四种贝母生物碱对离体心肌、血管及神经生理效应的影响

本文研究了四种贝母生物碱（ＦＨ１～ＦＨ４）对离体豚鼠及大鼠心肌、兔胸主动脉条和蟾蜍坐股神经干生理效应的影响。在左心房，ＦＨ１、ＦＨ４剂量依赖性地增强心肌收缩力，在右心房则减慢心率。ＦＨ２正肌作用微弱，ＦＨ３却表现为负性正肌作用。在离体血管上，ＦＨ１～ＦＨ４均可明显对抗甲氧胺引起的血管收缩作用；对神经动作电位无影响。

乙型肝炎病毒核心抗原及Flt3配体双表达核酸疫苗的小鼠免疫应答研究

目的构建乙型肝炎病毒核心抗原(HBcAg)和Flt3配体(FL)胞外段双表达核酸疫苗,并观察其免疫原性。方法分别将HBcAg、FL基因克隆入pJW4303载体,获得双表达核酸疫苗,体外转染293T细胞检测目的基因的表达。分组免疫BABL／c小鼠,酶联免疫吸附试验(ELISA)检测小鼠血清抗-HBc IgG效价,酶联免疫斑点试验(ELISPOT)检测HBcAg特异性Th1／Th2型细胞因子的分泌水平。结果所构建疫苗在体外均能表达HBcAg和FL,当基因位于内部核糖体切入位点(IRES)元件上游时表达水平明显较优。pJW4303／C／FL免疫组产生的抗-HBc IgG效价和Th1／Th2型细胞因子的分泌水平均显著优于pJW4303／C和pJW4303／FL／C组。结论成功构建双表达核酸疫苗,基因位于上游时表达水平高于下游。FL基因的引入明显增强了HBcAg核酸疫苗的免疫原性。

RT-PCR法检测白血病干细胞Flt3和N-ras基因的表达

目的:采用逆转录-聚合酶链反应(RT-PCR)法检测益气养阴方及其拆方后的扶正方组、祛邪方组急性白血病干细胞Flt3和N-ras基因的表达,以期阐明Flt3和N-ras基因表达与疾病发生、发展的关系。方法:RT-PCR法检测中药益气养阴方组、扶正方组、祛邪方组及对照组AML患者骨髓单个核细胞Flt3和N-ras基因表达的情况。结果:Flt3和N-ras基因表达阳性率益气养阴组、扶正组、祛邪组与对照组比较,差异有显著性意义(P均<0.01);益气养阴组与扶正组和祛邪组比较,差异有显著性意义(P均<0.01);扶正组与祛邪组比较,差异无显著性意义(P>0.05);各FAB亚型AML间Flt3与N-ras表达阳性率比较,差异无显著性意义(P>0.05)。结论:中药益气养阴方可降低Flt3和N-ras基因在AML细胞的表达水平,抑制AML细胞的克隆性增殖,对AML具有治疗作用。

FLT3基因在急性髓细胞白血病中的表达及临床意义

目的研究急性髓细胞白血病(AML)患者FLT3的表达水平,探讨Fms样的酪氨酸激酶3(FLT3)在AML中的作用机制及临床意义.方法采用半定量RT-PCR方法检测70例AML患者和11例良性血液病为对照组FLT3表达水平.老年AML36例,非老年AML34例,其中初治组31例,完全缓解(CR)组15例,难治复发组24例.结果70例AMLFLT3表达水平明显高于对照组,差别有统计学意义(P<0.01);36例老年AML组与34例非老年AML组间FLT3表达水平无显著性差异(P>0.05);复发难治组FLT3表达水平最高,初治组居中,CR组最低,三者表达水平具有显著性差异(P<0.05);AML初治组按FAB亚型分组,M3组表达水平最低,与其它亚型有显著性差异(P<0.05);M2、M4、M6居中,三者间表达水平无显著性差异(P>0.05);M5组表达水平最高,与其它亚型有显著性差异(P<0.05).结论FLT3在AML中过度表达,以M5最为明显,提示FLT3在白血病的发病机制中有一定作用,与疾病进展及预后有关,在检测微小残留病方面,也可能有一定价值.

[Li…X]e^(-[1])(X=FH，OH_2，NH_3)的光电性质从头算

在MP2理论水平上采用6-311G基组系列计算了一价阴离子van der Waals复合物[Li…X]e^(-[1])(X=FH,OH_2,NH_3)的偶极矩(μ)、平均极化率(α)以及平均一阶超极化率(β),讨论了基组效应和电子相关效应对计算结果的影响,比较了价电子对复合物一阶超极化率的贡献.在MP4(SDQ)/6-311++G(2df,2pd)水平上计算得到[Li…FH]e^(-[1])的μ=2.5633 a.u.,α=1.0476×10~3 a.u.,β=1.0948×10~5 a.u.;[Li…OH_2]e^(-[1])的μ=2.3204 a.u.,α=1.2201×10~3 a.u.,β= 2.1410×10~5 a.u.;[Li…NH_3]e^(-[1])的μ=2.4687 a.u.,α=1.4817×10~3 a.u.,β=3.4040×10~5 a.u.,计算结果表明,三种一价阴离子复合物分子均具有非常大的一阶超极化率,而一个价电子对复合物的一阶超极化率的贡献超过1.0×10~5 a.u..

人Flt3配体基因的克隆及在Hela细胞中的表达

目的:克隆人Flt3配体(FL)基因,检测其在Hela细胞中转录及表达蛋白的活性。方法:Trizol法提取K562细胞总RNA,经RT-巢式PCR得到FL的cDNA,PCR产物亚克隆入pGEM-T载体测序,构建pcDNA3/hFL。经Lipofectamine2000介导转入Hela细胞,RT-PCR法检测转染细胞中hFL基因的转录,ELISA法检测培养上清中hFL的含量,增殖和促生存实验鉴定hFL的活性。结果:所得FL基因序列正确。转染后的Hela细胞能转录FL基因,上清中hFL蛋白含量为56.8ng/ml/1,hFL能促Raji细胞生存及抑制凋亡(P<0.01),促进HL-60细胞增殖(P<0.05)。结论:构建的pcDNA3/hFL质粒在Hela细胞表达系统中能够有效转录,表达的hFL蛋白具有生物学活性。

Phenotypic analysis of a dwarf and deformed flower3 (ddf3) mutant in rice (Oryza sativa L.) and characterization of candidate genes

Dwarf mutants are the crucial resources for molecular biology research and rice breeding. Here, a rice mutant, dwarf and deformed flower3（ddf3）, was identified in tissue culture of Oryza sativa cv. Dongjin. Compared with wild type, the ddf3 mutant exhibited severe dwarfism, a greater number of tillers and significantly decreased fertility. In addition, leaf length, panicle length, and grain length, were significantly shorter. All internodes of ddf3 were shorter than those of wild type, and histological analysis revealed that internode cell elongation was significantly inhibited in ddf3. In the ddf3 mutant, pollen activity was significantly decreased, and the development of most stigmas was abnormal. Genetic analysis indicated that the ddf3 mutant phenotypes are controlled by a single or tightly linked nuclear genes. Using an F2 mapping population generated from a cross between ddf3 and Yangdao 6（9311）, the DDF3 gene was mapped to a 45.21-kb region between insertion-deletion（In Del） markers M15 and M16 on the long arm of chromosome 7. Sequencing revealed a 13.98-kbdeletion in this region in the ddf3 mutant genome that resulted in the complete or partial deletion of ZF（DHHC type zinc finger protein）, EP（expressed protein）, and FH2（actin-binding FH2 domain-containing protein） genes. Quantitative RT-PCR analyses revealed that in wild type, the transcript levels of FH2 were almost the same in all organs, while ZF was mainly expressed in the panicle, and no expression of EP was detected in any organ. Based on these results, ZF and FH2 could be potential DDF3 candidate genes involved in the regulation of rice morphology and flower organ development. Our work has laid the foundation for future functional analysis of these candidate genes and has provided a profitable gene resource for rice breeding for increased fertility in the future.