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Quantitative Recovery, Selective Removal and One‐Step Purification of Human Parotid and Leukemic Lysozymes by Immunoadsorption

  • Bruce J. MacKAY
  • , Vincent J. IACONO
  • , Joan M. ZUCKERMAN
  • , Elliot F. OSSERMAN
  • , Jerry J. POLLOCK
  • Stony Brook University
  • Government of New York

Research output: Contribution to journalArticlepeer-review

11 Scopus citations

Abstract

Immunoadsorption affinity chromatography was used to isolate and purify human lysozyme. The immunoadsorbent was prepared by coupling sheep anti‐(human leukemic lysozyme) IgG to epoxy‐activited Sepharose 6B. Lyophilized parotid saliva (21) was resupended in distilled water (325 ml, 50 mg/ml, w/v) and applied to a column which had a capacity to bind 4.25 mg human enzyme. Non‐adsorbed material did not contain lysozyme, as determined by enzymatic and immunological analyses. All lysozyme activity present in the applied sample (1.97 mg) bound to and was desorbed from the column by elution with 0.2 M sodium acetate HCl buffer, pH 1.8. The isolated material was homogeneous as determined by cationic and sodium dodecyl sulfate/polyacrylamide gel electrophoresis, ultracentrifugation, amino acid and amino‐terminal analyses, and immunoelectrophoretic analysis. The one‐step purification procedure yielded a 1370‐fold increase in specific activity. Human lysozyme was also selectively purified by this method from an ammonium sulfate precipitate of the urine of a patient with chronic monocytic leukemia. Amino acid and polyacrylamide gel electrophoretic analyses indicated that the purified enzyme was identical to human lysozyme isolated from leukemic urine by classical biochemical techniques.

Original languageEnglish
Pages (from-to)93-98
Number of pages6
JournalEuropean Journal of Biochemistry
Volume129
Issue number1
DOIs
StatePublished - Dec 1982

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