A stepwise approach for the reproducible optimization of PAMO expression in Escherichia coli for whole-cell biocatalysis

Edwin van Bloois; Hanna M. Dudek; Wouter A. Duetz; Marco W. Fraaije

doi:10.1186/1472-6750-12-31

A stepwise approach for the reproducible optimization of PAMO expression in Escherichia coli for whole-cell biocatalysis

Edwin van Bloois, Hanna M. Dudek, Wouter A. Duetz, Marco W. Fraaije^*

^*Corresponding author for this work

Biotechnology

Research output: Contribution to journal › Article › Academic › peer-review

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Abstract

Background: Baeyer-Villiger monooxygenases (BVMOs) represent a group of enzymes of considerable biotechnological relevance as illustrated by their growing use as biocatalyst in a variety of synthetic applications. However, due to their increased use the reproducible expression of BVMOs and other biotechnologically relevant enzymes has become a pressing matter while knowledge about the factors governing their reproducible expression is scattered.

Results: Here, we have used phenylacetone monooxygenase (PAMO) from Thermobifida fusca, a prototype Type I BVMO, as a model enzyme to develop a stepwise strategy to optimize the biotransformation performance of recombinant E. coli expressing PAMO in 96-well microtiter plates in a reproducible fashion. Using this system, the best expression conditions of PAMO were investigated first, including different host strains, temperature as well as time and induction period for PAMO expression. This optimized system was used next to improve biotransformation conditions, the PAMO-catalyzed conversion of phenylacetone, by evaluating the best electron donor, substrate concentration, and the temperature and length of biotransformation. Combining all optimized parameters resulted in a more than four-fold enhancement of the biocatalytic performance and, importantly, this was highly reproducible as indicated by the relative standard deviation of 1% for non-washed cells and 3% for washed cells. Furthermore, the optimized procedure was successfully adapted for activity-based mutant screening.

Conclusions: Our optimized procedure, which provides a comprehensive overview of the key factors influencing the reproducible expression and performance of a biocatalyst, is expected to form a rational basis for the optimization of miniaturized biotransformations and for the design of novel activity-based screening procedures suitable for BVMOs and other NAD(P)H-dependent enzymes as well.

Original language	English
Article number	31
Pages (from-to)	31-1-31-10
Number of pages	10
Journal	BMC Biotechnology
Volume	12
Issue number	1
DOIs	https://doi.org/10.1186/1472-6750-12-31
Publication status	Published - 21-Jun-2012

Keywords

Baeyer-Villiger monoxygenase
Escherichia coli
Biocatalysis
Square deep-well microtiter plates
Screening
BAEYER-VILLIGER MONOOXYGENASES
CATALYZED LACTONE SYNTHESIS
PHENYLACETONE-MONOOXYGENASE
CYCLOHEXANONE MONOOXYGENASE
KINETIC RESOLUTION
THERMOBIFIDA-FUSCA
OXIDATIONS
OVEREXPRESSION
REGENERATION
PYRUVATE

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@article{3ab0d1e028d54572a4ce7a1bcba3c67d,

title = "A stepwise approach for the reproducible optimization of PAMO expression in Escherichia coli for whole-cell biocatalysis",

abstract = "Background: Baeyer-Villiger monooxygenases (BVMOs) represent a group of enzymes of considerable biotechnological relevance as illustrated by their growing use as biocatalyst in a variety of synthetic applications. However, due to their increased use the reproducible expression of BVMOs and other biotechnologically relevant enzymes has become a pressing matter while knowledge about the factors governing their reproducible expression is scattered.Results: Here, we have used phenylacetone monooxygenase (PAMO) from Thermobifida fusca, a prototype Type I BVMO, as a model enzyme to develop a stepwise strategy to optimize the biotransformation performance of recombinant E. coli expressing PAMO in 96-well microtiter plates in a reproducible fashion. Using this system, the best expression conditions of PAMO were investigated first, including different host strains, temperature as well as time and induction period for PAMO expression. This optimized system was used next to improve biotransformation conditions, the PAMO-catalyzed conversion of phenylacetone, by evaluating the best electron donor, substrate concentration, and the temperature and length of biotransformation. Combining all optimized parameters resulted in a more than four-fold enhancement of the biocatalytic performance and, importantly, this was highly reproducible as indicated by the relative standard deviation of 1% for non-washed cells and 3% for washed cells. Furthermore, the optimized procedure was successfully adapted for activity-based mutant screening.Conclusions: Our optimized procedure, which provides a comprehensive overview of the key factors influencing the reproducible expression and performance of a biocatalyst, is expected to form a rational basis for the optimization of miniaturized biotransformations and for the design of novel activity-based screening procedures suitable for BVMOs and other NAD(P)H-dependent enzymes as well.",

keywords = "Baeyer-Villiger monoxygenase, Escherichia coli, Biocatalysis, Square deep-well microtiter plates, Screening, BAEYER-VILLIGER MONOOXYGENASES, CATALYZED LACTONE SYNTHESIS, PHENYLACETONE-MONOOXYGENASE, CYCLOHEXANONE MONOOXYGENASE, KINETIC RESOLUTION, THERMOBIFIDA-FUSCA, OXIDATIONS, OVEREXPRESSION, REGENERATION, PYRUVATE",

author = "{van Bloois}, Edwin and Dudek, {Hanna M.} and Duetz, {Wouter A.} and Fraaije, {Marco W.}",

year = "2012",

month = jun,

day = "21",

doi = "10.1186/1472-6750-12-31",

language = "English",

volume = "12",

pages = "31--1--31--10",

journal = "BMC Biotechnology",

issn = "1472-6750",

publisher = "BMC",

number = "1",

}

TY - JOUR

T1 - A stepwise approach for the reproducible optimization of PAMO expression in Escherichia coli for whole-cell biocatalysis

AU - van Bloois, Edwin

AU - Dudek, Hanna M.

AU - Duetz, Wouter A.

AU - Fraaije, Marco W.

PY - 2012/6/21

Y1 - 2012/6/21

N2 - Background: Baeyer-Villiger monooxygenases (BVMOs) represent a group of enzymes of considerable biotechnological relevance as illustrated by their growing use as biocatalyst in a variety of synthetic applications. However, due to their increased use the reproducible expression of BVMOs and other biotechnologically relevant enzymes has become a pressing matter while knowledge about the factors governing their reproducible expression is scattered.Results: Here, we have used phenylacetone monooxygenase (PAMO) from Thermobifida fusca, a prototype Type I BVMO, as a model enzyme to develop a stepwise strategy to optimize the biotransformation performance of recombinant E. coli expressing PAMO in 96-well microtiter plates in a reproducible fashion. Using this system, the best expression conditions of PAMO were investigated first, including different host strains, temperature as well as time and induction period for PAMO expression. This optimized system was used next to improve biotransformation conditions, the PAMO-catalyzed conversion of phenylacetone, by evaluating the best electron donor, substrate concentration, and the temperature and length of biotransformation. Combining all optimized parameters resulted in a more than four-fold enhancement of the biocatalytic performance and, importantly, this was highly reproducible as indicated by the relative standard deviation of 1% for non-washed cells and 3% for washed cells. Furthermore, the optimized procedure was successfully adapted for activity-based mutant screening.Conclusions: Our optimized procedure, which provides a comprehensive overview of the key factors influencing the reproducible expression and performance of a biocatalyst, is expected to form a rational basis for the optimization of miniaturized biotransformations and for the design of novel activity-based screening procedures suitable for BVMOs and other NAD(P)H-dependent enzymes as well.

AB - Background: Baeyer-Villiger monooxygenases (BVMOs) represent a group of enzymes of considerable biotechnological relevance as illustrated by their growing use as biocatalyst in a variety of synthetic applications. However, due to their increased use the reproducible expression of BVMOs and other biotechnologically relevant enzymes has become a pressing matter while knowledge about the factors governing their reproducible expression is scattered.Results: Here, we have used phenylacetone monooxygenase (PAMO) from Thermobifida fusca, a prototype Type I BVMO, as a model enzyme to develop a stepwise strategy to optimize the biotransformation performance of recombinant E. coli expressing PAMO in 96-well microtiter plates in a reproducible fashion. Using this system, the best expression conditions of PAMO were investigated first, including different host strains, temperature as well as time and induction period for PAMO expression. This optimized system was used next to improve biotransformation conditions, the PAMO-catalyzed conversion of phenylacetone, by evaluating the best electron donor, substrate concentration, and the temperature and length of biotransformation. Combining all optimized parameters resulted in a more than four-fold enhancement of the biocatalytic performance and, importantly, this was highly reproducible as indicated by the relative standard deviation of 1% for non-washed cells and 3% for washed cells. Furthermore, the optimized procedure was successfully adapted for activity-based mutant screening.Conclusions: Our optimized procedure, which provides a comprehensive overview of the key factors influencing the reproducible expression and performance of a biocatalyst, is expected to form a rational basis for the optimization of miniaturized biotransformations and for the design of novel activity-based screening procedures suitable for BVMOs and other NAD(P)H-dependent enzymes as well.

KW - Baeyer-Villiger monoxygenase

KW - Escherichia coli

KW - Biocatalysis

KW - Square deep-well microtiter plates

KW - Screening

KW - BAEYER-VILLIGER MONOOXYGENASES

KW - CATALYZED LACTONE SYNTHESIS

KW - PHENYLACETONE-MONOOXYGENASE

KW - CYCLOHEXANONE MONOOXYGENASE

KW - KINETIC RESOLUTION

KW - THERMOBIFIDA-FUSCA

KW - OXIDATIONS

KW - OVEREXPRESSION

KW - REGENERATION

KW - PYRUVATE

U2 - 10.1186/1472-6750-12-31

DO - 10.1186/1472-6750-12-31

M3 - Article

SN - 1472-6750

VL - 12

SP - 31-1-31-10

JO - BMC Biotechnology

JF - BMC Biotechnology

IS - 1

M1 - 31

ER -

A stepwise approach for the reproducible optimization of PAMO expression in Escherichia coli for whole-cell biocatalysis

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Keywords

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