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Featured researches published by Jeffrey A. Dietrich.


Annual Review of Biochemistry | 2010

High-Throughput Metabolic Engineering: Advances in Small-Molecule Screening and Selection

Jeffrey A. Dietrich; Adrienne E. McKee; Jay D. Keasling

Metabolic engineering for the overproduction of high-value small molecules is dependent upon techniques in directed evolution to improve production titers. The majority of small molecules targeted for overproduction are inconspicuous and cannot be readily obtained by screening. We provide a review on the development of high-throughput colorimetric, fluorescent, and growth-coupled screening techniques, enabling inconspicuous small-molecule detection. We first outline constraints on throughput imposed during the standard directed evolution workflow (library construction, transformation, and screening) and establish a screening and selection ladder on the basis of small-molecule assay throughput and sensitivity. An in-depth analysis of demonstrated screening and selection approaches for small-molecule detection is provided. Particular focus is placed on in vivo biosensor-based detection methods that reduce or eliminate in vitro assay manipulations and increase throughput. We conclude by providing our prospectus for the future, focusing on transcription factor-based detection systems as a natural microbial mode of small-molecule detection.


Chemistry & Biology | 2008

Redesigning enzymes based on adaptive evolution for optimal function in synthetic metabolic pathways

Yasuo Yoshikuni; Jeffrey A. Dietrich; Farnaz Nowroozi; Patricia C. Babbitt; Jay D. Keasling

Nature has balanced most metabolic pathways such that no one enzyme in the pathway controls the flux through that pathway. However, unnatural or nonnative, constructed metabolic pathways may have limited product flux due to unfavorable in vivo properties of one or more enzymes in the pathway. One such example is the mevalonate-based isoprenoid biosynthetic pathway that we previously reconstructed in Escherichia coli. We have used a probable mechanism of adaptive evolution to engineer the in vivo properties of two enzymes (3-hydroxy-3-methylglutaryl-CoA reductase [tHMGR] and many terpene synthases) in this pathway and thereby eliminate or minimize the bottleneck created by these inefficient or nonfunctional enzymes. Here, we demonstrate how we significantly improved the productivity (by approximately 1000 fold) of this reconstructed biosynthetic pathway using this strategy. We anticipate that this strategy will find broad applicability in the functional construction (or reconstruction) of biological pathways in heterologous hosts.


Microbial Cell Factories | 2012

Manipulation of the carbon storage regulator system for metabolite remodeling and biofuel production in Escherichia coli

Adrienne E. McKee; Becky J. Rutherford; Dylan Chivian; Edward K Baidoo; Darmawi Juminaga; Dwight Kuo; Peter I. Benke; Jeffrey A. Dietrich; Suzanne M. Ma; Adam P. Arkin; Christopher J. Petzold; Paul D. Adams; Jay D. Keasling; Swapnil R. Chhabra

BackgroundMicrobial engineering strategies that elicit global metabolic perturbations have the capacity to increase organism robustness for targeted metabolite production. In particular, perturbations to regulators of cellular systems that impact glycolysis and amino acid production while simultaneously decreasing fermentation by-products such as acetate and CO2 make ideal targets. Intriguingly, perturbation of the Carbon Storage Regulator (Csr) system has been previously implicated in large changes in central carbon metabolism in E. coli. Therefore, we hypothesized that perturbation of the Csr system through the CsrA-CsrB ribonucleoprotein complex might increase production of biofuels and their intermediates from heterologous pathways.ResultsWe engaged the CsrA-CsrB ribonucleoprotein complex of E. coli via overexpression of CsrB. CsrB is a 350-nucleotide non-coding RNA that antagonizes CsrA, an RNA-binding protein that regulates translation of specific mRNA targets. By using shotgun proteomics and targeted metabolomics we established that elevation of CsrB levels leads to alterations in metabolite and protein levels in glycolysis, the TCA cycle and amino acid levels. Consequently, we show that such changes can be suitably applied to improve the production of desired compounds through the native fatty acid and heterologous n-butanol and isoprenoid pathways by up to two-fold. We also observed concomitant decreases in undesirable fermentation by-products such as acetate and CO2.ConclusionsWe have demonstrated that simple engineering of the RNA-based Csr global regulatory system constitutes a novel approach to obtaining pathway-independent improvements within engineered hosts. Additionally, since Csr is conserved across most prokaryotic species, this approach may also be amenable to a wide variety of production hosts.


ACS Synthetic Biology | 2013

Transcription Factor-Based Screens and Synthetic Selections for Microbial Small-Molecule Biosynthesis

Jeffrey A. Dietrich; David L. Shis; Azadeh Alikhani; Jay D. Keasling


Archive | 2013

Host Cells and Methods for Producing Diacid Compounds

Eric J. Steen; Jeffrey L. Fortman; Jeffrey A. Dietrich; Jay D. Keasling


Archive | 2007

ARTEMISINIC EPOXIDE AND METHODS FOR PRODUCING SAME

Jeffrey A. Dietrich; Yasuo Yoshikuni; Jay D. Keasling; Michelle Chia-Yu Chang


Archive | 2008

Methods of generating protein variants

Jay D. Keasling; Yasuo Yoshikuni; Jeffrey A. Dietrich; Farnaz Nowroozi; Patricia C. Babbitt


Archive | 2013

Recombinant host cells for the production of malonate

Jeffrey A. Dietrich; Jeffrey L. Fortman; Eric J. Steen


Archive | 2012

TRANSCRIPTION FACTOR-BASED BIOSENSORS FOR DETECTING DICARBOXYLIC ACIDS

Jeffrey A. Dietrich; Jay D. Keasling


Archive | 2010

Novel transcription factor-based biosensor

Jeffrey A. Dietrich; Jay D. Keasling

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Adrienne E. McKee

Lawrence Berkeley National Laboratory

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Eric J. Steen

Lawrence Berkeley National Laboratory

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Adam P. Arkin

Lawrence Berkeley National Laboratory

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