Neoplasia: An International Journal for Oncology Research (Jan 2002)

Cellular Activation of the Self-Quenched Fluorescent Reporter Probe in Tumor Microenvironment

  • Alexei A. Bogdanov, Jr.,
  • Charles P. Lin,
  • Maria Simonova,
  • Lars Matuszewski,
  • Ralph Weissleder

DOI
https://doi.org/10.1038/sj.neo.7900238
Journal volume & issue
Vol. 4, no. 3
pp. 228 – 236

Abstract

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The effect of intralysosomal proteolysis of near-infrared fluorescent (NIRF) self-quenched macromolecular probe (PGC-Cy5.5) has been previously reported and used for tumor imaging. Here we demonstrate that proteolysis can be detected noninvasively in vivo at the cellular level. A codetection of GFP fluorescence (using two-photon excitation) and NIRF was performed in tumor-bearing animals injected with PGC-Cy5.5. In vivo microscopy of tumor cells in subdermal tissue layers (up to 160 μm) showed a strong Cy5.5 dequenching effect in GFP-negative cells. This observation was corroborated by flow cytometry, sorting, and reverse transcription polymerase chain reaction analysis of tumor-isolated cells. Both GFP-positive (81% total) and GFP-negative (19% total) populations contained Cy5.5-positive cells. The GFP-negative cells were confirmed to be host mouse cells by the absence of rat cathepsin mRNA signal. The subfraction of GFPnegative cells (2.5-3.0%) had seven times higher NIRF intensity than the majority of GFP-positive or GFPnegative cells (372 and 55 AU, respectively). Highly NIRF-positive, FP-negative cells were CD45-and MAC3-positive. Our results indicate that: 1) intracellular proteolysis can be imaged in vivo at the cellular level using cathepsin-sensitive probes; 2) tumor-recruited cells of hematopoetic origin participate most actively in uptake and degradation of long-circulating macromolecular probes.

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