人血清白蛋白纯品含量的同位素稀释质谱方法研究

doi:10.3969/j.issn.1000-1158.2016.03.22

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Abstract A mass balance method and a high performance liquid chromatography-isotope dilution mass spectrometry （HPLC-IDMS） method are established to determine the mass fraction of pure human serum albumin (HSA). With the mass balance method, the pure HSA is quantified by HPLC and its moisture and ash are quantified by Karl Fischer and ignition residue analysis, which give an average mass fraction of 0.861 g/g. By the HPLC-IDMS method, after the pure HSA is hydrolyzed by acid, the resulted Pro, Val and Phe are quantified. Consequently, the mass fraction of HSA is calculated by the average. Under the optimized conditions, the mass fraction of HSA is 0.853 g/g with a relative standard deviation (RSD) of 0.8% and an expanded uncertainty of 0.015 g/g (k=2). The limits of detection and quantification are 1.37×10^-5 g/g and 4.55×10^-5 g/g, respectively. Compared with the mass balance method, the relative bias of the HPLC-IDMS method is 0.9%.

Key words： metrology human serum albumin mass fraction high performance liquid chromatography-isotope dilution mass spectrometry mass balance method

Received: 15 November 2014 Published: 22 March 2016

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TB99

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	Articles by authors
	LI Jia-le
	WU Li-qing
	JIN You-xun
	WANG Jing
	YANG Bin
	YANG Yi

Cite this article:

LI Jia-le,WU Li-qing,JIN You-xun, et al. Determination of the Mass Fraction of Pure Human Serum Albumin by HPLC-IDMS[J]. Acta Metrologica Sinica, 2016, 37(3): 328-332.

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http://jlxb.china-csm.org:81/Jwk_jlxb/EN/10.3969/j.issn.1000-1158.2016.03.22 OR http://jlxb.china-csm.org:81/Jwk_jlxb/EN/Y2016/V37/I3/328

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