Literature DB >> 22314840

Metabolism of peptide reporters in cell lysates and single cells.

Angela Proctor1, Qunzhao Wang, David S Lawrence, Nancy L Allbritton.   

Abstract

The stability of an Abl kinase substrate peptide in a cytosolic lysate and in single cells was characterized. In the cytosolic lysate, the starting peptide was metabolized at an average initial rate of 1.7 ± 0.3 zmol pg(-1) s(-1) with a t(1/2) of 1.3 min. Five different fragments formed over time; however, a dominant cleavage site was identified. Multiple rational design cycles were utilized to develop a lead peptide with a phenylalanine and alanine replaced by an (N-methyl)phenylalanine and isoleucine, respectively, to attain cytosolic peptidase resistance while maintaining Abl substrate efficacy. This lead peptide possessed a 15-fold greater lifetime in the cytosolic lysate while attaining a 7-fold improvement in k(cat) as an Abl kinase substrate compared to the starting peptide. However, when loaded into single cells, the starting peptide and lead peptide possessed nearly identical degradation rates and an altered pattern of fragmentation relative to that in cell lysates. Preferential accumulation of a fragment with cleavage at an Ala-Ala bond in single cells suggested that dissimilar peptidases act on the peptides in the lysate versus single cells. A design strategy for peptide stabilization, analogous to that demonstrated for the lysate, should be effective for stabilization in single cells.

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Year:  2012        PMID: 22314840      PMCID: PMC3697743          DOI: 10.1039/c2an16162a

Source DB:  PubMed          Journal:  Analyst        ISSN: 0003-2654            Impact factor:   4.616


  47 in total

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Review 2.  Single-cell kinase assays: opening a window onto cell behavior.

Authors:  Christopher E Sims; Nancy L Allbritton
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4.  Measurement of kinase activation in single mammalian cells.

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5.  A family of protein-cutting proteins.

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6.  Effect of N-methylation and chain length on kinetic constants of trypsin substrates. Epsilon-N-methyllysine and homolysine derivatives as substrates.

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8.  Recognition of multiple substrate motifs by the c-ABL protein tyrosine kinase.

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9.  Translocation of c-ab1 oncogene correlates with the presence of a Philadelphia chromosome in chronic myelocytic leukaemia.

Authors:  C R Bartram; A de Klein; A Hagemeijer; T van Agthoven; A Geurts van Kessel; D Bootsma; G Grosveld; M A Ferguson-Smith; T Davies; M Stone
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Authors:  Jung Hwan Lee; Sandip K Nandy; David S Lawrence
Journal:  J Am Chem Soc       Date:  2004-03-24       Impact factor: 15.419

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  17 in total

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4.  Response of single leukemic cells to peptidase inhibitor therapy across time and dose using a microfluidic device.

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5.  Development of a protease-resistant reporter to quantify BCR-ABL activity in intact cells.

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6.  Fluorescence lifetime imaging of biosensor peptide phosphorylation in single live cells.

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7.  Development of a peptidase-resistant substrate for single-cell measurement of protein kinase B activation.

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8.  Microfluidic chemical cytometry of peptide degradation in single drug-treated acute myeloid leukemia cells.

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Review 9.  Measuring activity in the ubiquitin-proteasome system: from large scale discoveries to single cells analysis.

Authors:  Adam T Melvin; Gregery S Woss; Jessica H Park; Marcey L Waters; Nancy L Allbritton
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10.  Measurement of protein tyrosine phosphatase activity in single cells by capillary electrophoresis.

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