首页> 外文学位 >Characterization of the outer membrane proteins of Actinobacillus (Haemophilus) pleuropneumoniae. (Volumes I and II).
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Characterization of the outer membrane proteins of Actinobacillus (Haemophilus) pleuropneumoniae. (Volumes I and II).

机译:猪肺炎放线杆菌(嗜血杆菌)外膜蛋白的表征。 (第一和第二卷)。

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摘要

The outer membrane of Actinobacillus (Haemophilus) pleuropneumoniae (HPP) serotype 1 (Shope 4074) was separated using the EDTA, lithium chloride-lithium acetate and sarkosyl extraction methods. The sarkosyl method gave the highest yield of outer membrane protein (OMP) while the EDTA method gave the least. Six prominent OMPs were consistently observed in all sarkosyl extracts. Their nomenclature and corresponding molecular weight (approximate) were as follows: A - 71kD, B - 47kD, C - 39kD, D - 36.5kD, E - 29.5kD and F - 17kD. OMPs C, D and E were heat modifiable and A, D and F were resistant to trypsin digestion. Western blots using HPP serotype 1 hyperimmune rabbit and swine sera revealed intense reactivity to major bands corresponding to OMPs A, B, C and D. The {dollar}sp{lcub}125{rcub}{dollar}I radioimmuno-precipitation method extrinsically identified a 39kD (OMP C) and a 17 kD (OMP F) OMP. Intrinsic labeling with {dollar}sp{lcub}35{rcub}{dollar}S methionine identified OMPs with the following molecular weight: 100kD, 94kD, 91kD, 67kD and 39kD (OMP C). All three procedures identified OMP C to have antibody reactivity. The OMPs of HPP serotypes 1 to 7 had similar profiles except at the 35 to 50kD region (variable region). Despite difference in OMP patterns, Western blots probed with heterologous antiserum revealed cross reactivity amongst the OMP antigens of the seven A.(H.) pleuropneumoniae serotypes. Serotype specificity of high molecular weight non-protein antigens were demonstrated for all. Immunologic cross-reactivities were also demonstrated between A. (H.) pleuropneumoniae serotype 1 (App 1), Haemophilus minor strain 202 (202), H. parasuis (Hps), Pasteurella multocida serotype A (PmA) and serotype D (PmD) antigens using both the ELISA and Western blot methods. The cross reaction studies had strengthened Pohl et al's (1981) clarification of relationships among members of Haemophilus, Pasterurella, and Actinobacillus. This relatedness was most observed especially when B. bronchiseptica OMPs were rarely recognized by antisera against the other bacterial respiratory pathogens.
机译:使用EDTA,氯化锂-乙酸锂和沙糖基萃取法分离出1型胸膜肺炎放线杆菌(HPP)(Shope 4074)的外膜。 sarkosyl方法的外膜蛋白(OMP)产量最高,而EDTA方法的产量最低。在所有鲨鱼油提取物中均一致观察到六个突出的OMP。它们的命名法和相应的分子量(近似)如下:A-71kD,B-47kD,C-39kD,D-36.5kD,E-29.5kD和F-17kD。 OMP C,D和E是可热修饰的,而A,D和F对胰蛋白酶消化具有抗性。使用HPP血清型1超免疫兔和猪血清的Western印迹显示与对应于OMP A,B,C和D的主要条带具有强烈反应性。{dol} sp {lcub} 125 {rcub} {dollar} I放射免疫沉淀法是外部鉴定的39kD(OMP C)和17kD(OMP F)OMP。用{dol} sp {lcub} 35 {rcub} {dollar} S蛋氨酸进行内在标记可鉴定出具有以下分子量的OMP:100kD,94kD,91kD,67kD和39kD(OMP C)。所有这三个过程都将OMP C鉴定为具有抗体反应性。 HPP血清型1至7的OMP具有相似的分布图,但在35至50kD区域(可变区域)除外。尽管OMP模式有所不同,但用异源抗血清探测的Western印迹揭示了7种胸膜肺炎链球菌血清型的OMP抗原之间具有交叉反应性。所有人都证明了高分子量非蛋白抗原的血清型特异性。在猪肺炎支原体血清型1(App 1),小嗜血杆菌(202),副猪嗜血杆菌(Hps),多杀巴斯德氏菌血清型A(PmA)和血清型D(PmD)之间也显示出免疫学交叉反应性。使用ELISA和Western blot方法检测抗原。交叉反应研究加强了Pohl等人(1981年)对嗜血杆菌,巴斯德氏菌和放线杆菌成员之间关系的阐明。这种相关性最明显,特别是当支气管芽孢杆菌OMP很少被抗血清对其他细菌性呼吸道病原体识别时。

著录项

  • 作者

    Rovira, Hope Guerrero.;

  • 作者单位

    University of Minnesota.;

  • 授予单位 University of Minnesota.;
  • 学科 Biology Microbiology.; Biology Veterinary Science.; Biology Molecular.
  • 学位 Ph.D.
  • 年度 1990
  • 页码 367 p.
  • 总页数 367
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 微生物学;动物学;分子遗传学;
  • 关键词

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