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一种简单的液相色谱-串联质谱法,使用琥珀酰胆碱作为底物来测量血清胆碱酯酶活性。

A simple liquid chromatography linked to tandem mass spectrometry method for measurement of serum cholinesterase activity using succinylcholine as substrate.

机构信息

Department of Clinical Biochemistry, Leeds Teaching Hospitals NHS Trust, Britannia House, Morley, Leeds LS27 ODQ, UK.

出版信息

Ann Clin Biochem. 2010 May;47(Pt 3):217-22. doi: 10.1258/acb.2010.009169. Epub 2010 Apr 14.

Abstract

BACKGROUND

Individuals who are unable to metabolize the short-acting muscle relaxant succinylcholine due to abnormal cholinesterase activity are currently investigated via spectrophotometry using artificial substrates and enzyme inhibitors. Methods have been described using succinylcholine as substrate but with measurement of the product choline. However, choline may be released from other endogenous substrates within the serum. Direct measurement of the in vitro metabolism of succinylcholine as substrate may provide a better indication of the in vivo situation with regard to cholinesterase status.

METHODS

The rate of in vitro metabolism of succinylcholine by cholinesterase was measured using liquid chromatography linked to tandem mass spectrometry (LC-MS/MS). A comparison was made using serum samples in which cholinesterase activity had been measured using propionylthiocholine as substrate and phenotyped by enzyme inhibitor studies.

RESULTS

A good correlation (r = 0.9, P < 0.0001) was found between cholinesterase activity measured by LC-MS/MS using succinylcholine as substrate compared with propionylthiocholine as substrate measured spectrophotometrically. All serum samples with a cholinesterase activity of <1 IU/L, as measured using succinylcholine as substrate, were considered to be at increased risk of succinylcholine sensitivity. These latter results correlated well to the atypical phenotypes.

CONCLUSIONS

A simple and fast LC-MS/MS technique for the measurement of cholinesterase activity using succinylcholine as substrate has been described. This method clearly identifies patients at risk of prolonged apnoea following succinylcholine administration and compares favourably with existing spectrophotometric methods using artificial substrates.

摘要

背景

由于异常的胆碱酯酶活性,无法代谢短效肌肉松弛剂琥珀酰胆碱的个体目前通过使用人工底物和酶抑制剂的分光光度法进行研究。已经描述了使用琥珀酰胆碱作为底物的方法,但测量产物胆碱。然而,胆碱可能从血清中的其他内源性底物中释放出来。直接测量琥珀酰胆碱作为底物的体外代谢可能会更好地反映胆碱酯酶状态的体内情况。

方法

使用液相色谱串联质谱法(LC-MS/MS)测量胆碱酯酶体外代谢琥珀酰胆碱的速率。使用已使用丙酰硫代胆碱作为底物测量胆碱酯酶活性并通过酶抑制剂研究表型的血清样本进行了比较。

结果

用 LC-MS/MS 测量的琥珀酰胆碱作为底物的胆碱酯酶活性与分光光度法测量的丙酰硫代胆碱作为底物的活性之间存在良好的相关性(r = 0.9,P <0.0001)。所有用琥珀酰胆碱作为底物测量的胆碱酯酶活性<1IU/L 的血清样本均被认为有发生琥珀酰胆碱敏感性增加的风险。这些结果与非典型表型很好地相关。

结论

已经描述了一种使用琥珀酰胆碱作为底物测量胆碱酯酶活性的简单快速的 LC-MS/MS 技术。该方法可明确识别出在琥珀酰胆碱给药后有长时间呼吸暂停风险的患者,并且与使用人工底物的现有分光光度法相比具有优势。

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