Lysine-acetylation (LysAc) and its regulatory enzymes are broadly associated with cancers. Consequently, HDAC inhibitors have been developed to modulate the LysAc status, and are currently undergoing more than 80 clinical trials as anti-tumor therapeutics. Molecular biology and genetics approaches have been attempted to characterize LysAc pathway and the anti-tumor effects of HDAC inhibitors. However, such research provides limited insight into the functions of LysAc sites and their dynamics. LysAc sites among some substrate proteins have been elegantly analyzed by a candidate approach using mass spectrometry, generating key information for downstream biological studies to establish its known functions. Nevertheless, a large number of LysAc substrate proteins and their LysAc dynamics have not been globally studied in cancer-related environments before. This knowledge gap needs to be filled to improve our understanding of LysAc in cancer and other diseases. We hypothesize that dysregulation of LysAc plays a key role in cancer progression. The long-term objective of this research plan is to comprehensively elucidate the dynamic changes of lysine acetylation in cancer, and to use this knowledge to gain a better understanding of its biological functions. We propose to study global LysAc dynamics in cancer cells by a novel, integrated proteomics approach, consisting of (i) high- resolution protein pre-fractionation, (ii) efficient purification of LysAc peptides with anti- LysAc antibodies, and (iii) identification and quantification of the LysAc peptides by SILAC combined with 1D- HPLC/MS/MS or 2D-HPLC/MS/MS. This study is anticipated to identify a large number of non-nuclear LysAc proteins and to reveal their dynamics in cancer progression, therefore challenging the current concept that regulation of DNA-templated process is the major function of the modification. Given the difficulty in identifying new LysAc substrates, the novel, comprehensive LysAc datasets established in this study will address a critical barrier in the LysAc biology field.
Specific aims of this research are: (1) To define the aberrant changes in lysine acetylation in cancer cells. LysAc will be quantified between two sets of matched normal and cancer cells, with an emphasis on quantifying LysAc with the highest possible sensitivity. (2) To identify downstream protein targets of suberoylanilide hydroxamic acid (SAHA), the first HDAC inhibitor approved for clinical application. We will quantify LysAc, with or without SAHA, in both normal (SAHA-resistant cells) and matched cancer cells (SAHA-sensitive cells). (3) To identify the lysine-acetylation protein targets for p300 acetyltransferase. We will quantify LysAc proteins among transformed cell lines, with or without expression of the active p300 to generate an atlas of p300 substrates. And (4) to analyze and disseminate LysAc datasets to research community. The novel information from this study will be analyzed by bioinformatics tools and used to construct a LysAc database, providing an infrastructure to stimulate drug development and LysAc-biology research. ? Lysine acetylation, a post-translational modification in proteins, is dysregulated in cancer development. The proposed study aims to elucidate the dynamic changes of lysine acetylation in cancer progression. The resulting knowledge can be used to understand the biological functions of the modification, to assist development of novel biomarkers for diagnosis of cancer and development of novel anti-tumor drug with high potency and better safety profile. ? ? ?

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
7R01CA126832-02
Application #
7741585
Study Section
Enabling Bioanalytical and Biophysical Technologies Study Section (EBT)
Program Officer
Li, Jerry
Project Start
2008-06-01
Project End
2013-04-30
Budget Start
2008-12-01
Budget End
2009-04-30
Support Year
2
Fiscal Year
2008
Total Cost
$261,083
Indirect Cost
Name
University of Chicago
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
005421136
City
Chicago
State
IL
Country
United States
Zip Code
60637
Huang, He; Luo, Zhouqing; Qi, Shankang et al. (2018) Landscape of the regulatory elements for lysine 2-hydroxyisobutyrylation pathway. Cell Res 28:111-125
Huang, He; Lin, Shu; Garcia, Benjamin A et al. (2015) Quantitative proteomic analysis of histone modifications. Chem Rev 115:2376-418
Chen, Yue; Colak, Gozde; Zhao, Yingming (2013) SILAC-based quantification of Sirt1-responsive lysine acetylome. Methods Mol Biol 1077:105-20
Xie, Zhongyu; Dai, Junbiao; Dai, Lunzhi et al. (2012) Lysine succinylation and lysine malonylation in histones. Mol Cell Proteomics 11:100-7
Chen, Yue; Zhao, Wenhui; Yang, Jeong Soo et al. (2012) Quantitative acetylome analysis reveals the roles of SIRT1 in regulating diverse substrates and cellular pathways. Mol Cell Proteomics 11:1048-62
Choi, Moon-Chang; Cohen, Todd J; Barrientos, Tomasa et al. (2012) A direct HDAC4-MAP kinase crosstalk activates muscle atrophy program. Mol Cell 47:122-32
Chu, Chih-Wen; Hou, Fajian; Zhang, Junmei et al. (2011) A novel acetylation of ýý-tubulin by San modulates microtubule polymerization via down-regulating tubulin incorporation. Mol Biol Cell 22:448-56
Tan, Minjia; Luo, Hao; Lee, Sangkyu et al. (2011) Identification of 67 histone marks and histone lysine crotonylation as a new type of histone modification. Cell 146:1016-28
Zhang, Zhihong; Tan, Minjia; Xie, Zhongyu et al. (2011) Identification of lysine succinylation as a new post-translational modification. Nat Chem Biol 7:58-63
Lu, Zhike; Cheng, Zhongyi; Zhao, Yingming et al. (2011) Bioinformatic analysis and post-translational modification crosstalk prediction of lysine acetylation. PLoS One 6:e28228

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