Excitotoxic injury profiles of low-affinity kainate receptor agonists in cortical neuronal cultures.

Neurotoxic profiles of putative agonists for low-affinity kainate subtypes of L-glutamate receptors (GluR5-7) were determined in cultured cortical neurones. Rank order of neurotoxic potency (microM): (S)-5-iodowillardiine (9) approximately = (2S,4R,6E)-2-amino-4-carboxy-7-(2-naphthyl)hept-6-enoic acid (LY339434, 11) > (2S,4R)-4-methylglutamate (33) > kainate (100) > (RS)-2-amino-3-(hydroxy-5-tert-butylisoxazol-4-yl)propanoic acid (ATPA, 360). Using ionotropic glutamate receptor antagonists, neurotoxicity induced by kainate, ATPA and (S)-5-iodowillardiine appeared to involve a GluR5-7 component, unlike LY339434 and (2S,4R)-4-methylglutamate. These putative GluR5-7 agonists exhibited complex excitotoxic profiles highlighting the importance of studying native glutamate receptors.     

Excitotoxic profile of LY339434, a GluR5 agonist, in cultured murine cortical neurons

The neurotoxic profile of (2S,4R, 6E)-2-amino-4-carboxy-7-(2-naphthyl)hept-6-enoic acid (LY339434), a low-affinity kainate receptor subtype 5 (GluR5) agonist at recombinant human glutamate receptors, was evaluated to investigate the involvement of GluR5 in excitotoxic neuronal death. Murine cortical neurons were exposed to treatments for 24 h and assessed by a cell viability assay and phase-contrast microscopy. LY339434 (1-1000 microM) caused a concentration-dependent decrease in cell viability (EC(50)=11.4+/-1.2 microM) that was only attenuated by (5R, 10S)-(+)-5-methyl-10,11-dihydro-5H-dibenzo[a,d]cyclohepten-5, 10-imine (MK-801, 10 microM), but not by 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX; 50 microM) or 1-(4-aminophenyl)-4-methyl-7,8-methylenedioxy-5H-2,3-benzodiazepine (GYKI 52466, 20 microM). Labeling with nucleic acid binding dyes revealed that LY339434 induced few apoptotic-like characteristics. These findings indicate that in cultured murine cortical neurons, LY339434 acts predominantly through N-methyl-D-aspartate (NMDA) receptors rather than GluR5 to effect neuronal death that is rapid and involves predominantly necrosis rather than morphological apoptosis.     

联合术式治疗女性出口处梗阻性便秘57例

1临床资料我们1999-06/2004-10收治女性出口处梗阻性便秘176例,其中耻骨直肠肌肥厚、直肠黏膜内脱垂、直肠前突三者并存57例,占32.4%,均为经产妇;年龄26～76岁,分娩1～5胎;病程1～32 a.合理的肠道及阴道准备,体位为膀胱截石位.用络合碘消毒阴道及肛管直肠腔.     

成纤维细胞生长因子2的分子结构和生物学效应

目的:成纤维细胞生长因子2是一种多功能、作用广泛的细胞因子。就成纤维细胞生长因子2分子结构和生物学效应以及与骨髓间充质干细胞移植治疗大鼠急性心肌梗死的相关研究进行综述。资料来源:应用计算机检索PubMed数据库1990-01/2006-10有关成纤维细胞生长因子2的文章,检索词“FGF-2,molecular structure,biological effect,myocardial infarction and rat and marrows tem cell”,限定文章语言种类为English。同时计算机检索中国期刊全文数据库、万方数据库1990-01/2006-10期间的相关文章,检索词“碱性成纤维细胞生长因子”,限定文章语言种类为中文。资料选择:对资料进行初审,选取符合研究要求的有关文章找全文。纳入标准:①有关成纤维细胞生长因子2分子结构、生物学特性的研究。②有关骨髓间充质干细胞移植治疗急性心肌梗死的研究。资料提炼:共收集到34篇有关成纤维细胞生长因子2分子结构和生物学效应的文章,67篇有关骨髓间充质干细胞移植治疗大鼠急性心肌梗死的研究。选取其中31篇归纳总结。资料综合:①成纤维细胞生长因子2在人体内普遍存在,许多体外培养的细胞也自分泌成纤维细胞生长因子2。成纤维细胞生长因子2包括18000的低相对分子质量成纤维细胞生长因子2和高相对分子质量成纤维细胞生长因子2。成纤维细胞生长因子2翻译的起始密码子有两种:AUG和CUG。②成纤维细胞生长因子2有两种不同的受体,它们可与相应的受体结合发挥生物学功能。③在体外培养骨髓间充质干细胞的过程中,成纤维细胞生长因子2可促进其向心肌样细胞分化,在相对缺氧的环境下,提高心肌样细胞存活率。结论:成纤维细胞生长因子2作为一种多功能的细胞生长因子,在胚胎发育,创伤修复以及缺血、炎症、肿瘤等情况下,可作用于靶细胞上的特异性受体,发挥多种生理功能。它对新生血管形成过程中的毛细血管基底膜降解、内皮细胞迁移增殖、胶原合成及小血管腔形成等均有明显的促进作用。在相对缺氧的环境下,成纤维细胞生长因子2提高心肌样细胞存活率。     

应用质谱、红外光谱及核磁共振解析验证合成物9,10-二羟基硬脂酸的纯化性

目的：为获得大量的9,10-二羟基硬脂酸（Dihydroxy Stearic Acid,DHSA）,应用质谱、红外光谱及核磁共振解析验证合成物为DHSA。 方法：实验于2007-01/05在解放军总医院营养科实验室完成。在烧瓶中加入油酸后,再加入甲酸、过氧化氢,并不断搅拌。在整个反应过程中维持反应温度在40℃,反应四五小时后,反复水洗油层并收集。在油层中加入3mol/L NaOH溶液25mL,于100℃水浴加热1h,趁热加入3mol/L HCl50mL,剧烈搅拌,析出白色沉淀。用水反复清洗使清洗液pH值为中性,收集沉淀物。在沉淀物中加入体积分数为0.95的乙醇10mL,加热溶解,抽滤,将滤液于0℃析出结晶,抽滤,将抽滤物用体积分数为0.95的乙醇10mL加热溶解,于0℃结晶,抽滤。同样方法再结晶2次,最后得到白色结晶物,晾干,收率68.8%。将结晶物分别上FTS-65A红外光谱仪、ISONS EA1108型元素分析仪,Varian INOVA 600型核磁共振仪,安捷伦XCR-trap液相质谱（LC-MS）联用仪进行分析和结构鉴定。 结果：①LC-MS分析提示合成的DHSA经过多次重结晶后,纯度较高,可达95%。MS分析提示DHSA相对分子质量为315.1,与理论值316.48相近。②DHSA元素分析实验值C68.78%,H11.53%,与理论值C68.77%,H11.58%接近。③红外光谱分析提示DHSA为含有两个羟基的十八碳长链脂肪酸。④核磁共振的氢谱和碳谱均证实合成的化合物为9,10-二羟基十八碳脂肪酸。 结论：合成的DHSA经过3次重结晶后,纯度可95%以上,质谱、红外光谱及核磁共振解析结果证实合成的化合物是9,10-二羟基硬脂酸。     

阿魏酸钠对乙醇所致小鼠肝脏抗氧化功能改变的拮抗作用

研究了不同剂量乙醇对小鼠抗氧化和解毒功能的影响以及阿魏酸钠的拮抗作用。结果表明,大剂量乙醇(11.4g·kg^-1ig)引起肝脏GSH-Px活性升高的同时,肝脏GSH-Re,SOD和GST活性降低,GSH耗竭,而血清GST升高;阿魏酸钠(100mg·kg^-1ig,qd×10)预处理则明显拮抗大剂量乙醇所致的上述改变。表明阿魏酸钠对急性乙醇所致肝损害具有良好保护作用,其机理可能与提高GSH氧化还原酶功能、增加SOD活性和增强GSH结合反应有关。研究结果还提示,血清GST水平是反映乙醇性肝损害的灵敏指标。     

A yeast model of Down syndrome

The recent discovery that cellular proliferation was reduced in aneuploid haploid yeast supports a long-standing argument that the developmental neurophenotype of Down syndrome is not uniquely a result of the effects of increased gene dosage. Instead, some phenotypic outcomes appear to resemble those caused by disrupted cellular homeostasis induced by aneuploidy. Decreased cellular proliferation has been identified in the cerebellum and hippocampus of Down syndrome mouse models and in the post-mortem hippocampus and germinal matrix of Down syndrome fetuses. Consistent with predominantly stochastic gene expression and increased energy demands induced by aneuploidy, the “buffering” canalization processes in Down syndrome would be reduced thereby giving rise to increased variance to less stable developmental pathways such as proliferation. The nature and extent of phenotypes due to reduced canalization would depend on the tissue; which is also a question for future research to address. A conceptual model is presented here to demonstrate the nature of influences affecting phenotypes. Ultimately, in Down syndrome, exigent periods of neurodevelopment increasingly appear to reflect the burden of disrupted homeostasis.     

Serum creatinine is a poor marker of glomerular filtration rate in patients with spina bifida

Serum creatinine is used to estimate the glomerular filtration rate (GFR). The serum creatinine, however, may not accurately reflect the GFR in spina bifida patients, who often have decreased overall muscle mass resulting from spinal cord abnormalities. The relationship between the serum creatinine and GFR (obtained by [¹²⁵I]iothalamate clearance) was examined in a population of spina bifida patients. Age-matched patients without spina bifida were used as controls. Results demonstrate that, for serum creatinines above 0.5 mg/dL, serum creatinine is a very poor predictor of GFR. Two patients with serum creatinines of 2.2 mg/dL are near end-stage renal disease with GFRs of 12.5 and 13 mL/minute per 1.73m^z and two patients were initiated on dialysis at the conclusion of the study. It is concluded that obtaining a GFR from a clearance study and not serum creatinine is the only reliable method to assess renal function in spina bifida patients once the serum creatinine is greater than 0.5 mg/dL.