Expression of tumor-associated trypsinogens (TAT-1 and TAT-2) in prostate cancer

Anders Bjartell, Annukka Paju, Wan Ming Zhang, Virgil Gadaleanu, Jens Hansson, Göran Landberg, Ulf Håkan Stenman

    Research output: Contribution to journalArticlepeer-review

    Abstract

    BACKGROUND. Trypsinogens are pancreatic serine proteinases and expressed in several cancers as tumor-associated trypsinogens (TAT). Trypsin mediates activation of pro-uPA and pro-MMPs, thus promoting angiogenesis and tumor invasion. Recently, we described expression of TAT in the human male genital tract and now we studied TAT in relation to PSA in PCa. METHODS. TAT expression was studied by immunohistochemistry, in situ hybridization, RT-PCR, DNA-sequencing and IFMA. LNCaP cells were used to study secretion of TAT and PSA after androgen stimulation. RESULTS. Immunoreactive TAT was localized in all prostatic tumors (n = 109), lymph node (n = 16), and bone metastases (n = 17). Immunostaining intensity increased with higher Gleason's grade, whereas PSA immunostaining decreased significantly. PSA and TAT were not identically distributed in benign and malignant cells. Androgen stimulation of LNCaP cells decreased secretion of TAT and increased that of PSA. TAT mRNA was demonstrated in tissue sections and identified as TAT-1 and -2 by RT-PCR and DNA-sequencing. CONCLUSIONS. Expression of TAT is better preserved than PSA in high-grade PCa. Expression of TAT and PSA is regulated by different mechanisms as demonstrated in tissue sections and in vitro. Locally produced TAT may act in a paracrine mode to promote angiogenesis and tumor invasion in PCa by both activating and degrading of other proteinases. Further studies on the role of TAT in invasive PCa and on the mechanisms involved in the regulation of TAT expression are warranted. © 2005 Wiley-Liss, Inc.
    Original languageEnglish
    Pages (from-to)29-39
    Number of pages10
    JournalProstate
    Volume64
    Issue number1
    DOIs
    Publication statusPublished - 15 Jun 2005

    Keywords

    • Immunohistochemistry
    • In situ hybridization
    • Kallikreins
    • Proteases
    • RT-PCR

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