Literature DB >> 20145119

Tumor detection by imaging proteolytic activity.

Molly R Darragh1, Eric L Schneider, Jianlong Lou, Paul J Phojanakong, Christopher J Farady, James D Marks, Byron C Hann, Charles S Craik.   

Abstract

The cell surface protease membrane-type serine protease-1 (MT-SP1), also known as matriptase, is often upregulated in epithelial cancers. We hypothesized that dysregulation of MT-SP1 with regard to its cognate inhibitor hepatocyte growth factor activator inhibitor-1 (HAI-1), a situation that increases proteolytic activity, might be exploited for imaging purposes to differentiate malignant from normal tissue. In this study, we show that MT-SP1 is active on cancer cells and that its activity may be targeted in vivo for tumor detection. A proteolytic activity assay with several MT-SP1-positive human cancer cell lines showed that MT-SP1 antibodies that inhibit recombinant enzyme activity in vitro also bind and inhibit the full-length enzyme expressed on cells. In contrast, in the same assay, MT-SP1-negative cancer cell lines were inactive. Fluorescence microscopy confirmed the cell surface localization of labeled antibodies bound to MT-SP1-positive cells. To evaluate in vivo targeting capability, 0.7 to 2 nmoles of fluorescently labeled antibodies were administered to mice bearing tumors that were positive or negative for MT-SP1. Antibodies localized to MT-SP1-positive tumors (n = 3), permitting visualization of MT-SP1 activity, whereas MT-SP1-negative tumors (n = 2) were not visualized. Our findings define MT-SP1 activity as a useful biomarker to visualize epithelial cancers using a noninvasive antibody-based method.

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Year:  2010        PMID: 20145119      PMCID: PMC2823079          DOI: 10.1158/0008-5472.CAN-09-1640

Source DB:  PubMed          Journal:  Cancer Res        ISSN: 0008-5472            Impact factor:   12.701


  39 in total

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Journal:  Proc Natl Acad Sci U S A       Date:  1999-09-28       Impact factor: 11.205

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  20 in total

1.  Peptide length and leaving-group sterics influence potency of peptide phosphonate protease inhibitors.

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Journal:  Chem Biol       Date:  2011-01-28

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Review 3.  Fluorescent imaging of cancerous tissues for targeted surgery.

Authors:  Lihong Bu; Baozhong Shen; Zhen Cheng
Journal:  Adv Drug Deliv Rev       Date:  2014-07-24       Impact factor: 15.470

4.  Protein analytical assays for diagnosing, monitoring, and choosing treatment for cancer patients.

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Journal:  J Healthc Eng       Date:  2012-12       Impact factor: 2.682

5.  Proteinase-activated receptor 2 (PAR2) decreases apoptosis in colonic epithelial cells.

Authors:  Vadim Iablokov; Christina L Hirota; Michael A Peplowski; Rithwik Ramachandran; Koichiro Mihara; Morley D Hollenberg; Wallace K MacNaughton
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6.  A reverse binding motif that contributes to specific protease inhibition by antibodies.

Authors:  Eric L Schneider; Melody S Lee; Aida Baharuddin; David H Goetz; Christopher J Farady; Mick Ward; Cheng-I Wang; Charles S Craik
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Review 7.  Membrane-Anchored Serine Proteases and Protease-Activated Receptor-2-Mediated Signaling: Co-Conspirators in Cancer Progression.

Authors:  Nisha R Pawar; Marguerite S Buzza; Toni M Antalis
Journal:  Cancer Res       Date:  2019-01-04       Impact factor: 12.701

8.  Imaging a functional tumorigenic biomarker in the transformed epithelium.

Authors:  Aaron M LeBeau; Minhee Lee; Stephanie T Murphy; Byron C Hann; Robert S Warren; Romelyn Delos Santos; John Kurhanewicz; Samir M Hanash; Henry F VanBrocklin; Charles S Craik
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9.  Targeting uPAR with antagonistic recombinant human antibodies in aggressive breast cancer.

Authors:  Aaron M LeBeau; Sai Duriseti; Stephanie T Murphy; Francois Pepin; Byron Hann; Joe W Gray; Henry F VanBrocklin; Charles S Craik
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Authors:  Carly E Martin; Karin List
Journal:  Cancer Metastasis Rev       Date:  2019-09       Impact factor: 9.264

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