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Data-Independent Acquisition Phosphoproteomics of Urinary Extracellular Vesicles Enables Renal Cell Carcinoma Grade Differentiation

  • Marco Hadisurya
  • , Zheng Chi Lee
  • , Zhuojun Luo
  • , Guiyuan Zhang
  • , Yajie Ding
  • , Hao Zhang
  • , Anton B. Iliuk
  • , Roberto Pili
  • , Ronald S. Boris
  • , W. Andy Tao
  • Purdue University
  • West Lafayette Junior/Senior High School
  • Southeast University, Nanjing
  • Tymora Analytical Operations
  • Indiana University Bloomington

Research output: Contribution to journalArticlepeer-review

20 Scopus citations

Abstract

Translating the research capability and knowledge in cancer signaling into clinical settings has been slow and ineffective. Recently, extracellular vesicles (EVs) have emerged as a promising source for developing disease phosphoprotein markers to monitor disease status. This study focuses on the development of a robust data-independent acquisition (DIA) using mass spectrometry to profile urinary EV phosphoproteomics for renal cell cancer (RCC) grades differentiation. We examined gas-phase fractionated library, direct DIA (library-free), forbidden zones, and several different windowing schemes. After the development of a DIA mass spectrometry method for EV phosphoproteomics, we applied the strategy to identify and quantify urinary EV phosphoproteomes from 57 individuals representing low-grade clear cell RCC, high-grade clear cell RCC, chronic kidney disease, and healthy control individuals. Urinary EVs were efficiently isolated by functional magnetic beads, and EV phosphopeptides were subsequently enriched by PolyMAC. We quantified 2584 unique phosphosites and observed that multiple prominent cancer-related pathways, such as ErbB signaling, renal cell carcinoma, and regulation of actin cytoskeleton, were only upregulated in high-grade clear cell RCC. These results show that EV phosphoproteome analysis utilizing our optimized procedure of EV isolation, phosphopeptide enrichment, and DIA method provides a powerful tool for future clinical applications.

Original languageEnglish
Article number100536
JournalMolecular and Cellular Proteomics
Volume63
Issue number4
DOIs
StatePublished - May 2023

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