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1.
用细胞裂解计数法及超薄切片电镜观察法分析了迟缓爱德华氏菌侵袭Hep—2细胞的基本特性。在15株来源各异的迟缓爱德华氏菌中,有6株细菌具有对Hep—2细胞的侵袭能力。细菌侵入细胞后,主要位于空泡内。侵入细胞内的迟缓爱德华氏菌不仅可在细胞内增殖,而且可从细胞内释放出来。用细胞松弛素破坏微丝后可抑制其侵袭作用,而且表现出剂量依赖关系,而用秋水仙素破坏微管后不影响其侵袭力。这表明在迟缓爱德华氏菌对Hep—2细胞的侵袭过程中,细胞骨架中有微丝的参与,未发现微管的参与。  相似文献   

2.
Hui爱德华氏菌变异株C9605及对弊的致病性研究   总被引:1,自引:0,他引:1       下载免费PDF全文
从患白板综合症的病鳖分离到一株细菌(C9605),该菌为革兰氏阴性,直杆状,周生鞭毛。接触酶阳性,氧化酶阴性,还原硝酸盐,对多粘菌素不敏感,不利用柠檬酸盐和丙二酸盐作唯一碳源,不从甘露醇、蔗糖、海藻糖、L-阿拉伯糖产酸。根据这些特性,菌株可归于Hui爱德华氏菌。但是该菌发酵木糖产酸,产生H2S,耐青霉素,故鉴定为Hui爱德华氏菌变异株。人工感染实验证实,该菌株是鳖白板综合症的病原菌。  相似文献   

3.
邓佳  吴海珍 《微生物学通报》2017,44(10):2398-2406
【目的】迟缓爱德华氏菌甘油醛-3-磷酸脱氢酶(GAPDH)是糖酵解途径中关键酶之一,前期研究证实是一种广谱性抗原,可作为水产养殖细菌病免疫防治中疫苗的开发靶点。本文探究迟缓爱德华氏菌甘油醛-3-磷酸脱氢酶的胞外分泌机制。【方法】通过Western blot和ELISA方法考察迟缓爱德华氏菌经典分泌系统缺失株GAPDH胞外分泌情况;使用ELISA方法对迟缓爱德华氏菌突变体文库的GAPDH胞外分泌进行了大规模筛查,并结合q RT-PCR对筛查得到的插入失活株进行了表达分析。【结果】经典分泌系统与GAPDH的胞外分泌存在一定相关性。突变体文库的大规模筛查得到两株GAPDH分泌量明显增加的插入失活株Δesr A和Δesr C,这两个基因的失活会导致GAPDH的胞外分泌量显著上调。【结论】迟缓爱德华氏菌GAPDH的胞外分泌受Esr A和Esr C负调控。  相似文献   

4.
利用GFP示踪细胞内源性P53活性检测DNA损伤   总被引:2,自引:1,他引:1  
DNA损伤的检测对预防癌症和遗传病等非常重要。采用分子克隆技术,将报告基因—绿色荧光蛋白(GFP)置于SV40基本启动子调控下,构建成对照载体pSV-GFP。在SV40基本启动子上游插入寡核苷酸P53RE,构建成示踪载体p53RE-GFP。转染NIH3T3细胞,以GFP示踪细胞内源性P53的转录激活活性。紫外线照射或H2O2处理转化细胞使DNA损伤,诱导细胞内源性P53的表达。用激光扫描共聚焦成像系统(LSCIS)对细胞进行红、绿、蓝三色光融合成像,并测定GFP经488nm激发后发出的绿色荧光光密度,验证GFP示踪P53的特异性。p53RE-GFP转化细胞3T3-REG经紫外线照射或H2O2处理后,GFP的表达增高,处理后1hr光密度即达到最高水平,随后逐渐降低。血清“饥饿”—非DNA损伤处理的3T3-REG细胞,以及经紫外和H2O2处理的对照载体pSV-GFP转化细胞3T3-SVG,GFP的表达无明显增强。实验表明:GFP示踪内源性P53转录激活活性用于检测DNA损伤有很高的灵敏度和特异性,适宜推广应用。  相似文献   

5.
大鼠催乳素基因真核细胞可表达性质粒的构建及应用研究   总被引:4,自引:0,他引:4  
735bp的PRLcDNA片段从质粒PRL-SP65#1中回收后,用粘性末端连接法将其重组到真核表达载体pcDNA3上,筛选出正向连接重组体pcDNA3-PRLS和反向连接重组体pcDNA3-PRLAS。将重组体pcDNA3-PRLs和空载体pcDNA3分别转入NIH3T3细胞系,用G418筛选出阳性细胞后与未转染的NIH3T3细胞在加E2和不加E2的情况下,用原位杂交的方法,分别用PRLcDNA探针和原癌基因c-H-rascDNA探针进行检测,未转染的NIH3T3细胞在加E2和不加E2时都几乎无催乳素基因的表达,同样,转入空载体的NIH3T3细胞也无PRL的表达,而转入重组体pcDNA3-PRLS的NIH3T3细胞则有大量的PRL基因的表达,与对照组相比有显著差异(P<0.01)。正常和转入空载体的NIH3T3细胞有一定程度的原癌基因c-H-ras的表达,当分别加入E2和转入重组体pcDNA3-PRLS后,NIH3T3细胞中的c-H-ras基因表达水平都显著升高(P<0.05)。  相似文献   

6.
鳗鲡肝肾病病原菌的研究   总被引:33,自引:3,他引:30  
近年来,在广东潮州各养鳗场,每年3-5月和10-12月,广泛流行一种危害严重的鳗鲡肝肾病,给鳗鲡养殖业造成严重损失。本文记述了该病的症状,重点研究鳗肝肾病的病原菌。作者从患肝肾病的病鳗肝脏、肾脏和胃液中分离到10株致病菌。根据分离株的形态、培养、生化特性,8株致病菌特性一致,鉴定为迟饨爱德华氏菌(EdwardsiellatardaEwingetMcwhorter)另外两株菌特性相同被鉴定为运动性Aeronlonassp.。研究结果阐明了鳗鲡肝肾病主要是由E.tarda引起的爱德华氏菌病,部分病例是由E.tarda和运动性Aeromonas菌引起的并发症.E,tarda是鳗鲡肝肾病的病原菌。  相似文献   

7.
OSM是一种对黑色素瘤细胞显示抑制作用的细胞因子.为进行OSM针对黑色素瘤的基因-放射治疗研究,构建了小鼠Egr-1基因调控序列引导入OSMcDNA真核表达质粒(pEO),pEO质粒转染小鼠B-16黑色素瘤细胞,经G418和抗人OSM抗体的筛选,获得了稳定表达OSM的克隆细胞(pEO-1细胞),OSM表达量可达5.97ng每105细胞天,分子量为32kD.pEO-1细胞用一定浓度H2O2处理后OSM表达量可提高62%,表明pEO重组质粒可在氧自由基的刺激作用下增强OSM表达  相似文献   

8.
腹泻便中克吕沃尔氏菌的分离鉴定及致病性研究   总被引:1,自引:0,他引:1  
本文报告了自腹泻便分离到的18株克吕沃尔氏菌的生化鉴定。分子遗传学检测,药物敏感试验及致病性研究结果。18株菌中有11株为抗坏血酸克吕沃尔氏菌,7株栖冷克吕沃尔氏菌。其中溶血试验阳性率38.9%;乳鼠灌胃阳性率33。3%;Helo-2细胞病变22.2%;兔肠袢结扎阳性5.6%。豚鼠角膜侵袭试验及Vero细胞病变均呈阴性。以此证明,克吕沃尔氏菌中有部分菌株可致生物模型病变,与人腹泻有密切关系。该组细菌的抗药性已很广,临床可用药物不多,一旦发生感染,治疗将十分困难。  相似文献   

9.
利用λ-Red重组系统对福氏2a志贺氏菌301株ipaH4.5基因进行缺失突变,构建了福氏2a志贺氏菌301株ipaH4.5基因缺失突变株?ipaH4.5,利用低拷贝质粒构建ipaH4.5缺失突变株的回复突变株△ipaH4.5HF。PCR方法证实了ipaH4.5基因的缺失和回复。对野生株、突变株和回复突变株的生长代谢及细胞侵袭能力进行比较;ELISA方法检测3株菌侵袭鼠J774巨噬细胞后培养上清中炎性因子的水平。生长代谢实验表明缺失和回复ipaH4.5不影响志贺氏菌的生长速度,侵袭实验表明缺失和回复ipaH4.5也不影响志贺氏菌对HeLa细胞和鼠J774巨噬细胞的侵袭能力,表明ipaH4.5基因与志贺氏菌的生长代谢和侵袭能力无关;鼠J774巨噬细胞培养上清中细胞因子水平的改变提示该基因在志贺氏菌侵入细胞后抑制宿主细胞炎症反应。  相似文献   

10.
目的和方法构建EPO真核细胞表达载体(pcD2EPO),用缝线法和注射法将其直接导入肾性贫血大鼠股四头肌,观察EPO在骨骼肌细胞中的表达及其对贫血的治疗作用。结果:pcD2EPO导入股四头肌2周后,骨骼肌细胞内出现EPOmRNA,提示被导入的EPO基因在肌细胞内得到表达。贫血动物被治疗1周后,缝线组和注射组动物的HGB和RBC均显著升高;在第3周,缝线组的HGB和RBC接近健康大鼠的水平;至第4周,两个治疗组的HGB和RBC仍显著高于对照组。结论:经缝线法导入的pcD2EPO在骨骼肌中的表达效率及对贫血的治疗效果明显高于直接注射法,而两种治疗方法对改善肾性贫血动物肾脏清除BUN的功能无明显差异  相似文献   

11.
Streptococcus gordonii is a commensal bacterium that colonizes the hard and soft tissues present in the human mouth and nasopharynx. The cell wall-anchored polypeptides SspA and SspB expressed by S. gordonii mediate a wide range of interactions with host proteins and other bacteria. In this article we have determined the role of SspA and SspB proteins, which are members of the streptococcal antigen I/II (AgI/II) adhesin family, in S. gordonii adherence and internalization by epithelial cells. Wild-type S. gordonii DL1 expressing AgI/II polypeptides attached to and was internalized by HEp-2 cells, whereas an isogenic AgI/II- mutant was reduced in adherence and was not internalized. Association of S. gordonii DL1 with HEp-2 cells triggered protein tyrosine phosphorylation but no significant actin rearrangement. By contrast, Streptococcus pyogenes A40 showed 50-fold higher levels of internalization and this was associated with actin polymerization and interleukin-8 upregulation. Adherence and internalization of S. gordonii by HEp-2 cells involved beta1 integrin recognition but was not fibronectin-dependent. Recombinant SspA and SspB polypeptides bound to purified human alpha5beta1 integrin through sequences present within the NAV (N-terminal) region of AgI/II polypeptide. AgI/II polypeptides blocked interactions of S. gordonii and S. pyogenes with HEp-2 cells, and S. gordonii DL1 cells expressing AgI/II proteins inhibited adherence and internalization of S. pyogenes by HEp-2 cells. Conversely, S. gordonii AgI/II- mutant cells did not inhibit internalization of S. pyogenes. The results suggest that AgI/II proteins not only promote integrin-mediated internalization of oral commensal streptococci by host cells, but also potentially influence susceptibility of host tissues to more pathogenic bacteria.  相似文献   

12.
Lipoteichoic acid (LTA) is thought to play a role in the interactions between Streptococcus pyogenes and host cells. We have examined the effect of exogenous LTA on the adherence and entry of S. pyogenes JRS4 strain into HEp-2 epithelial cells. LTA markedly inhibited bacterial entry in a concentration-dependent manner, up to 250 microg ml(-1). In contrast, LTA had only a slight inhibitory effect on adherence. LTA also inhibited the entry but not adherence of Salmonella typhimurium strain into HEp-2 cells. Binding experiments showed a dose-dependent binding of LTA to cells up to 10 microg ml(-1). Confocal laser microscopy imaging and analysis revealed that LTA was internalized by the epithelial cells and colocalized with F-actin. These results might imply that, following binding, exogenous LTA enters HEp-2 cells and exerts a cytotoxic effect that interferes with bacterial internalization. A possible target for LTA activity might be the actin cytoskeleton, which is known to be essential for bacterial uptake.  相似文献   

13.
嗜水气单胞菌侵袭力与宿主细胞信号转导和骨架的关系   总被引:2,自引:0,他引:2  
嗜水气单胞菌(Aeromonas hydrophila,Ah)是淡水鱼暴发性败血症的主要病原,该菌能够引致淡水鱼等的败血症和人的腹泻等^[1]。嗜水气单胞菌有多种致病因子,如毒素、蛋白酶、S层蛋白等^[2],还发现它具有侵袭作用,有报道嗜水气单胞菌粪分离株能侵袭HEp-2细胞^[3],但对于鱼源菌株的侵袭特性知之甚少。仅有一些报道认为嗜水气单胞菌能引致细胞病变^[4,5]。  相似文献   

14.
The interaction with HeLa cells of an enteropathogenic Escherichia coli (EPEC) strain and its plasmid-cured derivative strain was examined. An O111:NM EPEC strain B171 harbours a 54 megadalton plasmid (pYR111) necessary for the expression of both localized adherence (LA) to HeLa cells and the O-repeating side chain of the lipopolysaccharide. Under light microscopy, the plasmid-cured derivative strain B171-4 was observed to interact with HeLa cells in a pattern distinct from LA. Transmission electron microscopy showed that the bacteria were internalized by HeLa cells. In contrast, strain B171 induced pedestal-like projections and invaginations of the plasma membrane, but was never completely internalized. A quantitative assay to determine the number of internalized bacteria revealed that strain B171-4 was internalized at levels 30-70-fold higher than those of avirulent E. coli strains. Cytochalasin B reduced the levels of internalization of both strain B171-4 and an enteroinvasive E. coli strain (E11), but did not affect LA by strain B171. These results suggest that EPEC strain B171 may carry a specific chromosomally determined surface factor needed to initiate internalization by HeLa cells. However, a plasmid-determined factor alters the nature of this interaction; the combined effects of the chromosomal and plasmid determinants lead to the characteristic attachment of the bacteria in clusters on the surface of the eukaryotic cell.  相似文献   

15.
Edwardsiella tarda is a pathogen with a broad host range infecting animals and humans. We have reported recently that the type III secretion system (TTSS) is essential for intracellular replication of the bacterium in murine macrophages. The present study shows that the TTSS is also needed for intracellular growth of the bacterium in human epithelial cells (HEp-2). However, different from the previous microarray analyses on murine macrophages, upregulation of the mRNA expression level of NF-kappaB target genes was not detected in the infected HEp-2 cells. The wild-type E. tarda, but not its TTSS mutant, actually repressed the tumor necrosis factor alpha-dependent NF-kappaB activation in an NF-kappaB reporter gene assay. These results suggest TTSS-dependent repression of the NF-kappaB activation in HEp-2 cells infected with E. tarda.  相似文献   

16.
Corynebacterium pseudodiphtheriticum is a well-known human pathogen that mainly causes respiratory disease and is associated with high mortality in compromised hosts. Little is known about the virulence factors and pathogenesis of C. pseudodiphtheriticum. In this study, cultured human epithelial (HEp-2) cells were used to analyse the adherence pattern, internalisation and intracellular survival of the ATCC 10700 type strain and two additional clinical isolates. These microorganisms exhibited an aggregative adherence-like pattern to HEp-2 cells characterised by clumps of bacteria with a "stacked-brick" appearance. The differences in the ability of these microorganisms to invade and survive within HEp-2 cells and replicate in the extracellular environment up to 24 h post infection were evaluated. The fluorescent actin staining test demonstrated that actin polymerisation is involved in the internalisation of the C. pseudodiphtheriticum strains. The depolymerisation of microfilaments by cytochalasin E significantly reduced the internalisation of C. pseudodiphtheriticum by HEp-2 cells. Bacterial internalisation and cytoskeletal rearrangement seemed to be partially triggered by the activation of tyrosine kinase activity. Although C. pseudodiphtheriticum strains did not demonstrate an ability to replicate intracellularly, HEp-2 cells were unable to fully clear the pathogen within 24 h. These characteristics may explain how some C. pseudodiphtheriticum strains cause severe infection in human patients.  相似文献   

17.
Yersinia enterocolitica cross the intestinal epithelium via translocation through M cells, which are located in the follicle-associated epithelium (FAE) of Peyer's patches (PP). To investigate the molecular basis of this process, studies were performed using a recently developed in vitro model, in which the enterocyte-like cell line Caco-2 and PP lymphocytes are co-cultured in order to establish FAE-like structures including M cells. Here, we demonstrate that Y. enterocolitica does not adhere significantly to the apical membrane of differentiated enterocyte-like Caco-2 cells that express binding sites for Ulex europaeus agglutinin (UEA)-1. In contrast, Y. enterocolitica adhered to, and was internalized by, cells that lacked UEA-1 binding sites and displayed a disorganized brush border. These cells were considered to be converted to M-like cells. Further analysis revealed that part of these cells expressed β1 integrins at their apical surface and, as revealed by comparison of wild-type and mutant strains, interacted with invasin of Y. enterocolitica . Consistently, anti-β1 integrin antibodies significantly inhibited internalization of inv -expressing yersiniae. Experiments with Yersinia mutant strains deficient in YadA or Yop secretion revealed that these virulence factors play a minor role in this process. After internalization, yersiniae were transported within LAMP-1-negative vacuoles to, and released at, the basal surface. Internalization and transport of yersiniae was inhibited by cytochalasin D, suggesting that F-actin assembly is required for this process. These results provide direct evidence that expression of β1 integrins at the apical surface of M cells enables interaction with the invasin of Y. enterocolitica , and thereby initiates internalization and translocation of bacteria.  相似文献   

18.
Invasiveness of Salmonella typhi strains in HeLa S3 monolayer cells   总被引:2,自引:0,他引:2  
The internalization and intracellular multiplication, i.e., the invasiveness, of Salmonella typhi strains recently isolated from typhoid fever patients were confirmed in HeLa cell monolayers. When stained with Giemsa solution, intracellular bacteria were 0.6 X 1.2 micron in size and stained purple, whereas extracellular bacteria associated or not with the HeLa cell surface were 1.0 X 3.0 micron and stained deep blue. Strain GIFU 10007 was internalized into 23% of the HeLa cells within 10 min after inoculation. About 90% of the HeLa cells were infected after 24 hr incubation in kanamycin (KM)-containing medium. Intracellular multiplication of the challenge organism was verified by a large number of intracellular bacteria after 24 hr incubation in KM-containing medium by both light-microscopy of the Giemsa stained preparation and viable counts of intracellular bacteria. The viable counts of strain 10007 showed an increase of more than 40-fold within 24 hr after inoculation, whereas in the four other less or non-infective strains, recovery of viable bacteria was poor or nil. Strains which were highly invasive usually failed to show strong adhesion. The contribution of Vi antigen to the internalization of challenge organisms was not proved. Infective strains, when killed by formalin were still adhesive, but were not internalized. The same strains, when killed by boiling, were neither adhesive nor internalized. From these findings it was concluded that the internalization and multiplication of infective S. typhi strains in cultured HeLa cells should be regarded as an invasion rather than phagocytosis by host cells, and such invasiveness could be an indicator to estimate the virulence of S. typhi strains.  相似文献   

19.
Earlier, we have shown that spontaneously isolated non‐pathogenic bacteria Serratia grimesii and Serratia proteamaculans invade eukaryotic cells, provided that they synthesize thermolysin‐like metalloproteases ECP32/grimelysin or protealysin characterized by high specificity towards actin. To address the question of whether the proteases are active players in entry of these bacteria into host cells, in this work, human larynx carcinoma Hep‐2 cells were infected with recombinant Escherichia coli expressing grimelysin or protealysin. Using confocal and electron microscopy, we have found that the recombinant bacteria, whose extracts limitedly cleaved actin, were internalized within the eukaryotic cells residing both in vacuoles and free in cytoplasm. The E. coli‐carrying plasmids without inserts of grimelysin or protealysin gene did not enter Hep‐2 cells. Moreover, internalization of non‐invasive E. coli was not observed in the presence of protealysin introduced into the culture medium. These results are consistent with the direct participation of ECP32/grimelysin and protealysin in entry of bacteria into the host cells. We assume that ECP32/grimelysin and protealysin mediate invasion being injected into the eukaryotic cell and that the high specificity of the enzyme towards actin may be a factor contributed to the bacteria internalization.  相似文献   

20.
Heparin-binding protein (HBP), also known as CAP37, is a proteolytically inactive serine protease homologue that is released from activated granulocytes. However, HBP is not a biologically inactive molecule but rather a multifunctional protein with properties that include the enhancement of LPS-induced TNF-alpha production from monocytes. We have previously demonstrated that HBP is internalized in monocytes. In the current study, we hypothesize that HBP is internalized in monocytes via endocytosis, and this internalization is an important mechanism by which HBP enhances LPS-induced TNF-alpha release. Using whole blood from healthy donors and flow cytometry, we found that colchicine (0.1-10 mM), cytochalasin D (1000 microM), NH4Cl (10-50 mM), and bafilomycin A1 (0.1-3 microM) significantly reduced the affinity of FITC-HBP for CD14-positive monocytes. Using isolated human monocytes and ELISA, we found that colchicine (0.1 mM), cytochalasin D (30 and 300 microM), NH4Cl (30 mM), and bafilomycin A1 (1 microM) significantly reduced the effect of HBP (10 microg/ml) to enhance LPS (10 ng/ml)-induced TNF-alpha release after 24 h. These findings demonstrate that internalization of HBP in monocytes is essential for the enhancement of LPS-induced TNF-alpha release. Transport of HBP to an activating compartment depends on intact F-actin polymerization and endosomal acidification, an important mechanism for endosomal protein sorting and trafficking.  相似文献   

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