通过体内基因转染改变Meis1在围着床期小鼠子宫中的表达影响胚胎着床

通过宫腔内脂质体转染改变小鼠子宫内Meis1基因的表达水平,研究其对子宫内膜容 受性的影响,从而推测Meis1基因在胚胎着床中的作用.选择8～12周龄昆明小鼠,于妊娠 第2 ｄ,通过向小鼠宫腔内注入Meis1基因表达质粒和siRNA表达质粒及其各自的对照质粒 ,在妊娠第5ｄ, 提取小鼠子宫mRNA 和蛋白质行半定量RT-PCR 和免疫组化分析,观察各组小鼠子宫内膜Meis1和整合素β3的表达变化.在妊娠第9 ｄ,观察Meis1基因上调组及其对 照组、Meis1基因下调及其对照组妊娠率和胚胎着床数的差异.结果显示,Meis1基因下调组胚胎着床率明显低于对照组（P<0.05）,Meis1基因上调组胚胎着床率略高于对照组,但无统计学意义（P>0.05）;Meis1基因上调组其整合素β3的表达高于其对照组,Meis1基因下调组 整合素β3的表达低于其对照组,差异均有显著性（P<0.05）.以上观察结果表明,Meis1基因表达下降可明显减少胚胎着床率,影响整合素β3的表达.Meis1基因表达提高则可促进整合素β3的表达. 因此,Meis1可能作为1种子宫内膜容受分子,在胚胎着床中发挥重要作用.     

粗毛栓菌cDNA文库的构建和漆酶基因的表达分析

粗毛栓菌（Trametes gallica）能够分泌多种胞外氧化酶并且快速降解木质纤维素.为了快速高效分离鉴定粗毛栓菌木质纤维素降解酶相关基因,用Trizol试剂提取不同培养条件下粗毛栓菌总RNA,用Creator^TM SMART^TM cDNA Library Construction Kit和Advantage^®2 PCR Kit成功构建了该菌全长cDNA文库.原始文库滴度为1.5×10⁵cfu,重组率达99%,插入片段在0.7～2.0 kb之间,平均大小约1 kb. 随机取16个重组子进行测序,全长cDNA序列完整性率为85.7%;并筛选到1个漆酶基因,编码区长1 551 bp,预测的蛋白质由517个氨基酸残基组成,分子量为55.41 kD,等电点为4.76.用半定量RT-PCR法分析了该漆酶基因在不同培养条件下的表达水平. 结果显示,高浓度的碳源,氮源,Cu^2＋均能诱导此基因的表达,该结果为漆酶基因的表达调控机制的深入研究奠定了基础.     

K14和CMV启动子驱动裸鼠体内HPV16 E6/E7基因表达的差异

人乳头瘤病毒（human papillomavirus,HPV）是一种无包膜的环状闭合双链DNA病毒,具有严格的嗜人组织的特性．为探讨不同启动子驱动HPV E6/E7癌蛋白在裸鼠体内不同组织的表达效率,构建了带有角蛋白(K14)启动子和带有巨细胞病毒（CMV）启动子的E6/E7腺病毒载体（pAd-K14-E6/E7和pAd-CMV-E6/E7）,pAd-K14-E6/E7和pAd-CMV-6/E7、以及作为对照的重组腺病毒空载体pAdtrack- K14和pAd-CMV同源重组后,分别在293细胞中包装,收集重组病毒Ad-K14-E6/E7 、Ad-CMV-E6/E7、Adtrack-K14和Ad-CMV,通过尾缘静脉注射到随机分组的裸鼠体内,并每d向裸鼠腹腔注射0.05 mg雌激素．采用RT-PCR和Western 免疫印迹检测不同实验组E6/E7 mRNA 和蛋白表达水平,免疫组化法检测P53和Bcl-2蛋白表达．结果显示,注射病毒Ad-K14-E6/E7（实验组1）裸鼠子宫体中E6/E7 mRNA、E6蛋白质、P53和Bcl-2蛋白高表达,而其它组织中低表达;注射病毒Ad-CMV-E6/E7（实验组2）裸鼠各组织E6/E7　mRNA、E6蛋白质、P53和Bcl-2蛋白均低表达．研究表明,在裸鼠体内角蛋白K14启动子可以调控E6/E7在子宫体中表达,CMV启动子未能诱导E6/E7在子宫体中表达．     

斜带石斑鱼2种胰脂肪酶基因全长cDNA序列的克隆与分析

利用RT-PCR和RACE方法克隆得到斜带石斑鱼（Epinephelus coioides）肝胰脏中胆盐活化的胰脂肪酶(bile salt-activated lipase,BSAL)和依赖于辅酶的胰脂肪酶(colipase-dependent pancreatic lipase,PL)基因的全长cDNA序列.BSAL基因全长cDNA序列1 796 bp,编码558个氨基酸,该蛋白序列含有BSAL的全部特征结构区,与其他脊椎动物BSAL的氨基酸序列同源性为49.9%～57.3%.PL基因的全长cDNA序列1 503bp,编码465个氨基酸,该蛋白序列含有PL全部的特征结构区,与其它脊椎动物PL的氨基酸同源性为49.1%～73.9%.系统树分析表明,斜带石斑鱼BSAL和PL与其它物种BSAL、PL和胰脂肪酶相关蛋白(PL-RP)聚于进化树的两个不同分支,属于2种不同的胰脂肪酶.结果证实,在同一鱼类体内也存在BSAL和PL两种胰脂肪酶基因.     

链孢囊菌属3种分子分类方法的对比

链孢囊菌属（Streptosporangium）是链孢囊菌科（Streptosporangiaceae）的模式属,包含13个种．种的鉴别通常是多相分类方法,其中尤以DNA同源性分析为国际公认的定种标准;全基因组杂交同源性在70%以下的为不同种．但在进行大量菌株的比对时操作比较复杂．本实验以链孢囊菌属15株标准菌株为实验菌株,选择适宜引物,对其基因组DNA的16S-23S rDNA 间隔区序列（ITS）和REP序列进行了扩增,分别获得了两种基因指纹图谱,并通过UPGMA聚类法构建了相应的进化距离树图．结果表明,对于链孢囊菌属中不同种的区分,两种基因图谱技术的分辨力相当,且两种方法呈现的菌株间同源性与DNA-DNA杂交的结果吻合,有望为链孢囊菌属分类学的研究提供简单、准确、快速的标准程序．     

福建地区小叶买麻藤遗传多样性ISSR分析

采用13条ISSR引物对福建地区小叶买麻藤11个种群共211个样本进行了种群遗传多样性检测。结果表明:(1)小叶买麻藤在物种水平上遗传多样性较高而在种群水平上较低,揭示该物种具有较强的生存、适应、发展潜力,但其种群遗传多样性已经受到生境片段化及人为活动的影响;(2)小叶买麻藤的遗传分化在裸子植物中处于中等水平,选择和基因流对种群遗传分化的作用大于遗传漂变的作用;(3)小叶买麻藤种群退化主要受人类活动影响,影响的时间较短,尚未表现出种群遗传结构的改变。     

人血小板生成素全长分子在酵母系统中的分泌表达及活性分析

外源基因可通过整合型载体被整合到毕赤酵母（Ｐｉｃｈｉａｐａｓｔｏｒｉｓ）染色体上,获得遗传性稳定分泌表达株．利用酵母信号肽ＭＦα,对该信号肽蛋白酶识别位点的相关序列进行重新设计,使天然人ＴＰＯ成熟肽在毕赤酵母系统中分泌表达成功．表达产物经Ｗｅｓｔｅｒｎ－ｂｌｏｔ进行分析,分子量约为６６ｋＤ处蛋白条带可被ＴＰＯ抗体识别;表达量约为０．１ｇ／Ｌ;Ｎ端氨基酸序列分析结果与设计的一致;表达产物对小鼠骨髓细胞形成巨核细胞集落形成单位（ｍｅｇａｋａｒｙ－ｏｃｙｔｅｃｏｌｏｎｙｆｏｒｍｉｎｇｕｎｉｔ,ＣＦＵ－Ｍｅｇ）具有明显的刺激作用．     

人肝金属硫蛋白-I_A基因在鱼腥藻中的克隆与表达

将人工合成的人肝金属硫蛋白（ｍｅｔａｌｏｔｈｉｏｎｅｉｎ,简称ＭＴ）－ＩＡ基因插入至中间载体ｐＲＬ－４３９上强启动子ｐｓｂＡ后,再将其与穿梭载体ｐＫＴ－２１０相连,得到大肠杆菌－蓝藻穿梭表达载体ｐＫＴ－ＭＴ,用三亲接合转移法将ｐＫＴ－ＭＴ转入丝状体蓝藻－鱼腥藻７１２０,经链霉素筛选,得到了稳定的转人肝ＭＴ－ＩＡ基因鱼腥藻．纯化单藻落,液体扩大培养．从鱼腥藻中提取的质粒经Ｓｏｕｔｈｅｒｎ印迹分析,确定人肝ＭＴ－ＩＡ基因已转入鱼腥藻７１２０中,Ｗｅｓｔｅｒｎ印迹分析表明,金属硫蛋白在转人肝ＭＴ－ＩＡ基因鱼腥藻中得到了表达．经原子吸收光谱法测定表达量约为７００μｇＭＴ／ｇ鲜藻,重金属耐受性实验表明,得到了能耐受重金属－镉的转人肝ＭＴ－ＩＡ基因鱼腥藻,它将在清除水域中重金属污染和医药研究方面发挥重要作用．     

HETEROCHRONY AND DEVELOPMENTAL INNOVATION: EVOLUTION OF FEMALE GAMETOPHYTE ONTOGENY IN GNETUM,A HIGHLY APOMORPHIC SEED PLANT

Seed plant female gametophytes are focal points for the evolutionary modification of development. From a structural perspective, the most divergent female gametophytes among all seed plants are found in Gnetum, a clade within Gnetales. Coenocytic organization at sexual maturity, absence of defined egg cells (free nuclei are fertilized), lack of centripetal cellularization, and postfertilization development of embryo-nourishing tissues are features of the female gametophytes of Gnetum unparalleled among seed plants. Although the female gametophyte of Gnetum retains the three basic phases of somatic development common to female gametophytes of plesiomorphic seed plants (free nuclear development, cellularization, cellular growth), the timing of fertilization has been accelerated relative to the rate of somatic development. As a consequence, the female gametophyte of Gnetum matures sexually (is fertilized) at a juvenile (compared with the ancestral somatic ontogeny) and free nuclear stage of somatic development, thereby precluding differentiation of egg cells. Unlike progenetic animals, where truncation of somatic ontogeny evolves in tandem with acceleration in the timing of sexual maturation, the female gametophyte of Gnetum completes the entire ancestral somatic ontogeny after precocious sexual maturation. This results in the evolution of postfertilization development of embryo-nourishing female gametophyte tissues, a phenomenon unique among seed plants. Nonheterochronic developmental innovations have also played important roles in the evolution of the female gametophyte of Gnetum. Centripetal cellularization, which is always associated with the phase change from coenocytic to cellular organization among plesiomorphic seed plant female gametophytes, is lacking in Gnetum. Instead, during early phases of development, apomorphic free nuclear organization is coupled with a highly anomalous pattern of cellularization. Stage-specific innovations during early development in the female gametophyte of Gnetum do not affect plesiomorphic aspects of later phases of development. Thus, a complex array of heterochronic and nonheterochronic developmental innovations have played critical roles in the ontogenetic evolution of the highly apomorphic female gametophyte of Gnetum.     

Studies on the Chemical Constituents of Gnetum montanum Markg

Six compounds had been isolated from the stem of Gnetum montanum Markgr, on the basis of spectral analysis (UV, IR, 1H NMR, 13C NMR and MS), physico-chemical constants and preparation of the derivative. They were identified as 2-hydroxy-3-methoxyl-4-methoxycarbonyl pyrrole (1), 2-hydroxy-3-methoxymethyl-4-methoxycarbonyl pyrrole (2), 3,4′-dihydroxy-4-methoxy-dibenzyl ether (3), 3, 3′,4′-trihydroxy-4-methoxy-dibenzy ether (4), 2,3-diphenyl-pyrrole (5) and aminemethyl-methyl alcohol (6). (1)—(4) are new compounds,