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建立采用选择反应监测(SRM)质谱法定量五种泪液蛋白的方法。

Method development for quantification of five tear proteins using selected reaction monitoring (SRM) mass spectrometry.

机构信息

Vision Cooperative Research Centre, Sydney, New South Wales, Australia.

出版信息

Invest Ophthalmol Vis Sci. 2014 Feb 10;55(2):767-75. doi: 10.1167/iovs.13-12777.

Abstract

PURPOSE

To establish the use of selected reaction monitoring (SRM) mass spectrometry for quantification of tear proteins.

METHODS

Tear samples were collected on multiple occasions (7-10 days) from healthy subjects with contact lens wear (CL = 3) and without contact lens wear (NCL = 4). Tear proteins were denatured using 8M urea, reduced with iodoacetamide, precipitated by acetone, and digested using trypsin. Internal standards were included by adding isotopically-labelled standards of known concentrations to the samples. Lactoferrin, lysozyme, prolactin-induced protein, lipocalin 1, and proline-rich protein 4 were quantified using liquid chromatography-triple quadruple mass spectrometry in conjunction with selected reaction monitoring.

RESULTS

The limits of quantification for the selected peptides were below 50 pg/μL. The recovery of peptides from spiked digested tears was greater than or equal to 56% and the coefficient of variation values were less than or equal to 16%. The concentration of lactoferrin (1.20 ± 0.77 μg/μL), lysozyme (2.11 ± 1.50 μg/μL), and lipocalin-1 (1.75 ± 0.99 μg/μL) were consistent with previous ELISA studies. Tear levels of prolactin-induced protein (0.09 ± 0.06 μg/μL) and proline-rich 4 (0.80 ± 0.50 μg/μL) are reported here for the first time.

CONCLUSIONS

The SRM method can be used for simultaneous detection and quantification of selected proteins in low volumes of human tear samples (2.5 μL per sample) without prior purification of each protein component or need for antibodies.

摘要

目的

建立使用选择反应监测(SRM)质谱法定量分析泪液蛋白。

方法

从佩戴隐形眼镜(CL=3)和不佩戴隐形眼镜(NCL=4)的健康受试者多次(7-10 天)收集泪液样本。使用 8M 尿素使泪液蛋白变性,用碘乙酰胺还原,用丙酮沉淀,然后用胰蛋白酶消化。通过向样品中加入已知浓度的同位素标记标准品来加入内标。使用液相色谱-三重四极杆质谱联用选择反应监测法定量测定乳铁蛋白、溶菌酶、催乳素诱导蛋白、脂钙蛋白 1 和富含脯氨酸蛋白 4。

结果

所选肽段的定量下限均低于 50pg/μL。从加标消化的泪液中回收肽段的比例大于或等于 56%,变异系数值小于或等于 16%。乳铁蛋白(1.20±0.77μg/μL)、溶菌酶(2.11±1.50μg/μL)和脂钙蛋白-1(1.75±0.99μg/μL)的浓度与之前的 ELISA 研究一致。催乳素诱导蛋白(0.09±0.06μg/μL)和富含脯氨酸蛋白 4(0.80±0.50μg/μL)的泪液水平是首次报道。

结论

SRM 方法可用于同时检测和定量分析低体积人泪液样本中的选定蛋白(每个样本 2.5μL),而无需对每种蛋白成分进行预先纯化或使用抗体。

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