中国苏铁属花粉形态研究

对中国苏铁属花粉进行了光镜和扫描电镜观察。花粉中等大,极轴长２６．５－３５．７μｍ,赤道轴长２０．６－２６．４μｍ;极面观椭圆形至近圆形,赤道面观船形或肾形,具远极单沟,达两端,其开闭和形状随花粉干燥或潮湿而变化,内部具多种不规则突起,两端具皱纹;远极面外壁光滑或稀具微突起,近极面具穿孔,孔穴或蜂窝状纹饰。     

绞股蓝属的染色体研究

报道了葫芦科绞股蓝属（Ｇｙｎｏｓｔｅｍｍａ Ｂ１．）８种共２０个居群的染色体数目,分别为２ｎ＝２２,３３,４４,６６,８８多倍体现象极为普遍。两个亚属;绞股蓝亚属（Ｓｕｂｇｅｎ．Ｇｙｎｏｓｔｅｍｍａ）和喙果藤亚属（Ｓｕｂｇｅｎ．Ｔｒｉｏｓｔｅｌｌｕｍ）的染色体基数均为Ｘ＝１１,并结合该属植物形态特征、繁殖方式和地理分布,对普遍出现的多倍体现象进行了讨论。     

ERK signaling is triggered by hepatitis C virus E2 protein through DC-SIGN

Dendritic cell-specific intercellular adhesion molecule-3-grabbing nonintegrin (DC-SIGN) is a binding receptor for hepatitis C virus (HCV). Binding of HCV envelope protein E2 to target cells is a prerequisite to DC-SIGN-mediated signaling. Using cell lines with stable or transient expression of DC-SIGN, we investigated effects of soluble HCV E2 protein on ERK pathway. MEK and ERK are activated by the E2 in NIH3T3 cells stably expressing DC-SIGN. Treatment of the cells with antibody to DC-SIGN results in inhibition of the E2 binding as well as the E2-induced MEK and ERK activation. In HEK293T cells transiently expressing DC-SIGN, activation of MEK and ERK is also induced by the E2. Activation of ERK pathway by HCV E2 through DC-SIGN provides useful information for understanding cellular receptor-mediated signaling.     

Characterization of two CTR-like protein kinases in Rosa hybrida and their expression during flower senescence and in response to ethylene

The expression of two CTR-gene homologues was investigated during flower senescence in two Rosa hybrida cultivars. A fragment of a gene for a protein kinase, termed RhCTR1 (GenBank Acc. No. AF271206), was amplified by PCR and used to isolate the corresponding full-length cDNA (Acc. No. AY032953) from a rose petal cDNA library. The protein RhCTR1 has 66% amino acid identity to Arabidopsis CTR1. A fragment of a second CTR homologue, termed RhCTR2 (Acc. No. AY029067) is 69% identical to the corresponding region of RhCTR1. RhCTR1 expression increased during flower senescence, while RhCTR2 was constitutively expressed during flower development. The expression of both RhCTR1 and RhCTR2 was increased in response to exogenous ethylene.     

丙型肝炎病毒F蛋白缺失对病毒复制及感染性的影响

探索了F蛋白缺失及核心蛋白(Core)二级结构改变对丙型肝炎病毒(HCV)复制和感染性的影响．利用定点突变方法,将J6JFH1的核心基因引进5个终止密码子以中断F蛋白的表达,从而获得F蛋白缺失的病毒复制子J6JFH1/ΔF．体外制备RNA转录体,并电穿孔转染Huh7.5.1细胞,采用免疫荧光、实时荧光定量PCR方法以及病毒感染等方法,观察F蛋白缺失对病毒复制、蛋白质表达及转染细胞上清感染性病毒颗粒产生的影响．在此基础上,构建5个单一突变病毒体,对HCV核心蛋白进行二级结构分析,观察核心蛋白二级结构对HCV复制和翻译的影响．结果显示,转染48 h后,J6JFH1/ΔF与野生型J6JFH1相比,J6JFH1/ΔF转染阳性细胞数明显降低,细胞内HCV RNA 水平降低约95%,J6JFH1/ΔF转染后不同时间点细胞上清中HCV RNA拷贝数和病毒颗粒也明显降低．5个单一突变体不影响核心基因二级结构,病毒在细胞内复制和感染性与野生型水平一致．J6JFH1/ΔF所产生的改变可能是由于5处突变导致核心基因二级结构改变而造成的．结果说明,HCV F蛋白缺失不影响病毒的复制翻译及病毒颗粒的包装释放,核心蛋白二级结构的改变对病毒复制和翻译则产生较大影响．     

携带HBV包膜大蛋白DNA疫苗的减毒沙门菌在小鼠诱导免疫应答

探索一种简便、有效的乙型肝炎病毒DNA疫苗免疫方法。将编码绿色荧光蛋白的真核表达质粒pEGFPN1转化到减毒鼠伤寒沙门菌SL7207,灌胃饲服BALB/c小鼠,流式细胞术检测出小鼠脾细胞内表达的绿色荧光蛋白;构建编码HBV包膜大蛋白的DNA疫苗pCIS1S2S,分别以SL7207为载体的口服途径或直接肌肉注射途径免疫BALB/c小鼠,检测小鼠的血清抗体、T细胞增殖和细胞毒性T淋巴细胞反应,结果表明两种免疫途径均能在小鼠体内诱生细胞和体液免疫应答,但口服途径诱导免疫应答的强度明显强于肌肉注射途径。口服携带HBV DNA疫苗的减毒伤寒沙门菌可能代表一种简便、有效的治疗乙型肝炎的新方法。      

烟草花叶病毒蚕豆株系基因组全序列分析及结构特征

根据已报道的TMV-U1株系核苷酸序列合成引物 ,利用RT-PCR技术获得了覆盖整个烟草花叶病毒蚕豆株系 (TMV-B)基因组的cDNA重组克隆 .结合末端测序技术 ,完成了TMV-B全基因组序列测定 .TMV-B全基因组共有 6 395个核苷酸组成 ,包括 4个开读框 (ORF) ,分别编码 1 2 6ku(含 1 1 1 6个氨基酸 )、1 83ku(含 1 6 1 6个氨基酸 )、30ku(含 2 6 8个氨基酸 )和 1 7.5ku蛋白 (含 1 5 9个氨基酸 ) .TMV-B与TMV-U1相比全基因组同源率达 99.4% ,两病毒基因组 5′ ,3′非编码区和CP基因完全相同 .TMV-B与TMV-U1之间在 1 2 6ku蛋白中有 6个氨基酸差异 ,5 4ku蛋白中有 2个差异 ,30ku蛋白中有 3个差异 .对导致TMV-B侵染蚕豆的可能致病机理进行了分析 .