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  4. Controlling localization of Escherichia coli populations using a two-part synthetic motility circuit: An accelerator and brake
 
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Controlling localization of Escherichia coli populations using a two-part synthetic motility circuit: An accelerator and brake

Journal
Biotechnology and Bioengineering
Journal Volume
114
Journal Issue
12
Pages
2883-2895
Date Issued
2017
Author(s)
McKay R
Hauk P
Wu H.-C
Pottash A.E
Shang W
Terrell J
Payne G.F
Bentley W.E.
HSUAN-CHEN WU  
DOI
10.1002/bit.26391
URI
https://www.scopus.com/inward/record.uri?eid=2-s2.0-85032023642&doi=10.1002%2fbit.26391&partnerID=40&md5=fd262769cd0c808f5efb64471c1c2921
https://scholars.lib.ntu.edu.tw/handle/123456789/573321
Abstract
Probiotics, whether taken as capsules or consumed in foods, have been regarded as safe for human use by regulatory agencies. Being living cells, they serve as “tunable” factories for the synthesis of a vast array of beneficial molecules. The idea of reprogramming probiotics to act as controllable factories, producing potential therapeutic molecules under user-specified conditions, represents a new and powerful concept in drug synthesis and delivery. Probiotics that serve as drug delivery vehicles pose several challenges, one being targeting (as seen with nanoparticle approaches). Here, we employ synthetic biology to control swimming directionality in a process referred to as “pseudotaxis.” Escherichia coli, absent the motility regulator cheZ, swim sporadically, missing the traditional “run” in the run:tumble swimming paradigm. Upon introduction of cheZ in trans and its signal-generated upregulation, engineered bacteria can be “programmed” to swim toward the source of the chemical cue. Here, engineered cells that encounter sufficient levels of the small signal molecule pyocyanin, produce an engineered CheZ and swim with programmed directionality. By incorporating a degradation tag at the C-terminus of CheZ, the cells stop running when they exit spaces containing pyocyanin. That is, the engineered CheZ modified with a C-terminal extension derived from the putative DNA-binding transcriptional regulator YbaQ (RREERAAKKVA) is consumed by the ClpXP protease machine at a rate sufficient to “brake” the cells when pyocyanin levels are too low. Through this process, we demonstrate that over time, these engineered E. coli accumulate in pyocyanin-rich locales. We suggest that such approaches may find utility in engineering probiotics so that their beneficial functions can be focused in areas of principal benefit. ? 2017 Wiley Periodicals, Inc.
Subjects
Brakes; Cells; Cytology; Escherichia coli; Industrial plants; Molecules; Timing circuits; C-terminal extensions; Drug delivery vehicles; motility; pseudotaxis; Synthetic biology; targeting; Therapeutic molecules; Transcriptional regulator; Synthesis (chemical); bacterial protein; clpxp enzyme; protein chez; proteinase; pyocyanine; transcription factor; transcriptional regulator ybaq; unclassified drug; cheZ protein, E coli; Escherichia coli protein; methyl accepting chemotaxis protein; pyocyanine; SoxS protein, E coli; transactivator protein; Article; bacterial gene; carboxy terminal sequence; cell motility; chez gene; Escherichia coli; nonhuman; chemotaxis; drug effects; Escherichia coli; gene regulatory network; genetic enhancement; genetics; physiology; procedures; synthetic biology; Chemotaxis; Escherichia coli; Escherichia coli Proteins; Gene Regulatory Networks; Genetic Enhancement; Methyl-Accepting Chemotaxis Proteins; Pyocyanine; Synthetic Biology; Trans-Activators
Type
journal article

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