Fine-Tuning of Photoautotrophic Protein Production by Combining Promoters and Neutral Sites in the Cyanobacterium Synechocystis sp. Strain PCC 6803

Ng, Andrew H.; Berla, Bertram M.; Pakrasi, Himadri B.

doi:10.1128/aem.01349-15

Cited by 77 publications

(82 citation statements)

References 43 publications

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“…Synechocystis 6803 strain expressing YFP [50] were cultivated as described above. Following the B-PER and control treatments, cell pellets and medium supernatants were diluted in the ratio of 3:1 (v/v) in 4× Laemmli sample buffer and loaded in equal proportion on a 12% (v/v) Criterion™ TGX Stain-Free™ Protein Gel, which contains trihalo compounds that can react with tryptophan residues under the UV irradiation and gives rise to fluorescence (BioRad, US).…”

Section: Methodsmentioning

confidence: 99%

An easy and efficient permeabilization protocol for in vivo enzyme activity assays in cyanobacteria

et al. 2016

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BackgroundCyanobacteria are photosynthetic bacteria that thrive in diverse ecosystems and play major roles in the global carbon cycle. The abilities of cyanobacteria to fix atmospheric CO2 and to allocate the fixed carbons to chemicals and biofuels have attracted growing attentions as sustainable microbial cell factories. Better understanding of the activities of enzymes involved in the central carbon metabolism would lead to increasing product yields. Currently cell-free lysates are the most widely used method for determination of intracellular enzyme activities. However, due to thick cell walls, lysis of cyanobacterial cells is inefficient and often laborious. In some cases radioisotope-labeled substrates can be fed directly to intact cells; however, label-free assays are often favored due to safety and practical reasons.ResultsHere we show an easy and highly efficient method for permeabilization of the cyanobacteria Synechococcus sp. PCC 7002 and Synechocystis sp. PCC 6803, and determination of two intracellular enzymes, ribulose-1,5-bisphosphate carboxylase/decarboxylase (Rubisco) and glucose-6-phosphate dehydrogenase (G6PDH), that play pivotal roles in the central carbon metabolism in cyanobacteria. Incubation of the cyanobacterial cells in the commercially available B-PER reagent for 10 min permeabilized the cells, as confirmed by the SYTOX Green staining. There was no significant change in the cell shape and no major loss of intracellular proteins was observed during the treatment. When used directly in the assays, the permeabilized cells exhibited the enzyme activities that are comparable or even higher than those detected for cell-free lysates. Moreover, the permeabilized cells could be stored at −20 °C without losing the enzyme activities. The permeabilization process and subsequent activity assays were successfully adapted to the 96-well plate system.ConclusionsAn easy, efficient and scalable permeabilization protocol was established for cyanobacteria. The permeabilized cells can be directly applied for measurement of G6PDH and Rubisco activities without using radioisotopes and the protocol may be readily adapted to studies of other cyanobacterial species and other intracellular enzymes. The permeabilization and enzyme assays can be performed in 96-well plates in a high-throughput manner.

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Section: Methodsmentioning

confidence: 99%

An easy and efficient permeabilization protocol for in vivo enzyme activity assays in cyanobacteria

et al. 2016

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“…Recently, a strong constitutive cpc560 promoter has been described, giving a 22‐fold increase in yield of 3‐hydroxypropionic acid relative to the widely used psbA2 promoter (Zhou et al ., ; Wang et al ., ). Heterologous genes are usually inserted into the genome at loci referred to as neutral sites, whose disruption does not affect cell integrity (Ng et al ., ; Pinto et al ., ), or cloned into customizable wide‐host‐range, self‐replicating expression vectors (Taton et al ., ). Issues such as genetic instability and extensive small RNA‐mediated transcriptional regulation also need to be considered when working with cyanobacteria (Mitschke et al ., ; Jones, ; Kopf and Hess, ).…”

Section: Tools For Synthetic Biology In Cyanobacteria and Chloroplastsmentioning

confidence: 98%

Extending the biosynthetic repertoires of cyanobacteria and chloroplasts

et al. 2016

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SUMMARYChloroplasts in plants and algae and photosynthetic microorganisms such as cyanobacteria are emerging hosts for sustainable production of valuable biochemicals, using only inorganic nutrients, water, CO 2 and light as inputs. In the past decade, many bioengineering efforts have focused on metabolic engineering and synthetic biology in the chloroplast or in cyanobacteria for the production of fuels, chemicals and complex, high-value bioactive molecules. Biosynthesis of all these compounds can be performed in photosynthetic organelles/organisms by heterologous expression of the appropriate pathways, but this requires optimization of carbon flux and reducing power, and a thorough understanding of regulatory pathways. Secretion or storage of the compounds produced can be exploited for the isolation or confinement of the desired compounds. In this review, we explore the use of chloroplasts and cyanobacteria as biosynthetic compartments and hosts, and we estimate the levels of production to be expected from photosynthetic hosts in light of the fraction of electrons and carbon that can potentially be diverted from photosynthesis. The supply of reducing power, in the form of electrons derived from the photosynthetic light reactions, appears to be non-limiting, but redirection of the fixed carbon via precursor molecules presents a challenge. We also discuss the available synthetic biology tools and the need to expand the molecular toolbox to facilitate cellular reprogramming for increased production yields in both cyanobacteria and chloroplasts.

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“…Pcpc560 (Huang et al, 2010;Zhou et al, 2014;Englund et al, 2016;Ruffing et al, 2016;Ferreira et al, 2018;Li et al, 2018;Liu and Pakrasi, 2018 Ptrc (Huang et al, 2010;Guerrero et al, 2012;Oliver et al, 2013;Markley et al, 2015;Ferreira et al, 2018;Li et al, 2018) TetR (aTc Inducible) L03 (Huang and Lindblad, 2013;Zess et al, 2016;Ferreira et al, 2018) efficient transformation using conjugation and electroporation (compared to homologous recombination); (2) avoidance of the need for time-consuming segregation to achieve incorporation of the transgenic sequence in all copies of the genome; and (3) increased orthogonality of the heterologous sequences, meaning no insertion in genomic loci that may not be neutral. A hybrid strategy that combines the advantages of using a shuttle vector and the stability of genomic insertion involves using native cyanobacterial plasmids, either as insertion sites (Ng et al, 2015) or as true shuttle vectors after isolation and modification (Jin et al, 2018). BioBricks and isothermal assembly techniques are adequate for the generation of a limited number of (Guerrero et al, 2012;Huang and Lindblad, 2013;Oliver et al, 2013;Camsund and Lindblad, 2014).…”

Section: Constitutivementioning

confidence: 99%