Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay

Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay

Abstract Background The split GFP assay is a well-known technology for activity-independent screening of target proteins. A superfolder GFP is split into two non-fluorescent parts, GFP11 which is fused to the target protein and GFP1-10. In the presence of both, GFP1-10 and the GFP11-tag are self-ass...

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Main Authors: Carolin Müller, Chika L. Igwe, Wolfgang Wiechert, Marco Oldiges
Format: Article
Language:English
Published: BMC 2021-09-01
Series:Microbial Cell Factories
Subjects:
Escherichia coli
Inclusion body
Fed-batch
Split GFP assay
Corynebacterium glutamicum
Signal peptide screening
Online Access:https://doi.org/10.1186/s12934-021-01672-6
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spelling doaj-6358c2e789154993bfb08083cb179b132021-10-03T11:55:42ZengBMCMicrobial Cell Factories1475-28592021-09-0120111110.1186/s12934-021-01672-6Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assayCarolin Müller0Chika L. Igwe1Wolfgang Wiechert2Marco Oldiges3Institute of Bio- and Geosciences, IBG-1: Biotechnology, Forschungszentrum Jülich GmbHInstitute of Bio- and Geosciences, IBG-1: Biotechnology, Forschungszentrum Jülich GmbHInstitute of Bio- and Geosciences, IBG-1: Biotechnology, Forschungszentrum Jülich GmbHInstitute of Bio- and Geosciences, IBG-1: Biotechnology, Forschungszentrum Jülich GmbHAbstract Background The split GFP assay is a well-known technology for activity-independent screening of target proteins. A superfolder GFP is split into two non-fluorescent parts, GFP11 which is fused to the target protein and GFP1-10. In the presence of both, GFP1-10 and the GFP11-tag are self-assembled and a functional chromophore is formed. However, it relies on the availability and quality of GFP1-10 detector protein to develop fluorescence by assembly with the GFP11-tag connected to the target protein. GFP1-10 detector protein is often produced in small scale shake flask cultivation and purified from inclusion bodies. Results The production of GFP1-10 in inclusion bodies and purification was comprehensively studied based on Escherichia coli as host. Cultivation in complex and defined medium as well as different feed strategies were tested in laboratory-scale bioreactor cultivation and a standardized process was developed providing high quantity of GFP1-10 detector protein with suitable quality. Split GFP assay was standardized to obtain robust and reliable assay results from cutinase secretion strains of Corynebacterium glutamicum with Bacillus subtilis Sec signal peptides NprE and Pel. Influencing factors from environmental conditions, such as pH and temperature were thoroughly investigated. Conclusions GFP1-10 detector protein production could be successfully scaled from shake flask to laboratory scale bioreactor. A single run yielded sufficient material for up to 385 96-well plate screening runs. The application study with cutinase secretory strains showed very high correlation between measured cutinase activity to split GFP fluorescence signal proofing applicability for larger screening studies.https://doi.org/10.1186/s12934-021-01672-6Escherichia coliInclusion bodyFed-batchSplit GFP assayCorynebacterium glutamicumSignal peptide screening
collection DOAJ
language English
format Article
sources DOAJ
author Carolin Müller
Chika L. Igwe
Wolfgang Wiechert
Marco Oldiges
spellingShingle Carolin Müller
Chika L. Igwe
Wolfgang Wiechert
Marco Oldiges
Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay
Microbial Cell Factories
Escherichia coli
Inclusion body
Fed-batch
Split GFP assay
Corynebacterium glutamicum
Signal peptide screening
author_facet Carolin Müller
Chika L. Igwe
Wolfgang Wiechert
Marco Oldiges
author_sort Carolin Müller
title Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay
title_short Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay
title_full Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay
title_fullStr Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay
title_full_unstemmed Scaling production of GFP1-10 detector protein in E. coli for secretion screening by split GFP assay
title_sort scaling production of gfp1-10 detector protein in e. coli for secretion screening by split gfp assay
publisher BMC
series Microbial Cell Factories
issn 1475-2859
publishDate 2021-09-01
description Abstract Background The split GFP assay is a well-known technology for activity-independent screening of target proteins. A superfolder GFP is split into two non-fluorescent parts, GFP11 which is fused to the target protein and GFP1-10. In the presence of both, GFP1-10 and the GFP11-tag are self-assembled and a functional chromophore is formed. However, it relies on the availability and quality of GFP1-10 detector protein to develop fluorescence by assembly with the GFP11-tag connected to the target protein. GFP1-10 detector protein is often produced in small scale shake flask cultivation and purified from inclusion bodies. Results The production of GFP1-10 in inclusion bodies and purification was comprehensively studied based on Escherichia coli as host. Cultivation in complex and defined medium as well as different feed strategies were tested in laboratory-scale bioreactor cultivation and a standardized process was developed providing high quantity of GFP1-10 detector protein with suitable quality. Split GFP assay was standardized to obtain robust and reliable assay results from cutinase secretion strains of Corynebacterium glutamicum with Bacillus subtilis Sec signal peptides NprE and Pel. Influencing factors from environmental conditions, such as pH and temperature were thoroughly investigated. Conclusions GFP1-10 detector protein production could be successfully scaled from shake flask to laboratory scale bioreactor. A single run yielded sufficient material for up to 385 96-well plate screening runs. The application study with cutinase secretory strains showed very high correlation between measured cutinase activity to split GFP fluorescence signal proofing applicability for larger screening studies.
topic Escherichia coli
Inclusion body
Fed-batch
Split GFP assay
Corynebacterium glutamicum
Signal peptide screening
url https://doi.org/10.1186/s12934-021-01672-6
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AT chikaligwe scalingproductionofgfp110detectorproteininecoliforsecretionscreeningbysplitgfpassay
AT wolfgangwiechert scalingproductionofgfp110detectorproteininecoliforsecretionscreeningbysplitgfpassay
AT marcooldiges scalingproductionofgfp110detectorproteininecoliforsecretionscreeningbysplitgfpassay
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