几种酶活抑制剂对红曲霉色素合成的影响

红曲色素是天然安全的色素和防腐剂,根据代谢数据库选择了6种代谢途径关键酶的抑制剂,在基本培养基中考察这些抑制剂对红曲霉生长和合成色素的影响。甲羟戊酸合成途径的抑制剂邻氨基苯甲酸和3,4-二羟苯甲酸对红曲霉生长和色素生物合成都没有影响;莽草酸途径关键酶氨基苯甲酸合成酶的抑制剂三甲胺不抑制红曲霉的生长和色素的合成。在不影响红曲霉生长的浓度范围内,聚酮途径中β-酮酯酰-ACP合成酶的专性抑制剂碘乙酰胺(0.5mmol/L)抑制红曲色素合成程度达64.7%,非专性抑制剂咪唑(1mmol/L)抑制幅度达60%,聚酮途径硫酯酶的抑制剂2,4-二硝基氟苯(0.5mmol/L)强烈抑制红曲霉合成色素的活性,抑制程度达91.5%。相关酶活抑制的试验数据显示红曲霉可能经过聚酮途径合成红曲色素。

枸杞叶蛋白提取物的特性表征与生物活性评价

为了探究枸杞叶蛋白提取物的特性表征与生物活性,采用碱提酸沉法提取枸杞叶蛋白提取物,通过持水性(water holding capacity,WA)、持油性(oil-holding property,FA)、热稳定性(thermal stability,TM)、溶解性(solubility,PS)、起泡性(froth capability,FC)、乳化性(emulsification capability,EC)等指标和十二烷基硫酸钠聚丙烯酰胺凝胶电泳(sodium dodecyl sulfate polyacrylamide gel electrophoresis,SDS-PAGE)、扫描电镜(scanning electron microscopy,SEM)、紫外可见光谱(ultraviolet-visible spectra,UV)、傅里叶变换红外光谱(Fourier Transform infrared spectroscopy,FT-IR)、X射线衍射(X-ray Diffraction,XRD)的方法及体外自由基清除试验和酶抑制试验对枸杞叶蛋白提取物的理化性质、功能特性、结构表征及生物活性进行分析。结果表明,枸杞叶蛋白提取物总氨基酸含量达344.00±10.49 mg/100 g,分子量在40~55 kDa,WA和FA分别为2.70、3.43 g/g,变性温度为85.73℃,随pH的升高,枸杞叶蛋白提取物溶液的PS、FC、EC、起泡稳定性(froth stability,FS)均呈现先下降后上升的趋势,而乳化稳定性(emulsion stability,ES)正好相反。枸杞叶蛋白提取物表面有紧密连接的小孔且呈大小不均一的块状,在270 nm附近有特征吸收峰,出现酰胺A、B、Ⅰ、Ⅱ、Ⅲ带,具有完整的三螺旋结构。枸杞叶蛋白提取物浓度为10 mg/mL时对超氧阴离子、羟基自由基的清除率分别为37.73%、35.38%,对α-葡萄糖苷酶、α-淀粉酶的IC50分别为9.88、21.09 mg/mL。综上所述,枸杞叶蛋白提取物的特性和结构稳定,有一定的体外抗氧化能力并能抑制与血糖代谢相关酶的活性。本试验为枸杞叶蛋白提取物的开发利用和深加工提供理论依据。

枸杞叶黄酮微胶囊的制备及消化稳定性与生物活性评价

本文以明胶和羧甲基纤维素钠(CMC)为壁材制备了枸杞叶黄酮微胶囊(M-LBLF),并对其稳定性和生物活性进行了探究。通过响应面试验优化M-LBLF制备工艺,采用扫描电镜(SEM)、傅里叶红外光谱(FTIR)、X-射线衍射(XRD)、热重分析和体外模拟消化等方法检测产物稳定性,通过自由基清除和酶活抑制实验评价产物生物活性。结果表明,M-LBLF的最佳制备工艺条件为芯壁比1:3.86,壁材浓度1.15%,搅拌温度45℃,包埋率为84.21%;SEM观察显示,微胶囊颗粒大部分表面光滑,囊壁的结构保持完整,壁材也无破裂痕迹;FTIR检测显示枸杞叶黄酮(LBLF)中1594 cm^(-1)处C=O发生偏移,推测与LBLF与CMC发生静电相互作用有关。XRD光谱显示,微胶囊化使非晶体结构部分转变为晶态,导致M-LBLF和LBLF的衍射峰强度上有细微的变化;热重分析发现微胶囊化改善了LBLF的高温分解,起到保护作用。体外模拟消化和抗氧化活性实验表明,微胶囊化提高了LBLF稳定性,可在消化过程中保留较好的抗氧化活性。此外,通过多元线性回归拟合方程得到微胶囊对胰脂酶的半抑制质量浓度(IC_(50))为2.2004±0.03 mg/mL,对α-淀粉酶半抑制质量浓度(IC_(50))为2.188±0.02 mg/mL,说明M-LBLF能够抑制胰脂肪酶活性和α-淀粉酶活性,提示其具有潜在的调节糖脂代谢活性,本实验为枸杞叶黄酮类提取物的稳定性提高及其相关营养健康产品开发提供了研究基础。

银杏达莫注射液对肾病综合征患者纤维蛋白原、D-二聚体、凝血酶激活的纤溶酶抑制物的影响

目的观察银杏达莫注射液对肾病综合征(NS)患者纤维蛋白原(FiB)、D-二聚体、凝血酶激活的纤溶酶抑制物的影响。方法选择40例入院时诊断为原发性NS的患者,观察组和对照组各20例,对照组采用常规治疗:泼尼松1 mg/(kg.d)及利尿消肿、调血脂治疗,并口服双嘧达莫。观察组在常规治疗基础上加用银杏达莫注射液治疗:5%葡萄糖250 mL+银杏达莫注射液25 mL静脉滴注,每日1次,疗程为10 d。分别于入院时及疗程满10 d时检测相关指标的浓度值。结果对照组FiB、D-二聚体、凝血酶激活的纤溶酶抑制物等治疗后变化无明显差异。观察组FiB、凝血酶激活的纤溶酶抑制物经治疗后有明显改善(P<0.05),D-二聚体无明显差异。两组治疗后比较,观察组FiB、凝血酶激活的纤溶酶抑制物较对照组有明显改善,但D-二聚体变化无统计学意义(P>0.05)。结论银杏达莫注射液对于纠正NS患者FiB、凝血酶激活的纤溶酶抑制物有一定疗效,可用于临床改善NS高凝状态。

果酒中多酚氧化酶及其性质的研究

对山楂酒中含有的六种分子量不同的多酚在多酚氧化酶作用下 ,测定氧化前后其涩度的变化。发现多酚物质的氧化作用能够加重果酒的苦涩味。并对山楂中的多酚氧化酶进行提取 ,测定其基本特性 ,确定了底物、温度、pH值对其活性的影响 ,并进一步测定其酶动力学曲线 ,发现多酚氧化酶催化的最适温度是 2 5℃ ,其最适pH是 6 5 ,其作用的最适底物是儿茶酚 ,其米氏常数是 1 0 77× 1 0 - 2 M。

重组组织因子途径抑制物对兔髂动脉粥样硬化新生内膜增生的抑制

目的:探讨兔髂动脉球囊剥脱术后局部灌注重组组织因子途径抑制物蛋白对血管内膜增生的抑制作用。方法:实验于2003-02/2004-11在哈尔滨医科大学附属第二医院实验动物中心及心内科完成。选择雄性日本大耳白兔24只,随机分为2组,重组组织因子途径抑制物组12只和生理盐水组12只。①建立髂动脉球囊损伤模型:将3.0～3.5mmOTW球囊导管沿导丝送入左髂动脉,使球囊近端距腹主动脉远端1cm。以606kPa扩张球囊,反复推拉3次,以剥脱血管内膜。撤出导丝,经OTW球囊按分组分别注入重组组织因子途径抑制物蛋白300μg和生理盐水1.5mL。球囊压力50kPa,保留20min后撤除。术后给予动物高胆固醇饮食(胆固醇、蛋黄粉、脂肪)4周。②测定横切面管腔面积、内弹力板内管腔面积、外弹力板内管腔面积、计算新生内膜面积(内膜面积=内弹力板内管腔面积-横切面管腔面积)、中膜面积(中膜面积=外弹力板内管腔面积-内弹力板内管腔面积)和新生内膜与中膜面积比,采用组织病理学方法,利用计算机图像处理。每段血管的数值均由2名人员读取3张切片(间隔30μm)数值计算均值而得。观察局部血管组织病理学变化,观察实验血管段新生内膜增生情况。结果:2组24只动物均进入结果分析,实验过程中无脱失值。①造膜结果:经过2周高胆固醇饮食饲养后兔血清总胆固醇水平高于饲养前犤(17.73±7.42),(1.10±0.26)mmol/L,P<0.01犦,经形态学观察确认为典型的髂动脉粥样硬化损伤模型。②组织病理图像分析:重组组织因子途径抑制物组外弹力板内管腔面积、内弹力板内管腔面积、横切面管腔面积分别高于生理盐水组犤(1.59±0.41),(1.21±0.40),(0.80±0.22)mm2,(1.16±0.36),(0.79±0.47),(0.24±0.19)mm2,P<0.01犦。重组组织因子途径抑制物组新生内膜面积、新生内膜与中膜面积比显著少于生理盐水组犤(0.23±0.21)mm2,0.74±0.64,(0.55±0.24)mm2,1.61±0.79,P<0.01犦。结论:应用重组组织因子途径抑制物灌注的方法,经病理学验证可以有效地抑制兔髂动脉球囊损伤后动脉粥样硬化血管的新生内膜增生。

冠心病患者血浆组织因子及组织因子途径抑制物变化分析

目的:探讨冠心病患者血浆组织因子及组织因子途径抑制物变化。方法:用酶联免疫吸附试验法测定48例冠心病患者其中稳定型心绞痛(SAP)患者16例;不稳定型心绞痛(UAP)患者16例;心肌梗死(AMI)患者16例;正常健康(NC)组11例血浆TF、TFPI。结果:AMI组血浆TF活性及TFPI含量与NC组、SAP组比较显著升高(P<0.01);AMI组与UAP组比较血浆TF活性和TFPI含量显著升高(P<0.05);AMI组的TF比UAP组显著升高(P<0.05);TFPI含量AMI组与UAP组比较两者差异无统计学意义(P>0.05)。结论:UAP、AMI发病期间存在异常增高的TFPI浓度TF活性增高,UAP、AMI的发病与斑块不稳定及血栓形成有关,TFPI可能是冠心病内皮细胞损伤后凝血的标志之一。

Study on Anti-oxidation and Inhibitory Effect on Nonenzymatic Glycation Reaction of Fermentation Extract from Biotransformation of Ginkgo biloba L. (EGB) by Hericium erinaceus

[ Objective] In order to study the anti-oxidation and inhibitory effect on nonenzymatic glycation reaction of EGB fermentation extraction biotransformed by Hericium erinaceus. [ Method ] The free radical scavenging ability and reducing capacity of DPPH as well as inhibitory rate of nonenzymatic glycation reaction were measured targets for comparing changes of anti-oxidation and inhibitory effect on nonenzymatic glycation reaction of fermentation lyophilizer and fermentation extraction before and after EGB fermention adsorbed by AB-8 macroporous resin. The EGB fermention was biotransformed by Hericium erinaceus. [ Result ] After adsorbed by AB-8 macroporous resin, the bioactive matters were concentrated and separated. The free radical scavenging rate, reducing capacity and inhibitory rate of nonenzymatic glycation reaction were increased significantly after adsorbed by AB-8 macroporous resin. [ Conclusion] AB-8 macroporous resin could be used for preliminary concentration of EGB fermentation which was biotransformed by Hericium erinaceus.

An Experimental Study of Pathogenesis of Steroid-induced Avascular Necrosis of Femoral Head

Objective: To explore the pathogenesis of avascular necrosis of femoral head(ANFH) and search an effective method for clinical practice. Methods: Twenty-four Japanese rabbitswere divided into 2 groups of models and controls. ANFH models were produced byintramuscular-injection of large dosage of steroid to rabbits for 8 weeks. From the 4th, 8th and12th week after production of models, 2 rabbits of each group were sacrificed to observe thestructure of femoral head through light microscope and scanning electron microscope. The contents ofNitric Oxide (NO), tissue-type plasminogen activator (t-PA) and -plasminogen activator inhibitor(PAI) in plasma of the 4 rabbits in each group were estimated at the same time. Results: Comparedwith control group, the rabbits of model group exhibited many differences: such as osteoporosis offemoral head, the presence of more bone lacuna and fat cell through light microscope observing; thebroken and sunk bone trabecula, the loosen and broken collagen fibers on the surface of bone matrixthrough scanning electron microscope observing. Compared with control group, the Concentration ofNO and t-PA in plasma of the model rabbits decreased obviously, but the Concentration of the PAIincreased obviously. Conclusion: The steroid-induced ANFH might be related to the lower level of NOand the descent of fibrinolytic activity.

细菌耐药拮抗剂的研究

本文介绍了具有拮抗细菌耐药性作用的物质的研究进展情况,包括灭活酶抑制剂、药物渗透促进剂、外输泵抑制剂、细菌生物被膜抑制剂、抗菌药物增强剂、耐药质粒消除剂等。

急性冠脉综合征合并糖尿病患者血浆TF、TFPI水平的研究

目的:探讨急性冠脉综合征(ACS)合并或不合并非胰岛素依赖性糖尿病(NIDDM)患者血浆组织因子(TF)?组织因子途径抑制物(TFPI)水平的特点?方法:选择ACS合并NIDDM患者22例?ACS不合并NIDDM患者21例?单纯NIDDM患者23例及正常对照组20例,应用ELISA法检测各组的TF?TFPI抗原水平,对比各组间指标,并对TF?TFPI水平进行相关性分析?结果:ACS合并或不合并NIDDM患者的TF和TFPI抗原水平皆显著高于对照组(P<0.01),且ACS合并NIDDM者高于不合并NIDDM者(P<0.05)及单纯NIDDM者(P<0.01);TF与TFPI抗原水平呈显著正相关(r=0.36, P<0.01)?结论:ACS患者存在凝血功能的异常状态,而ACS合并NIDDM患者的凝血功能异常更为明显,TF和TFPI水平升高可能是NIDDM患者发生ACS的预报因子?

Cantharidin and Its Analogues:Anticancer and Ser/Thr Protein Phosphatase Inhibitory Activities

This paper mainly describes the anticancer activities and Ser/Thr protein phosphatase inhibitory activities of cantharidin and its analogues.

INVESTIGATION OF THROMBOMODULIN AND PLASMINOGEN ACTIVATOR INHIBITOR TYPE-I IN PREGNANCY INDUCED HYPERTENSION AND ITS CLINICAL SIGNIFICANCE

Objective. To measure the circulating levels of thrombomodulin (TM) and plasminogen activator inhibitor type- I (PAI- I) in women with pregnancy induced hypertension (PIH). Methods. Blood samples were drawn from 97 pregnant women in their third trimester, grouped as 25 mild PIH,26 moderate PIH,22 severe PIH and 24 normotensive healthy pregnant women for determining levels of TM by ELISA,PAI- I by colorimetric assay methods, and creatinine (Cr) in serum by biochemical method. Results. Circulating levels of TM, PAI- I and TM/Cr ratio increased with increasing severity of PIH. There were no significant differences between mild and normotensive pregnant women. The parameters were significantly changed in the moderate and severe PIH groups. Conclusion. TM and PAI- I may serve as meaningful clinical markers for the assessment of the endothelial damage in PIH, which is very important in evaluating and following the development of PIH.

Effect of Dopamine Injection on the Hemocyte Count and Prophenoloxidase System of the White Shrimp Litopenaeus vannamei

Effects of dopamine injection on the hemocyte count, phenoloxidase activity, serine proteinase activity, proteinase in-hibitor activity and α2-macroglobulin-like activity in L. vannamei were studied. Results showed that dopamine injection resulted in a significant effect on the parameters measured (P < 0.05), while no significant difference was observed in the control group (0.85% NaCl). In the experimental groups,the hemocyte count reached the minimum in 3 h;granular and semi-granular cells became stable after 12 h and hyaline cells and the total hemocyte count became stable after 18 h. Phenoloxidase activity reached the minimum in 6 h, and then became stable after 9 h. Serine protease activity and proteinase inhibitor activity reached the minimum in 3 h, and α2-macro-globulin-like activity reached the maximum in 3 h,and all the three parameters became stable after 12 h. The results suggest that the activating mechanisms of the proPO system triggered by dopamine are different from those triggered by invasive agents or sponta-neously activated under a normal physical condition.

THE INCREASE IN PLASMINOGEN ACTIVATOR INHIBITOR TYPE-1 EXPRESSION BY STIMULATION OF ACTIVATORS FOR PEROXISOME PROLIFERATOR-ACTIVATED RECEPTORS IN HUMAN ENDOTHELIAL CELLS

Objective.To investigate the effect of peroxis ome proliferator-activated recept ors(PPARs )activators on plasminogen activator inhibitor ty pe-1(PAI-1)expression in human umbilical vein e ndothelial cells and the possi-ble mechanism.Methods.Human umbilical vein endothelial ce lls(HUVECs )were obtained from normal fetus,and cul-tured conventionally.Then the HUVECs were exposed to test agents(linolenic acid,linoleic acid,oleic acid,stearic acid and prostaglandin J 2 respectively)in varying concentrations with fresh media.RT -PCR and ELISA were applied to determine the expression of PPARs and PAI-1in HUVECs.Results.PPARα,PPARδand PPARγmRNA were detected by using RT-PCR in HUVECs.Treatment of HUVECs with PPARαand PPARγactivators---linolenic acid,linoleic acid,oleic acid and prostaglandin J 2 respectively,but not with stearic a cid could augment PAI-I mRNA expression and protein secretion in a concentration-dependent manner.However,the mRNA expressions of 3subclasses of PPAR with their activators in HUVECs were not changed compared w ith controls.Conclusion.HUVECs express PPARs.PPARs activators may increase PAI-1expression in ECs,but the underlying mechanism remains uncle ar.Although PPARs expression was not enhanced after stimulated by their activators in ECs,the role of functionally active PPARs in regulating PA I-1expression in ECs needs to be further investigated by using transient gen e transfection assay.

Effect of Lime Nitrogen on the Transformation of Ureain Soils

Laboratory incubation experiment was conducted to study the effect of lime nitrogen(LN) on transfor-mation of iirea-N in three paddy soils. The results showed that LN had an inhibitory effect on urease activityin these soils especially in the first 5 days, and that in the first 20 days of incubation, the amount of NH-Nderived from urea was lower in the soil with LN than in the soil without LN. While after 30 days the ainountof NH-N was higher in the mature haplic paddy soil developed on Quaternary red clay(MHPS) with LNthan that in the soil without LN. The amonnt of NH_3-N volatilized was decreased in the earlier stage andincreased in the later stage of incubation in the MHPS by the addition of LN.

Cysteine peptidase and its inhibitor activity levels and vitamin E concentration in normal human serum and colorectal carcinomas

AIM: Cysteine peptidase (CP) and its inhibitor (CPI) are a matrix protease that may be associated with colorectal carcinoma invasion and progression, and vitamin E is also a stimulator of the immunological system. Our purpose was to determine the correlation between the expression of cysteine peptidases and their endogenous inhibitors,and the level of vitamin E in sera of patients with colorectal cancer in comparison with healthy individuals.METHODS: The levels of cysteine peptidases and their inhibitors were determined in the sera of patients with primary and metastatic colorectal carcinoma and healthy individuals using fluorogenic substrate, and the level of vitamin E was determined by HPLC.RESULTS: The levels of cysteine peptidases and their inhibitors were significantly higher in the metastatic colorectal cancer patients than that in the healthy controls (P＜0.05).The activity of CP increased 2.2-fold, CPI 2.8-fold and vitamin E decreased 3.4-fold in sera of patients with metastasis in comparison with controls. The level of vitamin E in healthy individuals was higher, whereas the activity of cysteine peptidases and their inhibitors associated with complexes was lower than that in patients with cancer of the digestive tract.CONCLUSION: These results suggest that the serum levels of CP and their inhibitors could be an indicator of the prognosis for patients with metastatic colorectal cancer. Vitamin E can be administered prophylactically to prevent digestive tract neoplasmas.

Inhibition of Leukemic Cell Telomerase Activity by Antisense Phosphorothioate Oligodeoxynucleotides

Objective To evaluate the effect of human telomerase reverse transcriptase (hTERT) gene antisense oligodeoxynucleotide (ASODN) ontelomerase activity in K562 cells.Methods Telomerase activity was determined by polymerase chain reaction enzyme-linked immunoassay (PCR-ELISA) in K562 cellstreated with ASODN and hTERT mRNA expression was detected by reverse transcriptase polymerase chain reaction (RT-PCR).Results The hTERT mRNA level was decreased, and teloraerase activity was significantly inhibited when the K562 cells were treated withASODN for 48 h.Conclusion It is suggested that hTERT ASODN might specifically inhibit telomerase activity of K562 cells at translation level, and it isfurther proved that hTERT gene has significant correlation with telomerase activity.

The role and modulation of autophagy in experimental models of myocardial ischemia-reperfusion injury

A physiological sequence called autophagy qualitatively determines cellular viability by removing protein aggregates and damaged cyto-plasmic constituents, and contributes significantly to the degree of myocardial ischemia-reperfusion （I/R） injury. This tightly orchestrated cata-bolic cellular‘housekeeping’ process provides cells with a new source of energy to adapt to stressful conditions. This process was first described as a pro-survival mechanism, but increasing evidence suggests that it can also lead to the demise of the cell. Autophagy has been implicated in the pathogenesis of multiple cardiac conditions including myocardial I/R injury. However, a debate persists as to whether autophagy acts as a protec-tive mechanism or contributes to the injurious effects of I/R injury in the heart. This controversy may stem from several factors including the va-riability in the experimental models and species, and the methodology used to assess autophagy. This review provides updated knowledge on the modulation and role of autophagy in isolated cardiac cells subjected to I/R, and the growing interest towards manipulating autophagy to increase the survival of cardiac myocytes under conditions of stress-most notably being I/R injury. Perturbation of this evolutionarily conserved intracellular cleansing autophagy mechanism, by targeted modulation through, among others, mammalian target of rapamycin （mTOR） inhibitors, adenosine monophosphate-activated protein kinase （AMPK） modulators, calcium lowering agents, resveratrol, longevinex, sirtuin activators, the proapoptotic gene Bnip3, IP3 and lysosome inhibitors, may confer resistance to heart cells against I/R induced cell death. Thus, therapeutic ma-nipulation of autophagy in the challenged myocardium may benefit post-infarction cardiac healing and remodeling.