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Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum

Extracellular microvesicles are membranous nano-sized cellular organelles secreted by a variety of cells under normal and pathological conditions and heterogeneous in size ranging from 30 nm to 1 μm. They carry functional microRNAs that can influence immunity and development. For a particular applic...

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Autores principales: Maburutse, Brighton E., Park, Mi-Ri, Oh, Sangnam, Kim, Younghoon
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Korean Society for Food Science of Animal Resources 2017
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5686323/
https://www.ncbi.nlm.nih.gov/pubmed/29147088
http://dx.doi.org/10.5851/kosfa.2017.37.5.654
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author Maburutse, Brighton E.
Park, Mi-Ri
Oh, Sangnam
Kim, Younghoon
author_facet Maburutse, Brighton E.
Park, Mi-Ri
Oh, Sangnam
Kim, Younghoon
author_sort Maburutse, Brighton E.
collection PubMed
description Extracellular microvesicles are membranous nano-sized cellular organelles secreted by a variety of cells under normal and pathological conditions and heterogeneous in size ranging from 30 nm to 1 μm. They carry functional microRNAs that can influence immunity and development. For a particular application of microvesicles, choice of isolation method is particularly important; however, their isolation methods from colostrum in particular have not been described clearly. In this work, differential ultracentrifugation as a conventional method, ultracentrifugation with some modification such as additional precipitations, ultrafiltration, sucrose gradient separation and ExoQuick™ as a commercial reagent were compared. The goal was to compare mainly microvesicular total microRNA yield, distribution and purity among the methods then select the best isolation method for bovine colostrum microvesicles based largely on microRNA yield with the view of applying the vesicles in work where vesicular micro-RNA cargo is the target bioactive component. Highest yields for vesicular microRNA were obtained using conventional methods and among them, subsequent ultracentrifugation with 100,000 g and 135,000 g conventional method 2 was selected as it had the highest RNA to protein ratio indicating that it pelleted the least protein in relation to RNA an important factor for in vivo applications to assess microvesicle functionalities without risk of contaminating non-vesicular biomaterial. Microvesicles isolated using conventional method 2 were successfully internalized by cells in vitro showing their potential to deliver their cargo into cells in vitro and in vivo in case of functional studies.
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spelling pubmed-56863232017-11-16 Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum Maburutse, Brighton E. Park, Mi-Ri Oh, Sangnam Kim, Younghoon Korean J Food Sci Anim Resour Article Extracellular microvesicles are membranous nano-sized cellular organelles secreted by a variety of cells under normal and pathological conditions and heterogeneous in size ranging from 30 nm to 1 μm. They carry functional microRNAs that can influence immunity and development. For a particular application of microvesicles, choice of isolation method is particularly important; however, their isolation methods from colostrum in particular have not been described clearly. In this work, differential ultracentrifugation as a conventional method, ultracentrifugation with some modification such as additional precipitations, ultrafiltration, sucrose gradient separation and ExoQuick™ as a commercial reagent were compared. The goal was to compare mainly microvesicular total microRNA yield, distribution and purity among the methods then select the best isolation method for bovine colostrum microvesicles based largely on microRNA yield with the view of applying the vesicles in work where vesicular micro-RNA cargo is the target bioactive component. Highest yields for vesicular microRNA were obtained using conventional methods and among them, subsequent ultracentrifugation with 100,000 g and 135,000 g conventional method 2 was selected as it had the highest RNA to protein ratio indicating that it pelleted the least protein in relation to RNA an important factor for in vivo applications to assess microvesicle functionalities without risk of contaminating non-vesicular biomaterial. Microvesicles isolated using conventional method 2 were successfully internalized by cells in vitro showing their potential to deliver their cargo into cells in vitro and in vivo in case of functional studies. Korean Society for Food Science of Animal Resources 2017 2017-10-31 /pmc/articles/PMC5686323/ /pubmed/29147088 http://dx.doi.org/10.5851/kosfa.2017.37.5.654 Text en Copyright © 2017, Korean Society for Food Science of Animal Resources http://creativecommons.org/licences/by-nc/3.0 This is an open access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licences/by-nc/3.0) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Article
Maburutse, Brighton E.
Park, Mi-Ri
Oh, Sangnam
Kim, Younghoon
Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum
title Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum
title_full Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum
title_fullStr Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum
title_full_unstemmed Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum
title_short Evaluation and Characterization of Milk-derived Microvescicle Isolated from Bovine Colostrum
title_sort evaluation and characterization of milk-derived microvescicle isolated from bovine colostrum
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5686323/
https://www.ncbi.nlm.nih.gov/pubmed/29147088
http://dx.doi.org/10.5851/kosfa.2017.37.5.654
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