A toolkit for <i>Nannochloropsis oceanica </i><scp>CCMP</scp>1779 enables gene stacking and genetic engineering of the eicosapentaenoic acid pathway for enhanced long‐chain polyunsaturated fatty acid production

Poliner, Eric; Pulman, Jane A.; Zienkiewicz, Krzysztof; Childs, Kevin L.; Benning, Christoph; Farré, Eva M.

doi:10.1111/pbi.12772

Cited by 125 publications

(106 citation statements)

References 73 publications

Supporting

Mentioning

105

Contrasting

Order By: Relevance

“…The LDSP terminator (CCMP1779_4188) was PCR amplified from N. oceanica CCMP1779 genome using the primers LDSP term sac F+ and LDSP term afl R-(Figure S16), and digested with SacI and AflII to replace the 35S terminator as the terminator for the luciferase gene. The LUC+HA gene was then replaced by either N. oceanica CCMP1779 codon optimized coding sequences for firefly luciferase (FLUC) and, nanoluciferase (NLUC) (Hall et al , 2012, Poliner et al , 2018b) or a Chlamydomonas codon optimized renilla luciferase (RLUC) (Ferrante et al , 2008) to form pNOC-Fluc, pNOC-Nluc, and pNOC-Rluc respectively using AscI and SacI and the primers listed in Figure S16. The pNOC vectors were used to transform N. oceanica CCMP1779.…”

Section: Methodsmentioning

confidence: 99%

“…This cassette, which includes the CCMP537 EF promoter (NODE_7115_length_93819_cov_37.515949:78382..79716), the zeocin resistance gene and the CCMP1779 LDSP terminator, from N. salina selection construct pNSA-511 were cloned by restriction digest (AhdI/SbfI) generating the pNSA-FLUC and vector (Dataset 1). The pNSA-511 construct was generated by cloning the CCMP537 EF promoter into pNOC-411 using SnabI and XhoI (Poliner et al , 2018b). The promoters of the cellulose synthase (NannoCCMP1779|5780, NODE_11401_length_57650_cov_57.237450:4263..6099), LHC1 (NODE_14101_length_22726_cov_35.737923:17540..18097), and LHC8 (NannoCCMP1779|6809, NODE_11394_length_43512_cov_40.897591:1551..2663) promoters were amplified from the N. oceanica CCMP1779 and N. salina CCMP537 genomes using primers listed in Figure S16 and inserted into pENTR-D-Topo (Invitrogen).…”

Section: Methodsmentioning

confidence: 99%

“…Several Nannochloropsis strains from different worldwide locations have been sequenced and current data suggests that Nannochloropsis species are haploid with genome sizes of ~30 Mb, containing from ~6,500 to ~12,000 genes (Corteggiani Carpinelli et al , 2014, Radakovits et al , 2012, Schwartz et al , 2018, Vieler et al , 2012, Wang et al , 2014). Recent years have seen the development of a comprehensive set of molecular tools for working with these algae, such as homologous gene replacement, overexpression, gene silencing and CRISPR/Cas9 based genome editing (Kilian et al , 2011, Poliner et al , 2018a, Poliner et al , 2018b, Poliner et al , 2018c, Verruto et al , 2018, Wang et al , 2016, Wei et al , 2017). In this study, we describe the development of a bioluminescence reporter system for the long-term in vivo measurement of gene expression in two Nannochloropsis species.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Identification of circadian rhythms inNannochloropsisspecies using bioluminescence reporter lines

Poliner

Cummings

Newton

et al. 2019

Preprint

Self Cite

View full text Add to dashboard Cite

32Circadian clocks allow organisms to predict environmental changes caused by the rotation of the 33 Earth. Although circadian rhythms are widespread among different taxa, the core components of 34 circadian oscillators are not conserved and differ between bacteria, plants, animals and fungi. 35Stramenopiles are a large group of organisms in which circadian rhythms have been only poorly 36 characterized and no clock components have been identified. We have investigated cell division 37 and molecular rhythms in Nannochloropsis species. In the four strains tested, cell division 38 occurred principally during the night period under diel conditions, however, rhythms dampened 39 within 2-3 days after transfer to constant light. We developed firefly luciferase reporters for 40 long-term monitoring of in vivo transcriptional rhythms in two Nannochlropsis species, N. 41 oceanica CCMP1779 and N. salina CCMP537. The reporter lines express free-running 42 bioluminescence rhythms with periods of ~21-31 h that dampen within ~3-4 days under constant 43 light. Using different entrainment regimes, we demonstrate that these rhythms are regulated by a 44 circadian-type oscillator. In addition, the phase of free-running luminescence rhythms can be 45 modulated pharmacologically using a CK1 e/d inhibitor, suggesting a role of this kinase in the 46 Nannochloropsis clock. Together with the molecular and genomic tools available for 47 Nannochloropsis species, these reporter lines represent an excellent system for future studies on 48 the molecular mechanisms of stramenopile circadian oscillators. 49 50 Significance statement 51Stramenopiles are a large and diverse line of eukaryotes in which circadian rhythms have been 52 only poorly characterized and no clock components have been identified. We have developed 53 bioluminescence reporter lines in Nannochloropsis species and provide evidence for the presence 54 of a circadian oscillator in stramenopiles; these lines will serve as tools for future studies to 55 uncover the molecular mechanisms of circadian oscillations in these species. 56 57

show abstract

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Identification of circadian rhythms inNannochloropsisspecies using bioluminescence reporter lines

Poliner

Cummings

Newton

et al. 2019

Preprint

Self Cite

View full text Add to dashboard Cite

show abstract

“…This cassette, which includes the CCMP537 EF promoter (NODE_7115_length_93819_cov_37.515949:78382..79716), the zeocin resistance gene and the CCMP1779 LDSP terminator from N. salina selection construct pNSA-511 were cloned by restriction digest (AhdI/SbfI), generating the pNSA-FLUC and the vector (Dataset S1). The pNSA-511 construct was generated by cloning the CCMP537 EF promoter into pNOC-411 using SnabI and XhoI (Poliner et al, 2018b). The promoters of the cellulose synthase (NannoCCMP1779|5780, NODE_11401_length_57650_ cov_57.237450:4263..6099), LHC1 (NODE_14101_length_22726_ cov_35.737923:17540..18097) and LHC8 (NannoCCMP1779|6809, NODE_11394_length_43512_cov_40.897591:1551..2663) promoters were amplified from the N. oceanica CCMP1779 and N. salina CCMP537 genomes using the primers listed in Figure S16 and inserted into pENTR-D-Topo (Invitrogen, now ThermoFisher Scientific, https://www.thermofisher.com).…”

Section: Generation Of Luciferase Expressing Linesmentioning

confidence: 99%

Identification of circadian rhythms in Nannochloropsis species using bioluminescence reporter lines

et al. 2019

Self Cite

View full text Add to dashboard Cite

Utilization of microalgae has been hampered by limited tools for creating loss-of-function mutants. Furthermore, modified strains for deployment into the field must be free of antibiotic resistance genes and face fewer regulatory hurdles if they are transgene free. The oleaginous microalga, Nannochloropsis oceanica CCMP1779, is an emerging model for microalgal lipid metabolism. We present a one-vector episomal CRISPR/Cas9 system for N. oceanica that enables the generation of marker-free mutant lines. The CEN/ARS6 region from Saccharomyces cerevisiae was included in the vector to facilitate its maintenance as circular extrachromosal DNA. The vector utilizes a bidirectional promoter to produce both Cas9 and a ribozyme flanked sgRNA. This system efficiently generates targeted mutations, and allows the loss of episomal DNA after the removal of selection pressure, resulting in marker-free non-transgenic engineered lines. To test this system, we disrupted the nitrate reductase gene (NR) and subsequently removed the CRISPR episome to generate non-transgenic marker-free nitrate reductase knockout lines (NR-KO).

show abstract

“…Moreover, they are excellent research models for microalgal systems and synthetic biology, due to their small genome size and simple gene structure (Vieler et al 2012, Jinkerson et al 2013, Wei et al 2013, Corteggiani et al 2014). Moreover, a comprehensive set of genetic tools has been recently established that includes homologous recombination (Kilian et al 2011, Gee andNiyogi 2017), gene knockdown (Wei et al 2017b, Xin et al 2017, gene editing (Wang et al 2016, Ajjawi et al 2017) and overexpression (Kang et al 2015, Li et al 2016, Nobusawa et al 2017, Xin et al 2017, Poliner et al 2018. Thus, Nannochloropsis spp.…”

mentioning

confidence: 99%

Optimized methods of chromatin immunoprecipitation for profiling histone modifications in industrial microalgae Nannochloropsis spp.

Wei

2018

Journal of Phycology

View full text Add to dashboard Cite

Epigenetic factors such as histone modifications play integral roles in plant development and stress response, yet their implications in algae remain poorly understood. In the industrial oleaginous microalgae Nannochloropsis spp., the lack of an efficient methodology for chromatin immunoprecipitation (ChIP), which determines the specific genomic location of various histone modifications, has hindered probing the epigenetic basis of their photosynthetic carbon conversion and storage as oil. Here, a detailed ChIP protocol was developed for Nannochloropsis oceanica, which represents a reliable approach for the analysis of histone modifications, chromatin state, and transcription factor-binding sites at the epigenetic level. Using ChIP-qPCR, genes related to photosynthetic carbon fixation in this microalga were systematically assessed. Furthermore, a ChIP-Seq protocol was established and optimized, which generated a genome-wide profile of histone modification events, using histone mark H3K9Ac as an example. These results are the first step for appreciation of the chromatin landscape in industrial oleaginous microalgae and for epigenetics-based microalgal feedstock development.

show abstract

A toolkit for Nannochloropsis oceanica CCMP1779 enables gene stacking and genetic engineering of the eicosapentaenoic acid pathway for enhanced long‐chain polyunsaturated fatty acid production

Cited by 125 publications

References 73 publications

Identification of circadian rhythms inNannochloropsisspecies using bioluminescence reporter lines

Identification of circadian rhythms inNannochloropsisspecies using bioluminescence reporter lines

Identification of circadian rhythms in Nannochloropsis species using bioluminescence reporter lines

Optimized methods of chromatin immunoprecipitation for profiling histone modifications in industrial microalgae Nannochloropsis spp.

Contact Info

Product

Resources

About