Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions

Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions

Abstract Background The thorough understanding of the physiological and pathological processes mediated by extracellular vesicles (EVs) is challenged by purification methods which are cumbersome, not reproducible, or insufficient to yield homogeneous material. Chromatography based on both ion-exchan...

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Main Authors: Milica Popovic, Elisa Mazzega, Barbara Toffoletto, Ario de Marco
Format: Article
Language:English
Published: BMC 2018-01-01
Series:Microbial Cell Factories
Subjects:
Nanobodies
Extracellular vesicles
Panning strategy
Exosomes
Monolith chromatography
Online Access:http://link.springer.com/article/10.1186/s12934-017-0856-9
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spelling doaj-1fad06d6cb1941e68079ba6a22f4390b2020-11-25T00:39:01ZengBMCMicrobial Cell Factories1475-28592018-01-0117111310.1186/s12934-017-0856-9Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractionsMilica Popovic0Elisa Mazzega1Barbara Toffoletto2Ario de Marco3Faculty of Chemistry, Department of Biochemistry, University of BelgradeLaboratory for Environmental and Life Sciences, University of Nova GoricaAzienda Sanitaria Universitaria Integrata di Udine–Istituto di Anatomia PatologicaLaboratory for Environmental and Life Sciences, University of Nova GoricaAbstract Background The thorough understanding of the physiological and pathological processes mediated by extracellular vesicles (EVs) is challenged by purification methods which are cumbersome, not reproducible, or insufficient to yield homogeneous material. Chromatography based on both ion-exchange and immune-capture can represent an effective method to improve EV purification and successive analysis. Methods Cell culture supernatant was used as a model sample for assessing the capacity of anion-exchange chromatography to separate distinct EV fractions and to isolate nanobodies by direct panning on whole EVs to recover binders specific for the native conformation of EV-surface epitopes and suitable to develop EV immune-capture reagents. Results Anion-exchange chromatography of cell culture supernatant separated distinct protein-containing fractions and all of them were positive for CD9, a biomarker associated to some EVs. This suggested the existence of several EV fractions but did not help in separating EVs from other contaminants. We further isolated several nanobodies instrumental for implementing immune-affinity protocols. These were able to immobilize EVs from both cell culture supernatant and biological samples, to be used in ELISA, flow-cytometry, and immune-purification. Conclusions Here we report the first successful isolation of anti-EV nanobodies for the use in immunoaffinity-based EV capture by panning a phage library directly on partially purified EVs. This achievement paves the way for the application of direct EV panning for the discovery of novel antibody-vesicle surface biomarker pairs and represents the preliminary requirement for the development of selective immune-capture that, in combination with anion-exchange chromatography, can simplify the systematic stratification of EV sub-populations and their individual characterization.http://link.springer.com/article/10.1186/s12934-017-0856-9NanobodiesExtracellular vesiclesPanning strategyExosomesMonolith chromatography
collection DOAJ
language English
format Article
sources DOAJ
author Milica Popovic
Elisa Mazzega
Barbara Toffoletto
Ario de Marco
spellingShingle Milica Popovic
Elisa Mazzega
Barbara Toffoletto
Ario de Marco
Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
Microbial Cell Factories
Nanobodies
Extracellular vesicles
Panning strategy
Exosomes
Monolith chromatography
author_facet Milica Popovic
Elisa Mazzega
Barbara Toffoletto
Ario de Marco
author_sort Milica Popovic
title Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
title_short Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
title_full Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
title_fullStr Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
title_full_unstemmed Isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
title_sort isolation of anti-extra-cellular vesicle single-domain antibodies by direct panning on vesicle-enriched fractions
publisher BMC
series Microbial Cell Factories
issn 1475-2859
publishDate 2018-01-01
description Abstract Background The thorough understanding of the physiological and pathological processes mediated by extracellular vesicles (EVs) is challenged by purification methods which are cumbersome, not reproducible, or insufficient to yield homogeneous material. Chromatography based on both ion-exchange and immune-capture can represent an effective method to improve EV purification and successive analysis. Methods Cell culture supernatant was used as a model sample for assessing the capacity of anion-exchange chromatography to separate distinct EV fractions and to isolate nanobodies by direct panning on whole EVs to recover binders specific for the native conformation of EV-surface epitopes and suitable to develop EV immune-capture reagents. Results Anion-exchange chromatography of cell culture supernatant separated distinct protein-containing fractions and all of them were positive for CD9, a biomarker associated to some EVs. This suggested the existence of several EV fractions but did not help in separating EVs from other contaminants. We further isolated several nanobodies instrumental for implementing immune-affinity protocols. These were able to immobilize EVs from both cell culture supernatant and biological samples, to be used in ELISA, flow-cytometry, and immune-purification. Conclusions Here we report the first successful isolation of anti-EV nanobodies for the use in immunoaffinity-based EV capture by panning a phage library directly on partially purified EVs. This achievement paves the way for the application of direct EV panning for the discovery of novel antibody-vesicle surface biomarker pairs and represents the preliminary requirement for the development of selective immune-capture that, in combination with anion-exchange chromatography, can simplify the systematic stratification of EV sub-populations and their individual characterization.
topic Nanobodies
Extracellular vesicles
Panning strategy
Exosomes
Monolith chromatography
url http://link.springer.com/article/10.1186/s12934-017-0856-9
work_keys_str_mv AT milicapopovic isolationofantiextracellularvesiclesingledomainantibodiesbydirectpanningonvesicleenrichedfractions
AT elisamazzega isolationofantiextracellularvesiclesingledomainantibodiesbydirectpanningonvesicleenrichedfractions
AT barbaratoffoletto isolationofantiextracellularvesiclesingledomainantibodiesbydirectpanningonvesicleenrichedfractions
AT ariodemarco isolationofantiextracellularvesiclesingledomainantibodiesbydirectpanningonvesicleenrichedfractions
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