首页> 外文期刊>Analytical chemistry >Mass Spectrometric Quantitation of Tubulin Acetylation from Pepsin-Digested Rat Brain Tissue Using a Novel Stable-Isotope Standard and Capture by Anti-Peptide Antibody (SISCAPA) Method
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Mass Spectrometric Quantitation of Tubulin Acetylation from Pepsin-Digested Rat Brain Tissue Using a Novel Stable-Isotope Standard and Capture by Anti-Peptide Antibody (SISCAPA) Method

机译:用新型稳定同位素标准从胃蛋白酶消化的大鼠脑组织中致管酰胺的质谱定量,并通过抗肽抗体(SISCAPA)方法捕获

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摘要

Acetylation of alpha-tubulin at Lys-40 is a potential biomarker for cognitive deficits in various neurological disorders. However, this key post-translational modification (PTM) has not been previously studied with mass spectrometry, due to the inadequate distribution of tryptic cleavage sites. Following peptic digestion, a surrogate sequence containing this key PTM site was identified and was found to be stable and quantitatively reproducible. A highly sensitive and specific SISCAPA-LC-MS method for quantitating rat brain tubulin acetylation was developed, validated, and applied, and only required a small amount of tissue (2.2 mg). This workflow includes peptic digestion, stable-isotope dilution, capture with antiacetylated peptide antibody bound on protein G beads, and quantitation using LC-MS. The method allowed a lower limit of quantitation at 2.50 pmol/mg and provided a linear range of 2.50-62.50 pmol/mg. Selectivity, intra and interday precision and accuracy were also validated. This method has been successfully applied in a preclinical study of organophosphate neurotoxicity, and we found that chronic exposure to chlorpyrifos led to a significant and persistent inhibition of brain tubulin acetylation.
机译:Lys-40处的α-微管蛋白的乙酰化是用于各种神经系统疾病中的认知缺陷的潜在生物标志物。然而,由于胰蛋白酶切割位点的分布不足,此前尚未用谱分析术后改性(PTM)。在消化不良消化后,鉴定了含有该关键PTM位点的替代序列,并发现稳定和定量可再现。开发,验证和施加了一种用于定量大鼠脑微管蛋白乙酰化的高敏感和特异性的SISCAPA-LC-MS方法,并且仅需要少量组织(2.2mg)。该工作流程包括消化消化,稳定同位素稀释,捕获与蛋白G珠的抗抗乙酰化肽抗体,并使用LC-MS进行定量。该方法允许在2.50pmol / mg下定量下限,并提供2.50-62.50pmol / mg的线性范围。还验证了选择性,内部和白天精度和准确性。该方法已成功应用于有机磷酸酯神经毒性的临床前研究,并且我们发现慢性暴露于氯吡啶乳糖导致脑小管蛋白乙酰化的显着且持续的抑制。

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  • 来源
    《Analytical chemistry》 |2018年第3期|共9页
  • 作者单位

    Univ Georgia Dept Pharmaceut &

    Biomed Sci Coll Pharm 250 W Green St Athens GA 30602 USA;

    Augusta Univ Med Coll Georgia Dept Pharmacol &

    Toxicol Augusta GA 30912 USA;

    Univ Georgia Dept Pharmaceut &

    Biomed Sci Coll Pharm 250 W Green St Athens GA 30602 USA;

    Univ Georgia Dept Pharmaceut &

    Biomed Sci Coll Pharm 250 W Green St Athens GA 30602 USA;

    Univ Georgia Dept Pharmaceut &

    Biomed Sci Coll Pharm 250 W Green St Athens GA 30602 USA;

    Augusta Univ Med Coll Georgia Dept Pharmacol &

    Toxicol Augusta GA 30912 USA;

    Univ Georgia Dept Pharmaceut &

    Biomed Sci Coll Pharm 250 W Green St Athens GA 30602 USA;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分析化学;
  • 关键词

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