热应激心肌细胞损伤的线粒体机制探讨

目的：观察热应激对大鼠凡肌细胞线粒体氧化磷酸化和钙代谢功能的影响、研究线粒体膜渗透性转移（ＰＴ）的变化及其病理学意义、探索热应激心肌细胞损伤发生机制。方法：用Ｋｌａｒｋ氧电极极谱法测定线粒体呼吸功能,用生物发光法主肌ＡＴＰ含量及线粒体Ｃａ＾２＋。ＡＴＰ酶活性;用电感耦合等离子－原子发射光谱仪测定线粒体内Ｃａ＾２＋含量,用分光光度法测定线粒体膜ＰＴ。结果：热应激大鼠心肌细胞线粒体的呼吸控制率（ＲＣＰ     

活性氧对大豆下胚轴线粒体结构与功能的损伤

采用百草枯、H_2O_2和Fenton反应作为外源活性氧,探讨了活性氧对大豆下胚轴离体线粒体的部分功能与结构的伤害。结果表明,活性氧O_2~-,H_2O_2和·OH都能引起线粒体结构的迅速膨胀,呼吸控制比率和氧化磷酸化效率降低,以及细胞色素氧化酶活力下降。通过对线粒体膜脂氢过氧化物和脂质共轭二烯的吸收光谱分析,阐明了活性氧对线粒体的损伤是与膜脂过氧化作用密切相关的。     

线粒体钙单向转运体在心肌低氧/复氧损伤中的作用

目的:观察线粒体钙单向转运体在心肌低氧/复氧损伤中的作用并探讨其机制。方法:应用Langendorff大鼠心脏灌流模型,低氧/复氧(H/R)采用冠脉前降支结扎30 min、复灌120 min的方法。用生物信号采集系统记录左室发展压(LVDP)、左室压最大上升/下降速率(±dP/dtmax)、左室舒张末压(LVEDP);分光光度法分别检测冠脉流出液中乳酸脱氢酶(LDH)的含量和线粒体活性氧(ROS);TTC染色法检测心肌梗死面积。结果:与单纯低氧/复氧组相比,复氧起始给予线粒体钙单向转运体抑制剂钌红(5μmol/L)明显改善左心室各项功能指标,减小心肌梗死面积,降低线粒体ROS和冠脉流出液中LDH含量;而在复氧期起始给予线粒体钙单向转运体激动剂精胺(20μmol/L),显著升高了线粒体ROS活性,冠脉流出液中LDH含量在复氧5 min、20 min、30 min时显著增多,左心室各项功能指标与心肌梗死面积与单纯低氧/复氧组相比无显著差异。ROS清除剂MPG(1 mmol/L)与精胺联合应用则取消了精胺的作用。结论:抑制线粒体钙单向转运体可能通过减少线粒体ROS的生成减轻心脏低氧/复氧损伤。     

线粒体稳定高钙信号诱发超氧炫

线粒体对于细胞钙信号和活性氧信号转导有重要的调控作用．超氧炫是新近发现的单个线粒体超氧阴离子短时程爆发现象,反映了活性氧生成动力学的一种新形式．线粒体钙信号作为重要的细胞功能调控信号,能否及如何调控超氧炫尚待深入研究．本研究对HeLa细胞进行高胞外钙和离子霉素刺激,或用皂苷穿孔细胞质膜后置于高钙细胞内液中,两种方法均显著增加了超氧炫发生的频率．其中,穿孔细胞胞浆高钙诱导的超氧炫依赖于线粒体钙单向转运体,表明超氧炫由线粒体基质内高钙信号所诱发．重要的是,离子霉素诱导的超氧炫发生频率与线粒体稳态钙水平线性相关,而与瞬态线粒体钙无相关性,提示钙离子对超氧炫的调控是一个多步骤、相对缓慢的过程．综上,线粒体基质的稳态高钙是超氧炫的重要调控因子．     

鱼藤酮诱导线粒体轻度损伤细胞氧化应激时硫氧还蛋白转录水平降低

观察鱼藤酮诱导的线粒体轻度损伤细胞氧化应激时硫氧还蛋白转录水平的变化,探讨细胞氧化损伤的可能机制。通过荧光素发光法检测ATP生成、细胞内活性氧(ROS)水平的变化,流式细胞术检测线粒体膜电位,了解低剂量鱼藤酮对线粒体功能的影响;继而用H2O2诱导细胞氧化损伤,MTT法检测细胞活性,观察正常及线粒体缺陷细胞氧化应激时,胞内硫氧还蛋白(Trx)mRNA水平的变化。结果表明,鱼藤酮以剂量依赖方式抑制线粒体ATP的产生、降低线粒体膜电位,而细胞内ROS水平增高;当线粒体损伤细胞氧化应激时胞内Trx mRNA水平降低,提示鱼藤酮诱导线粒体轻度损伤细胞抗氧化能力降低与Trx转录受到抑制有关。     

内质网应激下的内质网-线粒体互作

内质网(endoplasmic reticulum,ER)在蛋白质质量控制体系中占据极其重要的地位.当未折叠和错误折叠蛋白质在ER中累积,会导致所谓"ER应激",进而启动未折叠蛋白响应(unfolded protein response,UPR)以恢复蛋白质稳态.如果ER应激不能得到缓解,UPR也会启动凋亡途径,清除累...     

硒拮抗超氧阴离子导致的心肌线粒体膜损伤

由黄嘌呤和黄嘌呤氧化酶体系产生的超氧阴离子作用于心肌线粒体后,其膜脂双层内产生了脂类自由基。在一定时间内,脂类自由基与自旋捕捉剂形成的加合物的ＥＳＲ信号强度随着孵育时间的增加而加强。１．０μｍｏｌ／Ｌ硒代蛋氨酸（Ｓｅ－Ｍｅｔ）或２．３μｍｏｌ／ＬｍＮａ２ＳｅＯ３可显著清除并抑制脂类自由基的产生。在的影响下,荧光探针ＤＰＨ在膜脂双层中的荧光寿合和膜脂流动性发生了明显改变。一定浓度的Ｓｅ－Ｍｅｔ或Ｎａ２ＳｅＯ３可明显拮抗的上述影响,前者的作用更为显著。     

缺氧及氧恢复对马铃薯块茎线粒体中活性氧及抗氧化酶的影响

选用马铃薯‘Favorita’品种,采用淹水及淹水后恢复通气的方法,研究了缺氧及氧恢复条件对马铃薯块茎亚细胞水平线粒体中活性氧（R0s）及抗氧化酶的影响。结果表明：缺氧胁迫会导致块茎线粒体中超氧阴离子（0;）的发生速率、过氧化氢（H202）及丙二醛（MDA）的含量先升高后下降,其中在缺氧第1天时分别比对照升高43．95％、49．18％、69．20％,在缺氧第3天时各项指标均达到最大值：而缺氧胁迫下超氧化物歧化酶（SOD）、抗坏血酸过氧化物酶（APX）、过氧化氢酶（CAT）活性呈现先降低、后升高、再降低的趋势,其中缺氧第1天分别比对照降低28．35％、31．48％、37．36％。氧恢复时07发生速率,H：O：及MDA含量,SOD、APX、CAT的活性同样呈现先升高后降低的趋势,其中与缺氧1d未恢复对照相比,氧恢复1d分别提高144．69％、63．45％、59．07％、39．29％、11．45％、2．88％。另外,上述各项指标因缺氧胁迫与氧恢复时间的不同而有较大的变化。由此推测：氧恢复比缺氧胁迫更能促进马铃薯块茎线粒体ROS的爆发,加剧膜脂过氧化,并增强线粒体抗氧化酶的短时防御性能。     

活性氧诱导线粒体损伤导致晶体上皮细胞凋亡

目的探讨线粒体损伤在活性氧诱导晶体上皮细胞凋亡中的作用。方法以过氧化氢为处理因素,MTT方法测定过氧化氢对晶体上皮细胞的半数致死浓度(IC50),使用确定的IC50处理培养的人晶体上皮细胞,琼脂糖凝胶电泳检测DNA片段化降解,流式细胞术检测细胞线粒体跨膜电位(Δψm)变化、透射电镜观察细胞线粒体形态,定量免疫印迹检测胞质溶胶中细胞色素c含量的变化及caspase-3的活化。结果过氧化氢对晶体上皮细胞的IC50是32.24μmol/L。32.24μmol/L的过氧化氢处理12h可以检测到晶体上皮细胞染色体DNA发生片段化降解;6h可以检测到线粒体跨膜电位去极化,且随时间延长逐渐加强;18h透射电镜观察可见明显的线粒体膜损伤。定量免疫印迹分析显示细胞色素c在胞质溶胶中的表达逐渐提高及caspase-3活化加强。结论活性氧可能是通过诱导线粒体结构和功能损伤导致晶体上皮细胞凋亡。     

毒黄素对线粒体呼吸耗氧的影响

毒黄素抑制线粒体的呼吸耗氧和氧化磷酸化活力,低浓度毒黄素下耗氧并不增加,也无过氧化氢的形成,此种效应在不同呼吸底物下是类似的。因此认为毒黄素对线粒体的抑制和微生物不同,其主要途径不是因递氢而产生过氧化氢。     

BAG5 Protects against Mitochondrial Oxidative Damage through Regulating PINK1 Degradation

Mutations in PTEN-induced kinase 1 (PINK1) gene cause PARK6 familial Parkinsonism, and loss of the stability of PINK1 may also contribute to sporadic Parkinson''s disease (PD). Degradation of PINK1 occurs predominantly through the ubiquitin proteasome system (UPS), however, to date, few of the proteins have been found to regulate the degradation of PINK1. Using the yeast two-hybrid system and pull-down methods, we identified bcl-2-associated athanogene 5 (BAG5), a BAG family member, directly interacted with PINK1. We showed that BAG5 stabilized PINK1 by decreasing the ubiquitination of PINK1. Interestingly, BAG5 rescued MPP⁺- and rotenone-induced mitochondria dysfunction by up-regulating PINK1 in vitro. In PINK1-null mice and MPTP-treated mice, BAG5 significantly increased in the substantia nigra pars compacta (SNpc) although PINK1 was decreased. Our findings indicated that BAG5, as a key protein to stabilize PINK1, is a promising therapeutic tool for preventing mitochondrial dysfunction following oxidative stress.     

GSK3beta-Mediated Drp1 Phosphorylation Induced Elongated Mitochondrial Morphology against Oxidative Stress

Multiple phosphorylation sites of Drp1 have been characterized for their functional importance. However, the functional consequence of GSK3beta-mediated phosphorylation of Drp1 remains unclear. In this report, we pinpointed 11 Serine/Threonine sites spanning from residue 634∼736 of the GED domain and robustly confirmed Drp1 Ser693 as a novel GSK3beta phosphorylation site. Our results suggest that GSK3beta-mediated phosphorylation at Ser693 does cause a dramatic decrease of GTPase activity; in contrast, GSK3beta-mediated phosphorylation at Ser693 appears not to affect Drp1 inter-/intra-molecular interactions. After identifying Ser693 as a GSK3beta phosphorylation site, we also determined that K679 is crucial for GSK3beta-binding, which strongly suggests that Drp1 is a novel substrate for GSK3beta. Thereafter, we found that overexpressed S693D, but not S693A mutant, caused an elongated mitochondrial morphology which is similar to that of K38A, S637D and K679A mutants. Interestedly, using H89 and LiCl to inhibit PKA and GSK3beta signaling, respectively, it appears that a portion of the elongated mitochondria switched to a fragmented phenotype. In investigating the biofunctionality of phosphorylation sites within the GED domain, cells overexpressing Drp1 S693D and S637D, but not S693A, showed an acquired resistance to H₂O₂-induced mitochondrial fragmentation and ensuing apoptosis, which affected cytochrome c, capase-3, -7, and PARP, but not LC3B, Atg-5, Beclin-1 and Bcl2 expressions. These results also showed that the S693D group is more effective in protecting both non-neuronal and neuronal cells from apoptotic death than the S637D group. Altogether, our data suggest that GSK3beta-mediated phosphorylation at Ser693 of Drp1 may be associated with mitochondrial elongation via down-regulating apoptosis, but not autophagy upon H₂O₂ insult.     

C-Phycocyanin Confers Protection against Oxalate-Mediated Oxidative Stress and Mitochondrial Dysfunctions in MDCK Cells

Oxalate toxicity is mediated through generation of reactive oxygen species (ROS) via a process that is partly dependent on mitochondrial dysfunction. Here, we investigated whether C-phycocyanin (CP) could protect against oxidative stress-mediated intracellular damage triggered by oxalate in MDCK cells. DCFDA, a fluorescence-based probe and hexanoyl-lysine adduct (HEL), an oxidative stress marker were used to investigate the effect of CP on oxalate-induced ROS production and membrane lipid peroxidation (LPO). The role of CP against oxalate-induced oxidative stress was studied by the evaluation of mitochondrial membrane potential by JC1 fluorescein staining, quantification of ATP synthesis and stress-induced MAP kinases (JNK/SAPK and ERK1/2). Our results revealed that oxalate-induced cells show markedly increased ROS levels and HEL protein expression that were significantly decreased following pre-treatment with CP. Further, JC1 staining showed that CP pre-treatment conferred significant protection from mitochondrial membrane permeability and increased ATP production in CP-treated cells than oxalate-alone-treated cells. In addition, CP treated cells significantly decreased the expression of phosphorylated JNK/SAPK and ERK1/2 as compared to oxalate-alone-treated cells. We concluded that CP could be used as a potential free radical-scavenging therapeutic strategy against oxidative stress-associated diseases including urolithiasis.     

Hydrogen Sulfide Protects HUVECs against Hydrogen Peroxide Induced Mitochondrial Dysfunction and Oxidative Stress

Background

Hydrogen sulfide (H₂S) has been shown to have cytoprotective effects in models of hypertension, ischemia/reperfusion and Alzheimer''s disease. However, little is known about its effects or mechanisms of action in atherosclerosis. Therefore, in the current study we evaluated the pharmacological effects of H₂S on antioxidant defenses and mitochondria protection against hydrogen peroxide (H₂O₂) induced endothelial cells damage.

Methodology and Principal Findings

H₂S, at non-cytotoxic levels, exerts a concentration dependent protective effect in human umbilical vein endothelial cells (HUVECs) exposed to H₂O₂. Analysis of ATP synthesis, mitochondrial membrane potential (ΔΨm) and cytochrome c release from mitochondria indicated that mitochondrial function was preserved by pretreatment with H₂S. In contrast, in H₂O₂ exposed endothelial cells mitochondria appeared swollen or ruptured. In additional experiments, H₂S was also found to preserve the activities and protein expressions levels of the antioxidants enzymes, superoxide dismutase, catalase, glutathione peroxidase and glutathione-S-transferase in H₂O₂ exposed cells. ROS and lipid peroxidation, as assessed by measuring H₂DCFDA, dihydroethidium (DHE), diphenyl-l-pyrenylphosphine (DPPP) and malonaldehyde (MDA) levels, were also inhibited by H₂S treatment. Interestingly, in the current model, D, L-propargylglycine (PAG), a selective inhibitor of cystathionine γ-lyase (CSE), abolished the protective effects of H₂S donors.

Innovation

This study is the first to show that H₂S can inhibit H₂O₂ mediated mitochondrial dysfunction in human endothelial cells by preserving antioxidant defences.

Significance

H₂S may protect against atherosclerosis by preventing H₂O₂ induced injury to endothelial cells. These effects appear to be mediated via the preservation of mitochondrial function and by reducing the deleterious effects of oxidative stress.     

Defence against multiple enemies

Although very common under natural conditions, the consequences of multiple enemies (parasites, predators, herbivores, or even 'chemical' enemies like insecticides) on investment in defence has scarcely been investigated. In this paper, we present a simple model of the joint evolution of two defences targeted against two enemies. We illustrate how the respective level of each defence can be influenced by the presence of the two enemies. Furthermore, we investigate the influences of direct interference and synergy between defences. We show that, depending on certain conditions (costs, interference or synergy between defences), an increase in selection pressure by one enemy can have dramatic effects on defence against another enemy. It is generally admitted that increasing the encounter rate with a second natural enemy can decrease investment in defence against a first enemy, but our results indicate that it may sometimes favour resistance against the first enemy. Moreover, we illustrate that the global defence against one enemy can be lower when only this enemy is present: this has important implications for experimental measures of resistance, and for organisms that invade an area with less enemies or whose community of enemies is reduced. We discuss possible implications of the existence of multiple enemies for conservation biology, biological control and chemical control.     

Defence against reactive oxygen species

As part of the European Commission Concerted Action on Functional Food which was managed by the International Life Sciences Institute (Europe) a series of Theme Papers was produced which examined the ‘state of the art’ with respect to the subject matter and made recommendations for research. This paper is a summary of the paper concerned with Defence Against Reactive Oxygen species. Having reviewed the scientific literature the authors concluded that certain stringent criteria, which they identified, would need to be satisfied in order to be able to conclude that free radical events are involved in certain human diseases, and that antioxidants are capable of modulating these events and thus reducing the risk of disease. Although there is some evidence that would lead to this conclusion the authors demonstrated that there is at present insufficient evidence available on which to base a firm conclusion that antioxidants are capable of reducing risk of disease, and very little evidence that addresses the important question as to how much of the nutrients concerned are required in the diet to achieve the objective of reducing risk. Research priorities address the need in particular for the development and validation of cellular markers of oxidative damage which are required before there can be new human studies that address the question. There is also a need for more information as to the pharmacokinetics of uptake from diet, distribution and cellular concentration of the antioxidants.