苦参碱的提取分离及对小鼠的毒性研究

采用酸性乙醇提取、乙醚萃取、硅胶柱层析分离等方法从苦参中分离到苦参碱单体.以小鼠为实验动物进行毒性测定,小鼠的死亡主要集中在48h内,48h后无小鼠的死亡现象.小鼠对苦参碱的耐受量大于30mg.k-g1,小于140mg.k-g1,致死中量LD50为64.01mg.kg-1,回归方程Y=-3.2370+4.5602X,LD50标准误差SE=6.14.适口性的测定表明,苦参碱对小鼠有较好的适口性,可以作为杀鼠剂使用.     

丙烯酰胺对小鼠血液毒性的研究

目的 为探明丙烯酰胺对小鼠血液的毒性效应.方法 采用丙烯酰胺溶液连续灌胃小鼠16天,记录小鼠体重、器官系数变化并对小鼠血液成分进行检测.结果 当染毒剂量为120、150 mg/kg时,小鼠体重增重率、肝系数、WBC、LYM、RBC、MCHC、PLT、P-LCR显著降低(P<0.05),GRAN显著增加(P<0.05);...     

氧化苦参碱对K562肿瘤细胞增殖的影响

目的:研究氧化苦参碱(OM)对人白血痛细胞系K562生长增殖的影响.方法:运用MTT比色法、活细胞计数法、集落形成法以及透射电镜观察检测OM对人白血病细胞系K562增殖抑制作用.结果:MTT实验、生长曲线及集落形成实验显示OM能明显抑制K562细胞的增殖.随着OM浓度的增加,K562细胞存活细胞显著降低,呈现明显的刺量依赖性,经相关分析,细胞抑制率与OM浓度呈正相关(r=0.9010),其半数抑制浓度(IC50)为0.33 mg/ml.透射电镜下显示在低浓度即有明显的诱导细胞凋亡的作用,出现核固缩、核碎裂、凋亡小体等典型的凋亡形态.结论:OM具有抑制K562白血病细胞增殖诱导肿瘤细胞凋亡的作用.     

恒定磁场对小鼠精子毒性作用的实验研究

观察不同强度恒定磁场对雄鼠睾丸、附睾重量、精子数量、精子活动度及精子形态的影响. 结果显示睾丸与附睾重量各组无显著差异, 精子数量在实验组与对照组中亦无明显改变. 在 0.12T磁场环境暴露下, 雄鼠精子畸形率增加及活动率下降, 与对照组相比有显著差异. (P< 0.01), 提示磁场对小鼠精子有一定毒性, 并且毒性与其强度有关.     

Th1／Th2类细胞因子在氧化苦参碱抗小鼠急性免疫性肝损伤的影响作用研究

本研究的目的是观察氧化苦参碱（OM）对ConA诱导的小鼠急性免疫性肝损伤干预过程中Th1／Th2细胞因子的变化,探讨OM抗急性免疫性肝损伤的分子机制。将Balb／c小鼠随机分为四组：正常对照组（NCG）,肝损伤组（LIG）,OM对照组（OMCG）,OM治疗组（OMTG）。除NCG及OMCG尾静脉注射生理盐水0．3ml外,LIG及OMTG尾静脉注射12．5mg／kg ConA（0．3ml）一次。此外OMCG和OMTG在造模前0．5h经腹腔注射OM（60mg／kg）,每24h注射一次。     

氧氟沙星对小鼠生殖毒性和致畸性的研究

目的研究氧氟沙星对昆明系小鼠胚胎和胎鼠发育的影响,确定其是否存在生殖毒性和致畸性。方法①雄鼠分别灌服各剂量氧氟沙星,连续10d,末次给药24h后与母鼠合笼,在妊娠第三天取胚胎,记录各剂量组胚胎发育率。②孕鼠妊娠零天给药,分别经口灌服高、中、低剂量[36、72和360mg(kg.bw)]氧氟沙星溶液,连续给药3d,在妊娠第三天收集胚胎,记录胚胎发育率。③孕鼠妊娠零天给药,分别经口灌服各剂量氧氟沙星溶液,连续给药10d,在妊娠第16天取出胎鼠,记录胎鼠体重、胎盘重、活胎数、胎鼠外观畸形和内脏畸形等指标。结果给药组与对照组相比,雄鼠服用高剂量组360mg(kg.bw)氧氟沙星对着床前胚胎发育影响显著(P<0.05),而中等剂量和低剂量组对着床前胚胎发育的影响不显著(P>0.05)。雌鼠服用不同剂量氧氟沙星对着床前胚胎发育影响不显著(P>0.05)。氧氟沙星对受孕鼠的活胎数和吸收胎数均无明显影响,给药组的活鼠体重、胎盘重均未见明显差异(P>0.05);药物组和对照组均未出现外观畸形和内脏畸形,也不存在剂量和效应关系。结论孕鼠服用不同剂氧氟沙星对昆明系小鼠胚胎和胎鼠发育无明显的影响,表明氧氟沙星对雌性鼠不具有明显的生殖毒性和致畸性;但雄鼠服用高剂量氧氟沙星对着床前胚胎发育影响显著。     

谷氨酰胺提取分离研究

谷氨酰胺是一种十分有用的氨基酸,它既可作为治疗药物,又可作为其它合成药物的前体。目前国内以谷氨酸为原料,采用化学合成法生产谷氨酰胺,供作试剂用,产量十分有限。日本用发酵法生产谷氨酰胺,年产1000吨,还有增加趋势。谷氨酰胺的销售价格比较高,经济效益可观。近年来国内有好几个研究小组都在进行谷氨酰胺发酵研究。我们是国内第一个谷氨酰胺研究组,已在5m~3发酵罐上取得中试成功。谷氨酰胺发酵液中混有谷氨酸,而这些少量的谷氨酸采用等电点沉淀法并不能将它们去除,影响谷氨酰胺的纯度。我们采用离子交换树脂法,成功地将谷氨酸从谷氨酰胺和谷氨酸的混合物中分离掉,得到单一的谷氨酰胺。在将发酵液上柱交换之前,必须对发酵液进行预处理,我们试验了4种不同方法,结果表明第4种方法更适合工厂使用。从我们使用过的几种树脂的分离效果及树脂的价格看,考虑到工     

氧化苦参碱对哮喘大鼠肺组织IL-10 表达的影响

目的:观察不同浓度氧化苦参碱(Oxymatrinem,Oxy)对哮喘大鼠肺组织IL~(-1)0表达的影响,并探讨其作用机制。方法:构建哮喘大鼠模型,将40只清洁级健康雌性SD大鼠随机分成5组,每组8只:A:哮喘组(仅卵蛋白(Ovalbumin,OVA)致敏)、B:低浓度组(Oxy 50 mg/kg)、C:中浓度组(Oxy 100 mg/kg)、D:高浓度组(Oxy 150 mg/kg)、E:对照组(生理盐水),末次激发24 h后处死全部大鼠,取大鼠肺脏,HE染色观察肺组织病理改变,采用RT-PCR、Western Blot测定各组肺组织中IL~(-1)0基因及蛋白水平的表达。结果:HE结果显示,哮喘组可见大量炎症细胞浸润,气管平滑肌明显增厚。对照组肺泡壁薄且光滑,未见明显炎性细胞的浸润,不同浓度氧化苦参碱药物干预组其肺组织炎症细胞浸润及气管平滑肌病变程度随着用药浓度的增高呈逐渐减轻趋势。RT-PCR以及Western blot检测IL~(-1)0发现,哮喘组、氧化苦参碱低浓度组、氧化苦参碱中浓度组与对照组相比IL~(-1)0的表达均有所减低(P0.05),而氧化苦参碱高浓度组与对照组比较,IL~(-1)0的表达无统计学意义(P0.05);氧化苦参碱中浓度组、氧化苦参碱高浓度组与哮喘组相比IL~(-1)0的表达均有所增高(P0.05),氧化苦参碱低浓度组与哮喘组相比IL~(-1)0的表达无统计学意义(P0.05)。结论:氧化苦参碱抑制、控制哮喘发作可能与促进肺组织中IL~(-1)0基因、蛋白的表达相关,且促进程度在一定范围内与浓度呈正比。     

氧化苦参碱对阿霉素所致大鼠心肌损伤的保护作用研究

目的：研究氧化苦参碱对阿霉素致大鼠心肌损伤的保护作用。方法：SD大鼠随机分成4组,阿霉素级（adriamycin,ADM）、阿霉素＋氧化苦参碱组（oxymatrine,OMT）,氧化苦参碱组,正常对照组。免疫组化染色法检测大鼠心肌Ⅰ Ⅲ型胶原的表达,用光镜及电镜观察心肌组织的病理改变及超微结构变化。结果：ADM组中大鼠心肌Ⅰ Ⅲ型胶原的表达显著增加,ADM＋OMT组也有相似改变,但较ADM组有显著下降,两组之间有显著差异（P〈0．05）;正常对照组与OMT组无变化。光镜及电镜结果显示ADM组与ADM＋OMT组大鼠心肌组织,均有损伤,但ADM＋OMT组较ADM组损伤明显减轻。OMT组动物未观察到心肌组织病理变化。结论：氧化苦参碱对阿霉素所致大鼠心肌损伤具有保护作用。     

氧化苦参碱对大鼠缺血再灌注心肌损伤的保护机制研究

目的:探讨氧化苦参碱(OMT)对大鼠缺血再灌注心肌损伤(MIRI)的保护机制。方法:随机将60只成年Wistar大鼠分成对照组、MIRI组和OMT组,每组20只,除对照组外,其他两组结扎30 min后松解结扎线灌注60 min。结扎前10 min,OMT组股静脉输入苦参注射液120 mg/kg,对照组、MIRI组则输入等容量生理盐水。造模后,记录两组心率(HR)、左心室收缩压(LVSP)、左室内压最大上升或下降速率(+dp/dt_(max)或-dp/dt_(min))及血清乳酸脱氢酶(LDH),检测两组心肌组织中一氧化氮(NO)、丙二醛(MDA)、一氧化氮合酶(NOS)、超氧化物歧化酶(SOD)、谷胱甘肽过氧化物酶(GSH-PX)水平。结果:与MIRI组相比,OMT组HR、LVSP和+dp/dt_(max)、-dp/dt_(min)均显著升高(P0.05),且OMT组上述指标与对照组比较,差异均无统计学意义(均P0.05)。与MIRI组相比,OMT组的NO、NOS、SOD、GSH-PX水平均显著升高,而MDA、血清LDH水平显著降低,比较差异均有统计学意义(均P0.05),且OMT组上述指标与对照组比较,差异均无统计学意义(均P0.05)。结论:OMT对MIRI大鼠具有心肌保护作用,其机制可能与提高抗氧自由基活性、改善微循环及舒张冠脉血管有关。     

年龄对小家鼠筑巢的影响

为研究不同年龄组小家鼠筑巢能力的差异,分别采用24-h等级法和连续4d巢材获取重量法,对幼年组、亚成年组、成年组小家鼠筑巢能力进行了测定。结果表明:1)小家鼠在亚成年期已具备较强的筑巢能力;2)成年组与亚成年组小家鼠能够快速完成筑巢,24h即可筑成稳定的杯状巢,而幼年组未能筑成稳定巢;3)小家鼠雄性与雌性筑巢能力相当;4)连续4d巢材获取重量表现为成年组>亚成年组,这与两组间身体大小有关,而4d后两组间筑巢等级无显著差异。研究结果提示,不同年龄组的小家鼠均有较强的筑巢需求,筑巢能力基本形成于亚成年期。     

小鼠精母细胞联会复合体RNA组分的电镜研究

本文运用常规染色和Bernhard染色方法对切片标本中小鼠粗线期精母细胞联会复合体(SC)的超微结构和电镜细胞化学特点进行了研究。经常规染色后,可见SC由侧生组分(LE)、中央组分(CE)和L-C纤维组成;SC宽约210nm,LE宽约60nm,中央间隔区宽约90nm。在Bernhard染色标本中,SC的LE、CE和L-C纤维着色较深,说明其中含有RNA;SC各结构组分的宽度和形态特点与常规染色标本中的基本一致。本文讨论了SC中存在有RNA等问题。     

Counterselection on sex chromosomes in the Mus musculus European hybrid zone

The extent to which alleles can disperse across a hybrid zone depends on the selection they are subjected to in the hybrid genetic background or, for those that are selectively neutral, on their ability to escape from the unfavourable environment by recombination. Three markers spanning a 45 cM segment in the center of the X chromosome were used to investigate the degree to which selection against X chromosome linked genes helps to maintain the barrier to gene flow in the hybrid zone between Mus musculus domesticus and M. m. musculus in Denmark. The introgression of all the sex chromosome specific markers was more limited than that of the autosomal enzymes (Idh1, Amy, Gpd1, Pgm1, Es1, Es2, Mpi, Np1, Es10, Sod1) and the mitochondrial DNA. The cline for DXPas2, which is in the center of the X chromosome, is extremely steep and shows that certain genes located in this region are strongly selected against in the hybrid background. The clines of the other two X-linked markers, Hprt and DXPas1, and of the Y chromosome are not as abrupt and all three have similar asymmetric introgression patterns. Although the musculus variants appear to behave in much the same way as those of the autosomal genes, the domesticus variants do not introgress. The results show that X-linked and to a lesser extent Y-linked genes are more strongly selected against in the hybrid genome than the mitochondrial genome or the different autosomal loci. This suggests that co-adapted gene systems involving the sex chromosomes may play an important role in the hybrid breakdown between the two subspecies.     

小家鼠和实验小鼠遗传特性的比较研究

本文用同工酶电泳法、微量细胞毒法和免疫双向扩散法对我国4个动物地理区的6个采集点的156个小家鼠(Mus musculus)进行了遗传特性的调查。结果发现:在全部被测的13个位点中,小家鼠在7个位点上存在着多种实验小鼠中罕见的基因组成;而不同动物地理区和亚区的小家鼠的遗传特性又各不相同。从而指出将小家鼠的特有基因导入实验小鼠,培育新品系的重大意义。     

Expression of glucose phosphate isomerase in interspecific hybrid (Mus musculus × Mus caroli)

Hybrid Mus musculus × Mus caroli embryos were produced by inseminating M. musculus (C57BL/Ola Ws) females with M. caroli sperm. Control M. caroli embryos developed more rapidly than did control M. musculus embryos and implanted approximately 1 day earlier. At 1 1/2 days, both the hybrid embryos and those of the maternal species (M. musculus) had cleaved to the 2-cell stage. By 2 1/2 days some of the hybrids were retarded compared to M. musculus, and by 3½ days most were lagging behind. This is consistent with the idea that the rate of development of hybrid embryos declines once it becomes dependent on embryo-coded gene products. We have used this difference in rate of preim-plantation development, between hybrid and M. musculus embryos, to try to determine whether the activation of embryonic Gpi-1s genes, that encode glucose phosphate isomerase (GPI-1), is age-related or stage-related. In control M. musculus embryos (both mated and Al groups), the GPI-1AB and GPI-1A allozyme, indicative of paternal gene expression, were detected in 7 of 9 samples of 3 1/2-day compacted morula stage embryos and were seen in all 19 samples of 31/2-day blastocysts. In hybrid embryos, these allozymes were detected 1 day later. They were not detected in any 31/2-day samples (12 samples of compacted morulae) but were consistently detected at 4½ days (4 samples of blastocysts and 2 samples of uncompacted morulae). Our interpretation of the results is that gene activation in hybrid embryos is stage-specific, rather than age-specific, and probably begins around the 8-cell stage, with detectable levels of enzyme accumulating later. Analysis of GPI-1 elec-trophoresis indicated that both the paternal (M. caroli) and maternal (M. musculus) Gpi-1s alleles were equally expressed in hybrid embryos and that the paternally derived allele was not activated before the maternally derived allele. © 1992 Wiley-Liss, Inc.     

Phylogeography of Chinese house mice (Mus musculus musculus/castaneus): distribution,routes of colonization and geographic regions of hybridization

House mice (Mus musculus) are human commensals and have served as a primary model in biomedical, ecological and evolutionary research. Although there is detailed knowledge of the biogeography of house mice in Europe, little is known of the history of house mice in China, despite the fact that China encompasses an enormous portion of their range. In the present study, 535 house mice caught from 29 localities in China were studied by sequencing the mitochondrial D‐loop and genotyping 10 nuclear microsatellite markers distributed on 10 chromosomes. Phylogenetic analyses revealed two evolutionary lineages corresponding to Mus musculus castaneus and Mus musculus musculus in the south and north, respectively, with the Yangtze River approximately representing the boundary. More detailed analyses combining published sequence data from mice sampled in neighbouring countries revealed the migration routes of the two subspecies into China: M. m. castaneus appeared to have migrated through a southern route (Yunnan and Guangxi), whereas M. m. musculus entered China from Kazakhstan through the north‐west border (Xinjiang). Bayesian analysis of mitochondrial sequences indicated rapid population expansions in both subspecies, approximately 4650–9300 and 7150–14 300 years ago for M. m. castaneus and M. m. musculus, respectively. Interestingly, the migration routes of Chinese house mice coincide with the colonization routes of modern humans into China, and the expansion times of house mice are consistent with the development of agriculture in southern and northern China, respectively. Finally, our study confirmed the existence of a hybrid zone between M. m. castaneus and M. m. musculus in China. Further study of this hybrid zone will provide a useful counterpart to the well‐studied hybrid zone between M. m. musculus and Mus musculus domesticus in central Europe.     

Morphometric stepwise discriminant analysis of the five genetically determined European taxa of the genus Mus

Univariate and multivariate analyses have been performed on skull and mandible measurements for the five biochemically defined groups of the genus Mus in Europe. Four of these taxa occur in Bulgaria; other samples came from France and Israel. This extensive biometrical analysis has allowed us to establish diagnostic keys for these taxa.     

重组小鼠血管内皮生长因子在毕赤酵母菌中的表达和纯化

目的：建立毕赤酵母重组小鼠血管内皮生长因子（mVEGF）的制备方法,为研究mVEGF的生物活性、抗原性等提供基础。方法：通过全基因合成方法获得编码mVEGF的基因片段,将其克隆至表达载体pPICZaA上,电转化整合到毕赤酵母GS115基因组中,用甲醇诱导表达目的蛋白,表达上清经硫酸铵沉淀、SephadexG25柱脱盐、阳离子交换层析三步纯化获得目的蛋白;用还原型和非还原型SDS-PAGE检测目的蛋白的聚体状态,用Westelqq印迹验证纯化蛋白;通过PNGaseF酶切分析目的蛋白的N-糖基化修饰;通过人脐静脉内皮细胞（HUVEC）增殖实验检测目的蛋白的生物活性。结果：获得mVEGF的重组毕赤酵母表达菌株,SDS-PAGE分析可见GSll5表达的重组mVEGF在还原状态下表观相对分子质量约为20×10^3,在非还原状态下约为40×10^3;经Western印迹检测,这些条带均为目的蛋白条带,能被兔抗mVEGF抗体特异性结合,PNGase F酶切后相对分子质量降至18×10^3左右,证明目的蛋白发生了Ⅳ-糖基化修饰;细胞测活实验表明,mVEGF具有刺激HUVEC增殖的生物活性。结论：利用毕赤酵母菌制备了具有生物活性的重组mVEGF。