IMMUNOLOGICAL CROSS-REACTIVITY TO LABORATORY-PRODUCED HPV-11 VIRIONS OF POLYSERA RAISED AGAINST BACTERIALLY DERIVED FUSION PROTEINS AND SYNTHETIC PEPTIDES OF HPV-6B AND HPV-16 CAPSID PROTEINS

被引：28

作者：

CHRISTENSEN, ND

KREIDER, JW

CLADEL, NM

GALLOWAY, DA

机构：

[1] FRED HUTCHINSON CANC RES CTR,SEATTLE,WA 98104

[2] PENN STATE UNIV,MILTON S HERSHEY MED CTR,DEPT MICROBIOL & IMMUNOL,HERSHEY,PA 17033

来源：

VIROLOGY | 1990年 / 175卷 / 01期

关键词：

D O I：

10.1016/0042-6822(90)90180-Y

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

Polysera raised in rabbits to bacterially derived fusion proteins and synthetic peptides of the Li and L2 ORFs of HPV-6b and -16 were tested for cross-reactivity to laboratory-produced infectious HPV-11 virions. The polysera were analyzed in a series of five different immunological assays including immunoperoxidase staining of the koilocytotic nuclei in sections of formalin-fixed, paraffin-embedded as well as fresh frozen sections of HPV-11 experimental condylomas generated in the athymic nude mouse xenograft system, ELISA, Western blots, and neutralization of infectious HPV-11 virions. ELISA and Western blot assays were used to determine whether the polysera identified external or internal epitopes on HPV-11 virions, and whether there was cross-reactivity to BPV-1 or laboratory-produced CRPV virions. Seven of a total of 12 sera were positive for reactivity to HPV-11 in one or more assays, but none of the reactivity was directed to external epitopes on the intact virions as determined by ELISA. None of the L1 products generated group-specific antigen (GSA) antisera including a synthetic peptide spanning the GSA site. The combination of assays clearly demonstrated that apparent false positive and false negative reactivities of different antisera were obtained for each assay system tested. Thus, no single assay could be used reliably to determine the true antiviral reactivity of a given polysera. © 1990.

引用

页码：1 / 9

页数：9

共 25 条

[1] ALMEIDA JD, 1969, MICROBIOS, V1, P225
[2] EXPRESSION OF HUMAN PAPILLOMAVIRUS TYPE-6 AND TYPE-16 CAPSID PROTEINS IN BACTERIA AND THEIR ANTIGENIC CHARACTERIZATION
BANKS, L
MATLASHEWSKI, G
PIM, D
CHURCHER, M
ROBERTS, C
CRAWFORD, L
[J]. JOURNAL OF GENERAL VIROLOGY, 1987, 68 : 3081 - 3089
[3] AUTOMATED CHEMICAL SYNTHESIS OF A PROTEIN-GROWTH FACTOR FOR HEMATOPOIETIC-CELLS, INTERLEUKIN-3
CLARKLEWIS, I
AEBERSOLD, R
ZILTENER, H
SCHRADER, JW
HOOD, LE
KENT, SBH
[J]. SCIENCE, 1986, 231 (4734) : 134 - 139
[4] COGGIN JR, 1979, CANCER RES, V39, P545
[5] COWSERT LM, 1987, J NATL CANCER I, V79, P1053
[6] IDENTIFICATION OF PROTEINS ENCODED BY THE L1 AND L2 OPEN READING FRAMES OF HUMAN PAPILLOMAVIRUS-1A
DOORBAR, J
GALLIMORE, PH
[J]. JOURNAL OF VIROLOGY, 1987, 61 (09) : 2793 - 2799
[7] A PAPILLOMAVIRUS DNA FROM A CERVICAL-CARCINOMA AND ITS PREVALENCE IN CANCER BIOPSY SAMPLES FROM DIFFERENT GEOGRAPHIC REGIONS
DURST, M
GISSMANN, L
IKENBERG, H
ZURHAUSEN, H
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1983, 80 (12): : 3812 - 3815
[8] PEPTIDES AS ANTIGENS - IMPORTANCE OF ORIENTATION
DYRBERG, T
OLDSTONE, MBA
[J]. JOURNAL OF EXPERIMENTAL MEDICINE, 1986, 164 (04) : 1344 - 1349
[9] STRUCTURAL POLYPEPTIDES OF RABBIT, BOVINE, AND HUMAN PAPILLOMAVIRUSES
FAVRE, M
BREITBURD, F
CROISSANT, O
ORTH, G
[J]. JOURNAL OF VIROLOGY, 1975, 15 (05) : 1239 - 1247
[10] DETECTION OF HUMAN PAPILLOMAVIRUS CAPSID ANTIGENS IN VARIOUS SQUAMOUS EPITHELIAL LESIONS USING ANTIBODIES DIRECTED AGAINST THE L1 AND L2 OPEN READING FRAMES
FIRZLAFF, JM
KIVIAT, NB
BECKMANN, AM
JENISON, SA
GALLOWAY, DA
[J]. VIROLOGY, 1988, 164 (02) : 467 - 477

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