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Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography. / Platonova, Galina A.; Pankova, Galina A.; Il'Ina, Irma Ye; Vlasov, Guennady P.; Tennikova, Tatiana B.

In: Journal of Chromatography A, Vol. 852, No. 1, 06.08.1999, p. 129-140.

Research output: Contribution to journalArticlepeer-review

Harvard

Platonova, GA, Pankova, GA, Il'Ina, IY, Vlasov, GP & Tennikova, TB 1999, 'Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography', Journal of Chromatography A, vol. 852, no. 1, pp. 129-140. https://doi.org/10.1016/S0021-9673(99)00672-X

APA

Platonova, G. A., Pankova, G. A., Il'Ina, I. Y., Vlasov, G. P., & Tennikova, T. B. (1999). Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography. Journal of Chromatography A, 852(1), 129-140. https://doi.org/10.1016/S0021-9673(99)00672-X

Vancouver

Platonova GA, Pankova GA, Il'Ina IY, Vlasov GP, Tennikova TB. Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography. Journal of Chromatography A. 1999 Aug 6;852(1):129-140. https://doi.org/10.1016/S0021-9673(99)00672-X

Author

Platonova, Galina A. ; Pankova, Galina A. ; Il'Ina, Irma Ye ; Vlasov, Guennady P. ; Tennikova, Tatiana B. / Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography. In: Journal of Chromatography A. 1999 ; Vol. 852, No. 1. pp. 129-140.

BibTeX

@article{d3b9ac9a673f4cc09dec456e40a336eb,
title = "Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography",
abstract = "A new affinity method for the direct quantitative analysis of monospecific anti-peptide immunoglobulins (antibodies) and, simultaneously, their semi-preparative isolation from blood serum of the immunized animals has been developed. Immunoaffinity discs based on macroporous poly(glycidyl methacrylate-co-ethylene dimethacrylate) were used as the supporting stationary phase. The specifically prepared synthetic peptides with biological activity imitating that of the immunoglobulin binding sites of various proteins were used as the selective ligands instead of native proteins. These ligands were immobilized by a single-step reaction that involves epoxy groups located on the pore surface of the porous polymer disc with amine groups of the peptide molecules. A spacer between biospecific ligands and the linking site was not required to achieve good separation. These novel immunosorbents characterized by large binding capacity are well suited for high throughput screening. Dissociation constants of the peptide-antibody complexes calculated from the experimental adsorption isotherms confirm the excellent selectivity of the proposed separation method. The discs were used in a single step enrichment of antibodies both from precipitated blood fraction and crude blood serum of immunized animals. The quantitative data of the immunoaffinity disc chromatography were compared to those obtained by an enzyme-linked immunosorbent assay. Gel electrophoresis was also used to demonstrate the high degree of purity of the final product. In contrast to typical techniques that involve proteins, this immunoaffinity approach allows for the first time direct determination of concentration of specific antibodies using the immunosorbent prepared from the short peptide molecules immobilized on the internal surface of reactive porous polymer discs. Copyright (C) 1999.",
keywords = "Antibodies, Immunoaffinity chromatography, Membrane chromatography",
author = "Platonova, {Galina A.} and Pankova, {Galina A.} and Il'Ina, {Irma Ye} and Vlasov, {Guennady P.} and Tennikova, {Tatiana B.}",
note = "Funding Information: The preparation of peptides by N.N. Skvortzova and S.V. Burov (Department of Physiologically Active Polymers of the Institute of Macromolecular Compounds of the Russian Academy of Sciences, St. Petersburg, Russia) and sera from immunized rabbits by L.V. Puchkova, M.M. Shavlovskii, T.D. Olejnikova and S.B. Ivanova (Department of Molecular Genetics of the Institute of Experimental Medicine of the Russian Academy of Medical Sciences, St. Petersburg, Russia) is gratefully acknowledged. This project is funded by grant {\textquoteleft}Scientific Schools{\textquoteright} (96-1597393) of the Russian Basic Research Foundation. ",
year = "1999",
month = aug,
day = "6",
doi = "10.1016/S0021-9673(99)00672-X",
language = "English",
volume = "852",
pages = "129--140",
journal = "Journal of Chromatography",
issn = "0021-9673",
publisher = "Elsevier",
number = "1",

}

RIS

TY - JOUR

T1 - Quantitative fast fractionation of a pool of polyclonal antibodies by immunoaffinity membrane chromatography

AU - Platonova, Galina A.

AU - Pankova, Galina A.

AU - Il'Ina, Irma Ye

AU - Vlasov, Guennady P.

AU - Tennikova, Tatiana B.

N1 - Funding Information: The preparation of peptides by N.N. Skvortzova and S.V. Burov (Department of Physiologically Active Polymers of the Institute of Macromolecular Compounds of the Russian Academy of Sciences, St. Petersburg, Russia) and sera from immunized rabbits by L.V. Puchkova, M.M. Shavlovskii, T.D. Olejnikova and S.B. Ivanova (Department of Molecular Genetics of the Institute of Experimental Medicine of the Russian Academy of Medical Sciences, St. Petersburg, Russia) is gratefully acknowledged. This project is funded by grant ‘Scientific Schools’ (96-1597393) of the Russian Basic Research Foundation.

PY - 1999/8/6

Y1 - 1999/8/6

N2 - A new affinity method for the direct quantitative analysis of monospecific anti-peptide immunoglobulins (antibodies) and, simultaneously, their semi-preparative isolation from blood serum of the immunized animals has been developed. Immunoaffinity discs based on macroporous poly(glycidyl methacrylate-co-ethylene dimethacrylate) were used as the supporting stationary phase. The specifically prepared synthetic peptides with biological activity imitating that of the immunoglobulin binding sites of various proteins were used as the selective ligands instead of native proteins. These ligands were immobilized by a single-step reaction that involves epoxy groups located on the pore surface of the porous polymer disc with amine groups of the peptide molecules. A spacer between biospecific ligands and the linking site was not required to achieve good separation. These novel immunosorbents characterized by large binding capacity are well suited for high throughput screening. Dissociation constants of the peptide-antibody complexes calculated from the experimental adsorption isotherms confirm the excellent selectivity of the proposed separation method. The discs were used in a single step enrichment of antibodies both from precipitated blood fraction and crude blood serum of immunized animals. The quantitative data of the immunoaffinity disc chromatography were compared to those obtained by an enzyme-linked immunosorbent assay. Gel electrophoresis was also used to demonstrate the high degree of purity of the final product. In contrast to typical techniques that involve proteins, this immunoaffinity approach allows for the first time direct determination of concentration of specific antibodies using the immunosorbent prepared from the short peptide molecules immobilized on the internal surface of reactive porous polymer discs. Copyright (C) 1999.

AB - A new affinity method for the direct quantitative analysis of monospecific anti-peptide immunoglobulins (antibodies) and, simultaneously, their semi-preparative isolation from blood serum of the immunized animals has been developed. Immunoaffinity discs based on macroporous poly(glycidyl methacrylate-co-ethylene dimethacrylate) were used as the supporting stationary phase. The specifically prepared synthetic peptides with biological activity imitating that of the immunoglobulin binding sites of various proteins were used as the selective ligands instead of native proteins. These ligands were immobilized by a single-step reaction that involves epoxy groups located on the pore surface of the porous polymer disc with amine groups of the peptide molecules. A spacer between biospecific ligands and the linking site was not required to achieve good separation. These novel immunosorbents characterized by large binding capacity are well suited for high throughput screening. Dissociation constants of the peptide-antibody complexes calculated from the experimental adsorption isotherms confirm the excellent selectivity of the proposed separation method. The discs were used in a single step enrichment of antibodies both from precipitated blood fraction and crude blood serum of immunized animals. The quantitative data of the immunoaffinity disc chromatography were compared to those obtained by an enzyme-linked immunosorbent assay. Gel electrophoresis was also used to demonstrate the high degree of purity of the final product. In contrast to typical techniques that involve proteins, this immunoaffinity approach allows for the first time direct determination of concentration of specific antibodies using the immunosorbent prepared from the short peptide molecules immobilized on the internal surface of reactive porous polymer discs. Copyright (C) 1999.

KW - Antibodies

KW - Immunoaffinity chromatography

KW - Membrane chromatography

UR - http://www.scopus.com/inward/record.url?scp=0032769641&partnerID=8YFLogxK

U2 - 10.1016/S0021-9673(99)00672-X

DO - 10.1016/S0021-9673(99)00672-X

M3 - Article

C2 - 10480238

AN - SCOPUS:0032769641

VL - 852

SP - 129

EP - 140

JO - Journal of Chromatography

JF - Journal of Chromatography

SN - 0021-9673

IS - 1

ER -

ID: 87865835