A Library of Phosphoproteomic and Chromatin Signatures for Characterizing Cellular Responses to Drug Perturbations

染色质 细胞生物学 磷酸蛋白质组学 计算生物学 生物 组蛋白 核小体 化学 蛋白质组学 转录因子 磷酸化 表观遗传学 蛋白质组
作者
Lev Litichevskiy,Ryan Peckner,Jennifer G. Abelin,Jacob K. Asiedu,Amanda L. Creech,John F. Davis,Desiree Davison,Caitlin M. Dunning,Jarrett D. Egertson,Shawn Egri,Joshua Gould,Tak Ko,Sarah A. Johnson,David L. Lahr,Daniel D. Lam,Zihan Liu,Nicholas J. Lyons,Xiaodong Lu,Brendan MacLean,Alison E. Mungenast,Adam Officer,Ted Natoli,Malvina Papanastasiou,Jinal Patel,Vagisha Sharma,Courtney Toder,Andrew A. Tubelli,Jennie Z. Young,Steven A. Carr,Todd R. Golub,Aravind Subramanian,Michael J. MacCoss,Li-Huei Tsai,Jacob D. Jaffe
出处
期刊:bioRxiv 卷期号:: 185918-
标识
DOI:10.1101/185918
摘要

Though the added value of proteomic measurements to gene expression profiling has been demonstrated, profiling of gene expression on its own remains the dominant means of understanding cellular responses to perturbation. Direct protein measurements are typically limited due to issues of cost and scale; however, the recent development of high-throughput, targeted sentinel mass spectrometry assays provides an opportunity for proteomics to contribute at a meaningful scale in high-value areas for drug development. To demonstrate the feasibility of a systematic and comprehensive library of perturbational proteomic signatures, we profiled 90 drugs (in triplicate) in six cell lines using two different proteomic assays -- one measuring global changes of epigenetic marks on histone proteins and another measuring a set of peptides reporting on the phosphoproteome -- for a total of more than 3,400 samples. This effort represents a first-of-its-kind resource for proteomics. The majority of tested drugs generated reproducible responses in both phosphosignaling and chromatin states, but we observed differences in the responses that were cell line- and assay-specific. We formalized the process of comparing response signatures within the data using a concept called connectivity, which enabled us to integrate data across cell types and assays. Furthermore, it facilitated incorporation of transcriptional signatures. Consistent connectivity among cell types revealed cellular responses that transcended cell-specific effects, while consistent connectivity among assays revealed unexpected associations between drugs that were confirmed by experimental follow-up. We further demonstrated how the resource could be leveraged against public domain external datasets to recognize therapeutic hypotheses that are consistent with ongoing clinical trials for the treatment of multiple myeloma and acute lymphocytic leukemia (ALL). These data are available for download via the Gene Expression Omnibus (accession GSE101406), and web apps for interacting with this resource are available at https://clue.io/proteomics.
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