4.6 Article

Kinetics from Indirectly Detected Hyperpolarized NMR Spectroscopy by Using Spatially Selective Coherence Transfers

期刊

CHEMISTRY-A EUROPEAN JOURNAL
卷 17, 期 2, 页码 697-703

出版社

WILEY-V C H VERLAG GMBH
DOI: 10.1002/chem.201002151

关键词

dynamic nuclear polarization; enzyme catalysis; NMR spectroscopy; spatial encoding; time-resolved spectroscopy

资金

  1. Israel Science Foundation [ISF 447/09]
  2. Helen and Martin Kimmel Award for Innovative Investigation
  3. Perlman Family Foundation
  4. Weizmann Feinberg Graduate School
  5. French Ministry of Foreign and European Affairs

向作者/读者索取更多资源

An important recent development in NMR spectroscopy is the advent of ex situ dynamic nuclear polarization (DNP) approaches, which are capable of yielding liquid-state sensitivities that exceed considerably those afforded by the highest-field spectrometers. This increase in sensitivity has triggered new research avenues, particularly concerning the in vivo monitoring of metabolism and disease by NMR spectroscopy. So far such gains have mainly materialized for experiments that focus on nonprotonated, low-gamma nuclei; targets favored by relatively long relaxation times T-1, which enable them to withstand the transfer from the cryogenic hyperpolarizer to the reacting centers of interest. Recent studies have also shown that transferring this hyperpolarization to protons by indirectly detected methods could successfully give rise to H-1 NMR spectra of hyperpolarized compounds with a high sensitivity. The present study demonstrates that, when merged with spatially encoded methods, indirectly detected H-1 NMR spectroscopy can also be exploited as time-resolved hyperpolarized spectroscopy. A methodology is thus introduced that can successfully deliver a series of hyperpolarized H-1 NMR spectra over a minutes-long timescale. The principles and opportunities presented by this approach are exemplified by following the in vitro phosphorylation of choline by choline kinase, a potential metabolic marker of cancer; and by tracking acetylcholine's hydrolysis by acetylcholine esterase, an important enzyme partaking in synaptic transmission and neuronal degradation.

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