Targeted anti-cancer therapy: Co-delivery of VEGF siRNA and Phenethyl isothiocyanate (PEITC) via cRGD-modified lipid nanoparticles for enhanced anti-angiogenic efficacy

Anti-tumor angiogenesis therapy, targeting the suppression of blood vessel growth in tumors, presents a potent approach in the battle against cancer. Traditional therapies have primarily concentrated on single-target techniques, with a specific emphasis on targeting the vascular endothelial growth factor, but have not reached ideal therapeutic efficacy. In response to this issue, our study introduced a novel nanoparticle system known as CS-siRNA/PEITC&L-cRGD NPs. These chitosan-based nanoparticles have been recognized for their excellent biocompatibility and ability to deliver genes. To enhance their targeted delivery capability, they were combined with a cyclic RGD peptide (cRGD). Targeted co-delivery of gene and chemotherapeutic agents was achieved through the use of a negatively charged lipid shell and cRGD, which possesses high affinity for integrin αvβ3 overexpressed in tumor cells and neovasculature. In this multifaceted approach, co-delivery of VEGF siRNA and phenethyl isothiocyanate (PEITC) was employed to target both tumor vascular endothelial cells and tumor cells simultaneously. The co-delivery of VEGF siRNA and PEITC could achieve precise silencing of VEGF, inhibit the accumulation of HIF-1α under hypoxic conditions, and induce apoptosis in tumor cells. In summary, we have successfully developed a nanoparticle delivery platform that utilizes a dual mechanism of action of anti-tumor angiogenesis and pro-tumor apoptosis, which provides a robust and potent strategy for the delivery of anti-cancer therapeutics.

PGE₂Generation in Myocardium from Isolated Rat Atrium under Hypoxia and Reoxygenation Conditions. Effect of Anti-<i>β</i>₁IgG from Patients with Chronic Severe Periodontitis

Background: Hypoxia is one of the most frequently encountered stresses in health and disease. Methods: We compared the effects of an anti-β1 periodontal IgG (pIgG) and an authentic β1 adrenergic agonist, xamoterol, on isolated myocardium from rat atria contractility. We used an ELISA assay to measure the generation of PGE2 in vitro after the addition of either the antibody or the adrenergic agonist. We analyzed the myocardium histopathologically in the presence of both the antibody and/or the adrenergic agonist drug during normoxia, hypoxia and reperfusion conditions. Results: PGE2 generation increased during the hypoxia and was unchanged during reoxygenation period compared with the production of this prostanoid in atria during normoxia condition. A β1 specific adrenoceptor antagonist atenolol and the β1 synthetic peptide abrogated the increment of the prostanoid in the presence of pIgG but only atenolol due to it in the presence of xamoterol. The increment of PGE2 was dependent on the activation of cox-1 and cox-2 isoforms. Moreover, cox-2 was more active and produced more increments in the production of PGE2 in the presence of the pIgG than cox-1 activation. Histopathologically, studies of myocardium specimens during these different periods of the experimental protocol: basal (B), hypoxia (H) and reoxygenation (R), were also performed and showed tissue necrosis and edematization at the myocardium level. Conclusion: The phenomenon studied here supports the notion that PGE2 may be responsible for tissue edematization. PGE2 maybe acts as a beneficial modulator in the myocardium and prevents a major injury of it. The inflammation damage to the heart organ and cardiomyocytes caused by the actions of the antibodies in the course of heart lesions provoked by cardiovascular autoimmune disease, explains some of these results obtained in the present experiments. Further studies will be needed to establish the real role of PGE2 during hypoxia injury of the heart in the course of autoimmune diseases.

基于3,5-二溴水杨醛席夫碱镍配合物-氧化石墨烯电化学免疫传感器检测Anti-IgG含量的研究

应用物理吸附法将羊抗人IgG抗原直接固定于3,5-二溴水杨醛席夫碱镍配合物-氧化石墨烯修饰的金电极表面,制备电化学免疫传感器。采用循环伏安法和交流阻抗法对传感器进行表征,结果表明该传感器适合检测Anti-IgG浓度。同时探讨了缓冲液pH值、扫描速度、免疫反应温度、抗原与抗体配比对循环伏安峰电流的影响,结果表明在5-100mV/s扫速范围内,峰电流与扫速呈线性。孵育最优条件为25℃,h-IgG与Anti-IgG配比为1∶1。循环伏安法研究还表明Anti-IgG浓度在0.01-260μg/L范围内,线性关系良好,相关系数r^2=0.993,检出限（S/N=3）为0.006μg/L,据此建立了检测Anti-IgG浓度的新方法。

信号分子IRAK1/4在antiβ-2GPI/β2GPI复合物诱导THP-1细胞表达TF中的作用探讨

目的:探讨IRAK1和IRAK4在antiβ-2GPI/β2GPI复合物诱导单核细胞株THP-1表达组织因子(TF)中的作用。方法:利用荧光定量PCR(Real-time PCR)、TF活性试剂盒分别检测THP-1细胞表达TF mRNA及TF活性;Western blot检测anti-β2GPI/β2GPI复合物诱导THP-1细胞表达IRAK1、磷酸化-IRAK1(p-IRAK1)、IRAK4情况;观察IRAK1/4抑制物是否干预anti-β2GPI/β2GPI复合物诱导THP-1表达TF。结果:Antiβ-2GPI/β2GPI复合物(100μg/ml)诱导THP-1细胞表达TF显著增加(P<0.05 vs control);Antiβ-2GPI/β2GPI复合物(100μg/ml)刺激THP-1细胞表达IRAK1、p-IRAK1、IRAK4(蛋白)显著升高(P<0.05 vscontrol);IRAK1/4抑制物(50μmol/L)能够阻断antiβ-2GPI/β2GPI复合物(100μg/ml)诱导THP-1表达TF及IRAK1磷酸化的效应。结论:antiβ-2GPI/β2GPI复合物诱导THP-1细胞表达TF过程中,信号分子IRAK1/4被激活进而发挥重要作用。

三维Anti de Sitter空间中Lorentzian曲面的S_t^1×S_s^1-值光锥Gauss映射的奇点分类

利用Arnol'd的Legendrian理论,对三维Anti de Sitter空间中Lorentzian曲面进行了研究.引入光维高度函数概念研究了三维Anti de Sitter空间Lorentzian曲面的S1t×S1s-值、光锥Gauss映射的奇点,进行了奇点分类,揭示了类光Causs-kronecker曲率之间的关系;并研究了Lorentzian曲面的一些基本几何性质.

The effect of alphastatin peptide suppressing the hypoxia-induced vasculogenic mimicry formation of glioma

Objective:To investigate the vasculogenic mimicry formation induced by hypoxia in Ⅱ-Ⅲ human glioma cell and the effect of alphastatin peptide suppressing the hypoxia-induced vasculogenic mimicry formation and the mechanism.Methods:MTT,Transwell and three-dimentional culture were used to detect the proliferation,migration and tubule formation of SHG44.The expression of vascular endothelial growth factor-α(VEGF-α),erythropoietin-producing hepatocellular carcinoma-A2 (EphA2) and matrix metalloproteinases 2 (MMP2) was detected by RT-PCR and Western blotting analysis.Results:The OD 490 in hypoxia group was 0.60±0.06 and in control group was 0.46±0.05.The number of cell migration was 178.71±18.81 in hypoxia group and 85.86±17.92 in control group.The tubule formation was 56.80±12.21 in hypoxia group and 4.20±2.62 in control group.The proliferation,migration and tubule formation in hypoxia group were significantly higher than that in control group.The expression of VEGF-α,EphA2 and MMP2 was upregulated in hypoxia.When various concentrations of alphastatin (100,1 000,10 000 nmol/L) were added to hypoxia group,the numbers of cell migration were 142.57±12.12,92.71±17.68,30.00±7.72 and the tubule formation were 47.71±10.58,18.86±8.40,8.43±5.62.The cell migration and tubule formation were significantly suppressed by alphastatin in a dose-dependent manner.In alphastatin group,the phosphorylation of EphA2 protein (P=0.037,F=4.629) and activation of MMP2 protein (P=0.005,F=9.331) were significantly suppressed but there was no change in VEGF-α protein.Conclusion:Ⅱ-Ⅲ human glioma cell is able to form vasculogenic mimicry induced by hypoxia and alphastatin peptide can suppress the hypoxia-induced vasculogenic mimicry.VEGF-α induced EphA2 phospharilation and MMP2 activation maybe the key pathway to form vasculogenic mimicry.

Hypoxia-associated circular RNA RPPH1 modulates triple-negative breast cancer cell growth via the miR-1296-5p/TRIM14 axis

Hypoxia affects the advancement,metastasis,and metabolism of breast cancer(BC).The circular RNA ribonuclease P RNA component H1(circRPPH1)(has_circ_0000515)is implicated in tumor progression.Nevertheless,the regulatory mechanism related to circRPPH1 in hypoxia-mediated triple-negative breast cancer(TNBC)progression is indistinct.The expression levels of circRPPH1,miR-1296-5p,tripartite motif-containing 14(TRIM14)mRNA in tissue samples and cells were examined through quantitative real-time polymerase chain reaction(qRT-PCR).Cell viability,migration,and invasion were determined with Cell Counting Kit-8(CCK-8)or transwell assays.The levels of glucose consumption and lactate production were assessed via the Glucose Assay Kit or Lactate Assay Kit.The protein levels of TRIM14,Glucose Transporter GLUT1(GLUT1),and lactic dehydrogenase A(LDHA)were detected by western blot analysis.The targeting relationship between circRPPH1 or TRIM14 and miR-1296-5p was verified with dual-luciferase reporter assay.The role of circRPPH1 was confirmed via xenograft assay.We verified that circRPPH1 and TRIM14 expression were increased while miR-1296-5p expression was decreased in BC tissues and hypoxia-cultured TNBC cells.Functionally,circRPPH1 silencing reversed the promoting effect of hypoxia on viability,migration,invasion,and glycolysis of TNBC cells.CircRPPH1 knockdown repressed decreased TNBC cell growth in vivo.Mechanistically,circRPPH1 sponged miR-1296-5p to modulate TRIM14 expression.Also,miR-1296-5p silencing restored circRPPH1 inhibition-mediated influence on the viability,migration,invasion,and glycolysis of hypoxia-treated TNBC cells.TRIM14 elevation overturned the inhibitory impact of miR-1296-5p mimic on viability,migration,invasion,and glycolysis of hypoxia-cultured TNBC cells.In conclusion,hypoxia-induced circRPPH1 fostered TNBC progression through regulation of the miR-1296-5p/TRIM14 axis,indicating that circRPPH1 was a promising target for TNBC treatment.

On the Construction of Deepening Anti - corruption Mechanism

It needs the foundation of system and the guarantee of organizational system for anti-corruption,but it is more necessary to build and form an effective anti-corruption mechanism,so that the anti-corruption can be really put into practice. Anti-corruption mechanism refers to a organic operation system of the interaction,interconnection and constraint between the constituent elements( parts) and elements of national anti-corruption,and as a system,anti-corruption mechanism should have the characteristics of system aticness,comprehensiveness,transparency,legalization,public participation,scientific dynam ic,and internationalism. The construction of deepening anti-corruption mechanism is the need for reconstructing the ruling legitimacy of the party and the governm ent. Adhering to the principle of treating both root causes and symptoms is necessary in the construction of anti-corruption m echanism,com bating and punishing corruption is an important part of anti-corruption,and the prevention and control of corruption is the basic project of anti-corruption. Therefore,the construction of prevention and control mechanism in the anti-corruption mechanism has a more far-reaching significance.

6-羟基染料木素及其甲基化衍生物的合成和抗氧化与抗缺氧活性

目的:缺氧是一种常见的病理现象,通常由机体组织供氧不足或无法有效利用氧导致。羟基化及甲氧基化黄酮类化合物具有显著的抗缺氧活性。本研究旨在探索6-羟基染料木素(6-hydroxygenistein,6-OHG)及其甲基化衍生物的合成方法和抗氧化与抗缺氧活性。方法:以鹰嘴豆芽素A为原料,经甲基化反应、溴化反应、甲氧基化反应及去甲基化反应得到6-OHG及其4个甲基化衍生物[4’,6,7-三甲氧基-5-羟基异黄酮(化合物3)、4’,5,6,7-四甲氧基异黄酮(化合物4)、4’,6-二甲氧基-5,7-二羟基异黄酮(化合物6)、4’-甲氧基-5,6,7-三羟基异黄酮(化合物7)]。采用氢-1核磁共振波谱法(1H-nuclear magnetic resonance spectroscopy,1H-NMR)和质谱法(mass spectrometry,MS)表征产物结构;高压液相色谱法检测化合物的纯度;1,1-二苯基-2-三硝基苯肼(1,1-diphenyl-2-picrylhydrazyl,DPPH)自由基清除实验检测化合物的体外抗氧化活性。将PC12细胞分为正常组、缺氧模型组、芦丁组(1×10-9~1×10^(-5)mol/L),以及常氧和缺氧条件下的目标化合物组(1×10-9~1×10^(-5)mol/L),采用细胞计数试剂盒-8(cell counting kit-8,CCK-8)检测细胞活力,筛选得到抗缺氧活性优异的目标化合物及其最佳抗缺氧活性时的药物浓度。分别用抗缺氧活性优异的目标化合物、芦丁的最佳药物浓度处理PC12细胞后,在光镜下观察细胞形态,采用流式细胞术测定细胞凋亡率,蛋白质印迹法检测缺氧诱导因子-1α(hypoxia inducible factor-1α,HIF-1α)和血管内皮生长因子(vascular endothelial growth factor,VEGF)的蛋白质表达水平。结果:6-OHG及其4个甲基化衍生物的结构无误,纯度均>97%。当浓度为4 mmol/L时,化合物7和6-OHG的DPPH自由基清除率分别为81.16%和86.94%,均高于阳性对照芦丁,而化合物3、4、6的清除率均低于20%。与正常组相比,缺氧模型组的细胞活力显著下降(P<0.01);与缺氧模型组相比,化合物3、4、6对缺氧条件下的细胞活力无显著影响;在所有实验浓度下,6-OHG组的细胞活力均显著高于缺氧模型组(均P<0.05);在给药浓度为1×10^(-7)或1×10^(-6)mol/L时,化合物7组的细胞活力显著高于缺氧模型组(均P<0.05)。6-OHG和化合物7的抗缺氧活性优异,最佳药物浓度分别为1×10^(-6)和1×10^(-7)mol/L。采用6-OHG(1×10^(-6)mol/L)和化合物7(1×10^(-7)mol/L)处理PC12细胞后,与缺氧模型组相比,细胞损伤明显减轻,细胞凋亡率显著下降(P<0.01),HIF-1α和VEGF蛋白质的表达水平显著下调(均P<0.01)。结论:优化后的合成路线可提高6-OHG的产率,通过甲基化和选择性去甲基化得到4个衍生物。6-OHG和其衍生物化合物7表现出优异的体外抗氧化和抗缺氧活性,该活性与其分子中存在的A环邻三酚羟基结构有关。

Circ-SMG6调节miR-132-3p/BTG2轴对缺氧/复氧诱导心肌细胞损伤的影响

目的探讨Circ-SMG6对缺氧/复氧诱导的心肌细胞损伤的影响及对miR-132-3p/BTG2轴的调节作用。方法心肌H9c2细胞分为:NC组(不做任何处理)、缺氧/复氧组、缺氧/复氧+si-NC组、缺氧/复氧+si-CircSMG6组、缺氧/复氧+si-Circ-SMG6+anti-NC组、缺氧/复氧+si-Circ-SMG6+anti-miR-132-3p组。RT-qPCR检测miR-132-3p、Circ-SMG6表达;Western blot检测BTG2、Bcl-2、Bax、cleaved-Caspase-3蛋白水平;ELISA法检测SOD、MDA以及IL-1β、IL-6、TNF-α水平CCK8法测定心肌细胞增殖;流式细胞术检测心肌细胞凋亡;双荧光素酶验证Circ-SMG6与miR-132-3p,miR-132-3p与BTG2靶向关系。结果与NC组相比,缺氧/复氧组、缺氧/复氧+si-NC组BTG2 mRNA及蛋白、Circ-SMG6水平、MDA、IL-1β、IL-6、TNF-α含量、凋亡率及Bax、cleavedCaspase-3蛋白水平显著增加(P<0.01),miR-132-3p水平、SOD含量、72 h的细胞活力、Bcl-2蛋白水平显著降低(P<0.01)。与缺氧/复氧组相比,缺氧/复氧+si-Circ-SMG6组BTG2蛋白、Circ-SMG6水平、MDA、IL-1β、IL-6、TNF-α含量、凋亡率及Bax、cleaved-Caspase-3蛋白水平显著降低(P<0.01),miR-132-3p水平、SOD含量、72 h的细胞活力、Bcl-2蛋白水平显著增加(P<0.01)。与缺氧/复氧+si-Circ-SMG6组相比,缺氧/复氧+si-Circ-SMG6+antimiR-132-3p组BTG2蛋白、MDA、IL-1β、IL-6、TNF-α含量、凋亡率及Bax、cleaved-Caspase-3蛋白水平显著增加(P<0.01),miR-132-3p水平、SOD含量、72 h的细胞活力、Bcl-2蛋白水平显著下降(P<0.01)。结论敲低CircSMG6可能通过调节miR-132-3p/BTG2轴减轻缺氧/复氧诱导的心肌细胞损伤。

Anti-Bacterial and Flame Retardant for Cotton Fabric by One-Bath Finishing

A research on the process of cotton fabric flame-re-tarding,anti-bacterial finishing and one-bath finish-ing of anti-bacterial and flame-retarding is discussed.The flame retardant agent was phosphorous-contained,and the bacteriostatic finishing agent named SFR-1 wassynthesized.The flame retardancy of the fabric finishedcan meet the DOC FF3-71 Children Sleepwear Stan-dard.Its bacterial inhibiting capacity can meet and ex-ceed the requirements of similar products

Testing of Anti-stripping Property of Friction Spun Core Yarn

Friction spun core yarn has two components: filament core and staple fiber sheath. Under axial rubbing action, the failure mode of the core yarn is the stripping of the sheath from the core. This paper introduces a method to test the anti - stripping property of the core yarn. With a modified Universal Testing Machine, the stripping resistance of friction spun core yarn can be continuously measured. Some factors Influencing the measurements are discussed in detail. The testing results are compared with those from a Y731 Yarn Abrasion Tester and fur - ther confirmed by weaving practice.

刺梨多糖RRTP-1的理化性质及抗缺氧活性

目的研究刺梨多糖RRTP-1的理化性质及抗缺氧活性。方法刺梨汁浓缩,乙醇沉淀,得粗多糖。粗多糖脱游离蛋白 质,脱色,DEAE-纤维素柱及Sepharose CL-6B凝胶柱色谱分离纯化得到刺梨多糖RRTP-1。应用凝胶渗透色谱法、气相色谱法 和红外光谱法分别测定其理化性质,并通过观察硫代硫酸钠损伤后各组神经干细胞死亡率和乳酸脱氢酶漏出率,研究其对神 经干细胞硫代硫酸钠损伤的保护作用。结果RRTP-1经凝胶柱色谱和聚丙烯酰胺凝胶电泳证明为相对分子质量分布均一的 多糖,由鼠李糖、阿拉伯糖、未知糖、木糖、甘露糖、半乳糖、葡萄糖和葡萄糖醛酸组成,相对分子质量为3 200。抗缺氧活性实验 表明,加入RRTP-1的实验组神经干细胞损伤有所减轻,高浓度实验组细胞死亡率和乳酸脱氢酶漏出率较低。结论 RRTP-1 对神经干细胞硫代硫酸钠损伤有明显的保护作用。

D-核糖对大鼠负载游泳后胰岛素、去甲肾上腺素、肾上腺素的影响及其抗疲劳、抗缺氧能力研究

通过灌服D-核糖,测定大鼠在负重游泳后血浆胰岛素、去甲肾上腺素和肾上腺素水平,研究D-核糖对运动后大鼠心脏及骨骼肌功能的恢复作用。灌服D-核糖,测定大鼠的抗疲劳游泳力竭时间与抗缺氧存活时间,探讨核糖的抗疲劳和抗缺氧能力。结果表明:运动后即刻核糖实验组胰岛素水平高于正常对照组和游泳对照组,恢复72h后,核糖组胰岛素水平均高于正常对照组;核糖实验组在运动后即刻去甲肾上腺素、肾上腺素水平高于游泳对照组,恢复72h后,核糖实验组肾上腺素水平低于游泳对照组和正常对照组;核糖组与对照组大鼠的抗疲劳游泳力竭时间、抗缺氧存活时间分别延长了50.21%和8.8%。结论:核糖可以调节激素水平,促进运动过程中的糖异生作用,对维持运动过程中血糖水平的稳定起重要作用,保护了心脑等重要器官的正常生理功能。补充核糖可以显著延长大鼠的抗疲劳游泳时间和缺氧状态下的存活时间。

5,6,7-三羟基-8-甲氧基黄酮的抗氧化及对高原缺氧小鼠的保护作用

目的对5,6,7-三羟基-8-甲氧基黄酮(TMF)的自由基清除及抗高原缺氧作用进行研究。方法采用1,1-二苯基-2-三硝基苯肼(DPPH)、羟自由基、超氧阴离子和一氧化氮清除方法评价TMF的抗氧化作用;利用常压密闭缺氧和低压性缺氧模型,通过测定缺氧小鼠心肌脑组织自由基代谢相关生化指标评价其抗缺氧活性。结果 TMF对4种自由基均表现出一定的清除活性。与缺氧模型组相比,TMF能够显著延长缺氧小鼠的存活时间,降低缺氧小鼠心脑组织中丙二醛(MDA)含量,提高超氧化物歧化酶(SOD)、过氧化氢酶(CAT)、谷胱甘肽过氧化物酶(GSH-Px)的活力(P<0.01)。结论 TMF是一种抗氧化活性优异的黄酮类化合物,能提高低压低氧小鼠抗氧化能力,减少自由基的损伤,表现出较好的抗缺氧活性。

氮氧自由基与γ-氨基丁酸偶联物的设计合成与抗缺氧活性研究

目的设计合成一种新型氮氧自由基与γ-氨基丁酸偶联物并研究其抗缺氧活性。方法以对羟基苯甲醛、溴乙酸乙酯、γ-氨基丁酸甲酯盐酸盐和2,3-二甲基-2,3-二羟氨基丁烷为原料,经醚化、酰胺化、缩合和氧化反应得到一种氮氧自由基与γ-氨基丁酸的偶联物(化合物3),并通过小鼠常压密闭耐缺氧实验对其抗缺氧活性进行评价。结果 3组在常压密闭缺氧实验下,与缺氧模型组比较,乙酰唑胺组和化合物3组存活时间均明显延长,差异有统计学意义(P<0.01),化合物3组与乙酰唑胺组比较存活时间延长(P<0.01)。与正常对照组比较,缺氧模型组中LD含量显著升高(P<0.01),LDH活性显著降低(P<0.01);与缺氧模型组比较,化合物3组小鼠血浆中LD含量差异无统计学意义,但是LD累积速率明显降低,差异有统计学意义(P<0.01)。结论氮氧自由基与γ-氨基丁酸偶联物的设计路线合理,合成方法简便,产率较高,并且表现出了较高的抗缺氧活性。

旺拉格-37味丸对正常小鼠抗疲劳作用的实验研究

目的:观察旺拉格-37味丸抗疲劳、恢复体力的作用。方法:取30只ICR小鼠,按体重随机分为空白对照组、抗衰复春片组、旺拉格-37组。空白对照组灌胃蒸馏水,抗衰复春片组灌胃抗衰复春片混悬液1.05g/kg,旺拉格-37组灌胃旺拉格-37混悬液2.1g/kg,以0.2mL/10g灌胃,日1次给药,连续灌胃16天。给药第14天观察小鼠疲劳棒耐力时间;第15天观察小鼠游泳至力竭时间和力竭运动后负重游泳的时间;第16天观察小鼠耐缺氧时间。结果:旺拉格-37可明显增加小鼠疲劳转棒落棒时间、增加小鼠负荷游泳时间和力竭运动小鼠负重游泳时间、增加耐缺氧时间,与空白对照组比较组间的差异具有统计学意义,P<0.05。结论:旺拉格-37味丸具有显著的抗疲劳、耐缺氧、恢复体力的作用。

5-甲基-7,4’-二羟基异黄酮水溶性衍生物的合成及其抗缺氧活性

目的5-甲基-7,4’-二羟基异黄酮水溶性衍生物的合成及其抗缺氧活性的比较。方法三氟化硼-乙醚催化的“一锅法”工艺制备母体化合物1,并通过甲基化和磺化反应合成衍生物2～4,常压耐缺氧试验评价其活性。结果化合物3和4水溶性强,且抗缺氧作用等价于母体化合物。结论新合成的水溶性化合物3和4具有明显的抗缺氧活性。

L-精氨酸耐缺氧效应的研究

通过模拟缺氧环境,试验灌胃L-精氨酸溶液对小白鼠耐缺氧时间、呼吸率、血浆和脑组织中NO水平的影响。对比结果显示灌胃L-精氨酸组减压耐缺氧和常压耐缺氧时间比空白组明显延长;肺组织切片显示L-精氨酸组血管明显舒张,耐缺氧效果显著。

胰高血糖素样肽-1对大鼠心肌缺血再灌注/细胞缺氧复氧损伤的保护作用及机制

目的:观察胰高血糖素样肽-1(GLP-1)对大鼠心肌缺血再灌注/细胞缺氧复氧损伤的作用并探讨其机制。方法:建立大鼠缺血再灌注模型,分别设假手术组(sham)、缺血再灌注组(IR)和IR+GLP-1(0.030nmol/L、0.16 nmol/L和0.30 nmol/L)组,缺血30 min后再灌注3 h,Evan's blue-TTC法检测心肌梗死范围;取左心室游离壁心肌组织,TUNEL法检测心肌细胞凋亡,同时测定心肌组织中氧化-抗氧化物质超氧化物歧化酶(SOD)活性及丙二醛(MDA)含量;培养乳鼠心肌细胞,随机分为正常对照组(control)、单纯缺氧复氧组(HR)、HR+GLP-1(1μmol/L、5μmol/L和10μmol/L)组,电镜下观察心肌细胞形态的变化,流式细胞术检测心肌细胞的凋亡,测定乳酸脱氢酶(LDH)释放、SOD活性、MDA含量、活性氧簇(ROS)水平以及线粒体膜电位(MMP)。结果:与IR组相比,IR+GLP-1(0.03 nmol/L、0.16 nmol/L和0.30 nmol/L)组剂量依赖性地减小心肌梗死面积,减轻线粒体超微结构改变及细胞凋亡,增加SOD活性,减少MDA含量(P<0.05或P<0.01);与HR组相比,HR+GLP-1(1μmol/L、5μmol/L和10μmol/L)组剂量依赖性地逆转HR诱导的细胞损伤,增加SOD活性,减少MDA含量,降低ROS水平,减轻HR诱导的MMP降低(P<0.05或P<0.01)。结论:GLP-1可以减轻大鼠心肌缺血再灌注/细胞缺氧复氧损伤;其作用机制可能与增强心肌抗氧化能力及保护线粒体结构和功能有关。