人参皂苷F1转化菌株的原生质体诱变育种

菌核青霉2246(Penicillium sclerotiorum)能够将人参皂苷Rg1转化为人参皂苷F1.以此菌为出发菌株,进行原生质体制备和再生的研究,确定原生质体的最佳形成条件:菌丝体培养24 h,用5 mg/mL溶壁酶、5mg/mL纤维素酶和5 mg/mL蜗牛酶的混合酶液进行酶解,以0.8 mol/L的KCI作为渗透压稳定剂,31℃水浴振摇2h.并对形成的原生质体进行亚硝基胍复合紫外线照射诱变,结果得到1株转化率显著提高、遗传性能稳定的诱变株( NU-1),其转化率由16.7％提高到30.5％.     

人参大片段DNA(100kb)转化灵芝的研究

为探讨人参大片段DNA转化灵芝的可能性,通过电击法将双元细菌人工染色体(BIBAC)载体上的100kb人参大片段DNA转化到灵芝原生质体内。研究发现,在电极间距为4mm,电压强度为240V时,将5μL的人参大片段DNA转化到75μL的灵芝原生质体,在选择培养基上获得了具有再生能力的转化子。根据克隆载体两侧的序列设计两对引物,对转化子进行PCR分析。试验结果表明人参大片段DNA已经转化到灵芝的基因组中。     

原生质体培养在芸薹属蔬菜作物中的研究进展

原生质体是遗传转化的优良受体。在原生质体培养过程中会产生很多无性系变异,还可以产生体细胞杂种,这些都为蔬菜育种提供了新的途径。介绍了原生质体培养及原生质体融合方法的研究进展,综述了原生质体培养在芸薹属蔬菜育种中所取得的研究成果,并对今后研究的方向进行了展望。     

影响谷子原生质体看护培养的一些因素

研究了谷子原生质体看护培养中的一些问题。结果表明：不同种植物愈伤组织做看护细胞对谷子原生质体培养植板率有不同的影响。用光头种草愈伤组织对谷子胚性、非胚性或中间型意伤组织的原生质体进行看护培养,以对胚性意伤组织原生质体的效果最好。看护培养主要是作用于原生质体形成完整细胞后的生长发育。试验没有观察到明显的看护细胞数量效应。     

木本植物的原生质体培养

木本植物的原生质体培养对于将生物技术应用于树木品种改良的研究具有重要意义,但难度较大。本文概述了近年来木本植物原生质体培养的进展,并针对木本植物原生质体培养过程中的问题进行了较详细的讨论。     

从棉花胚性细胞原生质体培养获得植株再生

原生质体培养植株再生是进行体细胞杂交与基因工程操作的重要基础工作。近年来,国内外已有一些关于棉花原生质体分离与培养的研究报告,1986年 Firoozabady 报道从陆地棉(Ghirsutum)叶肉原生质体培养获得2—3个细胞的微克隆,1987年 Ka~-     

影响谷子原生质体看护培养的一些因素

研究了谷子原生质体看护培养中一些问题。结果表明：不同种植物愈伤组织做看护细胞对谷子原生质体培养植板率有不同的影响。用光头稗草愈伤组织对谷子胚性、非胚性或中间型愈伤组织的原生质体进行看护培养,以对胚性愈伤组织原生质体的效果最好。看护培养主要是作用于原生质体形成完整细胞后的生长发育,试验没有观察到明显的看护细胞数量效应。     

不同培养条件对拟南芥根细胞膜片钳记录的影响

本文以沙培养法、蛭石培养法、土培养法、水培养法和MS培养基等不同的方法培养拟南芥(Arabidopsis thaliana),分析了不同培养方法对根生长发育的影响,并分别分离根的原生质体。在膜片钳记录中对不同来源的根原生质体状态进行了比较。结果表明,土培养法分离的原生质体最适于膜片钳记录。     

马铃薯实生苗子叶及下胚轴原生质体培养研究

用马铃薯普通栽培种（Ｓｏｌａｎｕｍ ｔｕｂｅｒｏｓｕｍ Ｌ．）３ 个品系的实生苗刚展开的子叶及下胚轴游离和培养原生质体。实验结果表明,子叶及下胚轴原生质体的分裂频率显著地高于经多次继代繁殖的试管苗顶部幼嫩叶片和茎尖的原生质体;在强连续光照下培养的实生苗,其原生质体的产量和质量都显著地高于弱光下培养的;在完全黑暗下培养的黄化实生苗不能游离出完整的原生质体;酶解前对子叶及下胚轴切段在酶液中进行真空渗透处理能显著地提高原生质体的产量,但此种处理对试管苗叶片无明显效果;下胚轴原生质体的产量显著地高于子叶,但在原生质体的质量方面,这两种组织间无明显的差异     

影响决明无菌苗子叶原生质体分离和培养因素的研究

以决明(Cassia obtusi folia)无菌苗子叶为材料,对酶组合、无菌苗日龄,植物激素组合和培养方法对其原生质体的分离和培养的影响进行了研究。结果表明:用3％的纤维素酶和0.2％Pectinase Y-23的酶组合处理决明无菌苗子叶块8小时可以高效分离出有活力的原生质体;约14日龄的决明无菌苗子叶比较适合于原生质体的分离;适当浓度的2,4-D 有利于原生质体的分离。促进原生质体分裂的理想的植物激素组合为0.4 mg/L 2,4-D,1.0 mg/L NAA and 0.1 mg/L KT;漂浮培养法最有利于原生质体的分裂和发育。找出了适合于决明无菌苗子叶原生质体的分离和培养的酶组合、植物激索组合、有效培养方法和决明无菌苗子叶日龄。这为有效地从决明无菌苗子叶原生质体再生植株奠定了基础。     

草木樨状黄芪单细胞培养再生植株及其影响因素的研究

从草木樨状黄芪的子叶和胚轴诱导的愈伤组织中选取结构松脆的颗粒状愈伤组织,用液体培养基Ｓ１２进行悬浮培养建立了悬浮细胞。取换液３天左右生长旺盛的悬浮系材料分离单细胞,用基本培养基Ｓ１２与不同浓度的植物血球凝集素组成的系列培养基ＭＣ１－ＭＣ６进行液体浅层静置暗培养;形成小愈伤组织后,经Ｍ３（ＭＳ＋２,４－Ｄ ２ｍｇ／Ｌ,ＮＡＡ ０．２ｍｇ／Ｌ,ＫＴ １ｍｇ／Ｌ）培养基增殖,ＭＲ２培养基诱导分化出苗,再     

Separate actions of different colony stimulating factors from human placental conditioned medium on human hemopoietic progenitor cell survival and proliferation

More than 20% of human granulocyte-macrophage and eosinophil colony-forming cells survived in agar culture for up to 4 days without the addition of exogenous colony stimulating factors (human placental-conditioned medium, HPCM). Survival was reduced slightly but not significantly, by the removal of adherent cell populations. Significant survival occurred even when only 100 cells enriched for colony-forming cells (CFCs) were cultured per dish. When individual colonies, initiated by stimulation with HPCM for 5 days, were transferred to dishes without HPCM, subsequent proliferation was significantly reduced compared with control cultures containing HPCM. Using the fluorescence-activated cell sorter and the fluoresceinated lectin from Lotus tetragonolobus, two populations of marrow cells were obtained, one enriched for day 7 and the other for day 14 colony-forming cells. Two colony-stimulating factors fractionated from HPLCM (CSF^β and CSF^α) have been shown previously to stimulate the day 7 and day 14 colony-forming cell populations, respectively. Developing clones from cultures initiated with CSFβ died between the fifth and tenth day of culture after transfer to dishes with CSFα or CSFβ or to dishes with no stimulus. Cells in clusters initiated with CSFα proliferated significantly between the fifth and tenth day of culture when transfered to CSFα or CSFβ but not when transfered to dishes with not stimulus. These studies provide further evidence for the existence of two subtypes of human granulocyte-macrophage progenitor cells each under the primary control of a specific regulator and indicate that these two regulators can both act on some developing clones of cells.     

Glio-neuronal aggregates in collagen gel: a model for studying the factors affecting development of central nervous system cells

Glio-neuronal aggregates of dissociated cells obtained from embryonic brain during cultivation in rotating flasks were transfered for further cultivation into collagen gel, containing balanced salt solution, serum-free amino acid medium, or complete nutrient medium. Active neurite growth and glial cell migration were observed during cultivation in collagen gel. The experiments have shown that glio-neuronal aggregates may serve as an experimental model for testing the activity of different neuronotrophic and neurite growth stimulating factors.     

Callus Induction And Triploid Plant Regeneration From Endosprm of ‘Hongjiang’ Sweet Orange

Endosperm at late stage of cell formation, excised from open-pollinated fruit of sweet orange (Citrus sinensis Osbeck. cv.‘Hongjiang’), was suitable for culture in vitro. The results indicated that 2,4-D was necessary for callus' induction, and supplemented with BA, CH in medium was more effective: the percentage of induction was as high as 33.3%. Endosperm tissues, excised from the fruits treated with low temperature (4–7℃) for 16 and 19 days, and from the young seeds precuhured on MT basal medium respectively with NAA, GA3, BA for 2–6 days, also stimulated to callus formation. When endosperm callus was transfered to the differentiation medium, embryoids and shoot-buds only developed in a sequence of culture conditions. Callus was first cultured on MT+BA/GA3, then transfered to different media with various nitrogen or hormone concentration, and finally transferred back to the first culture medium. Shoots were regenerated from shoot-buds in the medium in presence of hormones with only BA or with GA3. The whole plants were regenerated from embryoids in presence of GA3 or with BA. Analysis of endosperm plantlets showed that 79.4% of the observed celld have chromosome number of 2n=26–27, nearly the triploid number of 2n=3x=27. Through grafting on lemon seedlings as rootstocks in vitro, plantlets were growing successfully in soil.     

In vitro multiplication in liquid culture of Syngonium contaminated with Bacillus spp. and Rathayibacter tritici

Contaminated Syngonium clusters were multiplied in an air lift bioreactor in liquid medium containing sucrose with the medium being circulated through a sterilizing filter. After 30 days, the culture in filtered medium produced 19.5 shoot initials per gram fresh weight of inoculum compared to 8.7 shoot initials produced in unfiltered medium. Transfer to an elongation medium with 30 mg l^-1 Rifampicin produced shoots on 67% of the clusters, while transfer to elongation medium without Rifampicin poduced shoots on 40% of the clusters. Clusters grown for three subcultures in a reactor without medium filtration had lost their multiplication ability. Clusters grown for three subcultures in a reactor with filtration, however, continued to show a two-three fold increase in fresh weight and shoot production.Abbreviations MS Murashige and Skoog     

Plant Regeneration from Protoplasts of Peucedanum Terebinthaceum (Fisch.) Fisch. ex Turcz

Calll with many embryogenic cell colonies were produced from segments of seedlling of Peucedanum terebinthaceum (Fisch.) Fisch. ex Turcz. which were cultured on the 1/2MS agar medium (with half quantity of macronutrients) containing 1 mg/l 2,4-D. Cell suspension culture with high percentage of embryogenic cell colonies was established from the calli shaking in liquid medium. The cell suspension culture was used for protoplast preparation. Protoplasts were obtained with the enzyme mixture containing 1.5% Onozuka R-10, 0.3% Macerozyme R-10, 0.5% Snailase, 5 mmol/l CeCl2, 1 mmol/l KH2PO4, 0.6 mol/l mannital at pH 5.8 and 25℃. Cultured in a modified MS liquid medium containing 1 mg/l 2,4-D+ 0.5 mg/l zeatin, the protoplasts emered division after four days, and formed cell colonies of 0.5–1mm after about forty days. When transfered to 1/2 MS liquid medium supplemented with zeatin (0.5 mg/l), the cell colonies differentiated in to embryoids, then developed into plantlets with many green leaves and roots on the 1/2 MS agar medium devoid of phytohormones.     

黄槐叶片培养过程中器官发生的研究

以黄槐（ＣａｓｓｉａｓｕｒａｔｔｅｎｓｉｓＢｕｒｍ．ｆ．）幼嫩叶片为材料,接种于ＭＳ＋ＮＡＡ１ｐｐｍ＋２,４－Ｄ１ｐｐｍ＋６－ＢＡ２ｐｐｍ的培养基上,诱导形成两种形态的愈伤组织,即致密愈伤组织与雪花状愈伤组织．将愈伤组织转移到ＭＳ＋ＮＡＡ：１ｐｐｍ＋６－ＢＡ２ｐｐｍ的分化培养基上．仅致密型愈伤组织经过球状体至不定芽途径形成大量再生植株。扫描电镜及组织细胞学观察表明,致密愈伤组织表层细胞排列紧密,有许多分生细胞团,而雪花状愈伤组织表层细胞薄壁化,分裂能力很低。球状体起源于致密愈伤组织表层的分生细胞团,其细胞有极强的分生能力,顶端可以分化发育成不定芽原基,最后形成不定芽并发育成小植株。球状体可以看成是具有形成不定芽能力的繁殖单位．     

鹤望兰组织培养与工厂化快繁程序的研究

将材料接种于诱导愈伤组织手芽的培养基上,培养２个月后,胚芽外植体下出现白色颗粒状的愈伤组织,４个月后愈伤组织上出现小芽丛。将小芽丛转入不加植物激素的ＭＳ培养基上,芽的生长加快,２个月左右可长成３－６ｃｍ高的丛小植株。将小植株切下,插入根培养基中,一般３５ｄ左右基部突出很小的白色根尖。     

Selection and microculture of single embryogenic cell clusters in japanese conifers: Picea jezoensis, Larix leptolepis and Cryptomeria japonica

Summary A microculture method for single embryogenic cell clusters was established for several Japanese conifer species, namely Picea jezoensis, Larix leptolepis and Cryptomeria japonica. Individual small, dense cell clusters were identified and picked up by a micromanipulator and cultured in 50 μl liquid medium in a 96-well culture plate. In all three species studied, a majority of the cell clusters actively proliferated within the wells. Maturation of somatic embryos was successful when the newly proliferated cell clusters were transferred to solid abscisic acid-containing medium. Thus, the small, dense cell clusters could be a useful morphological marker for cells capable of proliferation and differentiation.     

SOMATIC EMBRYOGENESIS AND PLANT REGENERATION FROM IMMATURE ZYGOTIC EMBRYOS OF MUSCADINE GRAPE (VITIS ROTUNDIFOLIA) CULTIVARS

Embryogenic cell lines of Vitis rotundifolia were produced from immature zygotic embryo explants obtained by culturing ovules, harvested at 20 d postanthesis, for 8 wk and then dissecting embryos from them. Ovules cultured on Nitsch and Nitsch medium with naphthoxyacetic acid and benzyladenine (BA) produced a brown exudate, necessitating three transfers to fresh medium at 2-wk intervals during the 8-wk culture cycle. Zygotic embryos that were subsequently isolated from cultured ovules and placed on the same medium produced a heterogenous callus from which eventually emerged embryogenic cell lines. A higher percentage of ovules from cultivars ‘Dixie’, ‘Fry’, ‘Nesbitt’, and ‘Welder’ produced zygotic embryos (31%–39%) than did those from ‘Carlos’ (3%). A higher percentage of ‘Fry’ ovules produced embryogenic lines from cultured zygotic embryos (6.3%) than did those of the other four cultivars (1%–1.6%). Embryogenic cell lines were white and composed of variably sized cell clusters, somatic embryos, and embryonic tissue embedded in a watery matrix. These lines were maintained for over 1 yr on modified Murashige and Skoog (MS) medium lacking growth regulators by transfer of selected cell clusters every 6 wk. White, opaque somatic embryos grew directly from cell clusters and passed through recognizable developmental stages. Germination was induced by transfer of somatic embryos to MS medium with BA. Although 80%–100% of embryos germinated, plant recovery was low due to poor shoot development.