铜绿假单胞菌L型诱导血管内皮细胞凋亡机制的探讨

目的探讨铜绿假单胞菌L型诱导血管内皮细胞凋亡机制。方法 Annexin V-FITC/PI双染荧光法和流式细胞术法检测铜绿假单胞菌L型感染血管内皮细胞8 h时的凋亡率,分光光度法检测细胞Caspase-9活化情况。结果铜绿假单胞菌L型和血管内皮细胞共培养8 h时细胞凋亡率、Caspase-9活化程度较对照组增高（P〈0.05）。结论铜绿假单胞菌L型可通过活化Caspase-9的线粒体途径诱导血管内皮细胞凋亡。     

一氧化氮促进体外培养大鼠脑室下区神经干细胞的分化

目的：探讨一氧化氮（NO）对新生大鼠体外培养的神经干细胞（NSCs）分化的作用。方法：采用常规方法分离新生大鼠脑室下区（SVZ）组织,进行NSCs体外培养。用DETA／NO作为NO供体,用L-NAME作为一氧化氮合酶（NOS）抑制剂。免疫荧光法检测NSCs标志物-巢蛋白（nestin）、神经元标志物-8Ⅲ型微管蛋白（Tuj-1）和星型胶质细胞标志物-胶质原纤维酸性蛋白（GFAP）的表达,还检测了神经元型NOS的表达。用Greiss还原法检测培养液中总NO的浓度。结果：培养的神经球均为nestin阳性、BIdu阳性和nNOS阳性。NSCs和40μmol／L、50μmol／L、60μmol／LDEFA／N0共培养5d,实验组培养液中N0浓度较对照组显著增高（P〈0．01）,相应实验组分化的神经元数和星型胶质细胞数较对照组明显增加（P〈0．01和P〈0．05）。NSCs和100μmol／L、150μmol／L、200μmol／LL-NAME共培养5d,实验组培养液中NO浓度较对照组降低（P〈0．05）,相应实验组分化的神经元数和星型胶质细胞数也较对照组减少（P〈0．05）。结论：NO能直接促进大鼠SVZ体外培养的NSCs分化。     

短链脂肪酸作用下伤寒沙门菌诱导巨噬细胞凋亡机制的探讨

目的了解短链脂肪酸(SCFA)作用伤寒沙门菌诱导巨噬细胞凋亡机制。方法将SCFA作用伤寒沙门菌感染巨噬细胞8 h后,检测TNF-α、caspase3、caspase8、caspase9及NO的产生量,同时检测加入caspase3、caspase8、caspase9抑制剂和TNF-α抗体后的细胞凋亡率。结果作用8 h后caspase3、caspase8及NO、TNF-α的产生量均高于对照组(P0.01)。caspase3、caspase8抑制剂和TNF-α抗体均能不同程度抑制SCFA作用伤寒沙门菌诱导的巨噬细胞凋亡(P0.01)。结论 SCFA作用伤寒沙门菌诱导巨噬细胞凋亡可以通过NO及TNF-α介导,caspase3和caspase8参与的外源性凋亡途迳。     

葡萄糖氧化酶诱导肝细胞氧化应激模型的建立

目的：研究不同浓度葡萄糖氧化酶（GO）对人肝细胞L02氧化应激水平的影响,以确定建立肝细胞氧化应激模型的合适浓度。方法：用不同浓度GO干预L02肝细胞2h,MTT法检测细胞的存活率,流式细胞术检测细胞内活性氧簇（ROS）,荧光强度（FI）来表示ROS水平。分光光度法检测检测细胞MDA、GSH,速率法检测细胞培养液LDH、AST和ALT的水平。结果：①随GO浓度增加,肝细胞的存活率逐渐降低,其中75U/L、100U/L和125U/L组存活率显著低于对照组（P〈0.05）。②随GO浓度增加,MDA含量逐渐增高,其中50U/L、75U/L、100U/L、125U/L组MDA水平较对照组显著增高（P〈0.05）。GSH水平随GO浓度增高而逐渐减低,各干预组较对照组均显著降低（P〈0.05）。GO各干预组FI均较对照组显著降低（P〈0.05）。③各干预组LDH活性均显著高于对照组（P〈0.05）,50U/L、75U/L、100U/L、125U/L干预组AST与ALT水平均较对照组显著增高（P〈0.05）。结论：GO能引起的肝细胞氧化应激损伤有剂量依赖性,100U/L是建立肝细胞氧化应激的合适浓度。     

二苯乙烯苷抑制过氧化氢诱导的人脐静脉内皮细胞凋亡

目的：研究二苯乙烯苷（TSG）对过氧化氢（H2O2）诱导人脐静脉内皮细胞（HUVECs）凋亡的保护作用。方法：运用四甲基偶氮唑盐还原法（MTT法）和流式细胞术筛选建立细胞凋亡模型的H2O2合适浓度以及检测不同浓度TSG对H2O2诱导HUVECs的增殖率和凋亡率;Hoechst33258染色观察细胞凋亡形态。结果：MTT及流式法筛选300μmol/L为H2O2作用于细胞的最适凋亡浓度。MTT和流式结果显示,与H2O（2300μmol/L）损伤组比较,10μmol/L与100μmol/LTSG预处理组细胞的增殖率增加（P〈0.05）,凋亡率显著降低（P〈0.01）;Hoechst33258染色观察TSG能降低H2O2诱导的细胞凋亡,使细胞凋亡数减少。结论：TSG能抑制H2O2诱导的HUVECs凋亡,从而起到保护血管内皮细胞的作用。     

铜绿假单胞菌生物膜悬液和藻酸盐对小鼠巨噬细胞吞噬功能的影响

目的探讨铜绿假单胞菌（PA）生物膜和藻酸盐成分对小鼠巨噬细胞吞噬功能的影响。方法用具有生物膜成分的PA悬液分别感染肺部巨噬细胞缺乏小鼠和正常小鼠,比较组织中的细菌数量。提取小鼠腹腔巨噬细胞,藻酸盐作用后加入PA悬液,测定巨噬细胞对细菌的吞噬率。巨噬细胞经不同浓度的藻酸盐作用后,中性红法检测巨噬细胞吞噬能力。结果巨噬细胞缺乏组和对照组肺部组织的细菌数量分别为（4.16±3.36）×10^5/ml和（5.15±1.92）×10^5/ml,t=0.7211,P=0.483。生物膜细菌组的巨噬细胞吞噬率与对照组的吞噬率分别为（13.82±4.71）%和（42.73±11.00）%,Q=12.3231,P〈0.01。表明生物膜细菌组比对照组更能抵抗巨噬细胞的吞噬。加藻酸盐组的巨噬细胞吞噬率与对照组的吞噬率分别为（22.91±6.20）%和（42.73±11.00）%,Q=8.4465,P〈0.01。表明加藻酸盐组比对照组更能抵抗巨噬细胞的吞噬。当藻酸盐浓度为0、25、50、75、100、125、150μg/ml时,以吸光度A（540nm）值表示其巨噬细胞吞噬中性红的能力分别为：0.271±0.044、0.456±0.062、0.445±0.061、0.551±0.065、0.210±0.053、0.186±0.026、0.195±0.025。当藻酸盐≤75μg/ml时巨噬细胞吞噬中性红的能力增强,与0μg/ml组相比P〈0.05;当藻酸盐〉75μg/ml时巨噬细胞吞噬中性红的能力降低,与0μg/ml组相比P〈0.05。结论巨噬细胞有阻止PA入侵的作用。PA生物膜可以抑制巨噬细胞的吞噬。PA生物膜藻酸盐成分在〈75μg/ml时促进巨噬细胞的吞噬,而在较大剂量时抑制巨噬细胞的吞噬功能。     

解偶联蛋白2通过抗氧化应激反应预防酒精性心肌损害

目的：探讨解偶联蛋白2（uncouplingprotein2,UCP2）在酒精性心肌损害中的作用及其分子机制。方法：采用乙醇在体内的代谢产物乙醛作为刺激因素,将培养心肌细胞分为对照组,乙醛组和乙醛＋ucP2抑制剂京尼平组（京尼平组）,干预24小时后检测心肌细胞中超氧阴离子（superoxideanion,SOA）及一氧化氮（nitricoxide,NO）的水平,并检测UCP2的蛋白表达水平,另一组实验干预72小时后采用TUNEL法检测心肌细胞凋亡率。结果：与对照组比较,乙醛组心肌细胞中SOA水平显著升高（P〈0．01）,而NO水平显著降低（P〈0．01）,且UCP2的蛋白水平也较对照组显著增加（P〈0．01）。而与乙醛组比较,京尼平组心肌细胞中SOA的水平进一步增加（P〈0．01）,NO的水平也进一步降低（P〈0．01）。与对照组比较,乙醛可诱导培养心肌细胞凋亡（P〈0．01）,而京尼平组凋亡率较乙醛组则进一步升高（P〈0．01）。结论：UCP2在酒精性心肌损害中通过调控SOA／NO的水平发挥代偿性保护作用。     

Caspase-9抑制剂对SD大鼠椎间盘软骨终板细胞凋亡的影响

目的探讨caspase-9抑制剂对低胎牛血清培养诱导的大鼠椎间盘软骨终板细胞凋亡影响的研究。方法取3月龄SD大鼠椎间盘软骨终板,序贯消化法获取细胞原代培养,以1%FBS培养48 h为诱导凋亡条件。实验分为1%FBS凋亡组、caspase-9抑制剂组（Z-LEHD-FMK）及DMSO对照组,分别处理细胞48 h,后经流式细胞仪检测细胞凋亡率、Western blot检测procaspase-9,active caspase-9及active caspase-3的表达。结果流式细胞仪检测显示,caspases-9抑制剂组细胞凋亡率（26.3±2.56）%与1%FBS组（40.8±0.84）%及DMSO组（40.2±1.56）%相比凋亡率较低,有显著统计学差异（P〈0.05）;Western blot检测caspases-9抑制剂组active caspase-9及active caspase-3较1%FBS凋亡组及DMSO对照组表达均明显减少,有显著统计学意义（P〈0.05）。结论 Caspase-9抑制剂能明显抑制低胎牛血清培养诱导的大鼠椎间盘软骨终板细胞凋亡,有望成为治疗椎间盘退变的新型药物。     

草木犀石油醚提取物对小鼠巨噬细胞促炎介质的影响

目的研究草木犀石油醚提取物在体外的抗炎作用。方法采用小鼠巨噬细胞系RAW264．7建立炎症细胞模型,加入10μg/L的LPS培养液和不同浓度的草木犀石油醚提取物进行干预。ELISA法检测上清液中TNF-α,IL-1β,IL-6和NO的分泌量;实时荧光定量RT-PCR检测TNF-α,iNOS和COX-2的mRNA表达;Western印迹法检测COX-2蛋白的表达。结果草木犀提取物干预后细胞所分泌的炎性介质（TNF—α,IL-1β,IL-6和NO）与模型组相比均显著降低（P〈0．01）,并存在剂量依赖关系;RT-PCR结果显示干预后细胞TNF-α,iNOS和COX-2的mRNA表达水平显著降低（P〈0．01）,也存在剂量依赖关系;Western印迹结果显示草木犀石油醚提取物及地塞米松干预后COX-2蛋白水平明显降低（P〈0．01）。结论草木犀的石油醚提取物通过下调LPS诱导的巨噬细胞表达炎性介质而发挥其体外抗炎作用,且其下调作用呈剂量依赖性。     

β-淀粉样蛋白通过激活caspase-3诱导PC12细胞凋亡

目的探讨β-淀粉样蛋白25-35片段（Aβ25-35）对体外培养的大鼠嗜铬瘤细胞PC12细胞促凋亡机制。方法采用四甲基偶氮唑蓝（MTT）法观察不同浓度的Aβ25-35干预PC12细胞24h后的细胞活性;将细胞分为对照组、实验组（即20 mmol/L Aβ25-35组）,流式细胞技术观察两组PC12细胞凋亡率;免疫细胞化学染色法观察PC12细胞凋亡基因caspase-3的表达。结果PC12细胞活性呈Aβ25-35剂量依赖性降低,且浓度为20 mmol/L时降低最显著;PC12细胞实验组的凋亡率为23.03%±1.22%,对照组为2.42%±0.87%（P〈0.01）;caspase-3实验组的阳性表达较对照组明显增加（P〈0.01）。结论Aβ可通过激活促凋亡基因caspase-3诱导PC12细胞凋亡。     

Induction of neutrophil apoptosis by the Pseudomonas aeruginosa exotoxin pyocyanin: a potential mechanism of persistent infection

Pseudomonas aeruginosa colonizes and infects human tissues, although the mechanisms by which the organism evades the normal, predominantly neutrophilic, host defenses are unclear. Phenazine products of P. aeruginosa can induce death in Caenorhabditis elegans. We hypothesized that phenazines induce death of human neutrophils, and thus impair neutrophil-mediated bacterial killing. We investigated the effects of two phenazines, pyocyanin and 1-hydroxyphenazine, upon apoptosis of neutrophils in vitro. Pyocyanin induced a concentration- and time-dependent acceleration of neutrophil apoptosis, with 50 microM pyocyanin causing a 10-fold induction of apoptosis at 5 h (p < 0.001), a concentration that has been documented in sputum from patients colonized with P. aeruginosa. 1-hydroxyphenazine was without effect. In contrast to its rapid induction of neutrophil apoptosis, pyocyanin did not induce significant apoptosis of monocyte-derived macrophages or airway epithelial cells at time points up to 24 h. Comparison of wild-type and phenazine-deleted strains of P. aeruginosa showed a highly significant reduction in neutrophil killing by the phenazine-deleted strain. In clinical isolates of P. aeruginosa pyocyanin production was associated with a proapoptotic effect upon neutrophils in culture. Pyocyanin-induced neutrophil apoptosis was not delayed either by treatment with LPS, a powerfully antiapoptotic bacterial product, or in neutrophils from cystic fibrosis patients. Pyocyanin-induced apoptosis was associated with rapid and sustained generation of reactive oxygen intermediates and subsequent reduction of intracellular cAMP. Treatment of neutrophils with either antioxidants or synthetic cAMP analogues significantly abrogated pyocyanin-induced apoptosis. We conclude that pyocyanin-induced neutrophil apoptosis may be a clinically important mechanism of persistence of P. aeruginosa in human tissue.     

3种革兰氏阴性细菌及其L型内毒素含量的测定

本文采用鲎试剂对大肠杆菌（ＡＴＣＣ２５９２２）、伤寒杆菌、绿脓杆菌（ＡＴＣＣ７８５３）及它们的Ｌ型内毒素的含量进行测定。结果显示细菌型与细菌Ｌ型均具有内毒素,但细菌Ｌ型内毒素含量较细菌型低（约为１／３￣１／２）。因此,认为细菌Ｌ型仍有一定的致病性。     

Induction, growth and antibiotic production of Streptomyces viridifaciens L-form bacteria

AIMS: To induce, cultivate and investigate the characteristics of L-form bacteria derived from the filamentous actinomycete Streptomyces viridifaciens. METHODS AND RESULTS: L-forms were induced in a liquid medium supplemented with lysozyme and penicillin. A stable culture which no longer required inducing agents but could still revert, was obtained by the twelfth subculture. The specific growth rate of stable L-forms was faster (0.751) than unstable L-forms (0.361). After the exponential growth phase, the cell diameter continued to increase, as did the percentage of vacuoles. Morphologically, the L-forms appeared as spherical bodies with no signs of differentiation and were sensitive to osmotic stress, indicating removal of the cell wall. The L-forms produced secondary metabolites although much lower levels of antibiotic were assayed in the L-forms compared with the cell walled forms. CONCLUSION: Stable L-form bacteria were induced from S. viridifaciens and their growth characterized. The L-forms produced secondary metabolites. SIGNIFICANCE AND IMPACT OF THE STUDY: Stable Streptomyces L-forms were induced and have potential as biocontrol agents.     

咽部活组织中细菌L型的检出及意义

应用病原微生物培养、电镜、组织切片细菌学检查及Ｌ型抗体免疫组化染色等方法,检测６４例慢性咽炎组织的细菌Ｌ型。结果有４２例培养出细菌Ｌ型,其阳性率为６５．６％;它与切片革兰氏染色Ｌ型检出阳性率（６７．２％）无显著性差异,Ｐ＞０．０５。透射电镜在慢性咽炎组织的间质及上皮细胞、巨噬细胞等细胞内见皮细菌Ｌ型;且Ｌ型抗体免疫组化染色亦证实组织中有细菌Ｌ型抗原。提示,细菌Ｌ型感染与慢性咽炎关系密切,Ｌ型侵入组织并在宿主细胞内生长的特征,可能是慢性咽炎反复发作,迁延不愈的重要原因。     

Pseudomonas aeruginosa utilises its type III secretion system to kill the free-living amoeba Acanthamoeba castellanii

Pseudomonas aeruginosa is a free-living and common environmental bacterium. It is an opportunistic and nosocomial pathogen causing serious human health problems. To overcome its predators, such as macrophages and environmental phagocytes, it utilises different survival strategies, such as the formation of microcolonies and the production of toxins mediated by a type III secretion system (TTSS). The aim of this study was to examine interaction of TTSS effector proteins of P. aeruginosa PA103 with Acanthamoeba castellanii by co-cultivation, viable count, eosin staining, electron microscopy, apoptosis assay, and statistical analysis. The results showed that P. aeruginosa PA103 induced necrosis and apoptosis to kill A. castellanii by the effects of TTSS effector proteins ExoU, ExoS, ExoT, and ExoY. In comparison, Acanthamoeba cultured alone and co-cultured with P. aeruginosa PA103 lacking the known four TTSS effector proteins were not killed. The results are consistent with P. aeruginosa being a strict extracellular bacterium that needs TTSS to survive in the environment, because the TTSS effector proteins are able to kill its eukaryotic predators, such as Acanthamoeba.     

Burkholderia spp. alter Pseudomonas aeruginosa physiology through iron sequestration

Pseudomonas aeruginosa and members of the Burkholderia cepacia complex often coexist in both the soil and the lungs of cystic fibrosis patients. To gain an understanding of how these different species affect each other's physiology when coexisting, we performed a screen to identify P. aeruginosa genes that are induced in the presence of Burkholderia: A random gene fusion library was constructed in P. aeruginosa PA14 by using a transposon containing a promoterless lacZ gene. Fusion strains were screened for their ability to be induced in the presence of Burkholderia strains in a cross-streak assay. Three fusion strains were induced specifically by Burkholderia species; all three had transposon insertions in genes known to be iron regulated. One of these fusion strains, containing a transposon insertion in gene PA4467, was used to characterize the inducing activity from Burkholderia: Biochemical and genetic evidence demonstrate that ornibactin, a siderophore produced by nearly all B. cepacia strains, can induce P. aeruginosa PA4467. Significantly, PA4467 is induced early in coculture with an ornibactin-producing but not an ornibactin-deficient B. cepacia strain, indicating that ornibactin can be produced by B. cepacia and detected by P. aeruginosa when the two species coexist.     

人体病理组织中细菌L型的电镜观察

对9例细菌L型感染的人体病理组织进行透射电镜观察。结果显示:(1)L型可分布于组织间质或进入吞噬细胞、上皮细胞和癌细胞等细胞胞质;(2)L型具有多形态、大小不等、胞壁缺陷、电子密度低等特点,细胞胞质内的细菌L型尚有A、B两种形态区别;(3)L型在组织中形成了不完全箍缩分裂;(4)宿主细胞超微结构仅出现轻微改变。本结果与文献报道基本一致,提出了透射电镜下病理组织中细菌L型的形态特征及分布;并对L型感染与慢性炎症的关系等问题进行了讨论。     

Pseudomonas aeruginosa-induced human mast cell apoptosis is associated with up-regulation of endogenous Bcl-xS and down-regulation of Bcl-xL

Mast cells play a critical role in the host defense against bacterial infection. Recently, apoptosis has been demonstrated to be essential in the regulation of host response to Pseudomonas aeruginosa. In this study we show that human mast cell line HMC-1 and human cord blood-derived mast cells undergo apoptosis as determined by the ssDNA formation after infection with P. aeruginosa. P. aeruginosa induced activation of caspase-3 in mast cells as evidenced by the cleavage of D4-GDI, an endogenous caspase-3 substrate and the generation of an active form of caspase-3. Interestingly, P. aeruginosa treatment induced up-regulation of Bcl-x(S) and down-regulation of Bcl-x(L). Bcl-x(S), and Bcl-x(L) are alternative variants produced from the same Bcl-x pre-mRNA. The former is proapoptotic and the latter is antiapoptotic likely through regulating mitochondrial membrane integrity. Treatment of mast cells with P. aeruginosa induced release of cytochrome c from mitochondria and loss of mitochondrial membrane potentials. Moreover, P. aeruginosa treatment reduced levels of Fas-associated death domain protein-like IL-1beta-converting enzyme-inhibitory proteins (FLIPs) that are endogenous apoptosis inhibitors through counteraction with caspase-8. Thus, human mast cells undergo apoptosis after encountering P. aeruginosa through a mechanism that likely involves both the Bcl family protein mitochondrial-dependent and the FLIP-associated caspase-8 pathways.