缺氧预适应小鼠脑组织中缺氧诱导因子-1的表达

为探讨缺氧诱导因子 1 (HIF 1 )在缺氧预适应小鼠脑组织中的表达 ,用Western印迹法检测慢性缺氧 (H)和不缺氧 (C)HeLa细胞、急性重复性缺氧 0次 (H0 )、1次 (H1)、4次 (H4 )小鼠脑组织中的HIF 1α。结果 :慢性缺氧HeLa细胞中可检测到较多的HIF 1α,H0 组脑组织中检测不到HIF 1α ,H1组检测到微量HIF 1α,H4 组检测到较多HIF 1α。结果显示 :脑组织中HIF 1α的含量随缺氧预适应的产生而逐步增加 ,提示HIF 1可能参与缺氧预适应的形成。     

普鲁卡因对缺氧心肌细胞的影响

目的 探讨普鲁卡因对心肌细胞缺氧损伤的影响。方法 将原代培养成活48h的大鼠乳鼠心肌细胞分为三组：A组为对照组（氰化钠造成心肌细胞内缺氧模型）,B组为Prol组（缺氧＋7．4mg／L普鲁卡因）,C组为Pro2组（缺氧＋14．8mg／L普鲁卡因）。比较三组心肌细胞形态学（倒置相差显微镜、透射电镜观察）的变化及吸光度A值的改变。结果 缺氧12h后,对照组细胞搏动功能变化明显,呈散在细胞搏动,而实验组搏动频率减慢。随着时间的延长,细胞形态学变化逐渐明显,对照组较实验组变化更显著。结论 普鲁卡因对培养心肌细胞缺氧损伤有一定的保护作用。     

急性低压缺氧暴露后血脑屏障通透性的变化及其意义

目的：观察在急性低压缺氧条件下,大鼠血脑屏障通秀性的变化特点,为阐明低压缺氧作用下脑功能障碍的可能机理及临床上特殊病例治疗方案的确定提供生理学依据。方法：选择在雄性SD大鼠12只,随机分为对照组、5000m急性低压缺氧暴露组。实验组动物于低压舱内,以20m/s的速率上升,至5000m,停留5hm,而后以20m/s的速率下降至地面;出舱后立即经心脏灌注硝酸镧固定液,开颅取脑,制成切片,置透射电镜下观察。结果：急性低压缺氧暴露5h后即刻,即可见镧颗粒通过大鼠脑皮质的毛细血管内皮细胞膜,沉积于毛细血管内皮细胞浆内、细胞核膜上以及血管周围,弥漫性地分布于脑间质细胞间隙,并附着于神经细胞膜上,而对照组大鼠,镧颗粒仅滞留于大脑皮层的毛细血管腔内。结论：5000m以上低压缺氧连续暴露5h,可引起大鼠血脑屏障通透性增加。这可能在低压缺氧导致脑水肿的发生以及脑功能障碍的过程中起重要作用,对确定临床上特殊病例的治疗也有一定参考价值。     

The Effect of Erigeron Breviscapus on Proliferation of Pulmonary Artery Smooth Muscle Cells in Hypoxic Porcines

Erigeron breviscapus can relax microarteries,improve microcirculation,increase tissue bloodstream,enhance heart function and decrease bloodviscosity.Presently,good curative effects on is-chemia has been achieved,but few studies have beenconducted on the treatment of hypoxic pulmonaryhypertension( HPH) .In this study,MTT and ex-pression of PCNA was used to examine the prolifera-tion of PASMC and investigate the mechanism of ef-fectof EB on HPH.1　 MATERIALSAND METHODS1 .1　 Cult…     

人参皂甙Rg1对缺氧豚鼠心肌细胞游离钙浓度降低作用的研究

目的探讨人参皂甙(ginsentosides,Gin)单体Rgl及维拉帕米(verapamil,Ver)对豚鼠心肌细胞内游离钙浓度([Ca2+]i)变化的影响.方法采用离体豚鼠心脏Langendorff法灌注,胶原酶Ⅰ型分离心肌细胞,用荧光指示剂方法(Fura-2/AM)标记心肌([Ca2+]i)变化.将心肌细胞悬液分为3组对照组、Rgl组和Ver组.观察缺氧后心肌[Ca2+]i的变化.结果(1)正常氧状态心肌[Ca2+]i均值为(125.4±10.3)nmol/L(n=20).(2)缺氧状态下,心肌[Ca2+]i增加与缺氧时间(程度)直线相关,相关系数r为0.98左右.(3)Rgl对缺氧后心肌[Ca2+]i增加明显延缓.结论Rgl在缺氧条件下,使心肌[Ca2+]i明显下降,从而阻止心肌细胞内钙超载,其作用与Ver相似,我们认为Rgl具有心肌细胞的保护作用.     

不同抗炎药物对缺氧所致大鼠离体肺血管环张力变化的影响

为研究离体大鼠肺血管在缺氧时张力的变化,以及甾体、非甾体类抗炎药物对此变化影响的异同性,采用等长收缩技术,测定加入消炎痛或地塞米松前后张力改变的特点及两药作用的差异。结果发现Wistar大鼠与Sprague-Dawley大鼠肺血管环对缺氧的反应不同,后者仅出现收缩反应,而Wistar大鼠在收缩前出现一内皮依赖的舒张;COX非特异性抑制剂消炎痛对缺氧所致的舒张和收缩均有增强作用;COX-2特异性抑制剂地塞米松则在明显抑制舒张的同时轻度增强收缩反应。结果表明不同种属大鼠的肺血管缺氧反应可能存在差异;缩管性PGs和扩管性PGs分别调节急性肺血管缺氧的舒张和收缩反应,这一过程呈一定的内皮依赖性;非选择性和选择性的COX抑制剂对肺血管缺氧反应的作用不尽相同。     

Effects of cobalt and chromium ions on glycolytic flux and the stabilization of hypoxia‐inducible factor‐1α in macrophages in vitro

Implant wear and corrosion have been associated with adverse tissue reactions that can lead to implant failure. Wear and corrosion products are therefore of great clinical concern. For example, Co²⁺ and Cr³⁺ originating from CoCrMo‐based implants have been shown to induce a proinflammatory response in macrophages in vitro. Previous studies have also shown that the polarization of macrophages by some proinflammatory stimuli is associated with a hypoxia‐inducible factor‐1α (HIF‐1α)‐dependent metabolic shift from oxidative phosphorylation (OXPHOS) towards glycolysis. However, the potential of Co²⁺ and Cr³⁺ to induce this metabolic shift, which plays a determining role in the proinflammatory response of macrophages, remains largely unexplored. We recently demonstrated that Co²⁺, but not Cr³⁺, increased oxidative stress and decreased OXPHOS in RAW 264.7 murine macrophages. In the present study, we analyzed the effects of Co²⁺ and Cr³⁺ on glycolytic flux and HIF‐1α stabilization in the same experimental model. Cells were exposed to 6 to 24 ppm Co²⁺ or 50 to 250 ppm Cr³⁺. Glycolytic flux was determined by analyzing extracellular flux and lactate production, while HIF‐1α stabilization was analyzed by immunoblotting. Results showed that Co²⁺, and to a lesser extent Cr³⁺, increased glycolytic flux; however, only Co²⁺ acted through HIF‐1α stabilization. Overall, these results, together with our previous results showing that Co²⁺ increases oxidative stress and decreases OXPHOS, suggest that Co²⁺ (but not Cr³⁺) can induce a HIF‐1α‐dependent metabolic shift from OXPHOS towards glycolysis in macrophages. This metabolic shift may play an early and pivotal role in the inflammatory response induced by Co²⁺ in the periprosthetic environment.     

低氧环境对椎间盘自发性吸收的影响及其作用机制

目的探讨低氧环境对椎间盘自发性吸收的影响及其作用机制。方法取SPF级成年日本大耳兔9只,雌雄不限,平均体质量2 kg。将兔处死后取脊柱髓核组织,经消化、分离、培养后获得传代髓核细胞,将生长良好的髓核细胞制成细胞悬液。根据不同时效的低氧环境将细胞分为5组对照组(常氧浓度下培养6 h)、低氧6 h组(2%O2浓度下培养6 h)、低氧12 h组(2%O2浓度下培养12 h)、低氧24 h组(2%O2浓度下培养24 h)和低氧48 h组(2%O2浓度下培养48 h)。采用实时聚合酶链反应法检测缺氧诱导因子(HIF)-1α、3型酸敏感离子通道(ASIC3)及水通道蛋白3(AQP3)mRNA表达水平,采用流式细胞仪检测各组髓核细胞凋亡情况。采用SPSS 24.0软件对数据进行分析。结果与对照组比较,低氧各组细胞凋亡率均明显升高,差异均有统计学意义(均P<0.01);与低氧12、24和48 h组比较,低氧6 h组细胞凋亡率最高,差异均有统计学意义(均P<0.01)。与对照组比较,低氧各组细胞HIF-1α和ASIC3 mRNA表达水平均明显上升,AQP3 mRNA表达水平均明显下降,差异均有统计学意义(均P<0.01);与低氧12、24和48 h组比较,低氧6 h组HIF-1α和ASIC3 mRNA表达水平最高,差异均有统计学意义(均P<0.01)。结论短时间低氧环境可以促进髓核细胞凋亡,从而加速椎间盘突出组织自发性吸收进程,其机制可能与HIF-1α和ASIC3的表达增加及AQP3的表达下降有关。     

Combination of Methods for <Emphasis Type="Italic">in Vitro</Emphasis> Study of Antioxidant Properties of Chemical Compounds

Blood ammonia concentration increased in the portal vein (by 1.4 times) and inferior vena cava (caudal to the renal vein inflow, by 2.2 times; and cranial to the hepatic vein inflow, by 2.5 times) of rats 3 h after intragastric administration of 16.57 M ethanol solution (446 mmol/kg, ≈ 1.4 LD_{50/48 h}). Ammonia concentration in mixed blood samples (post-decapitation) increased by 39%. The rate of ammonia accumulation was 3-fold higher in an intraperitoneal lavage solution. Three-hour exposure of ethanol-treated animals to atmospheric ammonia (0.84–1.07 mg/liter, i.e. ≈ 1/8LC₅₀ for intact rats) was followed by a 2.4-fold increase in blood ammonia concentration as compared to specimens of the ethanol group. Ammonia inhalation potentiated the lethal effect of ethanol (dose variation factor 0.81), suppressed external respiration, and decreased oxygen consumption. Our results indicate that kinetic changes in endogenous ammonia have an adverse effect on the outcome of alcohol intoxication in rats. __________ Translated from Byulleten' Eksperimental'noi Biologii i Meditsiny, Vol. 145, No. 6, pp. 688–690, June, 2008