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1.
非洲猪瘟病毒p62蛋白单克隆抗体的制备及初步应用 总被引:1,自引:1,他引:0
为制备非洲猪瘟病毒(ASFV)p62蛋白的特异性单克隆抗体,并初步应用于感染组织样品中ASFV抗原的免疫组化(IHC)检测,本研究以杆状病毒表达的非洲猪瘟病毒重组p62蛋白免疫BALB/c小鼠,取其脾细胞与骨髓瘤细胞进行融合获得杂交瘤细胞。结果显示:基于纯化的p62蛋白建立的间接ELISA方法对杂交瘤细胞进行筛选和亚克隆,获得了18株可稳定分泌抗非洲猪瘟病毒p62蛋白单克隆抗体的杂交瘤细胞株。经IFA检测,制备的单克隆抗体均与非洲猪瘟病毒反应,且不与猪瘟病毒、猪繁殖与呼吸综合征病毒、猪伪狂犬病病毒、猪圆环病毒2型等猪源常见病毒反应,特异性良好。抗体识别蛋白的鉴定结果显示,3株MAbs识别p35蛋白,15株MAbs识别p15蛋白。14株MAbs重链亚类为IgG1型,4株MAbs重链亚类为IgG2a,轻链均为κ链。利用18株MAbs对ASFV感染猪的肺、扁桃体、淋巴结等组织进行IHC检测,结果显示5株MAbs均能够与感染ASFV的组织发生特异性的免疫反应。本研究获得的非洲猪瘟病毒p62蛋白单克隆抗体可为非洲猪瘟病毒免疫学检测方法的建立及p62蛋白的结构功能等基础研究提供重要的生物材料。 相似文献
2.
Virus yields from porcine alveolar macrophages (AM) infected with African swine fever virus (ASFV) were greater and were achieved more rapidly, when inoculated at a high multiplicity of infection (MOI) than at low MOI. The difference was related to a lower percentage of cells becoming infected after low MOI inoculation. The reduced yields after low MOI were not caused by prolongation of the culture time, by bacterial endotoxins or by production of inhibitory substances by infected AM. Virus-infected AM were not susceptible to lysis in antibody-dependent cell mediated cytotoxicity (ADCC) assays and this was apparently due to a paucity of viral antigen expressed on the cell surface. Uninfected AM did not act as effectors in ADCC.Porcine bone marrow (PBM) cells were effective in mediation of ADCC and their activity was reduced after ASFV infection. Cells separated into adherent and non-adherent populations, depleted by carbonyl iron treatment or separated by Ficoll-Hypaque centrifugation, all showed effector activity in ADCC. The effector cells were not mature neutrophils or lymphocytes and were probably granulocytic precursors. 相似文献
3.
Comparison of two antigens for use in an enzyme-linked immunosorbent assay to detect African swine fever antibody 总被引:3,自引:0,他引:3
Two African swine fever virus (ASFV) antigens were tested for use in an ELISA to detect antibody to ASFV. Antigens used were the cytoplasmic soluble fraction (CS-P) of infected cells grown in the presence of porcine serum and the semipurified viral structural protein VP73 (SVP73). Both antigens were tested by ELISA against 72 sera obtained during several ASF field episodes and from ASFV-inapparent carriers. Of the 72 sera, only 2.8% has positive results by ELISA against CS-P antigen; 60% of positive-reacting sera (to both antigens) had higher ELISA values when the CS-P antigen was used. Samples (with positive results) that reacted only to CS-P antigen had results confirmed by immunoblot analysis. Such sera reacted against ASFV-infection proteins IP25, IP25.5, and IP30, but not against IP73. In time-course experiments to detect appearance of ASFV-antibodies in infected miniature pigs, antibodies were detected by immunoblot analysis on postinoculation day (PID) 8. At that time, only the polypeptides IP25, IP25.5 IP30, and IP31 were recognized; IP73 and IP12 were first detected 3 and 4 days later, respectively. In the same experiments, ASFV antibodies were detected by ELISA, using CS-P or SVP73 antigens, on PID 7 and 9, respectively. These results could explain the percentage of sera not having positive results by ELISA using SVP73 antigen, if the sera were obtained from ASFV-infected pigs during the first days of infection before induction of antibody response against the IP73 protein. This feature makes the use of CS-P antigen advantageous in early serologic detection of ASFV-infected pigs. 相似文献
4.
Pamela Lithgow Haru Takamatsu Dirk Werling Linda Dixon Dave Chapman 《Veterinary microbiology》2014,168(2-4):413-419
The expression of surface markers on African swine fever virus (ASFV) infected cells was evaluated to assess their involvement in infection. Previous findings indicated CD163 expression was correlated with ASFV susceptibility. However, in this study the expression of porcine CD163 on cell lines did not increase the infection rate of these cells indicating other factors are likely to be important in determining susceptibility to infection. On adherent porcine bone marrow (pBM) cells the expression of CD45 was strongly correlated with infection. CD163 and CD203a expression correlated at intermediate levels with infection, indicating cells expressing these markers could become infected but were not preferentially infected by the virus. Most of the cells expressing MHCII were infected, indicating that they may be preferentially infected although expression of MHCII was not essential for infection and a large percentage of the infected cells were MHCII negative. CD16 showed a marked decrease in expression following infection and significantly lower levels of infected cells were shown to express CD16. Altogether these results suggest CD163 may be involved in ASFV infection but it may not be essential; the results also highlight the importance of other cell markers which requiring further investigation. 相似文献
5.
旨在研究非洲猪瘟病毒(African swine fever, ASFV)编码的D1133L基因功能,本文利用慢病毒表达系统构建了过表达D1133L的MA-104/D1133L细胞系,分析ASFV在MA-104/D1133L细胞系与MA-104细胞中的复制差异。利用RT-qPCR和Western blot技术分别检测了ASFV感染MA-104/D1133L细胞后p30和p72基因的转录和蛋白表达水平,同时测定病毒滴度和病毒拷贝数评价ASFV的复制能力。结果表明:ASFV p30和p72基因在MA-104/D1133L细胞系的转录和蛋白表达水平高于野生型细胞系,ASFV在MA-104/D1133L细胞系的病毒增殖能力高于野生型细胞。本研究成功构建了过表达ASFV D1133L基因的MA-104/D1133L细胞系,与野生型细胞相比,D1133L能促进ASFV增殖,MA-104/D1133L细胞系更利于ASFV的复制,本结果为进一步研究ASFV D1133L基因功能积累了生物材料。 相似文献
6.
A Fernández J Perez L Carrasco M A Sierra M Sanchez-Vizcaino A Jover 《American journal of veterinary research》1992,53(8):1462-1467
Tissues obtained from pigs inoculated with African swine fever virus (ASFV), fixed by vascular perfusion using glutaraldehyde, and embedded in paraffin or araldite were used for an immunohistologic electron microscopic study. To detect ASFV antigens, 4 methods were used on paraffin sections with or without pretreatment of the tissues. Use of biotinylated anti-ASFV antiserum combined with avidin-biotin complex and peroxidase proved to be the most suitable method, and antigen was detected in tissues infected with 2 ASF viruses of different virulence. Use of the glutaraldehyde fixation method should ensure optimal morphologic (structural and ultrastructural) data while allowing an immunohistologic study, and add to knowledge of the pathogenesis of ASF. 相似文献
7.
旨在初步探究非洲猪瘟病毒(African swine fever virus,ASFV)多基因家族MGF360-13L基因的功能。使用生物信息学软件对MGF360-13L基因进行分析;构建真核表达质粒pVAX1-MGF360-13L并转染至293T细胞进行表达;利用同源重组方法构建基因缺失毒株ASFV-ΔMGF360-13L,以相同的感染复数(MOI=0.01)在猪肺泡巨噬细胞(PAMs)中感染基因缺失毒株和亲本毒株(ASFV CN/GS/2018)后,利用红细胞吸附试验(HAD)计算病毒滴度并绘制体外生长曲线;以MOI=1将ASFV-ΔMGF360-13L和ASFV CN/GS/2018分别感染猪骨髓巨噬细胞(BMDM),利用qPCR和ELISA测定细胞炎性因子IL-1β、IL-6和TNF-α的表达水平。结果表明,MGF360-13L基因在ASFV基因Ⅱ型中相对保守,编码蛋白属于非分泌型、无跨膜区、亲水性好;构建的真核表达质粒pVAX1-MGF360-13L被293T细胞表达;成功获得MGF360-13L单基因缺失毒株ASFV-ΔMGF360-13L,与ASFV CN/GS/2018相比,其体外复制没有显著性差异;在ASFV-ΔMGF360-13L感染BMDM后,IL-1β、IL-6和TNF-α炎性细胞因子在转录和分泌水平都显著高于ASFV CN/GS/2018。本研究成功制备了ASFV的MGF360-13L基因缺失毒株,并证实了MGF360-13L基因作为ASFV复制非必需基因具有抑制炎性因子表达的功能,这为进一步注释ASFV MGF360-13L基因功能提供了线索。 相似文献
8.
A microculture assay is described for the titration of African swine fever virus (ASFV) using swine monocytes contained in mononuclear leucocyte (MNL) microcultures. Titration endpoints were determined by observing cytopathogenic effects (CPE) of ASFV infected monocytes with an inverted microscope at 40 X magnification. CPE was a late event following the detection of ASFV antigens in monocytes by radioimmune assay, immunofluorescence and hemadsorption. It began with the detachment, enlargement and rounding of monocytes which progressively formed into grape-like clusters of 3-20 or more cells which eventually lysed. The characteristic CPE was produced in monocyte microcultures by virulent, moderately virulent, Vero cell adapted, and nonhemadsorbing ASFV strains. The sensitivity and reproducibility of the CPE microassay was similar to that of the hemadsorption microassay. 相似文献
9.
J C Quintero R D Wesley T C Whyard D Gregg C A Mebus 《American journal of veterinary research》1986,47(5):1125-1131
The association of African swine fever virus (ASFV) with swine erythrocytes in vivo, in high titers, was verified by inoculating 30 pigs with 17 ASFV isolates and assaying their plasma and washed erythrocyte fractions for residual virus. Viral antigens were specifically localized on the surface of in vitro and in vivo swine erythrocytes, using the fluorescent antibody technique and 3 monoclonal antibodies specific for ASFV. The same monoclonal antibodies immunoprecipitated virus-specific polypeptides of molecular weights 13 kd and 73 kd from ASFV-infected Vero cells. Erythrocytes from viremic swine infected with Lisbon-60, Dominican Republic, Badajoz-M98, or Cameroon isolates of ASFV were studied by transmission electron microscopy. Virus was found in membrane depressions at the surface of erythrocytes. These surface depressions resembled stages of smooth surfaced pits. Erythrocytes from viremic pigs were fragile osmotically. 相似文献
10.
【目的】试验旨在表达与纯化非洲猪瘟病毒(African swine fever virus, ASFV)的结构蛋白p22,将其作为包被抗原建立ASFV抗体的间接ELISA检测方法,用于诊断非洲猪瘟。【方法】将ASFV p22编码基因KP177R的截短体(24―145位氨基酸)克隆至原核表达载体pET-32a(+)中,将重组质粒pET-32a-p22转化大肠杆菌BL21(DE3)感受态细胞,经0.1 mmol/L IPTG诱导表达5 h,利用镍柱亲和纯化p22蛋白,并进行Western blotting鉴定。利用p22蛋白免疫BALB/c小鼠制备抗血清,并以含p22全长基因的真核表达质粒pCAGGS-EGFP-fp22转染HEK293T细胞为抗原基质,利用间接免疫荧光(IFA)鉴定抗血清的反应性。以重组p22蛋白为包被抗原,优化最佳抗原包被浓度、待检血清稀释度、封闭条件、抗原抗体反应时间、酶标二抗工作浓度等参数,建立ASFV抗体间接ELISA检测方法,并对临床猪血清样品进行检测。【结果】ASFV p22截短蛋白在大肠杆菌中高水平表达,蛋白产量为0.85 mg/100 g菌体;p22蛋白具... 相似文献
11.
前期研究初步表明非洲猪瘟病毒(ASFV)编码的D1133L基因对ASFV复制至关重要,本研究拟进一步探究D1133L在ASFV复制中的作用。利用同源重组技术结合大肠杆菌lac阻遏操作系统实现条件性敲除D1133L基因,以pUC118为骨架重组转移载体ASFVΔi130,将重组转移载体转染骨髓源巨噬细胞(BMDMs),以ASFV CN/GS/2018为亲本毒株感染BMDM,在β-D-硫代半乳糖苷(IPTG)存在的条件下,经绿色荧光和PCR鉴定,获得条件性敲除D1133L重组毒株vD1133Li。利用荧光显微镜观察该重组毒株与亲本毒株在猪肺泡巨噬细胞(PAMs)中的复制差异,利用qPCR技术比较重组病毒与亲本毒株的复制差异,分析vD1133Li在无IPTG情况下回补D1133L蛋白后与在IPTG诱导情况下的复制差异。结果显示:本研究成功构建了条件性敲除D1133L的ASFV重组病毒vD1133Li,重组毒株不表达D1133L,在IPTG诱导下复制能力显著低于亲本毒株;在稳定表达D1133L的MA-104细胞系中,vD1133Li复制能力恢复。综上所述,D1133L基因对于ASFV复制至关重... 相似文献
12.
非洲猪瘟(ASF)自2018年8月在我国暴发,对养猪业构成巨大威胁.该病是由非洲猪瘟病毒(ASFV)引起的家养猪高热、急性和高死亡率的出血症和淋巴组织坏死症;认识和了解病原ASFV与宿主的相互作用是理解致病机制的基础和疫病防控的前提.本文对ASFV与宿主细胞受体和内体系统的互作、基因转录和蛋白合成系统的互作、细胞凋亡和内质网应激系统的互作、天然免疫干扰素应答系统的互作、抗原递呈细胞的互作五个方面现有研究进展进行综述;并试图在此基础上理解ASFV的免疫保护和免疫逃逸作用,思考ASFV与宿主互作中需要回答的问题,为研制保护性疫苗和深入认识ASF致病机制提供线索. 相似文献
13.
M Gonzalez Juarrero C A Mebus R Pan Y Revilla J M Alonso J K Lunney 《Veterinary immunology and immunopathology》1992,32(3-4):243-259
Swine leukocyte antigens (SLA) and a macrophage specific marker were monitored on porcine macrophages cultured with or without macrophage colony stimulatory factor (M-CSF) and on cells infected with African swine fever virus (ASFV). SLA expression was maximal either in the total cell extract or on the cell surface at 3-4 days of culture; after 4 days these values began to decrease. Fluorescence analyses of immunostained macrophages cultured with or without M-CSF indicated a major upward shift in the number of SLA Class I molecules on individual macrophages whereas for SLA Class II both a novel expression of Class II and an upward shift in the number of molecules per cell were evident. Infection of 3-day-old macrophage cultures with three different isolates of ASFV resulted in minor changes in surface expression of SLA Class I, SLA Class II, and macrophage markers. No differences in infection with ASFV was observed whether macrophages were SLA Class II positive or negative, nor was there blocking by anti-SLA Class I or Class II monoclonal antibodies of ASFV infection of cultured macrophages. 相似文献
14.
旨在探究雌二醇(β-estradiol,E2)和孕酮(progesterone,P4)对非洲猪瘟病毒(African swine fever virus,ASFV)体外复制的影响。采集空怀猪血清(non-pregnant swine serum,NPSS)和怀孕猪血清(pregnant swine serum,PSS)处理后,用添加胎牛血清(fetal bovine serum,FBS)、NPSS和PSS的培养液分别培养猪肺泡巨噬细胞(porcine alveolar macrophages,PAMs)和骨髓巨噬细胞(bone marrow-derived macrophages,BMDM)并感染ASFV,利用绝对定量PCR和Western blot检测ASFV复制差异;用E2和P4 ELISA试剂盒检测各组血清中E2和P4含量;并在FBS组中单独或者混合添加E2和P4后感染ASFV,检测ASFV复制差异;用NPSS和PSS培养BMDM 24 h后,相对定量检测β-干扰素及下游抗病毒因子转录差异。PSS培养组ASFV复制高于NPSS培养组;PSS中E2和P4的含量均高于NPSS,且FBS中E2和P4的含量很低;在FBS组中单独或者混合添加E2和P4后ASFV复制量增加;PSS培养BMDM后会抑制β-干扰素及下游抗病毒因子的转录。PSS中高含量的E2和P4促进ASFV复制,本研究为解释临床上猪群感染非洲猪瘟(African swine fever,ASF)后母猪首先发病且怀孕母猪病情较重的现象提供一定的科学依据。 相似文献
15.
Karalyan Z Zakaryan H Sargsyan Kh Voskanyan H Arzumanyan H Avagyan H Karalova E 《Veterinary immunology and immunopathology》2012,145(1-2):551-555
African swine fever virus (ASFV) is the causative agent of African swine fever that is the significant disease of domestic pigs, with high rates of mortality. ASFV is double-stranded DNA virus whose genes encode some proteins that are implicated in the suppression of host immune response. In this study, we have modeled in vivo infection of ASFV for determination of interferon (IFN) status in infected pigs. We measured the level of IFN-α, -β and -γ by enzyme-linked immunosorbent assay and showed that the level of IFN-α sharply decreased during infection. Unlike IFN-α, the level of IFN-β and -γ increased from the 2nd and 4th days post-infection, respectively. Also, we analyzed the population dynamics of peripheral white blood cells of infected pigs due to their important role in host immune system. We showed that the atypical lymphocytes appeared after short time of infection and this result is in accordance with our previous study done in vitro. At the last day of infection about 50% of the total white blood cells were destroyed, and the remaining cells were represented mainly by small-sized lymphocytes, reactive lymphocytes and lymphoblasts. 相似文献
16.
为建立检测血清中非洲猪瘟病毒(African swine fever virus,ASFV)抗体的间接ELISA方法,本试验将ASFV p30基因进行原核表达,采用SDS-PAGE和Western blotting方法对重组蛋白进行表达鉴定和免疫原性分析,随后以纯化的重组蛋白为包被抗原,经条件优化、特异性试验、敏感性试验和重复性试验,建立一种血清中ASFV抗体的检测方法。结果显示,ASFV p30基因成功克隆到原核表达载体pET-32a (+)中,获得pET-32a-p30重组质粒;转化大肠杆菌BL21(DE3)感受态细胞进行诱导表达,得到P30重组蛋白,重组蛋白大小约为42 ku,主要以包涵体形式存在;Western blotting结果显示,纯化后的蛋白具有良好的免疫原性;以纯化的P30重组蛋白为包被抗原,建立了检测ASFV抗体的间接ELISA方法,通过方阵试验对间接ELISA方法进行优化,最终确定了抗原最佳包被浓度为1.2 μg/mL,待检血清最佳稀释倍数为1:100,最佳封闭液为1% BSA,酶标抗体最佳稀释度为1:4 000,以此建立的ASFV间接ELISA方法临界值为0.322。本方法仅与ASFV阳性血清发生特异性反应,与猪瘟病毒、猪繁殖与呼吸综合征病毒、口蹄疫病毒、伪狂犬病病毒、猪圆环病毒2型及猪流行性腹泻病毒阳性血清均无交叉反应,具有较强的特异性。该方法检测ASFV阳性血清灵敏度可达到1:1 600;批内重复性和批间重复性变异系数均<10%。本试验建立的间接ELISA方法具有良好的特异性、灵敏度和重复性,可初步应用于ASFV抗体的检测。 相似文献
17.
Claire Guinat Ana Luisa Reis Christopher L Netherton Lynnette Goatley Dirk U Pfeiffer Linda Dixon 《Veterinary research》2014,45(1)
African swine fever virus (ASFV) is a highly virulent swine pathogen that has spread across Eastern Europe since 2007 and for which there is no effective vaccine or treatment available. The dynamics of shedding and excretion is not well known for this currently circulating ASFV strain. Therefore, susceptible pigs were exposed to pigs intramuscularly infected with the Georgia 2007/1 ASFV strain to measure those dynamics through within- and between-pen transmission scenarios. Blood, oral, nasal and rectal fluid samples were tested for the presence of ASFV by virus titration (VT) and quantitative real-time polymerase chain reaction (qPCR). Serum was tested for the presence of ASFV-specific antibodies. Both intramuscular inoculation and contact transmission resulted in development of acute disease in all pigs although the experiments indicated that the pathogenesis of the disease might be different, depending on the route of infection. Infectious ASFV was first isolated in blood among the inoculated pigs by day 3, and then chronologically among the direct and indirect contact pigs, by day 10 and 13, respectively. Close to the onset of clinical signs, higher ASFV titres were found in blood compared with nasal and rectal fluid samples among all pigs. No infectious ASFV was isolated in oral fluid samples although ASFV genome copies were detected. Only one animal developed antibodies starting after 12 days post-inoculation. The results provide quantitative data on shedding and excretion of the Georgia 2007/1 ASFV strain among domestic pigs and suggest a limited potential of this isolate to cause persistent infection. 相似文献
18.
Kleiboeker SB Scoles GA 《Animal health research reviews / Conference of Research Workers in Animal Diseases》2001,2(2):121-128
African swine fever virus (ASFV) is the only known DNA arbovirus and the sole member of the family Asfarviridae. It causes a lethal, hemorrhagic disease in domestic pigs. ASFV is enzootic in sub-Saharan Africa and is maintained in a sylvatic cycle by infecting both wild members of the Suidae (e.g. warthogs) and the argasid tick Ornithodoros porcinus porcinus. The pathogenesis of ASFV in O. porcinus porcinus ticks is characterized by a low infectious dose, lifelong infection, efficient transmission to both pigs and ticks, and low mortality until after the first oviposition. ASFV pathogenesis in warthogs is characterized by an inapparent infection with transient, low viremic titers. Thus O. porcinus porcinus ticks probably constitute the most important natural vector of ASFV, although both the mammalian and tick hosts are probably required for the maintenance of ASFV in the sylvatic cycle. The mechanism of ASFV transmission from the sylvatic cycle to domestic pigs is probably through infected ticks feeding on pigs. In addition to O. porcinus porcinus, a number of North American, Central American and Caribbean species of Ornithodoros have been shown to be potential vectors of ASFV. 相似文献
19.
E V Genovesi R C Knudsen T C Whyard C A Mebus 《American journal of veterinary research》1988,49(3):338-344
Blood samples of pigs infected with a moderately virulent African swine fever virus (ASFV) isolate, obtained from the Dominican Republic (DR-II), were monitored temporally for viremia, infective ASFV association with major blood components, differential changes in blood cell composition, and plasma antibodies to ASFV. After intranasal/oral virus inoculation, pigs underwent acute infection and illness that resolved. Acute illness began on postinoculation day (PID) 4 and continued to PID 11, and pigs were febrile, with maximal infective ASFV titers detected in blood. By PID 11, initial antibody titers to ASFV antigens were detected in plasma. The WBC numbers were maintained near preinoculation counts; however, lymphocyte counts decreased slightly with a compensatory increment in neutrophil and monocyte numbers. From PID 11 to PID 25, rectal temperatures gradually returned to preinoculation values, titers of viremia began to decrease, plasma antibody to ASFV antigens increased to peak titers, and WBC numbers increased slightly. Percentages of lymphocytes returned to preinoculation values, neutrophil percentages decreased to slightly below preinoculation values, monocyte percentages were mildly increased, and eosinophil percentages were unaffected. From PID 25 to PID 46, titers of viremia further decreased, and plasma titers of antibodies to ASFV antigens remained high. In pigs with DR-II viremia (PID 4 to PID 46), most viral infectivity (greater than 95%) was RBC associated. Plasma contained less than 1% infectivity, and less than 0.1% of virus was in the WBC fraction (monocytes, lymphocytes, and granulocytes). After PID 46, viremia was no longer detectable. 相似文献