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Design and assembly of the 117-kb Phaeodactylum tricornutum chloroplast genome
There is growing impetus to expand the repertoire of chassis available to synthetic biologists. Chloroplast genomes present an interesting alternative for engineering photosynthetic eukaryotes; however, development of the chloroplast as a synthetic biology chassis has been limited by a lack of effic...
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| Published in: | Plant physiology (Bethesda) 2024-03, Vol.194 (4), p.2217-2228 |
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| Main Authors: | , , , , |
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| container_end_page | 2228 |
| container_issue | 4 |
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| container_title | Plant physiology (Bethesda) |
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| creator | Walker, Emma J L Pampuch, Mark Chang, Nelson Cochrane, Ryan R Karas, Bogumil J |
| description | There is growing impetus to expand the repertoire of chassis available to synthetic biologists. Chloroplast genomes present an interesting alternative for engineering photosynthetic eukaryotes; however, development of the chloroplast as a synthetic biology chassis has been limited by a lack of efficient techniques for whole-genome cloning and engineering. Here, we demonstrate two approaches for cloning the 117-kb Phaeodactylum tricornutum chloroplast genome that have 90% to 100% efficiency when screening as few as 10 yeast (Saccharomyces cerevisiae) colonies following yeast assembly. The first method reconstitutes the genome from PCR-amplified fragments, whereas the second method involves precloning these fragments into individual plasmids from which they can later be released. In both cases, overlapping fragments of the chloroplast genome and a cloning vector are homologously recombined into a singular contig through yeast assembly. The cloned chloroplast genome can be stably maintained and propagated within Escherichia coli, which provides an exciting opportunity for engineering a delivery mechanism for bringing DNA directly to the algal chloroplast. Also, one of the cloned genomes was designed to contain a single SapI site within the yeast URA3 (coding for orotidine-5'-phosphate decarboxylase) open-reading frame, which can be used to linearize the genome and integrate designer cassettes via golden-gate cloning or further iterations of yeast assembly. The methods presented here could be extrapolated to other species-particularly those with a similar chloroplast genome size and architecture (e.g. Thalassiosira pseudonana). |
| doi_str_mv | 10.1093/plphys/kiad670 |
| format | article |
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| ispartof | Plant physiology (Bethesda), 2024-03, Vol.194 (4), p.2217-2228 |
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| source | Oxford Journals Online |
| title | Design and assembly of the 117-kb Phaeodactylum tricornutum chloroplast genome |
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