Human antibodies reactive with purified envelope antigens of primate type C tumor viruses.

Kurth, Reinhard; Mikschy, U

doi:10.1073/pnas.75.11.5692

Cited by 26 publications

(17 citation statements)

References 49 publications

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“…ized with R-MuLV (Hersh et al, 1974;Charman et al, 1975) were tested in the < assay, with similar results (Fig. 6) (Kurth et al, 1977;Kurth & Mikschy, 1978). Our interpretation of this binding is, however, very difficult, and conforms with that offered in more recent work (Barbacid et al, 1980;Snyder & Fleissner, 1980 (Yamaga et al, 1977).…”

Section: Methodssupporting

confidence: 68%

“…As most of these viruses are immunologically and biochemically similar, it was hoped that a putative human virus would follow the same pattern. The discrepancies between the reports have been ascribed to the use of different techniques, viral antigens and serum samples (Kurth et al, 1977;Kurth & Mikschy, 1978). Moreover, the specificity of these antibodies has been questioned (Hogg et al, 1979;Snyder et al, 1976).…”

mentioning

confidence: 94%

“…The widespread presence of anti-Type C virus antibodies in the human population (healthy and cancer patients) has been described (Aoki et al, 1976;Caldwell et al, 1975: Kurth et al, 1977Kurth & Mikschy, 1978;Loui et al, 1976;Snyder et al, 1976), but also questioned (Gardner et al, 1977; Krakower & Aaronson, 1978: Stephenson & Aaronson, 1976. In the absence of a Type C virus of indisputable origin, proteins from well characterized mammalian Type C viruses have been used in the above studies.…”

mentioning

confidence: 99%

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Heterophile binding of human antibodies to glycoproteins of retroviruses

Cardoso¹

1981

Br J Cancer

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Summary.-The binding of human immunoglobulin to Type C viruses has been analysed by radioimmunoassay. The assay is a double-antibody, solid-phase RIA, which has been optimized and calibrated using rabbit and human anti-MuLV sera.It detects varying concentrations of IgG binding to HL-23-V-1, a human Type C virus isolate, in all of a large number of human sera tested. As judged by inhibition with nonspecific glycoproteins, heterophile antigens and pure saccharides, this binding is to the glycoside moiety of the virus-envelope glycoproteins, in agreement with other recent reports. Nonspecific binding of this type stringently restricts the interpretation which can be placed on these and earlier data in man concerning antibodies to Type C viruses. It does not however exclude the possibility that Type C viruses do occur in man and do elicit antibody therein.

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Section: Methodssupporting

confidence: 68%

mentioning

confidence: 94%

mentioning

confidence: 99%

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Heterophile binding of human antibodies to glycoproteins of retroviruses

Cardoso¹

1981

Br J Cancer

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“…Recently, Kurth and Mikschy (20) reported that a large fraction of human sera were capable of precipitating, at relatively high titers, the purified major envelope glycoprotein (gp7O) of the woolly monkey type C virus. These workers ascribed discrepancies with previous reports (15) to the influence of variables on the antigen-antibody reactions (21).…”

mentioning

confidence: 99%

Humans have antibodies capable of recognizing oncoviral glycoproteins: demonstration that these antibodies are formed in response to cellular modification of glycoproteins rather than as consequence of exposure to virus.

Barbacid¹,

Bolognesi²,

Aaronson³

1980

Proc. Natl. Acad. Sci. U.S.A.

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There is controversy in the literature concerning the presence in humans of antibodies directed against the envelope glycoproteins of known oncoviruses. In the present report, we show that antibodies capable of precipitating a wide variety of oncoviral glycoproteins can be demonstrated under certain assay conditions. Substances as diverse as normal components of serum, extracts of bacteria, and even nonprotein molecules such as glycogen also shared the oncoviral glycoprotein determinants recognized by normal human sera. It was found that immunoprecipitation of a given viral glycoprotein by human sera was entirely dependent upon the cell in which the virus was grown. Human sera specifically did not recognize glycoproteins purified from oncoviruses grown in human or higher primate cells. These findings not only demonstrate that the antibodies were directed against cellular rather than the virus-coded antigenic determinants but also exclude the possibility that this immune response was elicited as a consequence of oncovirus exposure.

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“…Purified RSV antigens and pp60 ~-src were iodinated by the chloramine T method and employed in RIPAs to test directly the specificity of monoclonal antibodies (Kurth & Mikschy, 1978). It proved to be advantageous to use either fresh, unfrozen monoclonal antibodies from ascites (as also observed by Lipsich et al, 1983) or aliquots frozen once only.…”

Section: Methodsmentioning

confidence: 99%

Isolation of Monoclonal Antibodies Specific for Rous Sarcoma Virus Structural, Polymerase and Transforming Proteins and Their Use for the Study of Mutant Virus-infected Cells

Kurth

Tanaka

Moelling

1985

Journal of General Virology

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SUMMARYMonoclonal antibodies were developed that are specific for Rous sarcoma virus structural, polymerase (reverse transcriptase) and transforming proteins. The monoclonal antibodies were shown to bind to purified virus proteins in an indirect ~ :5I-labelled Protein A binding assay suitable for screening even very large numbers of hybridomas. Additional tests for specificity included radioimmunoprecipitation of purified virus structural proteins P 12 and P27, of reverse transcriptase subunits ~ and/~, and of the transforming protein pp60 ..... . Pilot immunofluorescence and protein kinase assays of the expression of virus proteins in avian and mammalian cells infected by wild-type virus as well as by temperature-sensitive, transformation-defective virus mutants revealed that synthesis of virus structural and transforming proteins is hardly affected by changes in temperature, whereas the pp60"-~c-associated kinase activity is temperature-sensitive in cells infected by most, but not all the virus mutants.

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Human antibodies reactive with purified envelope antigens of primate type C tumor viruses.

Cited by 26 publications

References 49 publications

Heterophile binding of human antibodies to glycoproteins of retroviruses

Heterophile binding of human antibodies to glycoproteins of retroviruses

Humans have antibodies capable of recognizing oncoviral glycoproteins: demonstration that these antibodies are formed in response to cellular modification of glycoproteins rather than as consequence of exposure to virus.

Isolation of Monoclonal Antibodies Specific for Rous Sarcoma Virus Structural, Polymerase and Transforming Proteins and Their Use for the Study of Mutant Virus-infected Cells

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