高原低氧条件下不同时间大鼠海马CA1区神经细胞粘附分子的表达

目的:观察高海拔低氧条件下不同时间大鼠海马CA1区神经细胞粘附分子的表达变化,探讨NCAM在机体对低氧应激反应中的作用。方法:将平原SD大鼠运至海拔(4100m)地区,在第2、5、9、15天取大鼠海马,常规免疫组化及RT-PCR检测高原环境下NCAM的表达变化。结果:NCAM在高海拔大鼠海马CA1区神经细胞NCAM的表达在第2、5、9天是明显低于正常(P0.05),在第15天达到正常(P0.05)。结论:高原低氧应激反应后NCAM基因表达先降低后升高,提示其在神经损伤修复过程中可能起重要作用。     

基因体外诱变*

综述了基因体外诱变的一般方法和技术,并将其分为不依赖于PCR体外诱变和依赖于PCR体外诱变两大类。着重介绍了基因体外诱变最新突破即DNA　Shuffling技术。     

荧光素酶研究进展*

荧光素酶 (Luciferase)可以分为萤火虫荧光素酶和细菌荧光素酶两大类。萤火虫荧光素酶是分子量为 60～ 64kD的多肽链 ,在Mg²⁺、ATP、O₂ 存在时 ,催化D 荧光素 (D Luciferin)氧化脱羧 ,发出光 (λ =550～580nm)。细菌荧光素酶是含α、β两个多肽亚基的加单氧酶 ,它催化长链脂肪醛、FMNH₂ 和O₂ 的氧化反应 ,发出绿蓝光 (λ =490nm)。萤火虫荧光素酶和细菌荧光素酶     

染料的生物降解研究*

生物降解法是染料污染治理的重要方法。针对目前使用量较大的偶氮染料、三苯基甲烷染料和蒽醌染料这3大类染料,重点介绍了厌氧和好氧条件下的偶氮还原及其机理、三苯基甲烷染料降解菌和蒽醌染料降解菌的研究进展。     

SIRT1功能及其对卵泡发育和卵母细胞成熟的调控作用 *

沉默信息调节因子1(silent information regulator1, SIRT1)是NAD⁺ 依赖的去乙酰化酶,通过使底物发生去乙酰化而参与细胞众多生理功能的调节,在糖脂代谢、衰老、细胞凋亡、氧化应激等过程中发挥了重要作用。另外,众多研究表明,SIRT1是调控动物卵巢老化、卵泡发育和卵母细胞成熟的重要因子,SIRT1 表达下降或活性改变将导致卵母细胞老化,降低动物的繁殖力。为了充分理解SIRT1功能,并通过调控SIRT1活性而延缓卵巢和卵母细胞老化,从而提高动物繁殖力,简述了SIRT1的激活及其参与细胞内调控的生物过程,并从能量代谢、抗氧化胁迫、染色质重塑的角度讨论了SIRT1的主要功能,重点阐述了SIRT1对动物卵泡发育和卵母细胞成熟的调控作用。     

螺旋藻的纯化*

观察了螺旋藻生长过程中藻丝和杂菌的生长规律,发现中性细菌和碱性细菌的数量始终是藻丝的10⁵～10⁶倍。采用常规的稀释平板法、毛细管法和挑单藻法均无法可靠地获得无菌纯藻。设计用低速离心法洗涤下沉性藻丝,用过滤法洗涤上浮性藻丝,对藻丝进行预处理洗去大量杂菌;对迁移性和非迁移性藻株分别采用夹层法和平板法纯化藻株,使得单根藻丝在平板上形成藻落,获得无菌纯藻。     

植物内生放线菌研究*

近年来从植物组织中发现一些新的放线菌菌种 ,有些内生放线菌产生新的生物活性代谢物 ,或产生具有新特性的酶 ;对植物内生放线菌与植物宿主及其他微生物之间的关系研究有新的发现 ,植物内生放线菌在植物病害防治中的作用已引起重视。本文将简单介绍近年来这方面的研究进展。     

神经肽Y 对炎症及低氧环境下不同癌细胞活力的影响

目的:研究神经肽Y对炎症反应及其对在低氧培养条件下的不同癌细胞活力的影响,探讨应激影响癌症发展的机制.方法:不同浓度神经肽Y(0,10-12M,10-10M,10-8M)与100 ng/ml LPS共孵育巨噬细胞24h后检测NO的浓度及iNOS表达的变化;不同浓度神经肽Y(0,10-9M,10-8M)刺激低氧培养条件下的肝癌细胞株HepG2与乳腺癌细胞株MCF-7 36h,采用cck-8检测细胞活力变化;不同浓度神经肽Y(0,10-9M,10-8)与LPS共孵育巨噬细胞24 h后取上清液离心,采用上清液培养两种癌细胞,并置于低氧条件下36h,cck-8检测细胞活力.结果:实验结果显示,神经肽Y可以抑制巨噬细胞NO的释放(P＜0.05),并降低iNOS的表达(P＜0.05);单独的神经肽Y对低氧培养条件下两种癌细胞的活力没有明显影响(P＞0.05);但在低氧培养条件中,相比于LPS组的条件培养基,LPS加神经肽Y组的条件培养基可明显增强MCF-7的活力(P＜0.05,P＜0.01),而HepG 2的活力则没有统计学差异.结论:神经肽Y可能通过抑制炎症反应,从而增强乳腺癌细胞MCF-7在低氧环境下的活力.     

Relating Cerebral Ischemia and Hypoxia to Insult Intensity

The contributions of five variables believed to influence the brain's metabolism of O2 during hypoxia [duration, PaO2, delta CMRO2 (the difference between normal and experimental oxygen uptake), O2 availability (blood O2 content.CBF), and O2 deficit (delta CMRO2.duration)] were assessed by stepwise and multiple linear regression. Levels of brain tissue carbohydrates (lactate, glucose, and glycogen) and energy metabolites [ATP, AMP, and creatine phosphate (CrP)] were significantly influenced by O2 deficit during hypoxia, as was final CMRO2. After 60 min of reoxygenation, levels of tissue lactate, glucose, ATP, and AMP were related statistically to the O2 deficit during hypoxia; however, CMRO2 changes were always associated more significantly with O2 availability during hypoxia. Creatine (Cr) and CrP levels in the brain following reoxygenation were correlated more to delta CMRO2 during hypoxia. Changes in some brain carbohydrate (lactate and glucose), energy metabolite (ATP and AMP) levels, and [H+]i induced by complete ischemia were also influenced by O2 deficit. After 60 min of postischemic reoxygenation, brain carbohydrate (lactate, glucose, and glycogen) and energy metabolite (ATP, AMP, CrP, and Cr) correlated with O2 deficit during ischemia. We conclude that "O2 deficit" is an excellent gauge of insult intensity which is related to observed changes in nearly two-thirds of the brain metabolites we studied during and following hypoxia and ischemia.     

Oxidative Stress, Hypoxia, and Ischemia-Like Conditions Increase the Release of Endogenous Amino Acids by Distinct Mechanisms in Cultured Retinal Cells

Abstract: The aim of this study was to elucidate the mechanisms by which retinal cells release endogenous amino acids in response to ascorbate/Fe²⁺-induced oxidative stress, as compared with chemical hypoxia or ischemia. In the absence of stimulation, oxidative stress increased the release of aspartate, glutamate, taurine, and GABA only when Ca²⁺ was present. Under hypoxia or ischemia, the release of aspartate, glutamate, glycine, alanine, taurine, and GABA increased mainly by a Ca²⁺-independent mechanism. The increased release observed in N -methyl- d -glucamine⁺ medium suggested the reversal of the Na⁺-dependent amino acid transporters. Upon oxidative stress, the release of aspartate, glutamate, and GABA, occurring through the reversal of the Na⁺-dependent transporters, was reduced by about 30%, although the release of taurine was enhanced. An increased release of [³H]arachidonic acid and free radicals seems to affect the Na⁺-dependent transporters for glutamate and GABA in oxidized cells. All cell treatments increased [Ca²⁺]_i (1.5 to twofold), although no differences were observed in membrane depolarization. The energy charge of cells submitted to hypoxia or oxidative stress was not changed. However, ischemia highly potentiated the reduction of the energy charge, as compared with hypoglycemia or hypoxia alone. The present work is important for understanding the mechanisms of amino acid release that occur in vivo upon oxidative stress, hypoxia, or ischemia, frequently associated with the impairment of energy metabolism.     

Hypoxia/Reoxygenation Stimulates Proliferation Through PKC-Dependent Activation of ERK and Akt in Mouse Neural Progenitor Cells

Cerebral ischemia increases neural progenitor cell proliferation and neurogenesis. However, the precise molecular mechanism is poorly understood. The present study was undertaken to determine roles of extracellular signal-regulated kinase (ERK) and phosphoinositide 3-kinase (PI3K)/Akt and their signaling pathways in neural progenitor cells exposed to hypoxia/reoxygenation (H/R), an in vitro model of ischemia/reperfusion. Neural progenitor cells were isolated from postnatal mouse brain. ERK and Akt were transiently activated during the early phase of reoxygenation following 4-h of hypoxia. The ERK activation was inhibited by U0126, a specific inhibitor of MEK, but not by LY294002, a specific inhibitor of PI3K, whereas the Akt activation was blocked by LY294002, but not by U0126. Reoxygenation following 4-h hypoxia stimulated cell proliferation, which was dependent on ERK and Akt activation. Inhibitors of growth factor receptor (AG1478) and Src (PP2) and the antioxidant N-acetylcysteine did not affect activation of ERK and Akt, while the Ras and Raf inhibitors inhibited activation of ERK, but not Akt. PKC inhibitors inhibited both ERK and Akt activation. Taken together, these results suggest that H/R induces activation of MEK/ERK and PI3K/Akt survival signaling pathways through a PKC-dependent mechanism. These pathways may be responsible for the repair process during ischemia/reperfusion.     

神经干细胞向神经元分化调控的研究进展

神经干细胞是一类具有分裂潜能和自更新能力的母细胞,它可以通过对称分裂和不对称分裂方式产生神经组织的各类细胞,包括神经元、星形胶质细胞和少突胶质细胞。中枢神经系统受到损伤后,神经元和胶质细胞的损伤导致了临床症状,内源性神经干细胞的修复作用不大,原因是干细胞的数量有限,微环境的不允许。移植的神经干细胞进入体内后,由于受到多种因素的影响,常保持未分化状态或大部分分化为胶质细胞。神经干细胞向神经元分化的调控机制及其影响因素直接决定神经干细胞源性神经元的比例和神经元之间功能性突触的数量。现就其研究进展做一综述。     

炎症和氧化应激对内皮祖细胞动员及其功能的影响

内皮祖细胞对于维持血管内皮完整性和血管稳态具有重要作用.增强EPC的数量和功能可使心血管疾病患者获益.炎症、氧化应激对内皮祖细胞动员及其功能发挥具有重要影响,本文着重综述炎症和氧化应激对内皮祖细胞动员的调控,并探讨增进内皮祖细胞数量和功能的相关治疗策略.     

小鼠不同组织及缺氧损伤后的大鼠心肌细胞中RIP3的表达

目的:检测小鼠组织中受体相互作用丝氨酸/苏氨酸蛋白激酶家族(RIPs)表达谱,并检测RIP3在大鼠心肌细胞缺氧损伤后的表达。方法:①采用荧光实时定量PCR分别检测RIPs家族基因在小鼠组织(心、肝、肺、肾、脑、小肠、骨骼肌、脾和主动脉)中的mRNA表达谱,并采用Western blot进一步检测RIP3在小鼠组织的蛋白表达谱。②将培养的大鼠心肌细胞分为缺氧组和对照组,缺氧组置于缺氧环境中培养48 h,采用western blot检测其中RIP3的表达变化。结果:①mRNA水平:RIP1 mRNA在脑组织中表达最高,心脏、肺、肾、骨骼肌较低;RIP2在心脏和肺表达量较其他组织高;RIP3在肠中表达较其他组织高出4倍以上,脑组织中未检测到RIP3表达;RIP4的表达以肺最高,而骨骼肌、脑和血管中表达量低。②蛋白水平:在小鼠组织中,RIP3表达以脑、骨骼肌中最高,心脏、肝、肺中表达较低。③培养的大鼠心肌细胞中,缺氧组心肌细胞的RIP3表达量显著高于对照组(P0.05)。结论:RIPs在小鼠组织中呈现差异表达,而在培养的大鼠心肌细胞缺氧损伤后RIP3表达升高。     

小鼠胚胎干细胞在单层粘附培养中向神经细胞的分化

目的 :探讨小鼠胚胎干 (ES)细胞在无血清培养基中以单层粘附培养方式向神经分化的方法。方法 :比较ES细胞在不同培养基中的生长情况 ,分析ES细胞在不同时间分化形成神经细胞的比例。结果 :( 1 )DMEM F1 2和Neurobasal B2 7的 1∶1混合培养基最适合ES的生长。 ( 2 )单层粘附的ES细胞表达神经细胞粘附分子 (NCAM)的比例随时间增长而增加 ,而nestin的表达先增加后下降。 ( 3)ES细胞可在两周分化为神经胶质及神经元 ,形成神经网络。结论 :小鼠ES细胞可在单层粘附培养中获得向神经的高效分化。     

BRCA-1 基因与神经干细胞

乳腺癌易感基因(Breast cancer susceptibility gene,Brca-1)是肿瘤抑制基因家族中的一员,它是乳腺癌特异性抑癌基因,1994年Miki等[1]采用定位克隆方法首次将Brca-1分离出来。Brca-1能防止细胞过快地或失去控制地生长和分化,在调节细胞进程、DNA损伤修复、细胞生长与凋亡及转录活化和抑制等多种生物学途径都发挥重要作用,Korhonen等2003年报道Brca-1基因可促进体外培养的大鼠来源的神经干细胞的增殖。