原发性血小板减少性紫癜模型小鼠血浆内皮素水平与加味小柴胡颗粒及其组方的干预

目的:建立原发性血小板减少性紫癜动物模型,观察加味小柴胡颗粒及其组方对造模小鼠血浆内皮素含量的调节。方法:实验于2006-07/12在南京中医药大学第一临床医学院实验中心完成。①实验动物与药品:选取SPF级BALB/C小鼠54只,随机数字表法分为5组:正常组10只、模型组12只、加味小柴胡颗粒组11只、小柴胡颗粒组11只、丹参三七颗粒组10只。小柴胡颗粒主要成份为柴胡、黄芩、法半夏、党参、炙甘草、生姜、大枣,每克颗粒含生药5.45g;丹参三七颗粒每克含生药2g;加味小柴胡颗粒:在小柴胡颗粒主要成份上添加丹参、三七,每克颗粒含生药4.18g;均由天江制药厂提供。②实验方法:除正常组外,各组均建立原发性血小板减少性紫癜动物模型。造模后7d灌胃给药,加味小柴胡颗粒组给予加味小柴胡颗粒16.7g生药/kg体质量,小柴胡颗粒组给予小柴胡颗粒13.8g生药/kg体质量,丹参三七颗粒组给予丹参三七颗粒4.4g生药/kg体质量,正常组及模型组均给予等容积蒸馏水。每天给药1次,共给药14d。③实验评估:各组小鼠眼球取血,分离血浆,取上清液用放射免疫法测定血浆内皮素含量。结果:54只BALB/C小鼠均进入结果分析。与正常组比较,模型组血浆内皮素含量明显升高(P<0.05)。与模型组比较,加味小柴胡颗粒组、丹参三七颗粒组明显下降(P<0.05),而小柴胡颗粒组无明显变化(P>0.05)。结论:原发性血小板减少性紫癜血管内皮功能异常,表现为血浆内皮素明显升高,加味小柴胡颗粒及丹参三七颗粒均对其有下调作用,而小柴胡颗粒无影响。     

不同孔径纳米羟基磷灰石人工骨修复兔桡骨缺损效果比较

目的:纳米级的羟基磷灰石材料与人体内组织成分更为相似,具有更佳的生物性能。评价不同孔径的多孔纳米羟基磷灰石人工骨的骨缺损修复能力,从而筛选出适合的孔径以达到骨传导功能与生物力学性能的良好统一。方法:实验于2005-10/2006-10在深圳市第二人民医院中心实验室完成。①实验材料:纳米羟基磷灰石人工骨以硝酸钙和磷酸二氢铵为原料,采用溶胶-絮凝法制备粉体,运用压力成型、木模成型和浸渍成型分别制得孔隙分布均匀的孔径分别为50～150μm、100～250μm和300～500μm的多孔纳米羟基磷灰石人工骨。②实验动物:雄性新西兰大白兔60只随机分为植入50～150μm孔径材料组、植入100～250μm孔径材料组、植入300～500μm孔径材料组、空白对照组,每组15只。实验过程中对动物处置符合动物伦理学要求。③实验方法:制备双侧桡骨骨缺损动物模型,然后用3种不同孔径的纳米羟基磷灰石人工骨材料植入骨缺损处进行修复,空白对照组不植入任何材料。④实验评估:术后4,8和12周分别行大体标本观察、X射线片观察、扫描电镜观察及生物力学测试,比较各组材料修复骨缺损的能力。结果:实验动物均进入结果分析。①X射线片检查结果:术后4周、8周、12周,植入100～250μm孔径材料组X射线评分高于植入50～150μm,300～500μm孔径材料组,差异有显著性意义(P<0.05)。②生物力学检测结果:术后4周、8周、12周,植入100～250μm孔径材料组生物力学强度高于植入50～150μm,300～500μm孔径材料组,差异有显著性意义(P<0.05)。③扫描电镜观察结果:植入100～250μm孔径材料组成骨效果明显优于植入50～150μm,300～500μm孔径材料组和空白对照组。结论:纳米羟基磷灰石人工骨具有良好的成骨能力,但其骨修复能力受孔径因素的影响,孔径100～250μm的纳米羟基磷灰石人工骨材料成骨能力较好。     

单侧输尿管梗阻大鼠肾脏组织基质金属蛋白酶3、基质金属蛋白酶2和金属蛋白酶组织抑制因子2的表达及益气活血法的影响

目的:肾间质纤维化是肾脏疾病进展到肾功能衰竭的共同通路。通过观察益气活血法中药制剂对肾间质纤维化大鼠肾组织基质金属蛋白酶3,基质金属蛋白酶2和金属蛋白酶组织抑制因子2表达的影响,探讨其抗肾间质纤维化的作用机制。方法:实验于2006-12/2007-06在首都医科大学解剖与组织胚胎学系实验室完成。①实验动物:Wistar雄性大鼠30只,采用随机数字法分为模型组、西药蒙诺组、中药小剂量组、中药中剂量组、中药大剂量组和假手术组。实验过程中对动物处置符合动物伦理学要求。②实验方法:其中前5组行单侧输尿管梗阻致肾小管间质纤维化模型手术,假手术组打开大鼠腹腔后,分离其左侧输尿管,不结扎即关闭腹腔。益气活血法中药制剂主要由生黄芪,当归,赤白芍,丹参,黄芩,车前草,牛膝等组成。西药组、中药小剂量组、中药中剂量组和中药大剂量组于手术前2d开始灌胃给药,1次/d,其药量分别为:西药组蒙诺10mg/(kg·d)、小剂量组0.018mL/(kg·d)、中剂量组0.036mL/(kg·d)、大剂量组0.072mL/(kg·d),连续给予2周。模型组及假手术组用相同体积的生理盐水灌胃。③实验评估:6组大鼠于术后14d麻醉后处死,观察梗阻肾脏病理改变,并用免疫组织化学方法检测肾组织对基质金属蛋白酶2、基质金属蛋白酶3和金属蛋白酶组织抑制因子2的表达,通过医学病理图像分析系统对基质金属蛋白酶2、基质金属蛋白酶3和金属蛋白酶组织抑制因子2的积分光密度进行统计学分析。结果:30只大鼠全部进入结果分析。肾组织切片免疫组织化学方法结果显示:基质金属蛋白酶2、基质金属蛋白酶3和金属蛋白酶组织抑制因子2主要表达部位在肾小管上皮,少量表达在肾间质和肾小球。基质金属蛋白酶2和基质金属蛋白酶3在模型组的表达较假手术组明显减弱,两组间积分光密度比较差异有显著性意义(P<0.05);中药大、中剂量组及西药蒙诺组的表达较模型组显著增强,积分光密度差异有显著性意义(P<0.05)。金属蛋白酶组织抑制因子2在模型组的表达较假手术组显著增强,两组间积分光密度比较差异有显著性意义(P<0.05);中药大、中剂量组及西药蒙诺组的表达较模型组有所减弱,两组间积分光密度比较差异有显著性意义(P<0.05);中药小剂量组无论基质金属蛋白酶2和基质金属蛋白酶3还是金属蛋白酶组织抑制因子2的表达与模型组相比均较为相似,两组间积分光密度比较差异无显著性意义(P>0.05)。结论:大鼠输尿管梗阻后呈现出的病理损害可能和肾组织基质金属蛋白酶3,基质金属蛋白酶2与金属蛋白酶组织抑制因子2的表达失衡有关,益气活血法可以上调基质金属蛋白酶2,基质金属蛋白酶3的表达,下调金属蛋白酶组织抑制因子2的表达,显示在抑制或延缓肾间质纤维化的进程中具有一定的作用。     

转化生长因子β细胞内信号转导负调控蛋白Smad6，7在肾间质纤维化大鼠肾脏表达与益气活血法的影响

目的:观察肾间质纤维化大鼠肾组织中转化生长因子β细胞内信号转导负调控蛋白Smad6,7表达变化与益气活血法中药制剂的影响。方法:实验于2006-12/2007-06在首都医科大学解剖与组织胚胎学系实验室完成。①实验动物:Wistar雄性大鼠30只,采用随机数字法随机分为模型组、中药大剂量组、中药中剂量组、中药小剂量组、西药蒙诺组、假手术组,每组5只。益气活血法中药提取液(生黄芪15g,当归10g,赤白芍10g,丹参30g,黄芩10g,车前草15g,牛膝15g等)经水提醇沉得4.4kg/L生药提取液。实验过程中对动物处置符合动物伦理学要求。②实验方法:其中前5组行单侧输尿管梗阻致肾小管间质纤维化模型手术。假手术组打开大鼠腹腔后分离左侧输尿管,并不结扎即关闭腹腔。中药大剂量组、中药中剂量组、中药小剂量组、西药蒙诺组,于手术前2d给予灌胃给药0.072mL/(kg·d),0.036mL/(kg·d),0.018mL/(kg·d),10mg/(kg·d),1次/d,连续2周。模型组及假手术组用相同体积的生理盐水灌胃。③实验评估:6组大鼠于术后14d麻醉后处死,观察梗阻肾组织病理改变,用免疫组化方法检测肾组织Smad6,7蛋白表达,通过医学病理图像分析系统对Smad6,7蛋白的积分光密度进行统计学分析。结果:30只大鼠全部进入结果分析。苏木精-伊红染色显示模型组肾小管上皮细胞萎缩,大部分肾小管管腔扩张,间质纤维组织增生,大量炎性细胞浸润,肾小球数目明显减少。中药大剂量组、中剂量组、西药蒙诺组较模型组肾间质炎性细胞浸润、纤维组织增生、肾小管扩张情况明显减轻。Smad6,7蛋白主要在肾皮质肾小管上皮细胞内表达,在模型组它们的表达较假手术组明显减弱且分布面积减少,两组间积分光密度差异具有统计学意义(P<0.05);中药中剂量组、大剂量组、西药蒙诺组Smad6,7蛋白的表达较模型组明显增强、面积增加,积分光密度差异具有统计学意义(P<0.05)。结论:益气活血法可以通过诱导肾组织Smad6,7蛋白表达而抑制肾间质纤维化。     

性腺切除及急性饥饿对大鼠垂体-甲状腺功能的影响

本实验采用性腺摘除或经假摘除手术的两性SD大鼠,其中部分动物分别予以睾酮(T)或雌二醇(E_2),观察它们在急性饥饿或非饥饿状态下血清T_4、TSH与T浓度变化。结果提示急性饥饿可使雄鼠甲状腺合成或分泌T_4和性腺分泌睾酮减少,从而不完全地抑制了雄激素所介导的对垂体TSH分泌的兴奋作用。外源性T替代虽然可以使去势雄鼠血清T浓度恢复正常,但却无兴奋TSH分泌的作用;饥饿组去势雄鼠接受外源性T后血清TSH更为减少。提示外源性T可抑制此组雄鼠垂体TSH合成及(或)释放。     

Fractionation of Spatial Memory in GRM2/3 (mGlu2/mGlu3) Double Knockout Mice Reveals a Role for Group II Metabotropic Glutamate Receptors at the Interface Between Arousal and Cognition

Group II metabotropic glutamate receptors (mGluR2 and mGluR3, encoded by GRM2 and GRM3) are implicated in hippocampal function and cognition, and in the pathophysiology and treatment of schizophrenia and other psychiatric disorders. However, pharmacological and behavioral studies with group II mGluR agonists and antagonists have produced complex results. Here, we studied hippocampus-dependent memory in GRM2/3 double knockout (GRM2/3^−/−) mice in an iterative sequence of experiments. We found that they were impaired on appetitively motivated spatial reference and working memory tasks, and on a spatial novelty preference task that relies on animals'' exploratory drive, but were unimpaired on aversively motivated spatial memory paradigms. GRM2/3^−/− mice also performed normally on an appetitively motivated, non-spatial, visual discrimination task. These results likely reflect an interaction between GRM2/3 genotype and the arousal-inducing properties of the experimental paradigm. The deficit seen on appetitive and exploratory spatial memory tasks may be absent in aversive tasks because the latter induce higher levels of arousal, which rescue spatial learning. Consistent with an altered arousal–cognition relationship in GRM2/3^−/− mice, injection stress worsened appetitively motivated, spatial working memory in wild-types, but enhanced performance in GRM2/3^−/− mice. GRM2/3^−/− mice were also hypoactive in response to amphetamine. This fractionation of hippocampus-dependent memory depending on the appetitive-aversive context is to our knowledge unique, and suggests a role for group II mGluRs at the interface of arousal and cognition. These arousal-dependent effects may explain apparently conflicting data from previous studies, and have translational relevance for the involvement of these receptors in schizophrenia and other disorders.     

Differential transport of platinum compounds by the human organic cation transporter hOCT2 (hSLC22A2)

Background:

Solute carriers (SLCs), in particular organic cation transporters (OCTs), have been implicated in the cellular uptake of platinum-containing anticancer compounds. The activity of these carriers may determine the pharmacokinetics and the severity of side effects, including neuro- and nephrotoxicity of platinum-based chemotherapy. As decreased drug accumulation is a key mechanism of platinum resistance, SLCs may also contribute to the development of resistance. Here, we define the role of hSLC22A2 (OCT2) in the cellular uptake of platinum compounds.

Experimental approach:

Human embryonic kidney (HEK) 293 cells stably expressing the hSLC22A2 gene (HEK293/hSLC22A2) were used in platinum accumulation studies. Following a 2 h exposure to various platinum compounds (100 µM), intracellular platinum levels were determined by flameless atomic absorption spectrometry.

Key results:

HEK293/hSLC22A2 cells, compared with HEK293/Neo control cells, displayed significant increases in oxaliplatin (28.6-fold), Pt[DACH]Cl₂ (20.6-fold), ormaplatin (8.1-fold), tetraplatin (4.5-fold), transplatin (3.7-fold) and cisplatin (1.3-fold), but not carboplatin. SLC22A2-mediated transport could be inhibited by 1-methyl-4-phenylpyridinium. Furthermore, hSLC22A2-mediated oxaliplatin and cisplatin accumulation was time- and concentration-dependent, but non-saturable. Expression of hSLC22A2 in HEK293 cells resulted in enhanced sensitivity to oxaliplatin (12-fold) and cisplatin (1.8-fold). Although, hSLC22A2 mRNA expression was frequently found in ovarian cancer cell lines, its expression in clinical ovarian cancer specimens (n= 80) was low and did not correlate with the treatment outcome of platinum-based regimens.

Conclusions and implications:

The hSLC22A2 drug transporter is a critical determinant in the uptake and cytotoxicity of various platinum compounds, particularly oxaliplatin.     

麦冬类中药组织切片计算机三维重建图鉴

利用计算机技术实现麦冬类中药组织连续切片三维重建与动态显示,为计算机辅助生药学鉴定和教学提供了新的三维图像技术和研究资料。