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Laurie Parker

Laurie Parker

· ProfessorVerified

University of Minnesota · Biochemistry, Molecular Biology, and Biophysics

Active 1909–2025

h-index26
Citations2.1k
Papers10526 last 5y
Funding$5.9M
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About

Laurie Parker, PhD, is a professor at the University of Minnesota Medical School. Her research focuses on assay development for post-translational modifications, with an emphasis on protein phosphorylation by tyrosine kinases. Her team utilizes chemical biology and proteomics techniques to develop tests that enable rapid screening for improved inhibitor drugs and to assess the effectiveness of inhibitors in order to enhance patient outcomes during cancer treatment.

Research topics

  • Biology
  • Computer Science
  • Internal medicine
  • Biochemistry
  • Cell biology
  • Chemistry
  • Medicine
  • Chromatography
  • Optics
  • Endocrinology
  • Computational biology
  • Biophysics
  • Physics
  • Database

Selected publications

  • Sorbate induces lysine sorbylation through noncanonical activities of class I HDACs to regulate the expression of inflammation genes

    Science Advances · 2025-05-30 · 4 citations

    articleOpen access

    Environmental factors may affect gene expression through epigenetic modifications of histones and transcription factors. Here, we report that cellular uptake of sorbate, a common food preservative, induces lysine sorbylation (Ksor) in mammalian cells and tissue mediated by the noncanonical activities of class I histone deacetylases (HDAC1-3). We demonstrated that HDAC1-3 catalyze sorbylation upon sorbate uptake and desorbylation in the absence of sorbate both in vitro and in cells. Sorbate uptake in mice livers significantly induced histone Ksor, correlating with decreased expressions of inflammation-response genes. Accordingly, sorbate treatment in macrophage RAW264.7 cells upon lipopolysaccharide (LPS) stimulation dose-dependently down-regulated proinflammatory gene expressions and nitric oxide production. Proteomic profiling identified RelA, a component of the NF-κB complex, and its interacting proteins as bona fide Ksor targets and sorbate treatment significantly decreased NF-κB transcriptional activities in response to LPS stimulation in RAW264.7 cells. Together, our study demonstrated a noncanonical mechanism of sorbate uptake in regulating epigenetic histone modifications and inflammatory gene expression.

  • Novel terbium-sensitizing peptide substrates for cyclin-dependent kinase 5 (CDK5) and their demonstration in luminescence kinase assays

    RSC Chemical Biology · 2025-01-01

    articleOpen accessSenior author

    Novel time-resolved terbium luminescence assays were developed for CDK5 and CDK2 by designing synthetic substrates which incorporate phospho-inducible terbium sensitizing motifs with kinase substrate consensus sequences. A substrate designed for CDK5 showed no phosphorylation by CDK2, opening the possibility for CDK5-specific assay development for selective drug discovery.

  • Novel approach to exploring protease activity and targets in HIV-associated obstructive lung disease using combined proteomic-peptidomic analysis

    Respiratory Research · 2024-09-10 · 1 citations

    articleOpen access

    BACKGROUND: Obstructive lung disease (OLD) is increasingly prevalent among persons living with HIV (PLWH). However, the role of proteases in HIV-associated OLD remains unclear. METHODS: We combined proteomics and peptidomics to comprehensively characterize protease activities. We combined mass spectrometry (MS) analysis on bronchoalveolar lavage fluid (BALF) peptides and proteins from PLWH with OLD (n = 25) and without OLD (n = 26) with a targeted Somascan aptamer-based proteomic approach to quantify individual proteases and assess their correlation with lung function. Endogenous peptidomics mapped peptides to native proteins to identify substrates of protease activity. Using the MEROPS database, we identified candidate proteases linked to peptide generation based on binding site affinities which were assessed via z-scores. We used t-tests to compare average forced expiratory volume in 1 s per predicted value (FEV1pp) between samples with and without detection of each cleaved protein and adjusted for multiple comparisons by controlling the false discovery rate (FDR). FINDINGS: We identified 101 proteases, of which 95 had functional network associations and 22 correlated with FEV1pp. These included cathepsins, metalloproteinases (MMP), caspases and neutrophil elastase. We discovered 31 proteins subject to proteolytic cleavage that associate with FEV1pp, with the top pathways involved in small ubiquitin-like modifier mediated modification (SUMOylation). Proteases linked to protein cleavage included neutrophil elastase, granzyme, and cathepsin D. INTERPRETATIONS: In HIV-associated OLD, a significant number of proteases are up-regulated, many of which are involved in protein degradation. These proteases degrade proteins involved in cell cycle and protein stability, thereby disrupting critical biological functions.

  • The lung proteome in HIV-associated obstructive lung disease

    ERJ Open Research · 2024-09-27 · 2 citations

    articleOpen access

    Rationale Obstructive lung disease is increasingly common among persons living with HIV (PLWH). There are currently no validated biomarkers that identify individuals at risk of developing obstructive lung disease (OLD), and specific mechanisms contributing to HIV-associated OLD remain elusive, independent of smoking. We sought to identify biomarkers and biological pathways associated with OLD using a broad proteomic approach. Methods We performed tandem mass tagging and mass spectrometry (MS) analysis on bronchoalveolar lavage fluid samples from persons living with HIV with OLD (n=26) and without OLD (n=26). We combined untargeted MS with a targeted SomaScan aptamer-based approach. We used Pearson correlation tests to identify associations between each protein and lung function (forced expiratory volume in 1 s (FEV 1 ) % pred). We adjusted for multiple comparisons using a false discovery rate adjustment. Significant proteins were entered into a pathway over-representation analysis. Protein-driven endotypes were constructed using K-means clustering. Measurements and main results We identified over 3800 proteins by MS and identified 254 proteins that correlated with FEV 1 % pred when we combined the MS and SomaScan proteomes when adjusting for smoking status. Pathway analysis revealed cell adhesion molecules as significant. Conclusions Protein expression differs in the lung of PLWH and decreased lung function (FEV 1 % pred). Pathway analysis reveals cell adhesion molecules having potentially important roles in this process.

  • Novel Approach to Exploring Protease Activity and Targets in Hiv-Associated Obstructive Lung Disease Using Combined Proteomic-Peptidomic Analysis

    SSRN Electronic Journal · 2024-01-01

    preprintOpen access
  • Antibody-free time-resolved terbium luminescence assays designed for cyclin-dependent kinase 5 (CDK5)

    bioRxiv (Cold Spring Harbor Laboratory) · 2024-04-24

    preprintOpen accessSenior authorCorresponding

    Novel time-resolved terbium luminescence assays were developed for CDK5 and CDK2 by designing synthetic substrates which incorporate phospho-inducible terbium sensitizing motifs with kinase substrate consensus sequences. Substrates designed for CDK5 showed no phosphorylation by CDK2, opening the possibility for CDK5-specific assay development for selective drug discovery.

  • Novel Approach to Exploring Protease Activity and Targets in HIV-associated Obstructive Lung Disease using Combined Proteomic-Peptidomic Analysis

    Research Square · 2024-06-04

    preprintOpen access
  • Additional file 1 of An optimized workflow for MS-based quantitative proteomics of challenging clinical bronchoalveolar lavage fluid (BALF) samples

    Figshare · 2023-01-01

    datasetOpen access

    Additional file 1: Figure S1. Representative spectra of contamination results; precipitation vs. S-traps.

  • Additional file 2 of An optimized workflow for MS-based quantitative proteomics of challenging clinical bronchoalveolar lavage fluid (BALF) samples

    Figshare · 2023-01-01

    datasetOpen access

    Additional file 2: Table S1. Protein and peptide yield at each step of the BALF processing workflow for 45 individual BALF samples.

  • Additional file 5 of An optimized workflow for MS-based quantitative proteomics of challenging clinical bronchoalveolar lavage fluid (BALF) samples

    Figshare · 2023-01-01

    datasetOpen access

    Additional file 5: Table S4. Quantitative protein and peptide identification across one TMT 16-plex group, comparing microfractionated vs. unfractionated analysis.

Recent grants

Frequent coauthors

  • Nur P. Damayanti

    40 shared
  • Joseph Irudayaraj

    University of Illinois Urbana-Champaign

    38 shared
  • Sampreeti Jena

    35 shared
  • Jackie Tan

    University of Minnesota System

    33 shared
  • Erica D. Pratt

    University of Minnesota

    32 shared
  • Christine Wendt

    VA Ann Arbor Healthcare System

    21 shared
  • Andrew M. Lipchik

    Eugene Applebaum College of Pharmacy and Health Sciences

    20 shared
  • C. Caroline O’Hare

    Weatherford (Norway)

    20 shared

Education

  • PhD, Chemistry

    University of Glasgow

    2003
  • B.A., Chemistry

    University of St. Thomas

    2000

Awards & honors

  • Dr. James E. Rubin Medical Memorial Award
  • Graduating Medical Student Research Award
  • Veneziale-Steer Award
  • Dr. Marvin and Hadassah Bacaner Research Awards
  • Schmidt Steer Award
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