红背山麻杆化学成分的研究

采用柱色谱技术从红背山麻杆叶子的60％乙醇提取物中分离得到4个黄酮苷和2个其他类化合物.根据理化性质及波谱方法分别鉴定为:芹菜素-6-C-D-葡萄糖苷(1)、芹菜素-7-O-芸香糖苷(2)、芹菜素-7-O-β-(2″-O-α-鼠李糖基)葡萄糖醛酸苷(3)、木犀草素-7-O-α-L-鼠李糖(1→6)-β-D-葡萄糖苷(4)、没食子酸乙酯(5)、β-胡萝卜苷(6).以上化合物均为首次从该植物中分离得到,其中化合物1～4为首次从山麻杆属中分离得到的黄酮苷.     

蒙药材莲座蓟化学成分的研究

从莲座蓟(Cirsium Esculentum C.A.Mey)植物的根及根茎中分离得到6个化合物,经波谱数据分析分别鉴定为β-谷甾醇(1)、5,7-二羟基-6,4’-二甲氧基黄酮(2)、刺槐素(3)、β-胡萝卜苷(4)、蒙花苷(5)、绿原酸(6)。上述化合物均为首次从该植物中分离得到。     

头花蓼化学成分研究

从苗药头花蓼(Polygonum capitatumBuch.-Ham.ex D.Don)乙酸乙酯部位中分离得到9个化合物,根据理化性质结合波谱学技术分别鉴定为槲皮素-3-O-(4″-O-乙酰基)-α-L-鼠李糖苷(1)、槲皮素(2)、槲皮苷(3)、杨梅苷(4)、槲皮素-3-O-(2″-没食子酰基)-鼠李糖苷(5)、原儿茶酸(6)、胡萝卜苷(7)、没食子酸(8)、没食子酸乙酯(9)。其中化合物1为首次从该属植物中分得,化合物4为首次从该植物中分得。同时,对黄酮苷类化合物中鼠李糖不同位置乙酰基取代后的1HNMR和13C NMR波谱数据进行了归纳总结。     

广藿香大极性化学成分的研究

从广藿香(Pogostemon cablin (Blance)Benth.)地上部分乙醇提取物的正丁醇萃取部位分离得到13个化合物.通过光谱和波谱分析,分别鉴定为:芹菜素(1)、3,5,4'-三羟基-7-甲氧基黄酮(2)、3,5-二羟基_4',7-二甲氧基黄酮(3)、Apigenin 7-galacturonide(4)、Apigenin 7-(O-methylghacuronide)(5),Luteolin 7-O-(6-O-methyl-β-D-glucuronopyranoside)(6),4',5-二羟基-3',7-二甲氧基二氢黄酮(7)、Quercetha-7-β-D-ghcoside(8),3,23-Dihydroxy-12-oleanen-28-oic acid(9)、Syringaresinol-β-D-glucoside(10),毛蕊花糖苷(11)、列当苷(12)、紫葳新苷(13),化合物2～13均为首次从该植物中分离得到.     

吊石苣苔中的化学成分

新鲜吊石苣苔全草用70%丙酮水溶液组织破碎提取,然后经Diaion HP-20,Toyopearl HW-40,硅胶等柱色谱技术进行分离纯化得到8个化合物,经波谱分析鉴定为5,7-二羟基-6,8,4′-三甲氧基黄酮(1),丁香酸(2),邻苯二甲酸-双-(2-乙基己基)酯(3),5,7-二羟基-6,8,4′-三甲氧基黄酮醇(4),7-羟基-6,8,4′-三甲氧基-5-O--βD-葡萄糖黄酮苷(5),7-羟基-6,8,4′-三甲氧基-5-O-[-βD-葡萄糖-(1→6)]--βD-葡萄糖黄酮苷(6),4′,5-二羟基-7-甲氧基-6-C--βD-葡萄糖黄酮苷(7)和4′,5-二羟基-6,7-二甲氧基-8-C-β-D-葡萄糖黄酮苷(8)。除7-羟基-6,8,4′-三甲氧基-5-O--βD-葡萄糖黄酮苷和7-羟基-6,8,4′-三甲氧基-5-O-[β-D-葡萄糖-(1→6)]--βD-葡萄糖黄酮苷外,其余6个化合物均为首次从该植物中分离得到。     

新疆蓝刺头化学成分研究

以新疆蓝刺头(Echinops ritro L.)全草为研究材料,通过硅胶柱色谱,Sephadex LH-20柱色谱,重结晶等技术对新疆蓝刺头化学成分进行分离纯化,通过理化性质分析及1H-NMR,13C-NMR等技术对化合物结构进行鉴定.结果表明,共分离出5个化合物,分别是三萜类化合物蒲公英甾醇乙酰酯(化合物1)、蒲公英甾醇(化合物2)、黄酮苷类化合物金丝桃苷(化合物3)、胡萝卜苷(化合物4)与β-豆甾醇葡萄糖苷(化合物5).其中化合物1,2,5首次从该种植物中分离,化合物3为首次从该属植物中分离.     

贯叶连翘中的新抗真菌黄酮苷

从贯叶连翘( Hypericum perforatum L.)地上部分的80%乙醇提取物中分离得到1个新的黄酮苷和6个已知黄酮类化合物.采用红外光谱、紫外光谱、质谱和核磁共振光谱等波谱技术测得新黄酮苷的结构为6″-O-乙酰基槲皮素-3-O-β- D -阿洛糖苷(1,6″-O-acetyl quercetin 3-O-β- D -alloside),6个已知化合物分别被鉴定为槲皮苷(quercitrin)、金丝桃苷(hyperoside)、蓄苷(avicularin)、芦丁(rutin)、槲皮素(quercetin)和山萘酚(kaemferol).体外抗真菌活性实验表明,新黄酮苷(1)、槲皮苷和槲皮素对植物病原菌 Helminthosporium sativum Pamel King et Bakke具有一定的抑制作用,三者的最小抑制浓度(MIC)分别为:25、50和50 μg/mL.另外,1和槲皮苷对禾赤色镰孢霉( Fusarium graminearum Schw.)的生长也有抑制作用(MIC值均为100 μg/mL).     

虎尾草化学成分研究

从虎尾草Lysimachia barystachys地上部分中分得8个已知黄酮苷类化合物,通过波谱解析其结构分别鉴定为槲皮素(1),山奈酚(2),金丝桃苷(3)、芦丁(4)、3,5,7,3',4'-五羟基黄酮-3-O-(2,6-二-O-α-L-吡喃鼠李糖)-β-D-吡喃半乳糖苷(5),3,5,7,3',4'-五羟基黄酮-7-O-α-L-吡喃鼠李糖-3-O-α-L-吡喃鼠李糖(1-2)-β-D-吡喃葡萄糖苷(6),3,5,7,4'-四羟基黄酮-3-O-(2,6-二-O-α-L-吡喃鼠李糖)-β-D-吡喃半乳糖苷(7),3,5,7,4'-四羟基黄酮-7-O-α-L-吡喃鼠李糖-3-O-α-L-吡喃鼠李糖(1-2)-β-D-吡喃葡萄糖苷(8).这些化合物除3,4外均为首次从该植物中分离得到.     

秃叶黄皮树叶子的化学成分研究(英文)

从秃叶黄皮树叶子(Phellodendron chinensevar.glabriusculumSchneid)分离到7个化合物,经波谱解析鉴定为6-O-乙酰基黄柏苷(1),6-O-乙酰基二氢黄柏苷(2),(2R)-4′,5-二羟基-7-O-β-D-吡喃葡萄糖基-8-异戊烯基-二氢黄酮(3),黄柏苷(4),2-O-β-D-吡喃葡萄糖基-6-羟基-苯甲酸苄酯(5),柑橘素C(6),3-羰基齐墩果烷(7),其中化合物1～3,5～7为首次从秃叶黄皮树叶子中分离得到。     

茎花葱臭木化学成分的研究

从茎花葱臭木种子中分离得到5个化合物,经理化与波谱分析鉴定为β-谷甾醇(1)、没食子酸乙酯(2)、胡萝卜苷(3)、1-O-β-D-吡喃葡萄糖基-(2S,3S,4R,8Z)-2-N-(2 ′-羟基二十四烷酰氨基)十八二氧鞘氨-8-烯(4)和2,3,2″,3″-四氢穗花杉双黄酮(5).这5个化合物均首次从该植物中分离得到.其中化合物5进行细胞毒活性测试,没有显示抑制活性.     

黄酮碳苷类化合物ESIMS-MS裂解规律初探

本研究通过ESIMS-MS技术分析一系列黄酮化合物的裂解情况,探讨黄酮碳苷类化合物ESIMS-MS的裂解规律。结果表明,六碳黄酮碳苷ESIMS-MS的子离子谱图中出现[M-H-60]-、[M-H-90]-和[M-H-120]-的离子碎片;五碳黄酮碳苷ESIMS-MS的子离子谱图中只能产生脱去60和90质量单位的碎片峰。该研究表明黄酮碳苷类化合物ESIMS-MS裂解具有一定的规律性,并有助于发现微量黄酮碳苷类成分。     

Development of a sandwich ELISA assay for measuring bovine soluble type II IL-1 receptor (IL1R2) concentration in serum and milk

The IL1R is composed of two kinds of molecule, type I (IL1R I) and type II (IL1R2). IL1R1 contributes to IL-1 signaling, whereas the IL1R2 has no signaling property and acts as a decoy for IL-1. In this study, we developed a bovine IL1R2-specific sandwich ELISA to examine the sIL1R2 concentration in serum and milk from dairy cows. The concentration of colostral IL-1beta was examined to estimate the correlation to sIL1R2. The results showed that the sIL1R2 concentration in sera and milk changes with the stages of lactation. The serum sIL1R2 concentrations were 5.56+/-0.69 ng/ml (colostrum), 3.14+/-0.72 ng/ml (the early stage of lactation) and 5.76+/-1.25 ng/ml (the late stage of lactation). The milk sIL1R2 concentrations were 1.83+/-0.47 ng/ml (colostrum), 0.73+/-0.22 ng/ml (the early stage of lactation) and 2.92+/-0.56 ng/ml (the late stage of lactation). The concentrations of IL1R2 in sera and milk were significantly higher at the late stage of lactation and colostrum than that of the early stage of lactation. The reduction rates of sIL1R2 levels from the colostrum to the early stage of lactation were 43.6% (serum) and 61% (whey). IL-1beta was detected in all the colostrum (995.9+/-346.6 ng/ml). Significant correlation was observed between the levels of colostral IL-1beta and IL1R2 (r=0.75).     

脊柱-骨盆固定系统的生物力学研究

目的:研究髂骨钉在脊柱-骨盆固定系统中对腰骶稳定性及螺钉应力分布的影响。方法:6具成人腰椎-骨盆防腐标本,分别按照三种不同的固定方式完成置钉连接操作,制成3个实验组:单纯腰椎后路长节段固定组(L2-L5组)、腰骶固定组(L2-S1组)、髂骨钉固定组(L2-S1-I组)。生物力学测试采用8 N·m纯力矩执行前屈、后伸、左右侧弯、左右旋转6个工况运动,比较各固定组L2、L5水平活动度以及L5椎弓根钉、S1螺钉应力。结果:L2-S1组、L2-S1-I组内固定系统以及腰骶关节活动度均明显降低(P0.05),L2-S1-I组的优势更加显著,尤其在抵抗固定系统旋转活动以及腰骶关节前屈活动时作用更明显。L2-S1-I组、L2-S1组L5椎弓根钉应力均较L2-L5组明显减小(P0.05);L2-S1-I组S1螺钉应力较L2-S1组显著减小(P0.05)。结论:髂骨钉技术能够提供良好的脊柱-骨盆固定效果,在维持腰骶稳定性方面优势明显;对近端固定螺钉有保护作用,在与S1螺钉联合使用时,能有效分担S1螺钉所受应力,显著降低螺钉松动、拔出的风险。     

Metabolic degradation of phenazine-1-carboxylic acid by the strain <Emphasis Type="Italic">Sphingomonas</Emphasis> sp. DP58: the identification of two metabolites

The biotransformation of phenazine-1-carboxylic acid (PCA) by PCA-degrading strain Sphingomonas sp. DP58 yielded small quantities of metabolites and was demonstrated for the first time. The metabolites were isolated by using preparative high-performance liquid chromatography (HPLC). In addition, these were subsequently characterized by gas chromatography (GC)-mass spectrum (MS) after N,O-bis(trimethylsilyl)trifluoroacetamide (BSTFA) derivatization and (1)H-nuclear magnetic resonance (NMR). They were identified as 4-hydroxy-1-(2-carboxyphenyl) azacyclobut-2-ene-2-carbonitrile (HPAEC) and 4-hydroxy-1-(2-carboxyphenyl)-2-azetidinecarbonitrile (HPAC). The two metabolites had transformational relationship between each other.     

不同类型缺血性脑血管病血清VCAM-1、MMP-2、TIMP-1的表达及与神经功能缺损的关系分析

摘要 目的：探讨不同类型缺血性脑血管病血清血管细胞粘附分子-1（VCAM-1）、基质金属蛋白酶-2（MMP-2）、基质金属蛋白酶抑制剂1（TIMP-1）的表达及与神经功能缺损的关系。方法：选择2016年1月至2020年1月我院接诊的98例缺血性脑血管病患者为本研究对象,其中脑梗死55例设为脑梗死组,短暂性脑缺血发作组43例,并选择我院同期体检中心健康者50作为对照组,分析三组血清VCAM-1、MMP-2、TIMP-1水平之间的差异及不同神经缺损程度血清VCAM-1、MMP-2、TIMP-1水平、美国国立卫生研究院卒中量表（NIHSS）评分变化情况,及其之间的相关性。结果：脑梗死组血清VCAM-1、MMP-2、TIMP-1水平及NIHSS评分显著高于短暂性脑缺血发作组和对照组,差异显著（P＜0.05）;短暂性脑缺血发作组血清VCAM-1、MMP-2、TIMP-1水平及NIHSS评分显著高于对照组,差异显著（P＜0.05）;重度神经缺损组血清VCAM-1、MMP-2、TIMP-1水平及NIHSS评分显著高于中度神经缺损组和轻度神经缺损组,差异显著（P＜0.05）;中度神经缺损组血清VCAM-1、MMP-2、TIMP-1水平及NIHSS评分显著高于轻度神经缺损组,差异显著（P＜0.05）;相关性分析结果中显示,血清VCAM-1、MMP-2、TIMP-1均和NIHSS评分呈正相关（r=0.603, 0.915, 0.778,P＜0.05）。结论：血清VCAM-1、MMP-2、TIMP-1在缺血性脑血管病患者中表达异常,神经缺损越严重血清VCAM-1、MMP-2、TIMP-1表达越高。     

Genetic Polymorphisms of Sulfotransferases (SULT1A1 and SULT1A2) in a Turkish Population

Sulfotransferases (SULTs) play a significant role in the biotransformation of a variety of xenobiotics and endogenous compounds. SULTs are genetically polymorphic enzymes; to date, 12 human cytosolic SULT isoforms have been identified. This study investigated SULT1A1 and SULT1A2 gene polymorphism using a PCR-RFLP method (n = 303). The frequency of the SULT1A1*1 allele was 76.2% and SULT1A1*2 was 23.8%. The SULT1A1*3 allele could not be identified. The SULT1A2 frequencies were 69.2% (SULT1A2*1), 18.3% (SULT1A2*2), and 12.5% (SULT1A2*3). The SULT1A1 and SULT1A2 loci were in Hardy-Weinberg equilibrium (SULT1A1 χ2 = 0.58, P = 0.44; SULT1A2 χ2 = 7.28, P = 0.06). Linkage analysis indicated a close linkage between these two genes (χ2 = 5.31, P < 0.01); therefore, the statistical hypothesis that SULT1A1 and SULT1A2 alleles are independently distributed was rejected. Additionally, a strongly positive linkage was detected between SULT1A1*2 and SULT1A2*2 alleles in this population (D' = 0.79, χ2 = 33.33).     

Transformation of arylamines into direct-acting mutagens by reaction with nitrite

Arylamines including aniline (I), 1-naphthylamine (II), 2-naphthylamine (III), 2-aminofluorene (IV), 1-aminoanthracene (V) and 1-aminopyrene (VI) were treated with 4 equivalent amounts of nitrite at pH3 and 37 degrees C for 4 h. The reaction mixtures of I, IV, V and VI showed mutagenicity to Salmonella typhimurium TA98 and TA100 strains without metabolic activation. The numbers of His+ revertant colonies to TA98 strain were 110/0.05 mumole I, 970/0.055 mumole IV, 620/0.10 mumole V and 870/0.02 mumole VI. These arylamines were converted into mutagens with diazoquinone, diazonium and nitro functions depending on their structures. The mutagen from I was p-diazoquinone (I2). The mutagen from IV was highly unstable fluorene-2-diazonium salt (IV1). The mutagens from V were N3O3-introduced anthracene (V1-1) and 1-nitroanthracene (V2), and those from VI were unidentified nitro-introduced compound (VI1) and 1-nitropyrene (VI2).     

下丘脑室旁核注射GLP-1 对糖尿病大鼠中枢GLP-1 受体表达

目的:探讨下丘脑室旁核(hypothalamic paraventricular nucleus,PVN)注射GLP-1(胰高血糖素样肽-1)对糖尿病大鼠胃排空的影响及机制。方法:30只Wistar大鼠随机分为正常对照组(NC组)、糖尿病组(DM组)和GLP-1干预组(GLP-1组),每组各10只。DM组和GLP-1组腹腔注射链脲佐菌素,三组大鼠均PVN区埋置套管,恢复7d,GLP-1组微量注射0.5μg/0.5μl的GLP-1,NC组和DM组大鼠PVN区微量注射等体积生理盐水。甲基纤维素-酚红灌胃法检测胃排空;半定量RT-PCR检测大鼠下丘脑GLP-1RmRNA的表达。结果:DM组胃排空率较NC组明显升高(P<0.05),GLP-1组胃排空明显低于DM组(P<0.05),GLP-1组和NC组差异无统计学意义(P>0.05)。GLP-1组下丘脑GLP-1RmRNA的表达明显高于DM组和NC组(P<0.05),并与胃排空率成负相关(P<0.05)。DM组和NC组差异无统计学意义(P>0.05)。结论:PVN区注射GLP-1可以抑制糖尿病大鼠早期胃排空加速,作用机制可能和促进下丘脑GLP-1受体表达有关。     

Treatment of halogenated organic compounds and monitoring of microbial dynamics in up-flow fixed bed reactors under sequentially alternating pollutant scenarios

Two up-flow fixed bed reactors (UFBR) were operated for 8 months treating a model synthetic wastewater containing 2-fluorobenzoate (2-FB) and dichloromethane (DCM). The stability of the reactors under dynamic conditions, that is, sequentially alternating pollutants (SAP), shock loads, and starvation periods was assessed. Two support materials were used: expanded clay (EC) that does not adsorb 2-FB or DCM, and granular-activated carbon (GAC) that adsorbs 180 mg g(-1) of 2-FB and 390 mg g(-1) of DCM. The reactors were inoculated with a 2-FB-degrading strain (FB2) and a DCM degrader (TM1). 2-FB was fed at organic loads ranging from 0 to 800 mg L(-1) d(-1), while DCM was fed at 0-250 mg L(-1) d(-1). 2-FB or DCM were never detected at the outlet of the GAC reactor, while in the EC reactor outlet small amounts were observed. Nevertheless, the highest biological elimination capacity was observed in the EC reactor (over 700 mg L(-1) d(-1) of 2-FB). DGGE analysis revealed a fairly stable bacterial community with the largest shifts occurring during starvation periods and changes in feed composition. Several bacterial strains isolated from the reactors showed capacity for 2-FB degradation, while only strain TM1 degraded DCM.     

O2 consumption of mechanically unloaded contractions of mouse left ventricular myocardial slices

Left ventricular (LV) myocardial slices were isolated from murine hearts (300 microm thick) and were stimulated at 1 Hz without external load. Mean myocardial slice O(2) consumption (MVo(2)) per minute (mMVo(2)) without stimulation was 0.97 +/- 0.14 ml O(2).min(-1).100 g LV(-1) and mean mMVo(2) with stimulation increased to 1.80 +/- 0.17 ml O(2).min(-1).100 g LV(-1) in normal Tyrode solution. Mean DeltamVo(2) (the mMVo(2) with stimulation - the mMVo(2) without stimulation) was 0.83 +/- 0.12 ml O(2).min(-1).100 g LV(-1). There were no differences between mean mMVo(2) with and without stimulation in Ca(2+)-free solution. The increases in extracellular Ca(2+) concentrations up to 14.4 mM did not affect the mMVo(2) without stimulation but significantly increased the mMVo(2) with stimulation up to 140% of control. The DeltamMVo(2) significantly increased up to 190% of the control in a dose-dependent manner. In contrast, the shortening did not increase in a dose-dependent manner. Cyclopiazonic acid (CPA; 30 microM) significantly reduced the DeltamMVo(2) to 0.27 +/- 0.06 ml O(2).min(-1).100 g LV(-1) (35% of control). The combination of 5 mM 2,3-butanedione monoxime (BDM) and 30 microM CPA did not further decrease DeltamMVo(2). Although BDM (3-5 mM) decreased the DeltamMVo(2) by 28-30% of control in a dose-independent manner, 3-5 mM BDM decreased shortening in a dose-dependent manner. Our results indicate that the DeltamMVo(2) of mouse LV slices during shortening under mechanically unloaded conditions consists of energy expenditure for total Ca(2+) handling during excitation-contraction coupling, basal metabolism, but no residual cross-bridge cycling.