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THE ANAPLASMA-MARGINALE MSP5 GENE ENCODES A 19-KILODALTON PROTEIN CONSERVED IN ALL RECOGNIZED ANAPLASMA SPECIES

被引:136
作者
VISSER, ES
MCGUIRE, TC
PALMER, GH
DAVIS, WC
SHKAP, V
PIPANO, E
KNOWLES, DP
机构
[1] USDA ARS,ANIM DIS RES UNIT,PULLMAN,WA 99164
[2] WASHINGTON STATE UNIV,DEPT VET MICROBIOL & PATHOL,PULLMAN,WA 99164
[3] ONDERSTEPOORT VET INST,ONDERSTEPOORT 0110,SOUTH AFRICA
[4] KIMRON VET INST,DEPT PATHOL,BET DAGAN,ISRAEL
来源
INFECTION AND IMMUNITY | 1992年 / 60卷 / 12期
关键词
D O I
10.1128/IAI.60.12.5139-5144.1992
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Immunization with Anaplasma marginale outer membranes induced immunity against clinical disease which correlated with antibody titer to outer membrane proteins, including a 19-kDa protein (N. Tebele, T. C. McGuire, and G. H. Palmer, Infect. Immun. 59:3199-3204, 1991). This 19-kDa protein, designated major surface protein 5 (MSP-5), was encoded by a single-copy 633-bp gene. The molecular mass of MSP-5, defined in immunoblots by binding to monoclonal antibody ANAF16C1, was conserved among all recognized species of Anaplasma: A. marginale, A. centrale, and A. ovis. Recombinant MSP-5, which absorbed the antibody reactivity of bovine immune serum to native MSP-5, was recognized by anti-A. marginale and anti-A. centrale immune sera in a competitive inhibition assay with monoclonal antibody ANAF16C1. The presence of antibody to the epitope defined by monoclonal antibody ANAF16C1 in all postinfection sera tested indicates that this epitope is a potential diagnostic antigen for use in identifying persistently infected cattle.
引用
收藏
页码:5139 / 5144
页数:6
相关论文
共 40 条
[1]  
ALDERINK FJ, 1981, 7TH P NAT AN C, P27
[2]   MOLECULAR-BASIS FOR SURFACE-ANTIGEN SIZE POLYMORPHISMS AND CONSERVATION OF A NEUTRALIZATION-SENSITIVE EPITOPE IN ANAPLASMA-MARGINALE [J].
ALLRED, DR ;
MCGUIRE, TC ;
PALMER, GH ;
LEIB, SR ;
HARKINS, TM ;
MCELWAIN, TF ;
BARBET, AF .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (08) :3220-3224
[3]   COMPARATIVE SEQUENCE-ANALYSIS OF A GENUS-COMMON RICKETTSIAL ANTIGEN GENE [J].
ANDERSON, BE ;
TZIANABOS, T .
JOURNAL OF BACTERIOLOGY, 1989, 171 (09) :5199-5201
[4]   SEQUENCE-ANALYSIS OF THE 17-KILODALTON-ANTIGEN GENE FROM RICKETTSIA-RICKETTSII [J].
ANDERSON, BE ;
REGNERY, RL ;
CARLONE, GM ;
TZIANABOS, T ;
MCDADE, JE ;
FU, ZY ;
BELLINI, WJ .
JOURNAL OF BACTERIOLOGY, 1987, 169 (06) :2385-2390
[5]   USE OF MONOCLONAL-ANTIBODY IN A BLOCKING ELISA TO DETECT GROUP-SPECIFIC ANTIBODIES TO BLUETONGUE VIRUS [J].
ANDERSON, J .
JOURNAL OF IMMUNOLOGICAL METHODS, 1984, 74 (01) :139-149
[6]   CHARACTERIZATION OF AN IMMUNOPROTECTIVE PROTEIN COMPLEX OF ANAPLASMA-MARGINALE BY CLONING AND EXPRESSION OF THE GENE CODING FOR POLYPEPTIDE AM105L [J].
BARBET, AF ;
PALMER, GH ;
MYLER, PJ ;
MCGUIRE, TC .
INFECTION AND IMMUNITY, 1987, 55 (10) :2428-2435
[7]   THE MSP1-BETA MULTIGENE FAMILY OF ANAPLASMA-MARGINALE - NUCLEOTIDE-SEQUENCE ANALYSIS OF AN EXPRESSED COPY [J].
BARBET, AF ;
ALLRED, DR .
INFECTION AND IMMUNITY, 1991, 59 (03) :971-976
[8]  
BEVAN LI. E. W., 1912, Veterinary Journal, V68, P400
[9]   CHARACTERIZATION OF THE GENE ENCODING THE PROTECTIVE PARACRYSTALLINE-SURFACE-LAYER PROTEIN OF RICKETTSIA-PROWAZEKII - PRESENCE OF A TRUNCATED IDENTICAL HOMOLOG IN RICKETTSIA-TYPHI [J].
CARL, M ;
DOBSON, ME ;
CHING, WM ;
DASCH, GA .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (21) :8237-8241
[10]  
DAVIS WC, 1981, 7TH P NAT AN C, P285
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