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核磁共振波谱法中脂溶性氮氧化物对脂质共振的选择性抑制

Selective suppression of lipid resonances by lipid-soluble nitroxides in NMR spectroscopy.

作者信息

Chen K, Lutz N W, Wehrle J P, Glickson J D, Swartz H M

机构信息

Department of Radiology and Radiological Sciences, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205.

出版信息

Magn Reson Med. 1992 May;25(1):120-7. doi: 10.1002/mrm.1910250112.

Abstract

The ability of lipid-soluble nitroxides to suppress selectively the peaks of lipid resonances in 31P, 1H, and 13C NMR spectra was investigated in serum as part of studies aimed at using these contrast agents for magnetic resonance imaging and magnetic resonance spectroscopy in vivo. Nitroxides are especially interesting potential contrast agents because they can reversibly be converted in cells to diamagnetic hydroxylamines, with conversion rates that are dependent on the redox potential and the intracellular concentration of oxygen; the characterization of nitroxide-dependent changes in NMR spectra may therefore be a useful means to measure oxygen-dependent redox metabolism in vivo. The fatty acid analogs, doxyl stearates, suppressed the methyl resonance of choline and the methyl and methylene peaks of lipids in the 1H NMR spectra of serum samples. As a consequence, lactate peaks, which were not readily detected became clearly resolved and could be evaluated quantitatively. The 31P resonance of phosphatidylcholine in the 31P NMR spectrum was suppressed by 5-doxyl stearate and 4-(N,N-dimethyl-N-hexadecyl)ammonium-2,2,6,6-tetramethylpiperidine-1-oxy l,iodid e (Cat16). In the 13C NMR spectrum, the resonances of the methyl groups of choline and the lipids also were broadened significantly by addition of 5-doxyl stearate. Differential suppression of lipid resonances can be employed to facilitate quantitation of lactate.

摘要

作为将这些造影剂用于体内磁共振成像和磁共振波谱研究的一部分,研究了脂溶性氮氧化物选择性抑制血清中31P、1H和13C NMR谱中脂质共振峰的能力。氮氧化物是特别有趣的潜在造影剂,因为它们可以在细胞中可逆地转化为抗磁性羟胺,其转化率取决于氧化还原电位和细胞内氧浓度;因此,NMR谱中依赖于氮氧化物的变化特征可能是测量体内氧依赖的氧化还原代谢的有用手段。脂肪酸类似物硬脂酰多昔,抑制了血清样品1H NMR谱中胆碱的甲基共振以及脂质的甲基和亚甲基峰。结果,原本不易检测到的乳酸峰变得清晰可辨,并可进行定量评估。在31P NMR谱中,磷脂酰胆碱的31P共振被5-硬脂酰多昔和4-(N,N-二甲基-N-十六烷基)铵-2,2,6,6-四甲基哌啶-1-氧基碘化物(Cat16)抑制。在13C NMR谱中,加入5-硬脂酰多昔后,胆碱和脂质甲基的共振也显著变宽。脂质共振的差异抑制可用于促进乳酸的定量分析。

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