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在体内 NMR 之前进行极化测量,实现对超极化分子的自动转移和注射。

Automated transfer and injection of hyperpolarized molecules with polarization measurement prior to in vivo NMR.

机构信息

Institute of Physics of Biological System, École Polytechnique Fédérale de Lausanne, Lausanne, Switzerland.

出版信息

NMR Biomed. 2013 Nov;26(11):1582-8. doi: 10.1002/nbm.2993. Epub 2013 Jul 25.

DOI:10.1002/nbm.2993
PMID:23893539
Abstract

Hyperpolarized magnetic resonance via dissolution dynamic nuclear polarization necessitates the transfer of the hyperpolarized molecules from the polarizer to the imager prior to in vivo measurements. This process leads to unavoidable losses in nuclear polarization, which are difficult to evaluate once the solution has been injected into an animal. We propose a method to measure the polarization of the hyperpolarized molecules inside the imager bore, 3 s following dissolution, at the time of the injection, using a precise quantification of the infusate concentration. This in situ quantification allows for distinguishing between signal modulations related to variations in the nuclear polarization at the time of the injection and signal modulations related to physiological processes such as tissue perfusion. In addition, our method includes a radical scavenging process that leads to a minor reduction in sample concentration and takes place within a couple of seconds following the dissolution in order to minimize the losses due to the presence of paramagnetic polarizing agent in the infusate. We showed that proton exchange between vitamin C, the scavenging molecule and the deuterated solvent shortens the long carboxyl (13)C longitudinal relaxation time in [1-(13)C]acetate. This additional source of dipolar relaxation can be avoided by using deuterated ascorbate. Overall, the method allows for a substantial gain in polarization and also leads to an extension of the time window available for in vivo measurements.

摘要

通过溶解动态核极化实现的超极化磁共振需要在体内测量之前将超极化分子从极化器转移到成像仪。在将溶液注入动物体内后,该过程会导致核极化不可避免地损失,这很难评估。我们提出了一种方法,即在注入时,即在溶液溶解后 3 秒内,通过对输注物浓度的精确定量,测量成像仪腔内超极化分子的极化。这种原位定量可以区分与注射时核极化变化相关的信号调制与组织灌注等生理过程相关的信号调制。此外,我们的方法包括一个自由基清除过程,该过程会导致样品浓度略有降低,并在溶液溶解后几秒钟内进行,以最大程度地减少输注物中顺磁极化剂存在所导致的损失。我们发现,维生素 C(清除分子)和氘化溶剂之间的质子交换会缩短[1-(13)C]乙酸盐中长羧基(13)C 纵向弛豫时间。通过使用氘化抗坏血酸可以避免这种额外的偶极弛豫源。总的来说,该方法可以大大提高极化度,并延长体内测量的可用时间窗口。

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