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Original Contribution

Separation of serum proteins by high performance liquid chromatography

Robert R. Harr, M.S., Paul S. Malchesky, D.Eng. and James Goldcamp, B.S.
Cleveland Clinic Journal of Medicine June 1986, 53 (2) 181-187;
Robert R. Harr
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Paul S. Malchesky
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James Goldcamp
Department of Artificial Organs, The Cleveland, Clinic Foundation
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ABSTRACT

This article describes the separation of serum proteins by isocratic HPLC using a polyvinyl alcohol gel as the stationary phase. The system separates immunoglobulins and other proteins by size exclusion and weak affinity bonding and gives a chromatogram that can be evaluated qualitatively, in a manner similar to serum protein electrophoresis scans. Peak heights measured for IgG, IgA, and IgM correlate closely with concentrations measured by radial immunodiffusion (RID). The separation, carried out without sample pretreatment, may prove to be a valuable technique for quantifying several serum proteins. The method may be used to screen hybridoma cultures for antibody production and to purify proteins without risk of denaturation.

Index terms
  • Blood proteins
  • Chromatography
  • high pressure liquid
  • Radioimmunoassay
  • Received November 1985.
  • Accepted March 1986.
  • Copyright © 1986 The Cleveland Clinic Foundation. All Rights Reserved.
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Cleveland Clinic Journal of Medicine: 53 (2)
Cleveland Clinic Journal of Medicine
Vol. 53, Issue 2
20 Jun 1986
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Separation of serum proteins by high performance liquid chromatography
Robert R. Harr, Paul S. Malchesky, James Goldcamp
Cleveland Clinic Journal of Medicine Jun 1986, 53 (2) 181-187;

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Separation of serum proteins by high performance liquid chromatography
Robert R. Harr, Paul S. Malchesky, James Goldcamp
Cleveland Clinic Journal of Medicine Jun 1986, 53 (2) 181-187;
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Keywords

  • Blood proteins
  • Chromatography
  • high pressure liquid
  • Radioimmunoassay

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