4.4 Article

Detection of the Prodrug-Activating Enzyme Carboxypeptidase G2 Activity with Chemical Exchange Saturation Transfer Magnetic Resonance

Journal

MOLECULAR IMAGING AND BIOLOGY
Volume 16, Issue 2, Pages 152-157

Publisher

SPRINGER
DOI: 10.1007/s11307-013-0680-5

Keywords

CEST MRI; Carboxypeptidase G2; Gene therapy; GDEPT

Funding

  1. MRC and Department of Health (England) [C1060/A10334]
  2. NHS
  3. Wellcome Trust [091763Z/10/Z]
  4. Christopher's Smile charity
  5. Cancer Research UK [C309/A8274, C107/A10433]
  6. Lewis Trust Ltd
  7. Head Neck Trust
  8. EPSRC [EP/H046526/1] Funding Source: UKRI
  9. Cancer Research UK [16464, 11566] Funding Source: researchfish
  10. Engineering and Physical Sciences Research Council [EP/H046526/1] Funding Source: researchfish

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The purpose of this study is to evaluate if the differential exchange rates with bulk water between amine and amide protons can be exploited using chemical exchange saturation transfer magnetic resonance (CEST-MR) to monitor the release of glutamate induced by carboxypeptidase G2 (CPG2), an enzyme utilized in cancer gene therapy. Z spectra of solutions of the CPG2 substrate, 3,5-difluorobenzoyl-l-glutamate (amide), and glutamate (amine) were acquired at 11.7 T, 37 A degrees C, across different pH (5-8). The ability of CEST-MR to monitor CPG2-mediated release of glutamate was assessed in extracts of CPG2-expressing cancer cells and purified solution of CPG2. The addition of CPG2 to a solution containing 3,5-difluorobenzoyl-l-glutamate led to a marked and progressively increasing CEST effect (+3 ppm), concomitant with the time-dependent release of glutamate induced by CPG2. CEST-MR allows the detection of CPG2 activity in vitro and supports the translation of CEST-MRI to assess CPG2-based gene therapy in vivo.

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