Subscribe to RSS
DOI: 10.1055/s-0038-1661211
Factors Influencing the Separation of Glu-Plasminogen Affinity Forms I and II by Affinity Chromatography
Publication History
Received 01 June 1984
Accepted 18 October 1984
Publication Date:
19 July 2018 (online)
Summary
Native human plasminogen, the proenzyme of plasmin (E. C. 3.4.21.7) occurs in blood in two well defined forms, affinity forms I and II. In this paper, the feasibility of separating these forms of human native plasminogen by affinity chromatography, is shown to be dependent on two factors: 1) the ionic composition of the buffer containing the displacing agent: buffers of varying contents of sodium, Tris, phosphate and chloride ions were compared, and 2) the type of adsorbent. Two adsorbents were compared: Sepharose-lysine and Sepharose-bisoxirane-lysine. Only in the phosphate containing buffers, irrespective of the type of adsorbent, the affinity forms can be separated. The influence of the adsorbent can be accounted for by a large difference in dissociation constants of the complex between plasminogen and the immobilized lysine.
-
References
- 1 Deutsch DG, Mertz ET. Plasminogen: Purification from human plasma by affinity chromatography. Science 1970; 170: 1095-1096
- 2 Brockway WJ, Castellino FJ. Measurement of the binding of antifibrinolytic amino acids to various plasminogens. Arch Biochem Biophys 1972; 151: 194-199
- 3 Castellino FJ, Sodetz JM. Rabbit plasminogen and plasmin isozymes. In: Methods in Enzymology. Lorand L. (ed) Academic Press; New York: 1976. 45 273-286
- 4 Castellino FJ, Powel JR. Human plasminogen. In: Methods in Enzymology. Lorand. (ed) Academic Press; New York: 1981. 80 365-378
- 5 Sundberg L, Porath J. Preparation of adsorbents for biospecific affinity chromatography. I. Attachment of group-containing ligands to insoluble polymers by means of bifunctional oxiranes. J Chromatogr 1974; 90: 87-98
- 6 Gelsema WJ, de Ligny CL, Roozen AM P, Wilms GP. Optimal conditions for the coupling of aromatic amines to epoxy-activated Sepharose 6B. J Chromatogr 1981; 209: 363-368
- 7 Dunn BM, Chaiken IM. Quantitative affinity chromatography. Determination of binding constants by elution with competitive inhibitors Proc Natl Acad Sci USA 1974; 71: 2382-2385
- 8 Gray WR. End-group analysis using dansyl chloride. In: Methods in Enzymology. Hirs CH W, Timasheff SN. (eds) Academic Press; New York: 1972. 25B 121-138
- 9 Weber K, Osborne M. The reliability of molecular weight determinations by dodecyl sulfate-polyacrylamide gel electrophoresis. J Biol Chem 1969; 224: 4406-4412
- 10 Hatton MW C, Regoeczi E. Some observations on the affinity chromatography of rabbit plasminogen. Biochim Biophys Acta 1974; 359: 51-65
- 11 Markus G, De Pasquale JL, Wissler FC. Quantitative determination of the binding of e-aminocaproic acid to native plasminogen. J Biol Chem 1978; 253: 727-732
- 12 Araki C. Structure of the agarose constituent of agar-agar. Bull Chem Soc Japan 1956; 29: 543-544
- 13 Van Ruyven-Vermeer IA M, Nieuwenhuizen W, Haverkate F, Timan T. A novel method for the rapid purification of human and rat fibrin(ogen) degradation products in high yields. Hoppe-Seyler’s Z physiol Chem 1979; 360: 633-637
- 14 Rickli EE, Cuendet PA. Isolation of plasmin-free plasminogen with N-terminal glutamic acid. Biochim Biophys Acta 1971; 250: 447-451