阿霉素纳米粒在肿瘤治疗中的应用研究

目的:观察阿霉素纳米粒对多耐受糖蛋白介导的膀胱移行细胞癌多耐药的逆转.方法:MTT法观察MDR逆转,采用流式细胞仪对细胞内阿霉素浓度进行检测.结果:阿霉素纳米对敏感株的细胞毒作用与阿霉素差异无显著性意义,耐药株对阿霉素纳米较对阿霉素纳米粒敏感4.8倍,表现细胞内阿霉素显著增高.结论:阿霉素纳米可有效逆转P-gp介导的多药耐药.     

人羊膜间充质干细胞移植对CCl_4诱导的小鼠损伤肝HGF、SIRT-1、α-SMA及P~(27kip1)表达的影响

人羊膜间充质干细胞(h AMSCs)具有自我增殖和多向分化潜能,有望为干细胞移植性治疗提供新来源,是病变组织器官损伤修复的理想种子细胞.但目前关于h AMSCs对肝损伤的修复机制仍不十分清楚.本研究采用胰蛋白酶-胶原酶消化法从羊膜组织中分离、纯化了间充质干细胞.免疫荧光检测表面标记波形丝蛋白(vimentin)和阶段特异表达抗原4(SSEA-4)均呈阳性.h AMSCs表达CD29、CD49d、CD73表面抗原,但不表达骨髓间充质表面抗原CD34、CD45和人类白细胞抗原DR位点(HLA-DR).实时定量PCR和Western印迹检测揭示,h AMSCs移植后可提高受损肝组织中肝细胞生长因子(HGF)和沉默信息调节因子1(SIRT-1)的表达,抑制α-平滑肌肌动蛋白(α-SMA)和周期性蛋白依赖性激酶抑制因子(P27kip1)的表达.因为上述蛋白质分子涉及肝细胞增殖、再生、凋亡调节,抑或肝纤维化过程,因此h AMSCs移植后所引起的上述分子表达变化可改善四氯化碳(CCL4)诱导的肝损伤,抑制肝细胞凋亡,促进肝细胞有丝分裂,对肝损伤有一定的修复作用.该研究为进一步探索调控肝再生、损伤修复信号通路(机制)及预防肝纤维化提供了新启示.     

不同批号蕲蛇酶在家兔血液凝固系统上的生物活性检测

目的：研究不同批号蕲蛇酶静脉给予家兔后,对血液凝固系统各项指标的影响,以判定其药效的稳定性。方法：取家兔,纯白色,体重1．5－2．5kg,雌雄兼用,每日静脉注入蕲蛇酶1．0u/kg.d^-1,连用3－5天,药前、药后从心脏取血6ml,取全血1ml作血栓形成;余血以3．0％枸橼酸钠按1：9抗凝,分离富血小板血浆（PRP）,测定其血小板数目和血小板聚集率,以贫血小板血浆（PPP）测定凝血酶时间（TT）,凝血酶原时间（PT）,部分凝血活酶时间（KPTT）以及纤维蛋白原（Fg)含量。结果：5个批号的蕲蛇酶药后3天或5天均可明显使血栓形成的重量减轻,长度缩短,Fg含量减少（P＜0．01）,TT,PT,KPTT均延长（P＜0．05－0．01）,血小板数轻度减少,聚集率抑制达20％－50％,结论：不同批号的蕲蛇酶静脉给予家兔,具有显著的作用于血液凝固系统,导致血栓形成减少,表明对心脑血管内血栓形成药学相同,说明用家 兔作为鉴定药品质量是可行而必须。     

溶藻菌株NP23的紫外诱变选育

应用紫外诱变技术对溶藻菌株NP23进行紫外诱变处理。经过粗筛后,从8株诱变株中选出2株对绿藻中小球藻和蓝藻中惠氏微囊藻的去除效果明显优于原始菌株的突变株NP23-1和NP23-4,其溶藻率(叶绿素a的去除率)比原始菌株提高30%-35%。连续6代测试,2株诱变菌株NP23-1和NP23-4溶藻率都很稳定,表明所得突变株是比原始菌株更优秀的溶藻菌株。     

枸杞脱落酸生物合成关键酶基因NCED的克隆及表达分析

脱落酸(abscisic acid,ABA)对植物的生长发育具有独特的调控功能,并在植物适应逆境环境中发挥重要作用。9-顺式环氧类胡萝卜素双加氧酶(NCED)是高等植物中ABA生物合成途径的一个关键酶。根据GenBank中的植物NCED基因的同源序列设计简并引物,通过RT-PCR及RACE技术从枸杞叶片中克隆到1个编码NCED的基因,命名为LbNCED。其cDNA全长为2316 bp,含有1个1824 bp的开放阅读框,编码1个含607氨基酸残基,分子量为67.38 kDa、等电点(pI)为6.43的假定蛋白,其氨基酸序列与番茄(Lycopersicon esculentum)和马铃薯(Solanum tuberosum)的同源性达90%,在N-末端具有1个含15个氨基酸的叶绿体转运肽。Southern杂交结果表明,该基因在枸杞基因组中以低拷贝形式存在。盐处理和脱水处理的枸杞叶片中LbNCED基因的表达与内源ABA的积累同步变化。     

Cynandione A mitigates ischemic injuries in rats with cerebral ischemia

Cynandione A, an acetophenone from the roots of Cynanchum auriculatum and other species in the genus attenuates neurotoxicity of a variety of neurotoxic agents such as l-glutamate in vitro. In this study, we sought to further characterize the neuroprotective effects of cynandione A and other acetophenones from the roots of C. auriculatum in pheochromocytoma tumor cell line PC12 and investigate whether cynandione A protected against ischemic injuries in rats with experimentally induced cerebral ischemia. Viability assays using the 2-(2-methoxy-4-nitrophenyl)-3-(4-nitrophenyl)-5-(2,4-disulfophen-yl)-2H-tetrazolium monosodium salt method and lactate dehydrogenase (LDH) release assays showed that cynandione A dose-dependently attenuated glutamate-induced cytotoxicity. Comparative proteomic analysis by two-dimensional gel electrophoresis and matrix-assisted laser desorption/ionization-time of flight MS/MS of PC12 cells treated with cynandione A showed 10 μM cynandione A caused broad changes in protein expression in PC12 cells including down-regulation of high mobility group box 1 (HMGB1) and dihydropyrimidinase-like 2 (DPYSL2). Immunoblotting studies showed that 10 μM cynandione A aborted glutamate-induced increase in DPYSL2 and HMGB1 levels in PC12 cells and 30 mg/kg cynandione A also attenuated the rise in HMGB1 levels and mitigated DPYSL2 cleavage in brain tissues of rats with cerebral ischemia. Furthermore, rats with cerebral ischemia treated with 30 mg/kg cynandione A exhibited markedly improved neurological deficit scores at 24 and 72 h compared with control and a 7.2% reduction in cerebral infarction size at 72 h (p < 0.05 vs. control). Our findings demonstrated that cynandione A mitigated ischemic injuries and should be further explored as a neuroprotective agent for ischemic stroke.     

紫茎泽兰的化学成分初报

紫茎泽兰(Eupalorium adenophorum Spreng)原产中美墨西哥,现在滇南一带广泛分布,对林、牧业生产造成严重危害。其化学成分研究未见报道。 从紫茎泽兰的叶和花序中,分到九个单体,经详细的光谱解析和与标准品对照,其中五个成分的化学结构分别为:正三十二烷n-dotriacontane(1),β-谷甾醇β-sitosterol(2),豆甾醇stigmasterol(3),蒲公英醇棕榈酸酯taraxasteryl palmitate(4),蒲公英醇乙酸酯taraxastcryl acetate(5)。     

Biodegradation of poly(ε-caprolactone) (PCL) by a new Penicillium oxalicum strain DSYD05-1

In this study, fungi isolated from soil were screened for their ability to form clear zones on agar plates with emulsified poly(ε-caprolactone) (PCL). The most active strain, designated as DSYD05, was identified as Penicillium oxalicum on the basis of morphological characteristics and phylogenetic analysis. Mutant DSYD05-1, obtained by ultraviolet-light mutagenesis from strain DSYD05, was more effective in PCL degradation. In liquid cultures of the mutant strain with PCL emulsion, DSYD05-1 showed the highest PCL-degrading activity after 4?days of cultivation. The products of PCL degradation were analysed by mass spectrometry; the results indicated that 6-hydroxyhexanoic acid was produced and assimilated during cultivation. The degradation of PCL film by DSYD05-1 was observed by scanning electron microscopy, and was indicative of a three-stage degradation process. The degradation of amorphous parts of the film preceded that of the crystalline center and then the peripheral crystalline regions. In addition, DSYD05-1 showed a wide range of substrate specificity, with capability to degrade PCL, poly(β-hydroxybutyrate), and poly(butylene succinate), but not poly(lactic acid), indicating that the strain could have potential for application in the treatment or recycling of bio-plastic wastes.     

N-糖基化移位对乙型肝炎病毒表面抗原中蛋白核酸疫苗的表达及免疫原性的影响

目的：研究N-糖基化移位对乙型肝炎病毒表面抗原中蛋白核酸疫苗体外蛋白表达及小鼠体内体液免疫及细胞免疫应答的影响。方法：通过基因工程中定点突变技术,将乙型肝炎病毒表面抗原中蛋白（MHBs）中第4位氨基酸上连接的糖链去除,或将糖链依次移位至第5、6或7位氨基酸,来构建N-糖基化去除及移位的核酸疫苗,分别命名为Adr—dN4、Adr-N4—5、Adr—N4．6、Adr—N4．7。用上述核酸疫苗与野生型MHBs核酸疫苗（pSW3891／MHBs／Adr,简称Adr）及空载体质粒pSW3891分别用脂质体瞬时转染293T细胞,应用蛋白印迹法检测MHBs的表达。采用肌肉注射法,以各组疫苗分别对BALB／c小鼠于第0、2、4和6周进行免疫．用ELISA法检测小鼠血清中抗．HBs抗体、ELISPOT法检测小鼠表面抗原多肽特异性分泌IFN-T的脾细胞数量。结果：蛋白印迹法结果显示Adr、Adr-dN4、Adr—N4．5、Adr—N4—6、Adr-N4—7体外转染293T细胞后,均可以在293T细胞内表达,且Adr、Adr-N4—5、Adr-N4—7可将表达产物分泌到细胞外。ELISA及EISPOT结果表明：Adr免疫组小鼠抗-HBs终点滴度及表面抗原特异性分泌IFN-γ的脾细胞数量,均略高于其他免疫组小鼠,但与Adr—N4—5、Adr．N4—7相比无统计学差异（P〉0．05）,与Adr-dN4和Adr—N4—6组相比有显著的统计学差异（P〈0．05）。结论：在第5或7位氨基酸附加N-连接糖链,能修补或替代Asn4连接糖链引导MHBs分泌的功能。HBs表达蛋白分泌到细胞外对诱导机体产生特异性细胞和体液免疫是至关重要的。