斑蝥素与去甲斑蝥素对昆虫细胞Sf9抑制作用比较

为探索斑蝥素的类似物去甲斑蝥素对昆虫的毒杀机理,本研究利用草地贪夜蛾Spodoptera frugiperda卵巢细胞系Sf9细胞作为实验材料,采用CCK-8法和AO/EB荧光染色法比较了斑蝥素(CTD)和去甲斑蝥素(NCTD)对细胞的增殖抑制和抑制方式。结果显示,3.125μg/mL的CTD处理细胞抑制率6h为20.00±1.10%,24h为66.33±0.81%;50μg/mL的CTD处理细胞抑制率6h为42.69±6.34%,24h为74.60±1.51%。3.125μg/mL的NCTD处理细胞抑制率6h为10.03±1.72%,24h为21.75±6.22%;50μg/mL的NCTD处理细胞抑制率6h为40.79±1.32%,24h为66.08±3.32%。结果表明,CTD与NCTD均能有效抑制Sf9细胞增殖和诱导细胞凋亡,且抑制率呈现出时间、剂量依赖性,较高剂量NCTD可以替代CTD达到相同效果。     

云南昆明和禄劝中缅树鼩体温调节和产热特征

为探讨不同地区中缅树鼩Tupaia belangeri的生理生态适应特征,对其体温调节和产热特征进行了测定,代谢率采用开放式呼吸仪进行测定。结果显示:A组中缅树鼩(禄劝县屏山镇)的体温(T b)与环境温度(T a)的关系为T b=38.0+0.07T a;B组中缅树鼩(昆明团结乡)的体温与环境温度的关系为T b=38.3+0.05T a;热中性区分别为30³5℃和27.535℃和27.5³5℃;基础代谢率分别为(1.40±0.03)mL/(g·h)和(1.66±0.06)mL/(g·h);平均最小热传导为(0.14±0.0034)mL/(g·h·℃)和(0.15±0.0041)mL/(g·h·℃);热中性区内F值,即(RMR/Kleiber期望RMR)/(C/Bradley期望C),分别为0.91±0.01和1.14±0.03。结果表明,昆明中缅树鼩较禄劝中缅树鼩有较高的基础代谢率和较宽的热中性区,并且有较好的调节体温的能力;它们的这种产热特征和体温调节方式的不同可能与它们的生活史和栖息地环境有关。     

辛伐他汀在大鼠体内药动学性别差异的研究

目的:研究Wistar大鼠单次灌服辛伐他汀后体内药代动力学的性别差异。方法:利用高效液相色谱方法检测大鼠血浆中辛伐他汀浓度,采用非房室模型法计算各自药动学参数。结果:雌、雄大鼠体内Cmax分别为(144.66±22.31)ng·mL~(-1)和(165.91±52.50)ng·mL~(-1);t_(1/2)分别为(4.74±1.19)h和(14.98±6.64)h;AUC_(0-10)分别为(0.990±0.19)μg.h·mL~(-1)和(0.726±0.15)μg·h·mL~(-1);AUC0-∞分别为(1.62±0.47)μg·h·mL~(-1)和(2.19±0.62)μg·h·mL~(-1);MRT分别为(9.69±1.60)h和(23.08±8.89)h,经t-检验,雌、雄大鼠主要药动学参数t_(1/2)、AUC_(0-10)、MRT均有统计学显著性差异(p<0.01)。结论:辛伐他汀在大鼠体内的药代动力学存在明显的性别差异,辛伐他汀在雌性大鼠体内代谢较快。     

始红蝽呼吸代谢的季节变化及对温度的适应性

为阐明始红蝽呼吸代谢的季节变化规律,探讨其对温度适应的呼吸代谢策略,运用多通道昆虫呼吸仪逐月测定始红蝽自然种群的O_2吸收率、CO_2释放率、代谢率和呼吸商。基于预实验获得始红蝽完成一次完整的呼吸代谢活动的时间为90 s,故每90 s记录1次数据。结果表明,始红蝽的呼吸代谢存在明显的季节变化。冬季种群(12—2月)呼吸代谢水平最弱,O_2吸收率、CO_2释放率和代谢率的平均值依次为(3.16±1.02)×10~(-5)mL/min、(2.09±0.78)×10~(-5)m L/min、(0.11±0.08)×10-3mLg~(-1)min~(-1);春季种群(3—5月)呼吸代谢水平迅速增加,夏季种群(6—8月)呼吸代谢水平最高,O_2吸收率、CO_2释放率和代谢率的平均值分别为(33.68±2.68)×10~(-5)mL/min、(36.00±3.07)×10~(-5)m L/min、(18.16±0.83)×10-3m Lg~(-1)min~(-1);秋季种群的呼吸代谢水平开始减弱并持续到冬季。始红蝽O_2吸收率、CO_2释放率和代谢率的值与栖息地的地表温度成正相关(r_1=0.914,r_2=0.909,r_3=0.836);春、夏、秋3个季节始红蝽以糖类物质作为呼吸代谢消耗的底物,冬季则消耗脂类物质。研究得出,随季节温度变化,始红蝽不仅能够调节呼吸代谢水平的强弱以提高自身对温度的适应能力,还可通过调整呼吸代谢消耗的底物类型以最大程度降低消耗,这对维持始红蝽种群数量和扩大其地理分布具有重要的生态学意义。     

恩诺沙星在罗氏沼虾体内的药物代谢动力学

应用反相高效液相色谱法(RP-HPLC)研究了恩诺沙星在罗氏沼虾(Macrobrachiumrosenbergii)体内的药物代谢动力学。实验结果表明,恩诺沙星在血淋巴、肝胰腺、肌肉中的平均回收率分别为86.54%±2.39%、85.43%±2.75%、95.01%±1.99%,其代谢产物环丙沙星在血淋巴、肝胰腺、肌肉中的平均回收率分别为94.34%±8.30%、75.17%±5.42%、80.42%±1.67%;恩诺沙星及其代谢产物环丙沙星在三种组织中的平均日内精密度分别为3.39%±0.53%和3.92%±1.24%,而日间精密度分别为5.11%±1.73%和5.28%±2.10%。恩诺沙星、环丙沙星的最低检测限分别为0.02μg/ml和0.01μg/ml。罗氏沼虾以10mg/kg虾体重剂量单次肌肉注射给药后,血液中药物浓度即刻达到峰值,并迅速向组织中分布。实验数据经MCPKP药动学软件分析,恩诺沙星在血淋巴中的主要药物代谢动力学参数为:t1/2α为0.581h、t1/2β为69.315h、Vd/F为7.230L/kg、CL/F为0.035L/h.kg、K12为0.01/h、K21为0.005/h、AUC为291.898μg/ml.h、Tmax为0.083h、Cmax为6.293μg/ml;恩诺沙星在肝胰腺、肌肉组织中主要药动学参数:t1/2α为1.941h、0.000h;t1/2β为70.732h、59.456h;AUC为308.07μg/ml.h、217.039μg/ml.h。三种组织中均能检测到恩诺沙星的活性代谢产物环丙沙星,但含量均处于较低水平,药物浓度-时间数据经MCPKP药动学软件处理后,不能用开放性一室模型或二室模型拟合。     

聚偏氟乙烯-丝氨酸血液灌流对感染性休克猪氧代谢的影响

目的:研究应用聚偏氟乙烯(polyvinylidene difluoride,PVDF)-丝氨酸(serine,Ser)吸附膜血液灌流对感染性休克氧代谢的影响.方法:雄性家猪16头,给予内毒素(lipopolysaccharides,LPS)1μg·kg-1·h-1静脉泵入4h复制感染性休克模型.随机分为实验组(E组),应用PVDF-Ser吸附膜进行血液灌流2h;对照组(C组),应用空白灌流器进行血液灌流2h.于基础期、注射内毒素后和血液灌流后分别测定中心静脉血氧饱和度(central venous oxygen saturation,ScvO2)、氧输送(oxygen delivery,DO2)、氧消耗(oxygen consumption,VO2)、氧摄取率(oxygen extraction ratio,O2ER)、血乳酸(lactation,LACT)和胃粘膜内pH(intramucosal pH,pHi).结果:血液灌流后E组ScvO2明显高于C组(68±1.7％vs62±3.1％,P=0.006);VO2、O2ER和LACT显著低于C组,分别为(204±28.1 mL·min-1·m-2 vs 249± 30.7 mL·min-1,m-2,p=0.017)、(33±3.3％vs 39±5.0％,P=0.031)和(3.1±1.0mmol/L vs 5.4±1.7mmol/L,P=0.022);E组的pHi较C组显著改善(7.29±0.09 vs 7.22±0.06,P=0.004).结论:应用PVDF-Ser吸附膜进行血液灌流,可以有效减少感染性休克的氧耗、纠正组织氧债和低灌注,改善机体氧代谢异常.     

核桃内生真菌抗氧化菌株的筛选及其代谢产物活性研究

本试验以29株核桃内生真菌为研究对象,采用总还原力(FRAP法)及DPPH·清除试验评价其代谢产物的抗氧化能力,从中筛选出高活性菌株,并对该菌株发酵液进行浓缩萃取,研究各萃取物的抗氧化活性。结果表明,供试29株菌的代谢产物都表现出一定的抗氧化活性,其中菌株LTS-6-6(Pyrenochaeta)为高活性菌株。该菌株发酵液乙酸乙酯萃取物(EAE)显示了较强的抗氧化活性,对DPPH·的EC₅₀为7μg/mL,总还原力为527.59±10.66 mg V_C/g,总酚和总黄酮含量分别达到641.14±7.50 mg没食子酸/g、100.30±8.44 mg芦丁/g。该结果表明,核桃内生真菌代谢产物具有一定的抗氧化活性,是寻找天然抗氧化活性物质的良好资源。     

RP-HPLC法测定阿托伐他汀在新西兰兔体内的药代动力学

目的:研究阿托伐他汀片在新西兰兔体内的药代动力学.方法:18只成年健康雄性新西兰兔.随机分为正常对照组、10mg/kg·d阿托伐他汀片组与15 mg/kg·d阿托伐他汀片组,每组6只,采用RP-HPLC法测定血药浓度,计算药代动力学参数.结果:10mg/kg·d组与15 mg/kg·d组的主要药代动力学参数分别为:AUC0～t/μ g·L-1·h为(619.58±215.45)与(1138.34±422.32)、AUC0～∞/μ g·L-1·h为(655.68±242.83)与(1216.57±353.64)、Cmax/μ g·L-1为(455.81±168.52)和(896.53±168.5.8)、MRT0～t/h为(3.68±0.75)与(5.73±0.56)、MRT0～∞/h为(3.83±0.91)与(5.25±0.48)、Tmax/h为(2.51±0.82)与(3.68±0.33)、T1/2/h为(4.22±0.55)与(9.51±0.67).结论:RP-HPLC法适用于阿托伐他汀片动物药代动力学的研究.     

Metabolic rate and evaporative water loss in the silky starling(Sturnus sericeus)

To better understand the physiological characteristics of the silky starling(Sturnus sericeus), its body temperature(Tb), basal metabolic rate(BMR), evaporative water loss(EWL) and thermal conductance(C) elicited by different ambient temperatures(Ta)(5-30 °C) were determined in the present study. Our results showed that they have a high Tb(41.6±0.1 °C), a wide thermal neutral zone(TNZ)(20-27.5 °C) and a relatively low BMR within the TNZ(3.37±0.17 mL O2/g·h). The EWL was nearly stable below the TNZ(0.91±0.07 mg H2O/g·h) but increased remarkably within and above the TNZ. The C was constant below the TNZ, with a minimum value of 0.14±0.01 mL O2/g·h·°C. These findings indicate that the BMR, Tb and EWL of the silky starling were all affected by Ta, especially when Ta was below 20 °C and the EWL plays an important role in thermal regulation.     

大蒜素体外抗白念珠菌生物膜作用的初步研究

目的研究大蒜素对体外白念珠菌生物膜的影响。方法 MTT法评价大蒜素对白念珠菌生物膜形成及细胞黏附的影响;血清芽管计数法评价大蒜素对白念珠菌芽管形成的影响。结果低浓度(4μg/mL)和高浓度(64μg/mL)大蒜素对白念珠菌生物膜形成的抑制率分别为(23.0±1.1)%和(95.6±0.3)%;32μg/mL大蒜素对早期(0h)、中期(12h)及成熟期(48h)生物膜的抑制率分别为(88.5±0.5)%、(63.3±0.8)%和(52.3±1.1)%;与空白对照组相比,不同浓度大蒜素(4～32μg/mL)对培养30min、60min、90min、120min的白念珠菌细胞黏附均有显著抑制作用(P0.05);空白对照组芽管形成率为(91.2±1.6)%,64μg/mL大蒜素组为(2.2±1.2)%。结论大蒜素对体外白念珠菌生物膜有较明显的抑制作用。     

维生素C保护Aβ1-40Cu(Ⅱ)复合物引起的神经元氧化损伤

老年斑中存在大量β 淀粉样蛋白（β-amyloid, Aβ）是老年痴呆症（Alzheimer′s disease, AD）的重要病理特征.大量数据表明,Aβ上具有与过渡态金属离子共价结合的位点,二者能结合成为寡聚复合物. Aβ_1-40Cu（Ⅱ）复合物通过Cu²⁺的还原催化O₂产生H₂O₂但反应机制不清.本文尝试以天然抗氧化剂维生素C（VC）来对抗Aβ_1-40及Aβ_1-40Cu（Ⅱ）复合物产生的H₂O₂对原代培养的神经细胞的毒性.结果表明,VC能够起到显著的保护作用,其有效浓度为1mmol/L.本文用胞外乳酸脱氢酶泄漏量和H₂O₂生成量的数据证实了细胞存活率（MTT实验）的实验结果.这些结果表明,Aβ_1-40Cu（Ⅱ）复合物能够释放更多的H₂O₂,引发细胞膜破裂并最终引起细胞死亡.加入VC后,神经元受到的损伤较轻,提示VC在保护细胞免受氧化损伤方面发挥了重要作用.     

Core RNAi machinery and gene knockdown in the emerald ash borer (Agrilus planipennis)

The RNA interference (RNAi) technology has been widely used in insect functional genomics research and provides an alternative approach for insect pest management. To understand whether the emerald ash borer (Agrilus planipennis), an invasive and destructive coleopteran insect pest of ash tree (Fraxinus spp.), possesses a strong RNAi machinery that is capable of degrading target mRNA as a response to exogenous double-stranded RNA (dsRNA) induction, we identified three RNAi pathway core component genes, Dicer-2, Argonaute-2 and R2D2, from the A. planipennis genome sequence. Characterization of these core components revealed that they contain conserved domains essential for the proteins to function in the RNAi pathway. Phylogenetic analyses showed that they are closely related to homologs derived from other coleopteran species. We also delivered the dsRNA fragment of AplaScrB-2, a β-fructofuranosidase-encoding gene horizontally acquired by A. planipennis as we reported previously, into A. planipennis adults through microinjection. Quantitative real-time PCR analysis on the dsRNA-treated beetles demonstrated a significantly decreased gene expression level of AplaScrB-2 appearing on day 2 and lasting until at least day 6. This study is the first record of RNAi applied in A. planipennis.     

Inhibition of thymidylate synthase by 2′,2′-difluoro-2′-deoxycytidine (Gemcitabine) and its metabolite 2′,2′-difluoro-2′-deoxyuridine

2′,2′-Difluoro-2′-deoxycytidine (dFdC, gemcitabine) is a cytidine analogue active against several solid tumor types, such as ovarian, pancreatic and non-small cell lung cancer. The compound has a complex mechanism of action. Because of the structural similarity of one metabolite of dFdC, dFdUMP, with the natural substrate for thymidylate synthase (TS) dUMP, we investigated whether dFdC and its deamination product 2′,2′-difluoro-2′-deoxyuridine (dFdU) would inhibit TS. This study was performed using two solid tumor cell lines: the human ovarian carcinoma cell line A2780 and its dFdC-resistant variant AG6000. The specific TS inhibitor Raltitrexed (RTX) was included as a positive control. Using the in situ TS activity assay measuring the intracellular conversion of [5-³H]-2′-deoxyuridine or [5-³H]-2′-deoxycytidine to dTMP and tritiated water, it was observed that dFdC and dFdU inhibited TS. In A2780 cells after a 4 h exposure to 1 μM dFdC tritium release was inhibited by 50% but did not increase after 24 h, Inhibition was also observed following dFdU at 100 μM. No effect was observed in the dFdC-resistant cell line AG6000; in this cell line only RTX had an inhibitory effect on TS activity. In the A2780 cell line RTX inhibited TS in a time dependent manner. In addition, DNA specific compounds such as 2′-C-cyano-2′-deoxy-1-beta-D-arabino-pentafuranosylcytosine and aphidicoline were utilized to exclude DNA inhibition mediated down regulation of the thymidine kinase.Inhibition of the enzyme resulted in a relative increase of mis-incorporation of [5-³H]-2′-deoxyuridine into DNA. In an attempt to elucidate the mechanism of in situ TS inhibition the ternary complex formation and possible inhibition in cellular extracts of A2780 cells, before and after exposure to dFdC, were determined. With the applied methods no proof for formation of a stable complex was found. In simultaneously performed experiments with 5FU such a complex formation could be demonstrated. However, using purified TS it was demonstrated that dFdUMP and not dFdCMP competitively inhibited TS with a Ki of 130 μM, without ternary complex formation. In conclusion, in this paper we reveal a new target of dFdC: thymidylate synthase.     

On the carbohydrate—protein linkage group in vitreous humor hyaluronate

Fractional molar ratios of serine, threonine and aspartic acid to neutral sugars in the purified bovine vitreous humor hyaluronate, and a 4–5-fold increase in the percentage of these amino acids and the absence of sugar alditols in hyaluronate reduced with NaBH₄---PdCl₂ after alkali treatment indicated the absence of a carbohydrate—protein linkage. Gel filtration behavior, a decrease in intrinsic viscosity of reduced hyaluronate to about one-half and a significant decrease in its specific rotation suggested that the two antiparallel chains of the hyaluronate double helix may come apart upo reduction. The vitreous humor hyaluronate contained 109.2 ppm of “bound” silicon. It is suggested that the bound silicon may bridge the two antiparallel chains through the neutral sugars and/or through the hydroxyl group of the uronic acid moiety.     

Discovery of 1,8-naphthyridin-2-one derivative as a potent and selective sphingomyelin synthase 2 inhibitor

Sphingomyelin synthase 2 (SMS2) has attracted attention as a drug target for the treatment of various cardiovascular and metabolic diseases. The modification of a high throughput screening hit, 2-quinolone 10, enhanced SMS2 inhibition at nanomolar concentrations with good selectivity against SMS1. To improve the pharmaceutical properties such as passive membrane permeability and aqueous solubility, adjustment of lipophilicity was attempted and 1,8-naphthyridin-2-one 37 was identified as a potent and selective SMS2 inhibitor. A significant reduction in hepatic sphingomyelin levels following repeated treatment in mice suggested that compound 37 could be an effective in vivo tool for clarifying the role of SMS2 enzyme and developing the treatment for SMS2-related diseases.     

Luminescence in Ba2Sr2Al2O7:RE (RE = Tb3+,Eu3+ and Dy3+) novel aluminate phosphors

The luminescence of novel rare earth ( Tb ^{3 +} , Eu ^{3 +} and Dy ^{3 +} )‐activated Ba ₂ Sr ₂ Al ₂ O ₇ phosphors for solid‐state lighting is presented. The aluminate phosphors were synthesized using a one‐step combustion method. X‐Ray diffraction, scanning electron microscopy and photoluminescence characterizations were performed to understand the mechanism of excitation and the corresponding emission in the as‐prepared phosphor, as characterized the phase purity and microstructure. Improvements in the luminescence properties of the phosphors with rare earth concentration were observed. The phosphor hue could be tuned from blue, green and red by proper selection of rare earth ions in typical concentrations. Effective absorption in the near‐ultraviolet region was observed, which makes the phosphor a potential candidate for ultraviolet light‐emitting diodes. Copyright © 2016 John Wiley & Sons, Ltd.     

Synthesis of 2′-O-Photocaged Ribonucleoside Phosphoramidites

The chemical synthesis and incorporation of the phosphoramidite derivatives of 2?′-O-photocaged ribonucleosides (A, C, G and U) with o-nitrobenzyl, α-methyl-o-nitrobenzyl or 4,5-dimethoxy-2-nitrobenzyl group into oligoribonucleotides are described. The efficiency of UV irradiated uncaging of these 2′-O-photocaged oligoribonucleotides was found in the order of α-methyl-o-nitrobenzyl < 4,5-dimethoxy-2-nitrobenzyl < 2′-O-o-nitrobenzyl.     

Development of a routine analysis method for liposome encapsulated recombinant interleukin-2

This paper describes the development of an isocratic reversed-phase high-performance liquid chromatographic method for the routine analysis of recombinant interleukin-2 (rIL-2) in liposome samples. The chromatographic system employed a C₄ column maintained at 30°C eluted with 52.5% (w/w) acetonitrile in water, containing 100 mM NaClO₄ and 10 mM HClO₄. To remove phospholipid interference the chromatographic method was combined with a lipid-extraction procedure. No significant loss of rIL-2 was noted upon inclusion of this extraction step. The protein eluted from the column with a capacity factor (k′) of 5.8. The method was validated for robustness, linearity, precision and reproducibility. It was shown that the method was linear over a sample concentration range of 1–100 μg/ml. Upon assessment of the intra-day and inter-day precision, the relative standard deviations (RSD) were within the range of the methodical error (approximately 5%), except at the lower concentration of 10 μg/ml, where the intra-day RSD was relatively high (17.8%). The recovery of rIL-2 upon liposome preparation and subsequent analysis of the samples was in the range 94±9%. The results indicate that the method is suitable for routine quantitation of rIL-2 in liposomal samples.     

2-Methylbutyryl CoA dehydrogenase from mitochondria of Ascarissuum and its relationship to NADH-dependent 2-methylcrotonyl CoA reduction

Acyl CoA dehydrogenase and electron-transfer flavoprotein have been isolated and partially purified from mitochondria of the anaerobic nematode, $\text{Ascaris}\text{suum}$. Dehydrogenase activity was greatest with 2-methylbutyryl CoA and the relative substrate specificities of the ascarid dehydrogenase(s) differ greatly from their mammalian counterparts. It appears that the ascarid dehydrogenase functions physiologically as a reductase, catalyzing the final step in the synthesis of branched-chain fatty acids. In fact, incubations of $\text{A}\text{.}\text{suum}$ mitochondrial membranes with electron-transfer flavoprotein, 2-methylbutyryl CoA dehydrogenase, 2-methylcrotonyl CoA and NADH resulted in a substantial, rotenone-sensitive, 2-methylbutyrate synthesis. These results suggest that the ascarid electron-transport chain and at least two soluble mitochondrial proteins are involved in the NADH-dependent reduction of 2-methylcrotonyl CoA.     

Design and synthesis of thiazolidine-2,4-diones hybrids with 1,2-dihydroquinolones and 2-oxindoles as potential VEGFR-2 inhibitors: in-vitro anticancer evaluation and in-silico studies

A thiazolidine-2,4-dione nucleus was molecularly hybridised with the effective antitumor moieties; 2-oxo-1,2-dihydroquinoline and 2-oxoindoline to obtain new hybrids with potential activity against VEGFR-2. The cytotoxic effects of the synthesised derivatives against Caco-2, HepG-2, and MDA-MB-231 cell lines were investigated. Compound 12a was found to be the most potent candidate against the investigated cell lines with IC₅₀ values of 2, 10, and 40 µM, respectively. Furthermore, the synthesised derivatives were tested in vitro for their VEGFR-2 inhibitory activity showing strong inhibition. Moreover, an in vitro viability study against Vero non-cancerous cell line was investigated and the results reflected a high safety profile of all tested compounds. Compound 12a was further investigated for its apoptotic behaviour by assessing the gene expression of four genes (Bcl2, Bcl-xl, TGF, and Survivin). Molecular dynamic simulations authenticated the high affinity, accurate binding, and perfect dynamics of compound 12a against VEGFR-2.