Assembly of eukaryotic algal chromosomes in yeast

BACKGROUND: Synthetic genomic approaches offer unique opportunities to use powerful yeast and Escherichia coli genetic systems to assemble and modify chromosome-sized molecules before returning the modified DNA to the target host. For example, the entire 1 Mb Mycoplasma mycoides chromosome can be st...

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Autores principales: Karas, Bogumil J, Molparia, Bhuvan, Jablanovic, Jelena, Hermann, Wolfgang J, Lin, Ying-Chi, Dupont, Christopher L, Tagwerker, Christian, Yonemoto, Isaac T, Noskov, Vladimir N, Chuang, Ray-Yuan, Allen, Andrew E, Glass, John I, Hutchison, Clyde A, Smith, Hamilton O, Venter, J Craig, Weyman, Philip D
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2013
Materias:
Methodology
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4029449/
https://www.ncbi.nlm.nih.gov/pubmed/24325901
http://dx.doi.org/10.1186/1754-1611-7-30
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author Karas, Bogumil J
Molparia, Bhuvan
Jablanovic, Jelena
Hermann, Wolfgang J
Lin, Ying-Chi
Dupont, Christopher L
Tagwerker, Christian
Yonemoto, Isaac T
Noskov, Vladimir N
Chuang, Ray-Yuan
Allen, Andrew E
Glass, John I
Hutchison, Clyde A
Smith, Hamilton O
Venter, J Craig
Weyman, Philip D
author_facet Karas, Bogumil J
Molparia, Bhuvan
Jablanovic, Jelena
Hermann, Wolfgang J
Lin, Ying-Chi
Dupont, Christopher L
Tagwerker, Christian
Yonemoto, Isaac T
Noskov, Vladimir N
Chuang, Ray-Yuan
Allen, Andrew E
Glass, John I
Hutchison, Clyde A
Smith, Hamilton O
Venter, J Craig
Weyman, Philip D
author_sort Karas, Bogumil J
collection PubMed
description BACKGROUND: Synthetic genomic approaches offer unique opportunities to use powerful yeast and Escherichia coli genetic systems to assemble and modify chromosome-sized molecules before returning the modified DNA to the target host. For example, the entire 1 Mb Mycoplasma mycoides chromosome can be stably maintained and manipulated in yeast before being transplanted back into recipient cells. We have previously demonstrated that cloning in yeast of large (> ~ 150 kb), high G + C (55%) prokaryotic DNA fragments was improved by addition of yeast replication origins every ~100 kb. Conversely, low G + C DNA is stable (up to at least 1.8 Mb) without adding supplemental yeast origins. It has not been previously tested whether addition of yeast replication origins similarly improves the yeast-based cloning of large (>150 kb) eukaryotic DNA with moderate G + C content. The model diatom Phaeodactylum tricornutum has an average G + C content of 48% and a 27.4 Mb genome sequence that has been assembled into chromosome-sized scaffolds making it an ideal test case for assembly and maintenance of eukaryotic chromosomes in yeast. RESULTS: We present a modified chromosome assembly technique in which eukaryotic chromosomes as large as ~500 kb can be assembled from cloned ~100 kb fragments. We used this technique to clone fragments spanning P. tricornutum chromosomes 25 and 26 and to assemble these fragments into single, chromosome-sized molecules. We found that addition of yeast replication origins improved the cloning, assembly, and maintenance of the large chromosomes in yeast. Furthermore, purification of the fragments to be assembled by electroelution greatly increased assembly efficiency. CONCLUSIONS: Entire eukaryotic chromosomes can be successfully cloned, maintained, and manipulated in yeast. These results highlight the improvement in assembly and maintenance afforded by including yeast replication origins in eukaryotic DNA with moderate G + C content (48%). They also highlight the increased efficiency of assembly that can be achieved by purifying fragments before assembly.
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spelling pubmed-40294492014-05-22 Assembly of eukaryotic algal chromosomes in yeast Karas, Bogumil J Molparia, Bhuvan Jablanovic, Jelena Hermann, Wolfgang J Lin, Ying-Chi Dupont, Christopher L Tagwerker, Christian Yonemoto, Isaac T Noskov, Vladimir N Chuang, Ray-Yuan Allen, Andrew E Glass, John I Hutchison, Clyde A Smith, Hamilton O Venter, J Craig Weyman, Philip D J Biol Eng Methodology BACKGROUND: Synthetic genomic approaches offer unique opportunities to use powerful yeast and Escherichia coli genetic systems to assemble and modify chromosome-sized molecules before returning the modified DNA to the target host. For example, the entire 1 Mb Mycoplasma mycoides chromosome can be stably maintained and manipulated in yeast before being transplanted back into recipient cells. We have previously demonstrated that cloning in yeast of large (> ~ 150 kb), high G + C (55%) prokaryotic DNA fragments was improved by addition of yeast replication origins every ~100 kb. Conversely, low G + C DNA is stable (up to at least 1.8 Mb) without adding supplemental yeast origins. It has not been previously tested whether addition of yeast replication origins similarly improves the yeast-based cloning of large (>150 kb) eukaryotic DNA with moderate G + C content. The model diatom Phaeodactylum tricornutum has an average G + C content of 48% and a 27.4 Mb genome sequence that has been assembled into chromosome-sized scaffolds making it an ideal test case for assembly and maintenance of eukaryotic chromosomes in yeast. RESULTS: We present a modified chromosome assembly technique in which eukaryotic chromosomes as large as ~500 kb can be assembled from cloned ~100 kb fragments. We used this technique to clone fragments spanning P. tricornutum chromosomes 25 and 26 and to assemble these fragments into single, chromosome-sized molecules. We found that addition of yeast replication origins improved the cloning, assembly, and maintenance of the large chromosomes in yeast. Furthermore, purification of the fragments to be assembled by electroelution greatly increased assembly efficiency. CONCLUSIONS: Entire eukaryotic chromosomes can be successfully cloned, maintained, and manipulated in yeast. These results highlight the improvement in assembly and maintenance afforded by including yeast replication origins in eukaryotic DNA with moderate G + C content (48%). They also highlight the increased efficiency of assembly that can be achieved by purifying fragments before assembly. BioMed Central 2013-12-10 /pmc/articles/PMC4029449/ /pubmed/24325901 http://dx.doi.org/10.1186/1754-1611-7-30 Text en Copyright © 2013 Karas et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated.
spellingShingle Methodology
Karas, Bogumil J
Molparia, Bhuvan
Jablanovic, Jelena
Hermann, Wolfgang J
Lin, Ying-Chi
Dupont, Christopher L
Tagwerker, Christian
Yonemoto, Isaac T
Noskov, Vladimir N
Chuang, Ray-Yuan
Allen, Andrew E
Glass, John I
Hutchison, Clyde A
Smith, Hamilton O
Venter, J Craig
Weyman, Philip D
Assembly of eukaryotic algal chromosomes in yeast
title Assembly of eukaryotic algal chromosomes in yeast
title_full Assembly of eukaryotic algal chromosomes in yeast
title_fullStr Assembly of eukaryotic algal chromosomes in yeast
title_full_unstemmed Assembly of eukaryotic algal chromosomes in yeast
title_short Assembly of eukaryotic algal chromosomes in yeast
title_sort assembly of eukaryotic algal chromosomes in yeast
topic Methodology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4029449/
https://www.ncbi.nlm.nih.gov/pubmed/24325901
http://dx.doi.org/10.1186/1754-1611-7-30
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