Clinical Chemistry
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Clinical Chemistry 50: 125-129, 2004. First published November 18, 2003; 10.1373/clinchem.2003.026146
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(Clinical Chemistry. 2004;50:125-129.)
© 2004 American Association for Clinical Chemistry, Inc.


Cancer Diagnostics

Immunopeptidometric Assay for Enzymatically Active Prostate-Specific Antigen

Ping Wua,1, Lei Zhu1, Ulf-Hkan Stenman1 and Jari Leinonen1

1 Department of Clinical Chemistry, Helsinki University Central Hospital, FIN-00029 Helsinki, Finland.

aAddress correspondence to this author at: Department of Clinical Chemistry, Biomedicum, A417a, Helsinki University Central Hospital, Haartmaninkatu 8, PB 700, FIN-00029 Helsinki, Finland. Fax 358-9-47171731; e-mail ping.wu{at}helsinki.fi.

Background: Determinations of certain forms of prostate-specific antigen (PSA) have been shown to increase the specificity for prostate cancer (PCa). One such variant, proteolytically active PSA, is a potentially useful tumor marker, but it is not specifically recognized by antibodies. Using phage display libraries, we previously identified a "family" of peptides that bind specifically to active PSA. We used these to develop an immunopeptidometric assay (IPMA) that specifically detects this form of PSA.

Methods: Microtitration plates coated with a PSA antibody were used to capture PSA, and a PSA-binding glutathione S-transferase (GST) fusion peptide was used as a tracer. Bound tracer was detected with an antibody to GST labeled with a europium chelate. PSA isoenzymes with high and low enzymatic activity were used to study binding specificity.

Results: The IPMA detected enzymatically active PSA but not internally cleaved PSA and pro-PSA, which are enzymatically inactive. The assay detected 1–10% of free PSA in serum from PCa patients.

Conclusions: Peptides identified by phage display can be used to develop assays with unique specificities for enzymatically active PSA. IPMA represents a new assay principle with wide potential utility.




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Novel Peptide Inhibitors of Human Kallikrein 2
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U.-H. Stenman
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