Literature DB >> 30038347

Quantitative analysis of newly synthesized proteins.

Yuanhui Ma1, Daniel B McClatchy1, Salim Barkallah2, William W Wood2, John R Yates3.   

Abstract

Measuring proteome response to perturbations is critical for understanding the underlying mechanisms involved. Traditional quantitative proteomic methods are limited by the large numbers of proteins in the proteome and the mass spectrometer's dynamic range. A previous method uses the biorthogonal reagent azidohomoalanine (AHA), a methionine analog, for labeling, enrichment and detection of newly synthesized proteins (NSPs). Newly synthesized AHA proteins can be coupled to biotin via CuAAC-mediated click chemistry and enriched using avidin-based affinity purification. The combination of AHA-mediated NSP labeling with metabolic stable isotope labeling allows quantitation of low-abundant, newly secreted proteins by mass spectrometry (MS). However, the resulting multiplicity of labeling complicates NSP analysis. We developed a new NSP quantification strategy, called HILAQ (heavy isotope-labeled azidohomoalanine quantification), that uses a heavy isotope-labeled AHA molecule to enable NSP labeling, enrichment, identification and quantification. In addition, the AHA-peptide enrichment used in HILAQ improves both the identification and quantification of NSPs over AHA-protein enrichment. Here, we provide a description of the HILAQ method that includes procedures for (i) pulse-labeling and harvesting NSPs; (ii) addition of biotin by click reaction; (iii) protein precipitation; (iv) protein digestion; (v) enrichment of AHA-biotin peptides by NeutrAvidin beads and four-step elution; (vi) MS analysis; and (vii) data analysis for the identification and quantification of NSPs by ProLuCID and pQuant. We demonstrate our HILAQ approach by identifying NSPs from cell cultures, but we anticipate that it can be adapted for applications in animal models. The whole protocol takes ~6 d to complete.

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Year:  2018        PMID: 30038347     DOI: 10.1038/s41596-018-0012-y

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  8 in total

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Journal:  Front Mol Biosci       Date:  2022-04-27

2.  Effective Method for Accurate and Sensitive Quantitation of Rapid Changes of Newly Synthesized Proteins.

Authors:  Ming Tong; Suttipong Suttapitugsakul; Ronghu Wu
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4.  Assessment of Streptavidin Bead Binding Capacity to Improve Quality of Streptavidin-based Enrichment Studies.

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Journal:  J Proteome Res       Date:  2020-12-03       Impact factor: 5.370

5.  Fishing for newly synthesized proteins with phosphonate-handles.

Authors:  Fleur Kleinpenning; Barbara Steigenberger; Wei Wu; Albert J R Heck
Journal:  Nat Commun       Date:  2020-06-26       Impact factor: 14.919

6.  Increased expression of NAF1 contributes to malignant phenotypes of glioma cells through promoting protein synthesis and associates with poor patient survival.

Authors:  Jing Wei; Qi Yang; Jing Shi; Bingyin Shi; Meiju Ji; Peng Hou
Journal:  Oncogenesis       Date:  2019-04-01       Impact factor: 7.485

7.  Automated High-Throughput Method for the Fast, Robust, and Reproducible Enrichment of Newly Synthesized Proteins.

Authors:  David Vargas-Diaz; Maarten Altelaar
Journal:  J Proteome Res       Date:  2021-12-03       Impact factor: 4.466

8.  Quantitative analysis of global protein stability rates in tissues.

Authors:  Daniel B McClatchy; Salvador Martínez-Bartolomé; Yu Gao; Mathieu Lavallée-Adam; John R Yates
Journal:  Sci Rep       Date:  2020-09-29       Impact factor: 4.379

  8 in total

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