人胸腺组织原代培养细胞与人类免疫缺陷病毒间的相互作用

背景:人类免疫缺陷病毒能够结合人胸腺的细胞CD4受体,从而导致CD4细胞活性降低。目的:观察人胚胎胸腺组织原代培养与人类免疫缺陷病毒相互作用关系。方法:取人胎胸腺组织进行原代细胞培养,取胸腺的细胞与人类免疫缺陷病毒1ⅢB混合培养设为实验组,设置不加人类免疫缺陷病毒培养的胸腺的细胞为对照组。结果与结论:透射电镜观察显示,培养40h,人类免疫缺陷病毒诱导的胸腺的细胞内即可发现大量艾滋病病毒颗粒。MTT法和免疫组织化学染色检测结果显示,培养40h^22d,HIV诱导胸腺的细胞吸光度值均显著低于对照组(r=0.9733,P<0.05),人类免疫缺陷病毒诱导胸腺的细胞膜上和细胞浆Fas-L阳性表达率均升高(P<0.05)。说明人类免疫缺陷病毒可致原代培养的人胚胎胸腺的细胞活性降低。

以异养细胞作为种子的椭圆小球藻产油脂光自养培养优化

异养细胞种子/光自养培养方法是一种可异养培养的能源微藻培养的有效方法,但已有文献尚未从工艺优化角度考察其发展潜力。为了获得较高细胞密度的用于光自养培养的种子和提高光自养培养的细胞密度与油脂产率,对异养细胞种子/光自养培养的培养基和培养条件进行了优化。结果表明,采用优化后的培养基,椭圆小球藻在摇瓶中异养培养的最高藻细胞密度可达11.04 g/L,比在初始培养基条件下提高了28.0%,在5 L发酵罐中异养培养的藻细胞密度达到73.89 g/L;在2 L柱式光生物反应器中光自养培养的藻细胞密度、油脂含量和油脂产率分别达1.62 g/L、36.34%和6.1 mg/(L·h),油脂成分主要为含C16-C18碳链的脂肪酸,是制备生物柴油的理想原料。经过优化,异养细胞种子/光自养培养这一方法能够显著地提高椭圆小球藻产油脂的能力,这进一步表明异养细胞种子/光自养培养方法有望成为可异养的能源微藻的高效培养方式。

原代肝细胞培养及其在药物代谢和毒理学研究中的应用进展

原代肝细胞培养技术已有四十几年的历史,随着技术水平的不断提高,其培养越来越成熟,并且已广泛用于研究药物对细胞色素P450酶的作用及其机制,药物相互作用,药物毒理学等多方面。因为其很好的维持和保留了肝脏的代谢能力,具有与体内一致的细胞色素P450酶的活性,成为日益重要和可信赖的评价药物和新化学实体的安全与有效的体外模型。该文对原代肝细胞培养技术及其在药物代谢和毒理学研究中的应用进展进行了综述。

健脾养胃方对人胃腺癌SGC7901细胞株的生长抑制和诱导凋亡作用的实验研究

目的:通过观察健脾养胃方对人胃腺癌SGC7901细胞株的生长抑制和诱导凋亡作用,探讨该方对人胃腺癌SGC7901细胞株生物学行为的影响。方法:通过四噻唑氮蓝(MTT)比色分析法,观察健脾养胃方对SGC7901细胞的增殖抑制作用;采用transwell小室法,研究健脾养胃方对SGC7901细胞侵袭力的影响;以Annexin-V/PI双染色,通过流式细胞仪,检测健脾养胃方对人胃腺癌SGC7901细胞凋亡的影响及其对细胞周期的影响。结果:健脾养胃方能抑制人胃腺癌SGC7901细胞增殖,以高剂量作用最为明显;健脾养胃方作用细胞24h后,肿瘤细胞侵袭力降低,高剂量组肿瘤细胞侵袭的细胞数最少;健脾养胃方作用细胞48h后可以诱导细胞凋亡;健脾养胃方可诱导SGC7901细胞G2/M期周期阻滞。结论:健脾养胃方对人胃腺癌SGC7901细胞株的生长抑制和诱导凋亡作用,是该方抑制胃癌细胞的重要机制。

滋养层细胞肿瘤P53蛋白的表达及其意义

目的：探讨P53蛋白在滋养层细胞肿瘤发生发展的作用。方法：用免疫组化LSAB法观察P53蛋白在绒毛膜癌、侵袭性葡萄胎及葡萄胎组织中的表达。结果：P53在56例良性葡萄胎、51例侵袭性葡萄胎和47例绒毛膜癌中均有过表达，且后两者明显高于前者（P＜0．01）。还发现29例具有恶变潜能的葡萄胎其P53蛋白的表达明显高于未发生恶变者（P＜0．05）。结论：提示P53蛋白的过表达与滋养层细胞肿瘤的增殖有一定意义，可作为判断良性肿瘤恶性变及鉴别良恶性肿瘤的指标之一，从基因水平推测P53基因在良性葡萄胎恶性变、绒毛膜癌及侵袭性葡萄胎发生发展中起重要作用。

光合细菌对养殖水体的生态调控作用

本文报道了养殖池施用光合细菌后，水中异养细菌、弧菌、发光细菌和光合细菌的消长情况，研究了它们的相互关系。结果表明，添加光合菌后，池水中光合细菌数量增加而弧菌和发光菌数量减少，表明了光合细菌具有调节养殖环境做生态系的作用。

海水网箱养殖水域异养细菌和弧菌的数量动态

1996年4月至1997年5月对浙江奉化、象山海水网箱养殖水域采用MPN法进行异养细菌和弧菌数量的检测。结果表明,细菌数量的变化受外界环境的影响较为明显,7～9月份细菌数量明显高于其它月份,网箱内菌数高于网箱外菌数。从异养细菌和弧菌数量的周年变化看,细菌数量变化与网箱养殖鱼类疾病的发生有密切关系。菌数的高峰期也是鱼病的频繁发生期。利用检测养殖水域异养细菌和弧菌的数量可预测鱼病的发生。

高密度温室与室外养鳖池中微生态环境的研究

对高密度温室养鳖池、室外发病和健康鳖池的理化指标、细菌数量、细菌种类、种群组成及溶血菌比例进行了研究 结果表明 ,溶氧量、氨氮值、COD值等指标 ,室外养鳖池优于高密度温室养鳖池 高密度温室养鳖池中共分离出 8个属的异养细菌 ,优势菌为气单胞菌属 ,在一个换水周期 (8d)中异养细菌数量由 2 5× 10 3个 /mL上升至 1 3× 10 5 个 /mL ,菌群逐渐单一化 ;室外发病鳖池共分离出 7个属的异养细菌 ,优势菌为气单胞菌属 ,异养细菌数量为 7 3× 10 3个 /mL ,而室外健康鳖池共分离出 8个属的异养细菌 ,优势菌为假单胞菌属 ,异养细菌数量为 8 3× 10 2 个

人体恶性肿瘤细胞体外抗癌药物敏感试验

用人癌细胞短期培养,以染料排除法(DEA),对21例恶性肿瘤患者的肿瘤细胞作体外抗癌药物敏感试验.结果能直观地反映出各类肿瘤细胞对化疗药物的作用特性.卵巢癌对DDP敏感占82%;MMC占36%;CTX占27%;TsPA占25%;对5-Fu89%不敏感.

蓖麻油甾醇组成及其对大鼠蜕膜细胞的影响

目的进一步探明蓖麻油中的抗生育物质成分。方法利用皂化和萃取,从蓖麻油中提取甾醇,用GC-MS分析蓖麻油甾醇成分;用MTT法检测蓖麻油甾醇对原代培养大鼠蜕膜细胞活力的影响。结果蓖麻油总甾醇的主要成分为γ-谷甾醇(43.02%)、豆甾醇(27.15%)、岩藻甾醇(11.43%)、麦角甾-5-稀-3-醇(6.00%)和普罗布考(7.46%)。蓖麻油甾醇对细胞活力有抑制作用,其半抑制剂(IC50)剂量为:(88.45±3.196)μg/ml,r=+0.9549;抑制作用具有量-效关系。结论在蓖麻油甾醇的主要成分中,γ-谷甾醇(r-Sitosterol)可能是抑制原代培养大鼠蜕膜细胞活力的主要成分,而豆甾醇(stigmasterol)可能起协助的作用。

Aurora-A激酶在人类肺癌细胞株中的表达

目的:探讨aurora -A基因在正常肺组织与不同肺癌细胞中的表达。方法:采用半定量RT- PCR、Western blot方法,检测Aurora- A在高转移的肺癌细胞PG、肺腺癌细胞A549、大细胞肺癌细胞NCI H460 三种肺癌细胞株的表达情况结果:RT -PCR结果显示,三种肺癌细胞与正常肺组织比较aurora -A mRNA均高表达,经图象分析,PG、A549、NCI H460 与正常肺组织中aurora A/βactin比值分别为1 14、1 16、0 84 和0 26Western blot结果经图象分析发现, A549、NCI H460 与PG 的aurora A/βactin 比值分别为21 .13、6 .43 与8 .96。三者比较,A549 最高, PG其次, NCI H460最低。结论:aurora -A在三种肺癌细胞中其mRNA及蛋白水平均呈高表达,不同细胞株其表达水平不同。aurora -A基因在肺癌细胞中高表达的结果提示,作为一种新的癌基因,aurora- A有可能成为肺癌新的肿瘤标记物及分子治疗靶点。

农杆菌介导的高羊茅高效遗传转化和转基因植株再生(英文)

用带有质粒pDBA121(含hpt基因和bar基因)的农杆菌EHA 105转化高羊茅(Festucaarundinacea Schreb.)胚性悬浮细胞,建立了可重复的、高效的农杆菌介导的高羊茅遗传转化系统.商业用的除草剂Basta直接用于转化细胞的筛选.基因型、受体材料的类型、培养基成分和筛选剂影响农杆菌介导的转化频率.悬浮细胞的农杆菌转化效率为每克悬浮细胞再生2.85～10.9株转基因植株,大大高于基因枪法的高羊茅转化效率(2～5株).经PCR分析和Southern杂交检测表明,bar基因已整合进入高羊茅基因组,转基因植株Basta喷洒试验表明bar基因已成功地实现高水平的表达.此转化系统的建立为高效地将外源有用基因导入高羊茅并高效稳定地表达奠定了基础.

Biotransformation of Gastrodin by Cell Suspension Cultures of Catharanthus roseus

应用长春花 (Catharanthusroseus (L .)G .Don)悬浮细胞培养体系对天麻素进行了生物转化反应研究。经过8d培养形成一个转化产物 ,应用光谱方法鉴定转化产物的结构为对羟基苯甲醇 ,为天麻素水解后形成的甙元。

Chemical Constituents of the Suspension Cell Cultures of Maytenus hookeri

Suspension cell cultures of Maytenus hookeri Loos. (Celastraceae) in SH media were established from the calli induced from the leaves and young steins of M. hookeri on MS media with the supplement of 2 mg/L 2,4-D and 0.1 mg/L KIN (kinetin). Ethyl acetate extract of the cultures showed inhibitory activities against Penicillium avellaneum UC-4376 which was sensitive to maytansinoids. Exhaustive isolation of natural products from a large scale of suspension cell cultures did not yield maytansine instead of affording nine compounds including one novel triterpenoid, named 2, 3-diacetoxyl maytenusone (1), and eight known ones including squalene (2), beta-sitosterol (3), 2', 3', 4-triacetyl-sitoindoside I (4), salaspermic acid (5), maytenonic acid (6), 2alpha-hydroxy-maytenonic acid (7), 6, 11,12-trihydroxy-8, 11, 13-abietrien-7-one (8) and 11, 12-dihydroxy-8, 11, 13-abietatrien-7-one (9) elucidated on the basis of 1D and 2D NMR data. The H-1-NMR and C-13-NMR assignments were made for 1, 5, 6 and 7, while the C-13-NMR assignments for 5 and 6 were revised. The chemical results suggested that the suspension cell cultures of M. hookeri did not produce maytansinoids under the reported experiment conditions.

Growth Differentiation Factor-9 Gene Expression of Mice Oocytes in Vitro and in Vivo

Mice preantral follicles were cultured in vitro for 12 days to achieve metaphase Ⅱ （M Ⅱ ） oocytes. Oocyte growth differentiation factor-9 （GDF-9） gene expression was measured during different growth stages to explore the relationship between oocyte maturation and GDF-9 gene expression. Preantral follicles of lO-day old mice were isolated from the ovaries and were cultured for 12 days. Oocytes from day 2 （D2）, D4, D6, D8, DIO, D12 cultured in vitro were named the in vitro group and oocytes of day 12 （D12）, D14, D16, D18, D20, D22 grown in vivo were named the in vivo group. Follicle survival, antrum formation and maturation rate were 89.5%, 51.8% and 56.6% respectively in follicles cultured in vitro. After RT-PCR and agarose gel electrophoresis, relative mRNA abundance of GDF-9 was measured in each group of oocytes. At day 8 - 12, the GDF-9 gene expression level of oocytes in vitro was significantly lower than that in vivo （P 〈 0.05）. We conclude that M Ⅱ oocytes can be obtained from in vitro culture of preantral follicles. The GDF- 9 gene expression of oocytes varies at different growth stages in vivo. The low expression of GDF-9 in oocytes cuhured in vitro may be the cause of their low developmental capacity.

Sugarcane Callus Culture and Cytological Characteristics

In order to obtain sugarcane embryogenic calli for transgenosis, the effects of different soaking time of explants, medium, culture conditions and sampling time on sugarcane callus culture were investigated. The results showed that soaking ex- plants with MS liquid medium for 20 min could significantly reduce the browning rate; MS＋3.0 mg/L 2.4-D was appropriate for induction and proliferation of embryo- genic calli; dark condition was suitable for the culture of sugarcane calli; calli differ- entiated from materials collected in August exhibited low browning rate, high callus induction rate and high embryogenic callus induction rate. Calli with different pheno- types were stained, prepared into slides and observed under a microscope to ana- lyze the cytological characteristics. The resultsshowed that milky-white granular em- bryogenic calli had closely arranged cells with large nucleus and exhibited strong differentiation capacity, which were appropriate receptor materials for genetic trans- formation of sugarcane.

ULTRASTRUCTURE OF THE VEGETATIVE CELLS OF NOSTOC FLAGELLIFORME PREPARED WITH HIGH PRESSURE FREEZING AND FREEZE SUBSTITUTION TECHNIQUE

The ultrastructure of the vegetative cells of Nostoc flagelliforme Born. et Flah. was investigated with high pressure freezing and freeze substitution technique and compared with the results obtained by using conventional preparation methods. During the processes of chemical fixation, dehydration and embedding, the cell structures might be more artificially modified than that obtained from high pressure freezing and freeze substitution. With the present method, the sheath of N. flagelliforme could be well penetrated and no extra big space could exist between the cell and the sheath. The cell protoplasm rarely shrinked. Some fine structures of cell inclusions and unit membranes became visualized. Many bacteria were harbored in the sheath. In addition, the presence of big vacuoles in the cell of N. flagelliforme as well as the presence of bacteria in the sheath shown in the present preparation for cyanobacteria has not been described so far in the literature.

苏联中学生物学教学改革动态

苏联从1986—87学年度起,按新的教学大纲进行中学生物学教学。苏联新的生物学教学大纲有着一系列特点,其中之一是将生物学作为一门课程而开设。这样在苏联中学里就不再有植物学、动物学、人体生理卫生学等课程。生物学由以下五个部分组成:植物(五—七年级)、细菌、真菌和地衣(七年级)、动物(七到八年级)、人体及其保健(九年级)、普通生物学(十到十一年级)。

体内外急性酒精性肝损伤模型的研究

目的:建立体内外急性酒精性肝损伤模型,为进一步研究药物对肝损伤的保护作用奠定基础。方法:测定乙醇的半数致死量,观察不同给药途径不同剂量下血清丙氨酸氨基转移酶(ALT)、门冬氨酸氨基转移酶(AST)活性变化。利用乙醇体外诱导原代培养的肝细胞损伤,检测不同时间和剂量下培养液上清乳酸脱氢酶(LDH)释放量。结果:小鼠灌胃乙醇的半数致死量为9．98 g·kg-1,乙醇灌胃剂量大于6．4 g·kg-1、腹腔注射剂量大于4．0 g·kg-1时,血清ALT、AST有升高趋势。50-400 mmol·L-1乙醇作用于大鼠肝细胞,培养液上清中LDH释放量有增加趋势。结论:体内、体外急性酒精性肝损伤的最适损伤剂量分别为7．2 g·kg-1和50～100 mmol·L-1。