Mutation of cytotoxin-associated gene A affects expressions of antioxidant proteins of Helicobacter pylori

AIM: To determine if disruption of the cagA gene of Helicobacter pylori (H pylori) has an effect on the expression of other proteins at proteome level. METHODS: Construction of a cagA knock out mutant Hp27 _△cagA (cagA -) via homologous recombination with the wild-type strain Hp27 (cagA+) as a recipient was performed. The method of sonication-urea-CHAPS-DTT was employed to extract bacterial proteins from both strains. Soluble proteins were analyzed by two-dimensional electrophoresis (2-DE). Images of 2-DE gels were digitalized and analyzed. Only spots that had a statistical signif icance in differential expression were selected and analyzed by matrix-assisted laser desorption/ionizationtime of flight mass spectrometry (MALDI-TOF-MS). Biological information was used to search protein database and identify the biological function of proteins. RESULTS: The proteome expressions between wild-type strain and isogenic mutant with the cagA gene knocked-out were compared. Five protein spots with high abundance in bacteria proteins of wild-type strains, down-regulated or absently expressed in bacteria proteins of mutants, were identified and analyzed. From a quantitative point of view, the identified proteins are related to the cagA gene and important antioxidant proteins of H pylori , including alkyl hydroperoxide reductase (Ahp), superoxide dismutase (SOD) and modulator of drug activity (Mda66), respectively, suggesting that cagA is important to maintain the normal activity of antioxidative stress and ensure H pylori persistent colonization in the host. CONCLUSION: cagA gene is relevant to the expressions of antioxidant proteins of H pylori, which may be a novel mechanism involved in H pylori cagA pathogenesis.

芝麻渣蛋白多肽抗氧化性研究

该研究考察了不同蛋白酶对芝麻渣中提取的芝麻蛋白水解度的影响。结果表明,中性蛋白酶、木瓜蛋白酶和风味蛋白酶对芝麻蛋白有较高的水解度,而中性蛋白酶水解度最高,达到10.54%,碱性蛋白酶水解度最低,只有2%。测定了水解后的芝麻蛋白多肽抗氧化活性,结果发现芝麻蛋白多肽表现出较强的清除DPPH、超氧阴离子、ABTS+·和羟基自由基的能力,表明芝麻蛋白多肽具有很强的抗氧化活性,是一种潜在的抗氧化剂。

Association between heat stress and oxidative stress in poultry;mitochondrial dysfunction and dietary interventions with phytochemicals

Heat as a stressor of poultry has been studied extensively for many decades; it affects poultry production on a worldwide basis and has significant impact on well-being and production. More recently, the involvement of heat stress in inducing oxidative stress has received much interest. Oxidative stress is defined as the presence of reactive species in excess of the available antioxidant capacity of animal cells. Reactive species can modify several biologically cellular macromolecules and can interfere with cell signaling pathways. Furthermore, during the last decade, there has been an ever-increasing interest in the use of a wide array of natural feed-delivered phytochemicals that have potential antioxidant properties for poultry. In light of this, the current review aims to（1） summarize the mechanisms through which heat stress triggers excessive superoxide radical production in the mitochondrion and progresses into oxidative stress,（2） illustrate that this pathophysiology is dependent on the intensity and duration of heat stress,（3） present different nutritional strategies for mitigation of mitochondrial dysfunction, with particular focus on antioxidant phytochemicals.Oxidative stress that occurs with heat exposure can be manifest in all parts of the body; however, mitochondrial dysfunction underlies oxidative stress. In the initial phase of acute heat stress, mitochondrial substrate oxidation and electron transport chain activity are increased resulting in excessive superoxide production. During the later stage of acute heat stress, down-regulation of avian uncoupling protein worsens the oxidative stress situation causing mitochondrial dysfunction and tissue damage. Typically, antioxidant enzyme activities are upregulated. Chronic heat stress, however, leads to downsizing of mitochondrial metabolic oxidative capacity, up-regulation of avian uncoupling protein, a clear alteration in the pattern of antioxidant enzyme activities, and depletion of antioxidant reserves.Some phytochemicals, such as various types of flavonoids and related compounds, were shown to be beneficial in chronic heat-stressed poultry, but were less or not effective in non-heat-stressed counterparts. This supports the contention that antioxidant phytochemicals have potential under challenging conditions. Though substantial progress has been made in our understanding of the association between heat stress and oxidative stress, the means by which phytochemicals can alleviate oxidative stress have been sparsely explored.

Induction of Antioxidant and Heat Shock Protein Responses During Torpor in the Gray Mouse Lemur, Microcebus murinus

A natural tolerance of various environmental stresses is typically supported by various cytoprotective mechanisms that protect macromolecules and promote extended viability. Among these are antioxidant defenses that help to limit damage from reactive oxygen species and chaperones that help to minimize protein misfolding or unfolding under stress conditions. To understand the molecular mechanisms that act to protect cells during primate torpor, the present study characterizes antioxidant and heat shock protein（HSP） responses in various organs of control（aroused）and torpid gray mouse lemurs, Microcebus murinus. Protein expression of HSP70 and HSP90 a was elevated to 1.26 and 1.49 fold, respectively, in brown adipose tissue during torpor as compared with control animals, whereas HSP60 in liver of torpid animals was 1.15 fold of that in control（P 〈 0.05）. Among antioxidant enzymes, protein levels of thioredoxin 1 were elevated to 2.19 fold in white adipose tissue during torpor, whereas Cu–Zn superoxide dismutase 1 levels rose to 1.1 fold in skeletal muscle（P 〈 0.05）. Additionally, total antioxidant capacity was increased to 1.6 fold in liver during torpor（P 〈 0.05）, while remaining unchanged in the five other tissues. Overall, our data suggest that antioxidant and HSP responses are modified in a tissue-specific manner during daily torpor in gray mouse lemurs. Furthermore, our data also show that cytoprotective strategies employed during primate torpor are distinct from the strategies in rodent hibernation as reported in previous studies.

红曲菌mrfA缺失突变株发酵过程中的生理生化特征

为了解红曲菌G蛋白信号调节子mrfA缺失突变株发酵过程中的生理生化特征,测定了该突变菌株在液态发酵过程中的生物量、葡萄糖利用率、pH值、蛋白酶、几丁质酶、过氧化氢酶、超氧化物歧化酶、谷胱甘肽过氧化物酶的活性。与原始菌株红色红曲菌M7相比较,mrfA缺失突变株在生长后期生物量会明显减少,在发酵过程中葡萄糖消耗率、蛋白酶和几丁质酶均高于出发菌株,其中蛋白酶活力在第6天达到最高。与此同时,mrfA缺失突变株的过氧化氢酶、超氧化物歧化酶、谷胱甘肽过氧化物酶酶活也均高于出发菌株M7。这些结果初步表明mrfA缺失突变株与原始菌株相比自溶特征更加明显,推测蛋白酶是诱发菌体自溶的主要水解酶,超氧化物歧化酶是其防御氧化应激的主要酶。研究结果为进一步理解mrfA介导的红曲菌自溶机理奠定了基础。

黑果枸杞子对过度训练大鼠骨骼肌MAPK信号通道蛋白表达及抗氧化应激损伤能力的影响

目的:研究黑果枸杞子对过度训练大鼠骨骼肌MAPK信号通道蛋白表达及抗氧化应激损伤能力的影响。方法:以等量负荷有氧运动训练和大强度耐力训练大鼠为模型,50只SPF级Wistar 49 d龄雄性大鼠为对象,随机分为4组,分别为正常组、有氧训练组、过度训练组、过度训练+黑果枸杞子组,每组12只(剔除不符合实验要求的大鼠)。每天灌胃(ig)给药1次,黑果枸杞子干预组剂量为4.48 mg·kg-1,ig体积为5 m L·kg-1,其他组ig等体积生理盐水。42 d负荷游泳训练后,测试各组大鼠骨骼肌丝裂素活化蛋白激酶(MAPK)信号系统蛋白表达及氧化应激损伤相关指标,分光光度法检测骨骼肌超氧化物歧化酶(SOD)活性及丙二醛(MDA)含量;蛋白质免疫印迹(Western blot)法检测MAPK信号通道蛋白表达;酶联免疫吸附测试法(ELISA)检测3-硝基酪氨酸(3-NT),8-羟基脱氧鸟苷(8-OHd G)含量;乙酰半胱氨酸法检测血清肌酸激酶(CK)活性;苯肼显色法检测乳酸脱氢酶(LDH)活性。结果:力竭游泳时间,有氧训练组较正常组有所延长,黑果枸杞子干预组较过度训练组显著增加(P<0.01)。骨骼肌SOD活性,有氧训练组略高于正常组;过度训练组较正常组和有氧训练组明显下降(P<0.05),黑果枸杞子干预组较过度训练组明显升高(P<0.05)。骨骼肌MDA含量,有氧训练组略低于正常组;过度训练组较正常组和有氧训练组显著升高(P<0.01),黑果枸杞子干预组较过度训练组显著降低(P<0.01)。骨骼肌3-NT,8-OHd G,有氧训练组略高于正常组;过度训练组较正常组和有氧训练组显著升高(P<0.01);黑果枸杞子干预组较过度训练组明显降低(P<0.05)。血清LDH活性,有氧训练组略高于正常组;过度训练组较正常组和有氧训练组均显著升高(P<0.01);黑果枸杞子干预组较过度训练组明显升高(P<0.05)。血清CK活性,有氧训练组略高于正常组;过度训练组较正常组和有氧训练组显著升高(P<0.01);黑果枸杞子干预组较过度训练组显著降低(P<0.01)。p38 MAPK,细胞外信号调节蛋白激酶(ERK)信号通路蛋白表达,有氧训练组高于正常组(P<0.05),低于过度训练组(P<0.05);过度训练组高于安静组(P<0.01);黑果枸杞子干预组高于正常组(P<0.05),低于过度训练组(P<0.05)。结论:补充黑果枸杞子可以有效缓解过度训练导致的机体内环境失衡,抑制MAPK信号通路蛋白的过度表达,激活过度训练大鼠骨骼肌MAPK信号转导系统诱导抗氧化酶基因表达,提高机体尤其是骨骼肌的氧自由基清除能力,调节机体的抗氧化应激损伤能力,预防和延缓氧化应激损伤及运动疲劳的发生与发展。

麦胚蛋白酶解物清除自由基及抗氧化作用的研究

研究麦胚蛋白酶解物的体外抗氧化活性。采用邻苯三酚自氧化、Fenton反应及FTC法分析酶解物清除自由基及抗脂质过氧化的效果。结果表明:麦胚蛋白酶解产物对三种自由基均有一定的清除活性,量效关系明显;其清除O2-·、·OH、DPPH·三种自由基的IC50分别为6.2、3.5、2.3mg/mL;在亚油酸体系中具有良好的抗氧化效果。麦胚蛋白酶解物是有效的、多功能的天然抗氧化剂和自由基清除剂,具有综合开发利用的价值。

高压均质对乳清蛋白糖基化产物抗氧化的影响

通过干法糖基化,以一定质量比例乳清蛋白和岩藻多糖(1︰3)作为糖基化反应原料,研究不同均质压力(0,70和120 MPa)条件下乳清蛋白和岩藻多糖糖基化产物反应特性以及体外抗氧化活性。试验结果表明,高压均质可促进蛋白质和多糖的糖基化反应,乳清蛋白-岩藻多糖混合物在294 nm和420 nm的吸光度随着均质压力的增加而显著变化(p<0.05),120 MPa条件处理下的样品的褐变程度要远大于未处理组。DPPH自由基清除率试验结果表明,乳清蛋白-岩藻多糖混合物经高压均质处理后可提高其抗氧化能力,但是随着糖基化反应进行,乳清蛋白-岩藻多糖糖基化产物DPPH自由基清除率无显著差异(p>0.05)。

新疆3种植物不同提取部位的抗氧化活性及其对PTP1B的抑制作用

目的:考察新疆树莓、黑果悬钩子和天山茶藨不同萃取部位的抗氧化活性及其对蛋白酪氨酸磷酸酶1B(PTP1B)的抑制作用,筛选具有抗氧化及降血糖活性的有效部位。方法:采用甲醇提取、分步萃取的方法分别制备了不同的极性部位。测定了3种植物不同部位的总黄酮含量,果实提取物经AB-8型大孔树脂纯化后制备了果实花青素部位;利用2,2'-联氮-二(3-乙基-苯并噻唑-6-磺酸)二铵盐法,1,1-二苯基-2-三硝基苯肼法及PTP1B抑制活性实验比较了不同部位的相关活性,并分析了黄酮含量和活性的相关性。结果:经AB-8型大孔树脂纯化后,树莓果实花青素含量由(12.72±0.14)mg·g-1提高到(238.13±1.18)mg·g-1,天山茶藨果实的花青素含量由(35.36±0.45)mg·g-1提高到(548.05±1.11)mg·g-1,随着花青素含量的升高,其抗氧化活性和PTP1B抑制活性也显著升高。黑果悬钩子茎乙酸乙酯部位总黄酮含量最高,为(658.65±11.43)mg·g-1;黑果悬钩子茎水部位抗氧化活性最高,ABTS和DPPH自由基清除能力分别为(4.53±0.07),(2.82±0.09)mmol Trolox·g-1当量;黑果悬钩子茎水部位对PTP1B的抑制率最高,半数抑制浓度为(0.08±0.01)mg·L-1。结论:这3种植物不同萃取部位均具有良好的抗氧化活性和PTP1B抑制作用,黑果悬钩子茎水部位为主要的抗氧化活性和PTP1B抑制活性的有效部位,树莓和天山茶藨果实中花青素是主要的活性成分,天山茶藨茎叶中黄酮是主要的抗氧化活性成分。