Proteomic fingerprints of damage in extracellular matrix assemblies

Proteomic fingerprints of damage in extracellular matrix assemblies

In contrast to the dynamic intracellular environment, structural extracellular matrix (ECM) proteins with half-lives measured in decades, are susceptible to accumulating damage. Whilst conventional approaches such as histology, immunohistochemistry and mass spectrometry are able to identify age- and...

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Main Authors: Alexander Eckersley, Matiss Ozols, Ronan O'Cualain, Emma-Jayne Keevill, April Foster, Suzanne Pilkington, David Knight, Christopher E.M. Griffiths, Rachel E.B. Watson, Michael J. Sherratt
Format: Article
Language:English
Published: Elsevier 2020-02-01
Series:Matrix Biology Plus
Online Access:http://www.sciencedirect.com/science/article/pii/S2590028520300089
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author Alexander Eckersley
Matiss Ozols
Ronan O'Cualain
Emma-Jayne Keevill
April Foster
Suzanne Pilkington
David Knight
Christopher E.M. Griffiths
Rachel E.B. Watson
Michael J. Sherratt
spellingShingle Alexander Eckersley
Matiss Ozols
Ronan O'Cualain
Emma-Jayne Keevill
April Foster
Suzanne Pilkington
David Knight
Christopher E.M. Griffiths
Rachel E.B. Watson
Michael J. Sherratt
Proteomic fingerprints of damage in extracellular matrix assemblies
Matrix Biology Plus
author_facet Alexander Eckersley
Matiss Ozols
Ronan O'Cualain
Emma-Jayne Keevill
April Foster
Suzanne Pilkington
David Knight
Christopher E.M. Griffiths
Rachel E.B. Watson
Michael J. Sherratt
author_sort Alexander Eckersley
title Proteomic fingerprints of damage in extracellular matrix assemblies
title_short Proteomic fingerprints of damage in extracellular matrix assemblies
title_full Proteomic fingerprints of damage in extracellular matrix assemblies
title_fullStr Proteomic fingerprints of damage in extracellular matrix assemblies
title_full_unstemmed Proteomic fingerprints of damage in extracellular matrix assemblies
title_sort proteomic fingerprints of damage in extracellular matrix assemblies
publisher Elsevier
series Matrix Biology Plus
issn 2590-0285
publishDate 2020-02-01
description In contrast to the dynamic intracellular environment, structural extracellular matrix (ECM) proteins with half-lives measured in decades, are susceptible to accumulating damage. Whilst conventional approaches such as histology, immunohistochemistry and mass spectrometry are able to identify age- and disease-related changes in protein abundance or distribution, these techniques are poorly suited to characterising molecular damage. We have previously shown that mass spectrometry can detect tissue-specific differences in the proteolytic susceptibility of protein regions within fibrillin-1 and collagen VI alpha-3. Here, we present a novel proteomic approach to detect damage-induced “peptide fingerprints” within complex multi-component ECM assemblies (fibrillin and collagen VI microfibrils) following their exposure to ultraviolet radiation (UVR) by broadband UVB or solar simulated radiation (SSR). These assemblies were chosen because, in chronically photoaged skin, fibrillin and collagen VI microfibril architectures are differentially susceptible to UVR. In this study, atomic force microscopy revealed that fibrillin microfibril ultrastructure was significantly altered by UVR exposure whereas the ultrastructure of collagen VI microfibrils was resistant. UVR-induced molecular damage was further characterised by proteolytic peptide generation with elastase followed by liquid chromatography tandem mass spectrometry (LC-MS/MS). Peptide mapping revealed that UVR exposure increased regional proteolytic susceptibility within the protein structures of fibrillin-1 and collagen VI alpha-3. This allowed the identification of UVR-induced molecular changes within these two key ECM assemblies. Additionally, similar changes were observed within protein regions of co-purifying, microfibril-associated receptors integrins αv and β1. This study demonstrates that LC-MS/MS mapping of peptides enables the characterisation of molecular post-translational damage (via direct irradiation and radiation-induced oxidative mechanisms) within a complex in vitro model system. This peptide fingerprinting approach reliably allows both the identification of UVR-induced molecular damage in and between proteins and the identification of specific protein domains with increased proteolytic susceptibility as a result of photo-denaturation. This has the potential to serve as a sensitive method of identifying accumulated molecular damage in vivo using conventional mass spectrometry data-sets. Keywords: Fibrillin microfibril, Collagen VI microfibril, Ultraviolet radiation, Photodamage, Mass spectrometry
url http://www.sciencedirect.com/science/article/pii/S2590028520300089
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spelling doaj-92276f7159764abd800a46e6ae8a6d4c2020-11-25T02:19:49ZengElsevierMatrix Biology Plus2590-02852020-02-015Proteomic fingerprints of damage in extracellular matrix assembliesAlexander Eckersley0Matiss Ozols1Ronan O'Cualain2Emma-Jayne Keevill3April Foster4Suzanne Pilkington5David Knight6Christopher E.M. Griffiths7Rachel E.B. Watson8Michael J. Sherratt9Division of Cell Matrix Biology & Regenerative Medicine, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UK; Corresponding authors at: 1.529 Stopford Building, The University of Manchester, Oxford Rd, Manchester M13 9PT, UK.Division of Cell Matrix Biology & Regenerative Medicine, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UKBiological Mass Spectrometry Core Research Facility, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UKBiological Mass Spectrometry Core Research Facility, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UKDivision of Musculoskeletal & Dermatological Sciences, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UKDivision of Musculoskeletal & Dermatological Sciences, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UKBiological Mass Spectrometry Core Research Facility, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UKDivision of Musculoskeletal & Dermatological Sciences, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UK; NIHR Manchester Biomedical Research Centre, Central Manchester University Hospitals NHS Foundation Trust, Manchester Academic Health Science Centre, Manchester, UKDivision of Musculoskeletal & Dermatological Sciences, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UK; NIHR Manchester Biomedical Research Centre, Central Manchester University Hospitals NHS Foundation Trust, Manchester Academic Health Science Centre, Manchester, UKDivision of Cell Matrix Biology & Regenerative Medicine, School of Biological Sciences, Faculty of Biology, Medicine and Health, The University of Manchester, Manchester, UK; Corresponding authors at: 1.529 Stopford Building, The University of Manchester, Oxford Rd, Manchester M13 9PT, UK.In contrast to the dynamic intracellular environment, structural extracellular matrix (ECM) proteins with half-lives measured in decades, are susceptible to accumulating damage. Whilst conventional approaches such as histology, immunohistochemistry and mass spectrometry are able to identify age- and disease-related changes in protein abundance or distribution, these techniques are poorly suited to characterising molecular damage. We have previously shown that mass spectrometry can detect tissue-specific differences in the proteolytic susceptibility of protein regions within fibrillin-1 and collagen VI alpha-3. Here, we present a novel proteomic approach to detect damage-induced “peptide fingerprints” within complex multi-component ECM assemblies (fibrillin and collagen VI microfibrils) following their exposure to ultraviolet radiation (UVR) by broadband UVB or solar simulated radiation (SSR). These assemblies were chosen because, in chronically photoaged skin, fibrillin and collagen VI microfibril architectures are differentially susceptible to UVR. In this study, atomic force microscopy revealed that fibrillin microfibril ultrastructure was significantly altered by UVR exposure whereas the ultrastructure of collagen VI microfibrils was resistant. UVR-induced molecular damage was further characterised by proteolytic peptide generation with elastase followed by liquid chromatography tandem mass spectrometry (LC-MS/MS). Peptide mapping revealed that UVR exposure increased regional proteolytic susceptibility within the protein structures of fibrillin-1 and collagen VI alpha-3. This allowed the identification of UVR-induced molecular changes within these two key ECM assemblies. Additionally, similar changes were observed within protein regions of co-purifying, microfibril-associated receptors integrins αv and β1. This study demonstrates that LC-MS/MS mapping of peptides enables the characterisation of molecular post-translational damage (via direct irradiation and radiation-induced oxidative mechanisms) within a complex in vitro model system. This peptide fingerprinting approach reliably allows both the identification of UVR-induced molecular damage in and between proteins and the identification of specific protein domains with increased proteolytic susceptibility as a result of photo-denaturation. This has the potential to serve as a sensitive method of identifying accumulated molecular damage in vivo using conventional mass spectrometry data-sets. Keywords: Fibrillin microfibril, Collagen VI microfibril, Ultraviolet radiation, Photodamage, Mass spectrometryhttp://www.sciencedirect.com/science/article/pii/S2590028520300089

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