循环加载作用下皮肤应力软化的连续介质模型

皮肤组织作为富含纤维的非均匀材料,具有复杂的力学特性．皮肤组织在循环加载作用下,随着循环次数的增加,加载过程的应力响应逐渐降低,并最终达到不随循环次数增加而改变的稳定状态,这种现象被称为应力软化行为．本文对加载过程中纤维的延展机制对宏观力学响应的影响进行研究,认为在外界载荷较小时该机制主导了宏观层次上的应力软化行为,随着外界载荷的增大,拉伸过程中微观结构损伤的演化开始产生影响,而且此时内部微观结构的演化由两种机制共同影响,据此建立了连续介质模型,将宏观尺度上应力软化行为和微观结构的演化相关联．将所获得的应力响应理论结果与猪离体头部皮肤在循环加载作用下的实验结果进行对比分析,证明了该模型能够合理地描述皮肤组织在循环加载作用下的应力软化行为．     

马氏珠母贝(Pinctada martenssi Dunker)外套膜组织培养基的设计

分析了培养基中的小牛血清、贝血清、水解乳蛋白等几种天然成分和合成培养基ＴＣ１９９对中国马氏珠母贝外套膜组织细胞在体外的生长情况和珍珠质分泌功能的影响，并确定了它们在组成培养基时的适宜含量．其中，贝组织提取物、鸡胚汁对细胞的生长和珍珠质的分泌具有十分重要的作用；５％的小牛血清和１０％的贝血清共同使用对维持细胞形促进细胞生长有很好的作用，但单独使用则有一定的负作用．     

牙齿组织光热动态特性仿真与试验研究

调制激光作用牙齿组织发生散射形成光子密度波, 而由于光热效应产生热波, 基于一维介质辐射传输漫射近似方程与一维热传导方程建立了调制激光作用牙齿组织半透明混合介质的一维热波数学模型. 利用该模型仿真分析了牙齿龋损特性参数(牙釉质龋损层光吸收系数、散射系数、热扩散系数及龋损深度)对光热辐射动态响应特性的影响与规律. 利用红外探测器(HgCdTe, 2–12 μm)记录808 nm半导体激光激发牙齿组织产生的热波信号, 由锁相放大器计算热波信号的幅值与相位. 通过频率扫描试验获得了牙齿组织的光热动态响应, 利用多参数最佳统计拟合方法得到了牙齿组织特性参数. 结果表明光热辐射测量对牙齿组织不均匀性和龋损特性均具有较高敏感性与特异性.     

频域近红外光谱法研究生物组织内部光子传输特性

基于光子在生物组织中的辐射传输理论以及Feng模型,应用频域近红外光谱法研究生物组织中异质体位置的变化,对出射光的光强和相位变化的影响及规律。设计了一仿真实验,用牛奶代替强散射性质的生物组织,并在牛奶中放置一个高度可控的具有一定吸收系数和散射系数的小球。移动小球在牛奶中的高度,检测出射光的交流幅度AC、直流光强DC和相位延迟Phase的值,绘制小球位于不同深度时AC,DC和Phase的曲线,并探讨其变化规律。结果表明,随着小球在牛奶中深度的变化,光强AC,DC和相位Phase呈现一定的相关性;随着光源和检测器之间距离的增加,检测到的光强和相位曲线的波谷点均向右偏移;当小球偏离光源和检测器越远,对检测到的光强和相位的影响越小。验证了光子在生物组织中的传输规律,为用频域近红外光谱法进行组织光学参数的检测及组织中异质体位置的定位奠定了基础。     

聚乳酸组织工程支架结构的精密调控

采用糖球模板法结合热致相分离技术,制备了孔径尺寸、内连通度及孔隙率高度可控的左旋聚乳酸(PLLA)支架材料,并通过扫描电镜(SEM)、红外光谱(FTIR)以及示差扫描量热法(DSC)对其空间结构及性能进行了系统研究.支架材料孔径从50μm到800μm及内连通孔径从10μm到200μm连续可调,微观孔壁结构根据不同溶剂可形成各异的微纳米结构.支架的制备对PLLA化学结构无显著影响,但相分离过程会不同程度地降低PLLA的结晶度.     

Application of a liquid chromatography–tandem mass spectrometry method to the pharmacokinetics,tissue distribution and excretion in the study of anemoside B4, a novel antiviral agent candidate,in rats

A simple, sensitive and reliable LC–MS/MS method was developed and validated for the quantification of anemoside B4, a potential antiviral constituent isolated from Pulsatilla chinensis in rat plasma, tissue, bile, urine and feces. All biological samples were prepared by protein precipitation method, and ginsenoside‐Rg1 was chosen as the internal standard (IS). The analyte and IS were separated using a C₁₈ column (2.1 × 50 mm, 1.8 μm) and a mobile phase consisting of 0.1% formic acid in water (v /v) and acetonitrile running at a flow rate of 0.2 mL/min for 5 min. The multiple reaction monitoring transitions were monitored at m /z 1219.5–749.5 for anemoside B4 and 845.4–637.4 for ginsenoside‐Rg1 in electrospray ionization negative mode. The calibration curve was linear in the range of 10–2000 ng/mL for all biological matrices with a lower limit of quantification of 10 ng/mL. The validated method was successfully applied to a pharmacokinetics, tissue distribution and excretion study. These preclinical data will be beneficial for further development of anemoside B4 in future studies.     

新辅助化疗在软组织肉瘤治疗中的应用分析

目的研究并探讨新辅助化疗在软组织肉瘤治疗中的应用效果。方法选取2013年1月—2016年6月期间甘肃中医药大学临床医学院收治的软组织肉瘤共80例作为研究对象,采取单盲随机分组法随机分为对照组和观察组各40例,对照组实施手术治疗,观察组在手术前实施新辅助化疗,比较两组患者的保肢率、治疗效果、术后半年复发情况。结果观察组患者的保肢手术率为77.50%,对照组患者为55.00%,差异具有统计学意义(P0.05);观察组患者的治疗总有效率明显高于对照组(P0.05);术后半年随访发现,观察组的复发率明显低于对照组(P0.05);观察组患者在新辅助化疗期间未出现严重的不良反应。结论在软组织肉瘤患者行手术治疗前实施新辅助化疗,可提高患者的保肢率,提高治疗效果,减少复发,有利于改善预后。     

Tissue distribution of capilliposide B,capilliposide C and their bioactive metabolite in mice using liquid ‐tandem mass spectrometry

Lysimachia capillipes Hemsl (Primulaceae), a folk medicinal plant in China, showed significant anti‐tumor activities in vivo and in vitro . Capilliposide B (LC‐B) and capilliposide C (LC‐C) are the main bioactive components in this plant. To explore their tissue distribution, a reliable bioanalytical method for the quantification of LC‐B, LC‐C and their bioactive metabolite, capilliposide A (LC‐A), in mouse tissues was developed and validated. In this study, the tissue distribution profiles of the three compounds were examined after intravenous administration of pure LC‐B and oral administration of total saponins of L. capillipes Hemsl extract (LCE) for 10 days. Method validation was conducted over the curve range 10.0–5000 ng/mL for all three analytes in various tissue homogenates. The relative standard deviation of intra‐day and inter‐day precision of the QC samples was <14.7%, and the accuracy ranged from 85.9 to 114.0%. The results indicated that LC‐B was rapidly and widely distributed throughout the whole body except for muscle following intravenous administration of LC‐B. In addition, LC‐A was only in liver, intestine, lung and stomach. After oral administration of LCE, LC‐B and LC‐C were distributed into various tissues. The highest levels were observed in stomach and intestine.     

Development of solid‐phase microextraction coupled with liquid chromatography for analysis of tramadol in brain tissue using its molecularly imprinted polymer

In this work, performance of a molecularly imprinted polymer (MIP) as a selective solid‐phase microextraction sorbent for the extraction and enrichment of tramadol in aqueous solution and rabbit brain tissue, is described. Binding properties of MIPs were studied in comparison with their nonimprinted polymer (NIP). Ten milligrams of the optimized MIP was then evaluated as a sorbent, for preconcentration, in molecularly imprinted solid‐phase microextraction (MISPME) of tramadol from aqueous solution and rabbit brain tissue. The analytical method was calibrated in the range of 0.004 ppm (4 ng mL⁻¹) and 10 ppm (10 μg mL⁻¹) in aqueous media and in the ranges of 0.01 and 10 ppm in rabbit brain tissue, respectively. The results indicated significantly higher binding affinity of MIPs to tramadol, in comparison with NIP. The MISPME procedure was developed and optimized with a recovery of 81.12–107.54% in aqueous solution and 76.16–91.20% in rabbit brain tissue. The inter‐ and intra‐day variation values were <8.24 and 5.06%, respectively. Finally the calibrated method was applied for determination of tramadol in real rabbit brain tissue samples after administration of a lethal dose. Our data demonstrated the potential of MISPME for rapid, sensitive and cost‐effective sample analysis.