机构:[1]Hubei Collaborative Innovation Center for Green Transformation of Bio-resources, Hubei Key Laboratory of Industrial Biotechnology,school of Life Sciences, Hubei University, Wuhan, 430062, China.[2]Genecreate Biological Engineering Co., Ltd., National Bio-industry Base, Wuhan, 430071, Hubei, China.[3]Department of Orthopedic Surgery, The People's Hospital of Yuxi City, The 6th Affiliated Hospital of Kunming Medical University, 21 Nieer Road, Yuxi, 653100, Yunan, China.[4]Center for Reproductive Medicine, Tongji Medical College, Huazhong University of Science and Technology, Wuhan, 430030, Hubei, China.[5]Center for Reproductive Medicine, The First Affiliated Hospital, Wenzhou Medical University, Wenzhou, 325000, China.[6]Department of Gynecology, The Tumor Hospital of Yunnan Province, The 3th Affiliated Hospital of Kunming Medical University, Kunzhou Road, Kunming, 650106, Yunan, China.[7]Department of Nephrology, Health Screening Center, The People's Hospital of Yuxi City, The 6th Affiliated Hospital of Kunming Medical University, 21 Nieer Road, Yuxi, 653100, Yunan, China.
MicroRNAs (miRNAs) bind to the 3'-untranslated region of target mRNAs in a sequence-specific manner and subsequently repress gene translation. Human miR-26a has been studied extensively, but the target transcripts are far from complete. We first employed the CRISPR-Cas9 system to generate an miR-26a-knockout line in human cervical cancer HeLa cells. The miR26a-knockout line showed increased cell growth and altered proliferation. Proteomics technology of sequential window acquisition of all theoretical mass spectra (SWATH-MS) was utilized to compare the protein abundance between the wild-type and the knockout lines, with an attempt to identify transcripts whose translation was influenced by miR-26a. Functional classification of the proteins with significant changes revealed their function in stress response, proliferation, localization, development, signaling, etc. Several proteins in the cell cycle/proliferation signaling pathway were chosen to be validated by western blot and parallel reaction monitoring (PRM). The satisfactory consistency among the three approaches indicated the reliability of the SWATH-MS quantification. Among the computationally predicted targets, a subset of the targets was directly regulated by miR-26a, as demonstrated by luciferase assays and Western blotting. This study creates an inventory of miR-26a-targeted transcripts in HeLa cells and provides fundamental knowledge to further explore the functions of miR-26a in human cancer.
基金:
National Natural Science Foundation of China (31300074 and
81760136), the Natural Science Foundation of Hubei Province (2014CFB541), the Specialized Research Fund for
the Doctoral Program of Higher Education (20124208120004), and the Science and Technology Support Program
of Hubei Province (2014BCB031).
语种:
外文
PubmedID:
中科院(CAS)分区:
出版当年[2019]版:
大类|3 区综合性期刊
小类|3 区综合性期刊
最新[2023]版:
大类|2 区综合性期刊
小类|2 区综合性期刊
第一作者:
第一作者机构:[1]Hubei Collaborative Innovation Center for Green Transformation of Bio-resources, Hubei Key Laboratory of Industrial Biotechnology,school of Life Sciences, Hubei University, Wuhan, 430062, China.[2]Genecreate Biological Engineering Co., Ltd., National Bio-industry Base, Wuhan, 430071, Hubei, China.
通讯作者:
推荐引用方式(GB/T 7714):
Shen Hexiao,Li Li,Teng Zhaowei,et al.Label-free Quantitative Analysis of Protein Expression Alterations in miR-26a-Knockout HeLa Cells using SWATH-MS Technology.[J].Scientific reports.2019,9(1):1399.doi:10.1038/s41598-018-34904-8.
APA:
Shen Hexiao,Li Li,Teng Zhaowei,Meng Tianqing,Kong Xiangbin...&Ma Lixin.(2019).Label-free Quantitative Analysis of Protein Expression Alterations in miR-26a-Knockout HeLa Cells using SWATH-MS Technology..Scientific reports,9,(1)
MLA:
Shen Hexiao,et al."Label-free Quantitative Analysis of Protein Expression Alterations in miR-26a-Knockout HeLa Cells using SWATH-MS Technology.".Scientific reports 9..1(2019):1399
