: including collagen; polyornithine-, polylysine-, and polyglutamate-coated surfaces, and tissue culture dishes. The air-blaster method was used to measure growth cone-substratum adhesion.Growth cones adhere much more strongly to polyornithine- or polylysine-coated surfaces and to the upper surfaces of glial cells than to tissue culture plastic. Axons, too, adhere tightly to these substrata, and are crooked, whereas on tissue culture plastic, axons are not adherent and are straight. The fraction of neurons that form axons and the rates of axonal elongation and branching are markedly increased when cells are cultured on polyornithine-coated dishes as compared to tissue culture dishes.This correlation of strong adhesion and enhanced neuronal morphogenesis suggests that adhesive interactions between the growth cone and the microenvironment in an embryo are crucial parts of the initiation and elongation of neuronal processes. Regulation of neuronal morphogenesis may be expressed through the physicochemical properties of the interacting cell surfaces and extracellular environment.     

Monolayer cell expansion conditions affect the chondrogenic potential of adipose-derived stem cells

Adipose-derived stem cells (ASCs) are an abundant, readily available population of multipotent progenitor cells that reside in adipose tissue. Isolated ASCs are typically expanded in monolayer on standard tissue culture plastic with a basal medium containing 10% fetal bovine serum. However, recent data suggest that altering the monolayer expansion conditions by using suspension culture plastic, adding growth factors to the medium, or adjusting the seeding density may affect the self-renewal rate, multipotency, and lineage-specific differentiation potential of the ASCs. We hypothesized that variation in any of these expansion conditions would influence the chondrogenic potential of ASCs. ASCs were isolated from human liposuction waste tissue and expanded through two passages with different tissue culture plastic, feed medium, and cell seeding densities. Once expanded, the cells were cast in an agarose gel and subjected to identical chondrogenic culture conditions for 7 days, at which point cell viability, radiolabel incorporation, and gene expression were measured. High rates of matrix synthesis upon chondrogenic induction were mostly associated with smaller cells, as indicated by cell width and area on tissue culture plastic, and it appears that expansion in a growth factor supplemented medium is important in maintaining this morphology. All end-point measures were highly dependent on the specific monolayer culture conditions. These results support the hypothesis that monolayer culture conditions may "prime" the cells or predispose them towards a specific phenotype and thus underscore the importance of early culture conditions in determining the growth and differentiation potential of ASCs.