Synthetic Biology: engineering complexity and refactoring cell capabilities

Editorial

21 August 2015

Editorial – Synthetic Biology: Engineering Complexity and Refactoring Cell Capabilities

Francesca Ceroni

Pablo Carbonell

Jean-Marie François

and

Karmella A. Haynes

7,429 views

6 citations

Editors

Francesca Ceroni

Imperial College London

Karmella Ann Haynes

Arizona State University

Pablo Carbonell

Universitat Politècnica de València

Jean Marie François

Institut Biotechnologique de Toulouse (INSA)

Impact

Example of a Boolean signal with values that cannot be perfectly distinguished: (A,B) show histograms for 50,000 cells sampled from typical distributions for Boolean true and false states, respectively. These distributions overlap, however, and in the overlapping range it is difficult or impossible to distinguish between true and false values.

Original Research

30 June 2015

Signal-to-Noise Ratio Measures Efficacy of Biological Computing Devices and Circuits

Jacob Beal

11,837 views

23 citations

Original Research

08 April 2015

A Sense of Balance: Experimental Investigation and Modeling of a Malonyl-CoA Sensor in Escherichia coli

Tamás Fehér

, 2 more and

Jean-Loup Faulon

11,033 views

11 citations

Review

10 March 2015

Can the Natural Diversity of Quorum-Sensing Advance Synthetic Biology?

René Michele Davis

, 1 more and

Karmella Ann Haynes

15,652 views

56 citations

Original Research

28 October 2014

New Transposon Tools Tailored for Metabolic Engineering of Gram-Negative Microbial Cell Factories

Esteban Martínez-García

, 2 more and

Pablo I. Nikel

Re-programming microorganisms to modify their existing functions and/or to bestow bacteria with entirely new-to-Nature tasks have largely relied so far on specialized molecular biology tools. Such endeavors are not only relevant in the burgeoning metabolic engineering arena but also instrumental to explore the functioning of complex regulatory networks from a fundamental point of view. À la carte modification of bacterial genomes thus calls for novel tools to make genetic manipulations easier. We propose the use of a series of new broad-host-range mini-Tn5-vectors, termed pBAMDs, for the delivery of gene(s) into the chromosome of Gram-negative bacteria and for generating saturated mutagenesis libraries in gene function studies. These delivery vectors endow the user with the possibility of easy cloning and subsequent insertion of functional cargoes with three different antibiotic-resistance markers (kanamycin, streptomycin, and gentamicin). After validating the pBAMD vectors in the environmental bacterium Pseudomonas putida KT2440, their use was also illustrated by inserting the entire poly(3-hydroxybutyrate) (PHB) synthesis pathway from Cupriavidus necator in the chromosome of a phosphotransacetylase mutant of Escherichia coli. PHB is a completely biodegradable polyester with a number of industrial applications that make it attractive as a potential replacement of oil-based plastics. The non-selective nature of chromosomal insertions of the biosynthetic genes was evidenced by a large landscape of PHB synthesis levels in independent clones. One clone was selected and further characterized as a microbial cell factory for PHB accumulation, and it achieved polymer accumulation levels comparable to those of a plasmid-bearing recombinant. Taken together, our results demonstrate that the new mini-Tn5-vectors can be used to confer interesting phenotypes in Gram-negative bacteria that would be very difficult to engineer through direct manipulation of the structural genes.

18,044 views

114 citations

Challenges of lignocellulose conversion. Lignocellulose regularly needs pretreatment to release its sugar components for biocatalysts to make fuels and chemicals. This is a sustainable approach to reduce our dependence on petroleum and to prevent carbon dioxide emission. At least three major challenges remain to be solved for a cost-effective lignocellulose conversion.

Review

18 February 2015

Engineering Sugar Utilization and Microbial Tolerance toward Lignocellulose Conversion

Lizbeth M. Nieves

, 1 more and

Xuan Wang

8,680 views

57 citations

Original Research

20 August 2014

Optimization of the IPP Precursor Supply for the Production of Lycopene, Decaprenoxanthin and Astaxanthin by Corynebacterium glutamicum

Sabine A. E. Heider

, 3 more and

Volker F. Wendisch

Scheme of the MEP pathway (A) and of decaprenoxanthin biosynthesis in C. glutamicum (B) with heterologous astaxanthin biosynthesis. Gene names from C. glutamicum (and gene IDs for MEP pathway genes) as well as gene names from Pantoea ananatis and Brevundimonas aurantiaca (gray boxes) are indicated. The structures of the endogenous C50 carotenoid decaprenoxanthin and the heterologous C40 carotenoid astaxanthin are given (GAP, glyceraldehyde 3-phosphate; DXP, 1-deoxy-d-xylulose 5-phosphate; MEP, 2-methylerythritol 4-phosphate; CDP-ME, 4-diphosphocytidyl-2-methylerythritol; CDP-MEP, 4-diphosphocytidyl-2-methylerythritol 2-phosphate; ME-cPP, 2-methylerythritol 2,4-cyclopyrophosphate; HMBPP, 4-hydroxy-3-methyl-but-2-enyl pyrophosphate; IPP, isopentenyl pyrophosphate; DMAPP, dimethylallyl pyrophosphate).

The biotechnologically relevant bacterium Corynebacterium glutamicum, currently used for the million ton-scale production of amino acids for the food and feed industries, is pigmented due to synthesis of the rare cyclic C50 carotenoid decaprenoxanthin and its glucosides. The precursors of carotenoid biosynthesis, isopenthenyl pyrophosphate (IPP) and its isomer dimethylallyl pyrophosphate, are synthesized in this organism via the methylerythritol phosphate (MEP) or non-mevalonate pathway. Terminal pathway engineering in recombinant C. glutamicum permitted the production of various non-native C50 and C40 carotenoids. Here, the role of engineering isoprenoid precursor supply for lycopene production by C. glutamicum was characterized. Overexpression of dxs encoding the enzyme that catalyzes the first committed step of the MEP-pathway by chromosomal promoter exchange in a prophage-cured, genome-reduced C. glutamicum strain improved lycopene formation. Similarly, an increased IPP supply was achieved by chromosomal integration of two artificial operons comprising MEP pathway genes under the control of a constitutive promoter. Combined overexpression of dxs and the other six MEP pathways genes in C. glutamicum strain LYC3-MEP was not synergistic with respect to improving lycopene accumulation. Based on C. glutamicum strain LYC3-MEP, astaxanthin could be produced in the milligrams per gram cell dry weight range when the endogenous genes crtE, crtB, and crtI for conversion of geranylgeranyl pyrophosphate to lycopene were coexpressed with the genes for lycopene cyclase and β-carotene hydroxylase from Pantoea ananatis and carotene C(4) oxygenase from Brevundimonas aurantiaca.