. 2017 May 11;23(27):6514-6517.

doi: 10.1002/chem.201700721. Epub 2017 Apr 20.

Detection of DT-diaphorase Enzyme with a ParaCEST MRI Contrast Agent

Iman Daryaei¹, Kyle M Jones², Mark D Pagel³

Affiliations

¹ Department of Chemistry and Biochemistry, University of Arizona, 1306 E. University Blvd., Room 221, Tucson, Arizona, 85721-0041, USA.
² Department of Biomedical Engineering, University of Arizona, 1127 E James E. Rogers Way P.O. Box 210020, Tucson, AZ, 85721-0020, USA.
³ Department of Medical Imaging, University of Arizona, 1501 N. Campbell, P.O. Box 245067, Tucson, Arizona, 85724, USA.

PMID: 28370655
PMCID: PMC6010184
DOI: 10.1002/chem.201700721

Detection of DT-diaphorase Enzyme with a ParaCEST MRI Contrast Agent

Iman Daryaei et al. Chemistry. 2017.

. 2017 May 11;23(27):6514-6517.

doi: 10.1002/chem.201700721. Epub 2017 Apr 20.

Authors

Iman Daryaei¹, Kyle M Jones², Mark D Pagel³

Affiliations

¹ Department of Chemistry and Biochemistry, University of Arizona, 1306 E. University Blvd., Room 221, Tucson, Arizona, 85721-0041, USA.
² Department of Biomedical Engineering, University of Arizona, 1127 E James E. Rogers Way P.O. Box 210020, Tucson, AZ, 85721-0020, USA.
³ Department of Medical Imaging, University of Arizona, 1501 N. Campbell, P.O. Box 245067, Tucson, Arizona, 85724, USA.

PMID: 28370655
PMCID: PMC6010184
DOI: 10.1002/chem.201700721

Abstract

A responsive magnetic resonance (MRI) contrast agent has been developed that can detect the enzyme activity of DT-diaphorase. The agent produced different chemical exchange saturation transfer (CEST) MRI signals before and after incubation with the enzyme, NADH, and GSH at different pH values whereas it showed good stability in a reducing environment without enzyme.

Keywords: CEST MRI; NQO1; dt-diaphorase; molecular imaging; trimethyl lock.

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Conflict of interest statement

Conflict of interest

The authors declare no conflict of interest.

Figures

**Figure 1**
Yb-DO3A-oAA-TML-Q was reacted with DT-diaphorase enzyme at pH 8.1 ± 0.1 and 37 °C for 15 h. CEST spectra were acquired with 6 μT, saturation power applied for 4 sec. (A) No reaction was detected when no enzyme, GSH, and NADH were added to the solution. (B) A new CEST signal at 9 ppm (solid red line) was detected when the CEST MRI agent was reacted with the enzyme, GSH, and NADH. The absence of NADH (C) or GSH (D) did not allow formation of the desired product whereas the CEST signal of unactivated CEST MRI agent (dashed lines in C and D) was clearly detected.

**Figure 2**
Yb-DO3A-oAA-TML-Q showed stability under anaerobic conditions (A) whereas the presence of DT-diaphorase enzyme and NADH in presence (B) or absence (C) of GSH activated the agent and produced a CEST signal at 9 ppm at pH 7.0 ± 0.25, 37 °C for 15 h, power level of 6 μT, and saturation time of 4 sec. The agent showed good stability in a reducing environment even in the presence of the enzyme and GSH in an anaerobic chamber (D).

**Scheme 1**
The quinone functional group in Yb-DO3A-oAA-TML-Q was reduced to hydroquinone in the presence of DT-diaphorase enzyme, NADH, and GSH. The newly formed hydroxy group attacked and dissociated the amide bond as a result of the steric effect between the methyl group on the benzene ring and the two adjacent methyl groups, consequently resulting in the release of the CEST agent.

**Scheme 2**
Synthesis of Yb-DO3A-oAA-TML-Q. The caboxylic acid form of quinone was prepared in 2 steps. Then it was reacted with *tert*-butyl protected DO3A-oAA that was prepared in 3 steps. The resulting product was de-protected and then used to chelate Yb^III.

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Detection of DT-diaphorase Enzyme with a ParaCEST MRI Contrast Agent

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Detection of DT-diaphorase Enzyme with a ParaCEST MRI Contrast Agent

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