数字化大鼠动脉血管系统三维模型的建立

采用含造影剂及显色剂的填充剂对成年SD大鼠动脉血管系统进行灌注,并借助数字X射线成像设备对灌注效果进行实时监测,通过断层解剖成像系统获取切削间距为100 μm的二维断面解剖数据集(图像分辨率为4917×3446×24 bit,共1 464张),最后利用Visual C 结合可视化工具包编程实现数据集的动脉分割及三维可视化,得到数字化SD大鼠动脉血管系统的三维模型.该模型能提供大鼠动脉血管系统的空间结构信息,为实验大鼠血管系统的研究提供了更为准确可靠的形态学参考.     

Phage-displayed mimotopes recognizing a biologically active anti-HIV-1 gp120 murine monoclonal antibody

Antibody-dependent cellular cytotoxicity (ADCC) is a host defense mechanism in which Fc receptor-bearing effector cells in combination with antigen-specific antibodies recognize and kill antigen-expressing target cells. The authors previously described a murine monoclonal antibody (MAb-ID6) that mediated ADCC activity against HIV-infected cells. It was demonstrated that the specificity of MAb-ID6 maps to the first 204 amino acids of gp120; however, the exact epitope was not identified. In the present work, by screening phage display libraries with MAb-ID6, the authors have mapped the corresponding epitope to amino acids 86-100 (HIV-1 gp120 sequence). This epitope lies within the C1 region of gp120 and is highly conserved among all subtypes and circulating recombinant forms of HIV-1. Thus, these phage mimotopes of C1 may serve as components of a vaccine for the induction of gp120-specific antibodies mimicking MAb-ID6.     

Bone-specific antibodies in sera from patients with celiac disease: characterization and implications in osteoporosis

Osteopenia and osteoporosis are well-known complications detected in celiac disease patients with still obscure pathogenesis. In the present study we investigated the presence of circulating anti-bone autoantibodies in patients with celiac disease and explored their role in the associated bone disease. We evaluated serum samples from 33 patients at the time of diagnosis and from 20 of them after treatment. Sera from patients with inflammatory bowel disease (n = 9), nonceliac osteoporotic (n = 18), and healthy individuals (n = 10) were used as controls. The presence of IgA specific anti-bone antibodies was first investigated using indirect immunofluorescence on cryosections of fetal rat tibia (20-day pregnancy). Furthermore, samples were homogenized and total tissue extracts were subjected to Western blot analysis to confirm immunoreactivity. At diagnosis, sera from 51.5% (17/33) of celiac patients had antibodies that recognized antigenic structures in chondrocytes and the extracellular matrix along mature cartilage, bone interface, and perichondrium of fetal rat bone. Among controls, only two osteoporotic patients showed very low titles of anti-bone autoantibodies. The immunostaining was localized in areas where an active mineralization process occurred and was similar to the distribution of the native bone tissue transglutaminase. The frequency of patients with positive baseline titers of anti-bone antibodies diminished significantly after treatment (P = 0.048). Western blot assays confirmed the presence of autoantibodies in sera from patients with a positive immunofluorescence staining. Autoantibodies recognized a major protein band on tissue extracts with a molecular weight of 77–80 kDa, which could be displaced when sera were preadsorbed with human recombinant tissue transglutaminase. We provide original evidence that patients with celiac disease have IgA-type circulating autoantibodies against intra- and extracellular structures of fetal rat tibia. Our findings suggest that these antibodies recognize bone tissue transglutaminase as the autoantigen, and based on the localization of the immunoreactivity we speculate that they might have an active role in the pathophysiology of celiac disease-associated bone complications.     

Genetic Conservation of Hemagglutinin Gene of H9 Influenza Virus in Chicken Population in Mainland China

The hemagglutinin (HA) genes of 12 H9N2 influenza virus strains isolated from chickens in Mainland China during the period 1995–2002 were genetically analyzed. All the isolates possessed the same amino acid motif -R-S-S-R/G-L- at the cleavage site of HA. Except for the conserved amino acids, as is the case in the other avian influenza viruses, located in the receptor binding site, all of the 12 isolates possessed N at amino acid position 183; A, T, or V at position 190; K at position 137, whereas the representative strains of the other lineage (except Dk/HK/Y280/97-like lineage) virus of H9N2 viruses had H, E, and R at these positions respectively. These could be considered as the partial molecular markers of the H9 viruses isolated from chickens in Mainland China. Phylogenetic analyses showed HA genes of these isolates belonged to that of A/duck/Hong Kong/Y280/97-like virus lineage. No A/quail/Hong Kong/Gl/97-like virus was found in chicken, population since the outbreak of H9N2 influenza in Mainland China in 1992. The available evidence indicates that HA genes of H9 influenza virus circulating in Mainland China during the past years were well conserved.     

Influence of food on the intravenous and oral dose kinetics of propranolol in the dog

The intravenous and oral dose kinetics of propranolol were studied in the dog both in a fasted state and immediately after a meal consisting of 100 g of cooked beef liver. Fifty Ci of³H-propranolol was administered intravenously simultaneously with a 40-mg oral dose of unlabeled propranolol. Plasma³H-propranolol was measured by specific extraction and liquid scintillation spectrometry, and unlabeled plasma propranolol was determined by gas chromatography-mass spectrometry. Feeding significantly reduced (25%) the elimination half-life and increased (52%) the systemic clearance of intravenous propranolol. The increase in the systemic clearance of propranolol after feeding was mostly due to an increase (60%) in apparent hepatic blood flow, which appeared to remain elevated for 5–7 hr. The meal had no influence on the apparent volume of distribution or plasma binding. Feeding did not affect the area under the concentration-time curve of oral propranolol, but significantly delayed the rate of oral propranolol absorption, shifting the time to reach peak plasma levels from 60 to 158 min. The results of this study suggest that feeding alters the disposition of propranolol in the dog by producing a sustained increase in hepatic blood flow.This work was supported by National Institute of Health grants GM 07534, GM 20387, and HL 29566.     

催经止孕药Ru-486的临床药代动力学

应用高效液相色谱法(HPLC)研究了抗孕激素药,Ru-486的临床药代动力学。六名志愿受试者,一次口服Ru-486 50毫克后测得该药的药代动力学各项参数,血药半寿期t 1/2 33.0小时,一级消除速率常数Kel 0.021 hr~(-1),血药表观容积Vd 120.1 Liter,体内血药总廓清率Cl2.5 Liter/hr,药-时曲线下面积Auc 19825.1 ng/ml/hr。实验表明,服药后一小时血药浓度迅即达高峰,随后转入消除期,血浆药物浓度在消除相的头4～8小时消除较快,而后逐渐减慢,持续24小时,到48小时血药浓度已较低(0.15±0.07μg/ml)。     

1H-NMR技术结合多元统计分析鉴别降香及其伪品

目的：采用核磁共振氢谱(¹H-NMR)技术结合多元统计分析建立降香及其伪品的鉴别方法。方法：获得降香及其伪品的¹H-NMR图谱,建立全成分信息并转化为数据矩阵,检测条件为以含0.03%四甲基硅烷(TMS)的氘代二甲基亚砜(DMSO-d₆)为溶剂,恒温298 K(1 K=-272.15℃),脉冲间隔1.00 s,谱宽12 019.23 Hz,扫描数16次,采样时间1.08 s。对降香及其伪品数据矩阵进行相似度考察和层次聚类分析(HCA),采用正交偏最小二乘法-判别分析(OPLS-DA)对数据矩阵进行分析,找出降香与其伪品之间的差异性成分;建立OPLS-DA类别变量值模型,设定降香类别变量值为1,降香伪品类别变量值为0,阈值±0.3,用于市售降香的真伪鉴别;以OPLS-DA得分图确定市售降香中伪品的种类,并通过薄层色谱法(TLC)进行验证。结果：相似度分析与HCA结果表明,降香与其伪品之间差异明显;OPLS-DA发现降香与其伪品显著性差异成分为反式-橙花叔醇;建立的类别变量值模型可成功对市售降香进行真伪鉴别;OPLS-DA得...     

基于血清药物化学和网络药理学的泽漆抗慢阻肺药效物质基础分析

目的：对泽漆水提物的入血成分进行分析,探讨该水提物抗慢性阻塞性肺疾病（COPD）的药效物质基础。方法：采用超高效液相色谱-四极杆-飞行时间串联质谱法（UPLC-Q-TOF-MS/MS）检测大鼠灌胃泽漆水提物后入血成分,检测条件为Agilent RRHD SB-C18色谱柱（3 mm×100 mm,1.8μm）,流动相0.1%甲酸水溶液（A）-乙腈（B）梯度洗脱（0～15 min,5%～30%B;15～20 min,30%～50%B;20～30 min,50%～95%B;30～35 min,95%～5%B）,检测波长190～800 nm,柱温40℃,流速0.3 mL·min-1,进样量4μL,电喷雾离子源（ESI）,正、负离子模式检测,检测范围m/z 50～1 250。利用网络药理学方法对入血成分的靶点与COPD的靶点进行交互分析,通过网络拓扑分析筛选关键成分和关键靶点,运用Metascape数据库预测泽漆抗COPD主要涉及的分子功能、生物过程、细胞组成及信号通路,并采用分子对接技术判断关键靶点与关键成分的亲合力。结果：大鼠灌胃泽漆水提物后,从其含药血清中检测出了29个入血成分,9个为原...     

上海市预防接种工作人员疑似预防接种异常反应监测认知和报告影响因素

目的了解上海市预防接种工作人员疑似预防接种异常反应(Adverse events following immunization,AEFI)监测的知识和态度以及影响AEFI报告的因素。方法采用方便抽样在上海市所有459个预防接种门诊选择预防接种工作人员开展问卷调查,分析AEFI监测知识得分(满分6分)和态度,采用多因素Logistic回归分析AEFI报告的影响因素。结果1379名调查对象的AEFI监测知识平均得分为3.30±1.31分;认为开展AEFI监测有必要、报告AEFI是自身职责、AEFI监测是额外工作负担的调查对象分别占98.84%、92.75%、30.38%。69.62%的调查对象近1年报告过AEFI;社区接种门诊、免疫规划专职人员、近1年接受过AEFI培训、AEFI监测知识得分高的调查对象报告AEFI的比例高[OR(95%CI):19.55(14.16-26.98)、1.95(1.45-2.64)、3.14(1.76-5.59)、1.91(1.38-2.63)]。结论上海市预防接种工作人员AEFI监测知识水平不高,对AEFI监测存在一定认识误区;需加强AEFI监测培训,进一步提高其AEFI报告意识。