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1.
冯少珍  李娇  曹伟胜  廖明 《微生物学报》2011,51(12):1663-1668
[目的]毒株NX0101是骨髓瘤病变型J亚群禽白血病病毒,其早期感染细胞能诱导PI3 K/Akt信号转导通路的激活,本文针对NX0101毒株是否存在YXXM基序及其作用进行了探讨.[方法]利用TMpred软件对NX0101毒株囊膜蛋白(Env)的氨基酸序列进行生物信息学分析,通过搭桥PCR方法将YXXM基序相应的核苷酸序列突变后,构建突变质粒并转染DF-1细胞,拯救出YXXM突变体毒株NX0101 mt( Y/F,M/A),利用real-time PCR和ELISA方法检测并比较YXXM突变前后毒株在RNA水平和蛋白水平的复制情况.[结果]NX0101毒株Env胞浆区554 -557位氨基酸存在典型的PI3K结合基序YXXM.YXXM基序突变后,病毒RNA转录水平和病毒蛋白合成水平都显著下降.[结论]YXXM基序对NX0101毒株在体外宿主细胞中复制发挥重要的作用.  相似文献   

2.
韩静  陈晨  曹红  陈福勇 《病毒学报》2005,21(4):293-297
将禽白血病病毒(ALV)的p27基因克隆人表达性载体pET28a,在大肠杆菌以His Tag融合蛋白的形式获得了高效表达。以表达产物免疫家兔,制备了抗ALV p27的多克隆抗体,经亲和纯化后,用此抗体建立了对ALV抗原的双抗体夹心法ELISA,并对疑似病料进行了实验室诊断。检测结果与IDEXX的禽白血病抗原检测试剂盒符合率达到98.6%,证明表达产物保留了天然p27蛋白的相关抗原性。交叉试验和群特异性试验证明,此方法具有良好的特异件,并且可以检测出A、B、J亚群的禽白血病病毒p27抗原。用此ALV抗体和所建立的ELISA方法成功地进行了禽白血病病毒抗原的实验室诊断。  相似文献   

3.
将鸡J亚群白血病病毒(ALV-J)中国分离株NX0101接种到已长成单层鸡胚成纤维细胞(CEF)的六孔细胞培养板上, 分为A组(培养基中无抗体)和B组(培养基中含抗体), 每组设3个独立的传代系列. 分别对第10代、20代和30代病毒的囊膜糖蛋白基因(env)进行了克隆和测序. 序列比较结果表明: 原始病毒与无抗体A组不同传代系列的不同代次之间gp85氨基酸序列同源性为97.7%~99.7%; 而原始病毒与有抗体B组不同传代系列的不同代次之间gp85的氨基酸序列同源性为93.8%~96.1%. 对gp85高变区上有义突变(NS)与沉默突变(S)的比例计算分析表明, 无抗体A组三个传代系列在110~120, 141~151和189~194 aa这3个高变区域上NS/S的值分别为2(8/4), 1(3/3)和1.3(4/3); 有抗体B组三个传代系列在110~120, 140~150和188~193 aa这3个高变区域上NS/S的值分别为4.1(13/3), 4.7(14/3)和3.3(11/3). 该结果是在严格实验条件下显示特异性抗体这一免疫选择压对gp85基因变异的影响.  相似文献   

4.
我国地方品种鸡分离到的一个禽白血病病毒新亚群的鉴定   总被引:2,自引:0,他引:2  
王鑫  赵鹏  崔治中 《病毒学报》2012,(6):609-614
为探明我国地方品种鸡群禽白血病病毒(Avian leukosis virus,ALV)的特点,通过接种DF-1细胞及细胞培养上清液p27抗原的检测,从芦花鸡中分离得到三株外源性ALV禽白血病病毒,分别是JS11C1、JS11C2和JS11C3,并对其进行亚群鉴定分析。用PCR方法扩增env基因测序,并与已知鸡源各亚群ALV的囊膜蛋白(gp85)作氨基酸同源性比较。这三株ALV的env基因的gp85大小为1 005bp,编码335个氨基酸;env基因的gp37大小为609bp,编码203个氨基酸。三个毒株之间gp85的同源性为91.9%~97.0%。与A、B、C、D和E五个经典亚群在GenBank中已发表的18个毒株的gp85的同源性仅在77.7%~84.6%间,显著低于鸡群中常见的A、B、E各亚群内的同源性范围(分别为88.2%~98.5%,91.6%~98.8%和97.9%~99.4%),而与J亚群参考株的同源性更是只有34.2%~36.5%。上述结果表明,芦花鸡分离到的三株病毒可能是不同于鸡源ALV已知6个亚群的一个新亚群,按国际上对ALV亚群分类的习惯,初步将其定名为K亚群。  相似文献   

5.
[目的]制备鼠抗fps单因子血清,检测急性致瘤性ALV诱发肉瘤组织中的fps肿瘤抗原.[方法]以J亚群相关禽白血病/肉瘤病毒Fu-J株RNA为模板,分两段扩增v-fps肿瘤基因,利用大肠杆菌表达系统表达这两段蛋白,纯化后将两种蛋白同时免疫小鼠,获得抗血清,间接免疫荧光试验检测肉瘤组织滤过液感染的CEF和肿瘤细胞中的fps抗原,免疫组织化学方法检测肿瘤组织中的fps抗原.[结果]该单因子血清具有较好特异性,不与经典ALV-J发生交叉反应.被感染的CEF细胞、肿瘤细胞及纤维肉瘤组织切片均显示阳性.[结论]该实验制备了鼠抗fps单因子血清,建立了fps肿瘤抗原的检测方法,为进一步研究该病毒的生物学特性及其致瘤机制奠定了基础.  相似文献   

6.
禽白血病病毒J亚群内蒙株的分离与鉴定   总被引:4,自引:0,他引:4  
本研究从曾见典型禽骨髓性白血病(Myeloid Leukosis, ML)病例的内蒙古某肉种鸡场随机选取的淘汰肉种鸡中,分离出一株J亚群禽白血病病毒(Avian leukosis virus Subgroup J, ALV-J).利用PCR和间接免疫荧光反应进行鉴定,J亚群禽白血病病毒内蒙株可以被两对ALV-J特异性引物扩增(特异条带约2.2kb和545bp);且在特异性单抗的间接免疫荧光检测中呈现强阳性荧光反应.此外,对山东一例肉种鸡骨髓性白血病病例亦进行了J亚群禽白血病病毒的分离与鉴定.2.2kb PCR扩增物的测序结果表明,两株分离病毒的同源性为96.9%,与已分离的SD9901和YZ9901株ALV-J同源性达94.2%~95.4%.  相似文献   

7.
本研究从曾见典型禽骨髓性白血病(Myeloid Leukosis,ML)病例的内蒙古某肉种鸡场随机选取的淘汰肉种鸡中,分离出一株J亚群禽白血病病毒(Avian leukosis virus Subgroup J.ALV-J)。利用PCR和间接免疫荧光反应进行鉴定,J亚群禽白血病病毒内蒙株可以被两对ALV—J特异性引物扩增(特异条带约2.2kb和545bp);且在特异性单抗的间接免疫荧光检测中呈现强阳性荧光反应。此外,对山东一例肉种鸡骨髓性白血病病例亦进行了J亚群禽白血病病毒的分离与鉴定。2.2kb PCR扩增物的测序结果表明,两株分离病毒的同源性为96.9%,与已分离的SD9901和YZ9901株ALV-J同源性达94.2%~95.4%。  相似文献   

8.
Wu ZC  Zhu MZ  Bian XM  Ma CT  Zhao P  Cui ZZ 《病毒学报》2011,27(5):447-455
本研究比较了从山东地方品系鸡群分离到的二株B亚型禽白血病病毒(ALV)SDAU09E3和SDAU09C2的全基因组序列及它们在细胞培养上的复制动态。这二株ALV-B的同源性为95.4%,与GenBank中3株B亚群参考株之间的同源性也均在91.0%~94.9%间,而与其它亚群参考株的同源性均低于87.9%。与亚群无关的gag、pol基因和LTR的核苷酸序列比较表明,这二株ALV-Bgp85基因的gag和pol基因与所有比较的参考株的同源性均在93%以上。LTR与其他外源性ALV参考株的LTR间的同源性在72.6%~88.3%范围内,但与E亚群内源性ALV的LTR的同源性只有51.5%。然而,这二个ALV-B的LTR的同源性也只有74.8%,远低于其他基因组部分的同源性,特别是它们的LTR的U3区同源性只有68.8%,二者在二个CAAT分布上也显著不同。对这二株ALV-B在DF-1细胞上的复制动态比较表明,它们在细胞培养上清液中的TCID50值非常类似,但SDAU09E3株核衣壳蛋白p27抗原的含量显著高于SDAU09C2株。这表明,同一亚群的不同毒株在复制过程中,所表达的p27抗原量与所形成的具有传染性的病毒量间没有平行关系。这一差异与LTR-U3区的相关性则有待应用感染性克隆技术来做进一步深入研究。  相似文献   

9.
采用PCR方法分3段扩增出J亚群白血病病毒NX0 10 1株的前病毒cDNA ,PCR产物经克隆后顺次连接,获得一个含有完整ALV J前病毒cDNA的重组质粒,命名为pALV J NX。将此质粒DNA纯化后转染鸡胚成纤维细胞,以针对ALV J的单克隆抗体JE9对转染后的细胞作间接免疫荧光反应,证明获得了具有感染性的病毒。测定原始野毒和分子克隆化病毒的半数组织感染量(TCID50 ) ,分别人工接种1日龄商品代肉鸡并隔离饲养17周。接种野毒组死亡率为2 6 % ,髓细胞瘤发病率为2 4 %。接种分子克隆化病毒组死亡率为2 2 % ,髓细胞瘤发病率为2 2 %。结果表明,克隆化病毒具有天然病毒的致病性并对肉用型鸡表现致瘤性  相似文献   

10.
根据GenBank数据库K亚群禽白血病病毒(Subgroup K avian leukosis virus,ALV-K)特异性抗原gp85的基因序列,设计一组ALV-K特异性的引物和探针,并构建阳性重组质粒。在对反应体系进行优化的基础上,建立了ALV-K的实时荧光RT-PCR检测方法并进行了特异性试验、敏感性试验和重复性试验。结果显示,本方法能对ALV-K进行特异性扩增,而对A亚群、B亚群、J亚群、E亚群禽白血病毒和新城疫病毒(NDV)、鸡传染性支气管炎病毒(IBV)、禽网状内皮组织增生病病毒(REV)、禽流感病毒(AIV)等禽病病原未见扩增。该方法最低能够检测到3.4×10~1拷贝数/μL的阳性质粒,灵敏度是RT-PCR的100倍。应用本方法对人工攻毒ALV-K的SPF鸡各脏器进行病毒定量分析,结果显示,在攻毒鸡体内心、肝、脾、肺、肾等脏器中均能检测到ALV-K,且肝、肾和脾中的病毒含量显著高于心和肺(P0.01)。  相似文献   

11.
Subgroup J Avian leucosis virus (ALV-J) strain NX0101 was inoculated into chicken embryo fibroblasts (CEF) monolayers in 6-well plates. The six wells of CEF inoculated with NX0101 were divided into groups A (without anti-ALV-J serum in the medium) and B (with anti-ALV-J serum in the medium), then viruses from each well of both groups were separately passed in CEF every 6 d and formed their independent passage lineages. For each lineage of both groups, gp85 genes of the viruses in the 10th, 20th and 30th passages were amplified, cloned and sequenced. The sequence data indicated that the homologies of gp85 at aa level between the primary virus and the passed viruses of different passages of 3 lineages in group A were 97.7%-99.7%; and the homologies of gp85 between the primary virus and the passed viruses of different passages of 3 lineages in group B were 93.8%-96.1%. Analysis of the ratios of nonsynonium (NS) vs synonium (S) mutations of nucleic acids demonstrated that NS/S in 3 highly variable (hr-) regions at aa#110-120, aa#141-151 and aa#189-194 of gp85 in 3 lineages of group A were 2 (8/4), 1(3/3) and 1.3 (4/3), however, NS/S in the same 3 hr-regions of group B were 4.1 (13/3), 4.7 (14/3) and 3.3 (11/3). This study is the first demonstration of influence of immune selective pressure on evolution of ALV-J gp85 by specific antibodies under the controlled in vitro experiments.  相似文献   

12.
Subgroup J Avian leucosis virus (ALV-J) strain NX0101 was inoculated into chicken embryo fibroblasts (CEF) monolayers in 6-well plates. The six wells of CEF inoculated with NX0101 were divided into groups A (without anti-ALV-J serum in the medium) and B (with anti-ALV-J serum in the medium), then viruses from each well of both groups were separately passed in CEF every 6 d and formed their independent passage lineages. For each lineage of both groups, gp85 genes of the viruses in the 10th, 20th and 30th passages were amplified, cloned and sequenced. The sequence data indicated that the homologies of gp85 at aa level between the primary virus and the passed viruses of different passages of 3 lineages in group A were 97.7%–99.7%; and the homologies of gp85 between the primary virus and the passed viruses of different passages of 3 lineages in group B were 93.8%–96.1%. Analysis of the ratios of nonsynonium (NS) vs synonium (S) mutations of nucleic acids demonstrated that NS/S in 3 highly variable (hr-) regions at aa#110–120, aa#141–151 and aa#189–194 of gp85 in 3 lineages of group A were 2 (8/4), 1(3/3) and 1.3 (4/3), however, NS/S in the same 3 hr-regions of group B were 4.1 (13/3), 4.7 (14/3) and 3.3 (11/3). This study is the first demonstration of influence of immune selective pressure on evolution of ALV-J gp85 by specific antibodies under the controlled in vitro experiments.  相似文献   

13.
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14.
【目的】为了研究出一种能够针对A亚群禽白血病的快速特异性诊断试剂。【方法】将A亚群禽白血病病毒(ALV-A)SDAU09E1株接种于DF1细胞上,以感染细胞DNA为模板,通过PCR方法扩增出1023bp的ALV-A-gp85基因。将其正确阅读框架插入表达载体PET-32a(+)中,实现在BL21(Rosetta)宿主菌中表达。将纯化的融合蛋白常规免疫小鼠,制备得抗血清。【结果】实验成功获得52.8kDa的重组融合蛋白,且具有良好的免疫原性。间接免疫荧光试验(IFA)表明该血清可与ALV-A和ALV-B反应,但不与ALV-J反应。【结论】该实验首次在国内外研制出能用于鉴别性检测经典的A/B亚群ALV的单因子血清,可与ALV-J特异性单抗互补作用于外源性ALV感染的鉴别性诊断。我国鸡群同时受经典的ALV-A/B和新出现的ALV-J困扰,鉴别诊断非常必要,研究这种试剂具有较高的实用价值。  相似文献   

15.
Christman SA  Kong BW  Landry MM  Kim H  Foster DN 《FEBS letters》2005,579(30):6705-6715
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16.
目的 确定DEAE-葡聚糖对CEMx174细胞的半数抑制浓度,明确其在SHIV病毒TCID50滴定及病毒扩增中的促进作用.方法 分别使用含DEAE和无DEAE的DMEM完全培养基测定SHIVchn19p7的TCID50.用无血清DMEM培养基系列稀释DEAE,加入CEMx174细胞,使用cck-8测定细胞破坏率.分别选取DEAE浓度为28.125μg/mL和14.0625μg/mL的无血清DMEM培养基对CEMx174细胞预处理3 h.再加入SHIV-KB9病毒液,定期测定培养上清中的P24水平,同时做正常病毒对照和DEAE-1640对照,比对不同处理下的病毒扩增情况.结果 使用了DEAE后,SHIVchn19p7的TCID50达到了3.16×104TCID50/mL,不使用DEAE,病毒的TCID50测定为阴性.DEAE对CEMx174细胞的IC50为44.85μg/mL.经浓度为28.125μg/mL和14.0625 μg/mL的DEAE预处理后,SHIV-KB9病毒扩增在13 d~17 d达到高峰.而用不含DEAE的1640生长液培养的实验孔在19 d才开始出现阳性反应.结论 高浓度的DEAE对细胞有较强的杀伤作用,低浓度的DEAE对细胞的破坏率较低,并且能显著促进病毒扩增.DEAE在病毒进入细胞的过程中确实起了重要的作用.  相似文献   

17.
The propagation of hepatitis A virus (HAV), CF53 strain, released without any cytopathic effect into the PLC/PRF/5 cells supernatant, was studied in the course of six serial passages (6th to 11th). The decrease (from 5 to 1 week) of incubation time required to detect HAV, by RIA, in culture supernatant, the increase in Hepatitis A antigen (from 777 to 10,038 c.p.m./50 microliter) and infectivity titre (from 10(3.0) TCID 50/ml to 10(4.5) TCID 50/ml) were consistent with the adaptation of this virus to the cell line PLC/PRF/5.  相似文献   

18.
Chickens bearing tumors which have been induced by avian retroviruses express cellmediated immune responsiveness against antigens which are associated with these neoplasms. We have employed a peripheral lymphocyte stimulation test to characterize antigens which are found in the supernatant fluids of avian retrovirus-infected chicken embryo fibroblast (CEF) cells and in the plasma of birds which have been inoculated with avian myeloblastosis virus (AMV). The results indicated that the antigenic activity being measured was virus group specific, cell transformation independent, and nonvirion in nature. Paradoxically, expression of such antigen(s) was restricted to cells which were actively synthesizing progeny avian retrovirus particles, and was absent in mammalian nonproducer cells which had been transformed by avian sarcoma viruses. Ability to respond immunologically to such antigen(s) was present in animals which had been inoculated with either leukosis or sarcoma viruses. Thymectomy, but not bursectomy, was stimulatory to tumor growth and abolished sensitized lymphocyte immune responsiveness in this system.  相似文献   

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