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人垂体组织中甲硫氨酸脑啡肽的快原子轰击质谱定量分析。

Fast atom bombardment mass spectrometric quantitative analysis of methionine-enkephalin in human pituitary tissues.

作者信息

Kusmierz J J, Sumrada R, Desiderio D M

机构信息

Department of Immunology-Virology, University of Tennesse--Memphis 38163.

出版信息

Anal Chem. 1990 Nov 1;62(21):2395-400. doi: 10.1021/ac00220a026.

Abstract

Picomole amounts of endogenous methionine-enkephalin (ME = YGGFM) were quantified in 11 individual human pituitaries by fast atom bombardment mass spectrometry methods. Quantification was based either upon the comparison of the molecular ion (MH+) current of endogenous ME versus the current of a deuterated ME internal standard (d5-ME) or, similarly, upon the unimolecular decomposition MH+----YGGF-+ In the first field-free region to produce the unique tetrapeptide fragment ion. The latter method used the multiple reaction monitoring (MRM) mode. Native ME was purified with an octadecylsilyl (ODS) disposable cartridge and with multidimensional reversed-phase high-performance liquid chromatography. The amounts of ME determined were 18.26 +/- 19.98 ng of ME/mg of protein with the MH+ method and 15.28 +/- 16.59 ng of ME/mg of protein with the MRM method. A fraction (ca. 4%) of the total amount of ME from one pituitary was used to acquire these quantitative data, and ca. half of the remaining amount of a separate sample (no d5-ME added) was used to obtain a linked scan at constant B/E (B, magnetic field; E, electric field) of the ME MH+ at 574 u to produce the amino acid sequence determining fragment ions at m/z 297, 354, 411, 397, 278, and 425 u corresponding to Y2", Y3", Y4", A4, B3, and B4, respectively. That product ion spectrum was similar to a scan of 100 ng of synthetic ME. We calculated that the amount of pentapeptide for the MRM experiments corresponded to a total of 30 ng (52 pmol) of ME on the probe tip during quantification. On the other hand, we estimated that 3 times more, or 90 ng (156 pmol), ME was on the probe tip during acquisition of the product ion spectrum.

摘要

采用快原子轰击质谱法对11个个体的人垂体中皮摩尔量的内源性甲硫氨酸脑啡肽(ME = YGGFM)进行了定量分析。定量分析是基于内源性ME的分子离子(MH⁺)电流与氘代ME内标(d⁵ - ME)电流的比较,或者类似地,基于在第一个无场区中产生独特四肽碎片离子的单分子分解MH⁺→YGGF⁺。后一种方法使用多反应监测(MRM)模式。天然ME用十八烷基硅烷(ODS)一次性柱和多维反相高效液相色谱进行纯化。用MH⁺法测定的ME量为18.26±19.98 ng ME/mg蛋白质,用MRM法测定的ME量为15.28±16.59 ng ME/mg蛋白质。来自一个垂体的ME总量的一小部分(约4%)用于获取这些定量数据,另一个单独样品(未添加d⁵ - ME)剩余量的约一半用于在574 u处对ME MH⁺进行恒定B/E(B,磁场;E,电场)的连锁扫描,以产生对应于Y²⁺、Y³⁺、Y⁴⁺、A⁴、B³和B⁴的m/z 297、354、411、397、278和425 u的氨基酸序列确定碎片离子。该产物离子谱与100 ng合成ME的扫描谱相似。我们计算得出,MRM实验中五肽的量在定量过程中相当于探针尖端上总共30 ng(52 pmol)的ME。另一方面,我们估计在产物离子谱采集过程中,探针尖端上的ME是其三倍多,即90 ng(156 pmol)。

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