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一种从人颅骨中分离全蛋白的方法。

A method for whole protein isolation from human cranial bone.

作者信息

Lyon Sarah M, Mayampurath Anoop, Rogers M Rose, Wolfgeher Donald J, Fisher Sean M, Volchenboum Samuel L, He Tong-Chuan, Reid Russell R

机构信息

The Pritzker School of Medicine, United States.

Computation Institute, United States; Center for Research Informatics, United States.

出版信息

Anal Biochem. 2016 Dec 15;515:33-39. doi: 10.1016/j.ab.2016.09.021. Epub 2016 Sep 25.

Abstract

The presence of the dense hydroxyapatite matrix within human bone limits the applicability of conventional protocols for protein extraction. This has hindered the complete and accurate characterization of the human bone proteome thus far, leaving many bone-related disorders poorly understood. We sought to refine an existing method of protein extraction from mouse bone to extract whole proteins of varying molecular weights from human cranial bone. Whole protein was extracted from human cranial suture by mechanically processing samples using a method that limits protein degradation by minimizing heat introduction to proteins. The presence of whole protein was confirmed by western blotting. Mass spectrometry was used to sequence peptides and identify isolated proteins. The data have been deposited to the ProteomeXchange with identifier PXD003215. Extracted proteins were characterized as both intra- and extracellular and had molecular weights ranging from 9.4 to 629 kDa. High correlation scores among suture protein spectral counts support the reproducibility of the method. Ontology analytics revealed proteins of myriad functions including mediators of metabolic processes and cell organelles. These results demonstrate a reproducible method for isolation of whole protein from human cranial bone, representing a large range of molecular weights, origins and functions.

摘要

人体骨骼中致密的羟基磷灰石基质限制了传统蛋白质提取方案的适用性。到目前为止,这阻碍了对人类骨骼蛋白质组的完整和准确表征,导致许多与骨骼相关的疾病仍未得到充分了解。我们试图改进一种现有的从小鼠骨骼中提取蛋白质的方法,以从人类颅骨中提取不同分子量的全蛋白。通过机械处理样品,采用一种通过尽量减少蛋白质受热来限制蛋白质降解的方法,从人类颅缝中提取全蛋白。通过蛋白质印迹法确认了全蛋白的存在。使用质谱对肽段进行测序并鉴定分离出的蛋白质。数据已存入蛋白质组交换库,标识符为PXD003215。提取的蛋白质被鉴定为细胞内和细胞外蛋白质,分子量范围为9.4至629 kDa。颅缝蛋白质光谱计数之间的高相关性得分支持了该方法的可重复性。本体分析揭示了具有多种功能的蛋白质,包括代谢过程介质和细胞器。这些结果证明了一种可重复的方法,用于从人类颅骨中分离全蛋白,这些全蛋白具有广泛的分子量、来源和功能。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/930b/5584578/3b3d9ae317fe/nihms-821758-f0001.jpg

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