1. Evaluation of the C-terminal C5a effector site with short synthetic C5a analog peptides.
- Author
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Köhl J, Lübbers B, Klos A, Bautsch W, and Casaretto M
- Subjects
- Acetylglucosaminidase metabolism, Adenosine Triphosphate metabolism, Amino Acid Sequence, Animals, Blood Platelets metabolism, Complement C5a chemistry, Humans, In Vitro Techniques, Molecular Sequence Data, Neutrophils metabolism, Peroxidase metabolism, Rats, Recombinant Proteins, Structure-Activity Relationship, Tumor Cells, Cultured, Complement C5a metabolism
- Abstract
Biological activities have been determined for a series of 18 peptides based on the C-terminal sequence of human or rat C5a. Lysosomal enzyme release was tested in two cell types, the promyelotic leukemia cell line U937 and polymorphonuclear leukocytes. In addition, an ATP-release assay with guinea pig platelets was performed. It was demonstrated that the C-terminal octapeptide 67-74 of human C5a represents the minimal sequence required to induce a measurable biological signal in all assays. Extending this peptide to a length of 21 amino acids produced at best only a slight enhancement of potency. Amino acid replacements with either tryptophanyl or phenylalanyl residues in positions between 65-69 either increased potency (at position 67), or abrogated potency (at position 66) in the two lysosomal enzyme assays. N-terminal acylation with the fluorenylmethoxy-carbonyl-aminohexanoyl group slightly enhanced C5a potency. In desensitization experiments with guinea pig platelets all peptides with a C5a activity were able to desensitize not only the C5a but also the C3a responses.
- Published
- 1993
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