机构:[1]Capital Med Univ, Beijing Tian Tan Hosp, Dept Neurosurg, Beijing, Peoples R China;[2]China Natl Clin Res Ctr Neurol Dis, Beijing, Peoples R China;国家神经系统疾病临床医学研究中心国家神经系统疾病临床医学研究中心首都医科大学附属天坛医院[3]Chinese Acad Sci, Inst Genet & Dev Biol, Beijing 100864, Peoples R China
Objective. To screen differentially expressed proteins of saccular intracranial aneurysms and superficial temporal artery by the proteomics analysis using isobaric tags for relative and absolute quantification (iTRAQ) combined with reverse phase high-performance liquid chromatography. Methods. Collecting 17 samples from intracranial aneurysm patients undergoing aneurysmectomy as experiment group and 17 matched STA as control group. After quantification and enzymolysis of the protein, the iTRAQ were used to label the peptides of the 2 groups respectively. Then, the mixture of the peptides was fractioned by RP-HPLC and analyzed by LC-MS/MS to identify the differential expression proteins. Results. A total of 1699 proteins were identified from the ProteinPilot 4.5 software (AB SCIEX) using the Paragon database search algorithm. Comparing with STA, 54 proteins were significantly up-regulated (115:114 < 0.5-fold) and 37 were significantly down-regulated in sIAs (115:114 > 2.0-fold). Furthermore, Integrin beta 3, Secreted frizzled-related protein 2 were significantly up-regulated (2.3 fold and 2.1 fold, respectively), whereas MyosinIIb, Alpha-actinin-1, Laminin beta 2, and Carboxypeptidase A3 were down-regulated (3.01 fold, 2.1 fold, 2.07 fold, and 2.01 fold, respectively) in sIAs. GO Ontology analysis showed that most differential proteins expressed in cytoskeletal; up-regulated proteins in sIAs play an important role in inflammatory reaction, enzymatic hydrolysis, cell adhesion and invasion, and cellular immune reaction; down-regulated proteins in slAs involved in cytoskeletal protein, enzyme, and structural protein. ITGB3, ACTN1 and MYL2 play a role in aneurysm formation via focal adhesion pathway. The results of Western-blot assay were consistent with the proteomic changes of those 6 proteins. Conclusion. The differentially expressed proteins in slAs that showed aneurysm formation are related to cytoskeleton abnormal and extracellular matrix changes. The iTRAQ technology provides scientific foundation for the further study to explore the pathogenic mechanism of slAs. (C) 2015 Elsevier B.V. All rights reserved.
基金:
This work was conducted at Beijing Tian Tan Hospital, Capital Medical University, and Institute of Genetics and Developmental Biology, Chinese Academy of Sciences. The authors have no proprietary interest in any of the products mentioned in this manuscript.
第一作者机构:[1]Capital Med Univ, Beijing Tian Tan Hosp, Dept Neurosurg, Beijing, Peoples R China;
通讯作者:
通讯机构:[1]Capital Med Univ, Beijing Tian Tan Hosp, Dept Neurosurg, Beijing, Peoples R China;[2]China Natl Clin Res Ctr Neurol Dis, Beijing, Peoples R China;
推荐引用方式(GB/T 7714):
Wang Jia,Yu Lanbing,Huang Xiahe,et al.Comparative proteome analysis of saccular intracranial aneurysms with iTRAQ quantitative proteomics[J].JOURNAL OF PROTEOMICS.2016,130:120-128.doi:10.1016/j.jprot.2015.09.014.
APA:
Wang, Jia,Yu, Lanbing,Huang, Xiahe,Wang, Yingchun&Zhao, Jizong.(2016).Comparative proteome analysis of saccular intracranial aneurysms with iTRAQ quantitative proteomics.JOURNAL OF PROTEOMICS,130,
MLA:
Wang, Jia,et al."Comparative proteome analysis of saccular intracranial aneurysms with iTRAQ quantitative proteomics".JOURNAL OF PROTEOMICS 130.(2016):120-128
