SUPERINFECTION OF CATS WITH FELINE IMMUNODEFICIENCY VIRUS SUBTYPE-A AND SUBTYPE-B

被引:34
|
作者
OKADA, S
PU, RY
YOUNG, E
STOFFS, WV
YAMAMOTO, JK
机构
[1] UNIV FLORIDA,COLL VET MED,DEPT COMPARAT & EXPTL PATHOL,GAINESVILLE,FL 32610
[2] KITASATO INST,CTR BASIC RES,DEPT VIROL,MINATO KU,TOKYO 108,JAPAN
[3] CAMBRIDGE BIOTECH CORP,WORCESTER,MA 01605
关键词
D O I
10.1089/aid.1994.10.1739
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
The ability of feline immunodeficiency virus (FIV) isolates from subtypes A and B to superinfect cats and cell cultures was tested, Three specific pathogen-free (SPF) cats were first inoculated with 10 ID50 of subtype B virus (FIVBang) and 30 weeks later inoculated with 100 ID50 of subtype A virus (FIVPet). On the basis of subtype-specific PCR analysis, both FIV subtypes were detected in the peripheral blood lymphocytes (PBLs) of two of three cats from 9 to 30 weeks following the second inoculation. Only the first virus was detected in the bone marrow (BM) cells of these two cats until 30 weeks following the second inoculation, at which time the second virus was finally detected in their BM cells. Both cats developed significant virus-neutralizing (VN) antibodies to the second virus by 15 weeks following the second inoculation; but only one cat had high VN titers to the first virus, which remained at the same level even after the second inoculation. The two control cats inoculated with only the second virus developed VN titers specifically to the second virus and were consistently PCR positive for the virus in PBLs and BM cells starting 9 weeks postinoculation. Thus a delay in BM infection with the second virus was observed in the two superinfected cats. In contrast, one of three cats had neither VN antibodies to the second virus nor PCR signal of the second virus in its PBLs, BM, and lymph node throughout the 30 weeks of study and it appeared to be resistant to superinfection. However, this cat bad high constant levels of both the first virus and VN antibodies to the first virus. In the in vitro superinfection studies, both FIVPet and FIVBang were detected in the primary PBL cultures after either simultaneous coinfection or superinfection (second virus infected 1 week later) and in the FIVPet-producer cell line after superinfection with FIVBang. Thus our in vitro results support our in vivo findings, which suggest that at a certain stage of initial FIV infection infected cats can be superinfected with another FIV subtype. These findings present the complexity of the FIV immunopathogenicity during multiple FIV exposure and shed some concern as to whether an FIV vaccine developed from a single subtype can completely protect cats against infection with other FIV subtypes. As a small animal AIDS model, our findings should also provide some insight into the events that occur during multiple HIV exposure in humans and in identifying approaches for HIV vaccine development.
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页码:1739 / 1746
页数:8
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