Synthetic genomes

Recombinant DNA Technology

Soon after the discovery of restriction endonucleases and ligases, the field of genetics began using these molecular tools to assemble artificial sequences from smaller fragments of synthetic or naturally-occurring DNA. The advantage in using the recombinatory approach as opposed to continual DNA synthesis stems from the inverse relationship that exists between synthetic DNA length and percent purity of that synthetic length. In other words, as you synthesize longer sequences, the number of error-containing clones increases due to the inherent error rates of current technologies.[1] Although recombinant DNA technology is more commonly used in the construction of fusion proteins and plasmids, several techniques with larger capacities have emerged, allowing for the construction of entire genomes.[2]

Polymerase Cycling Assembly

Polymerase Cycling Assembly. Blue arrows represent oligonucleotides 40 to 60 bp with overlapping regions of about 20 bp. The cycle is repeated until the final genome is constructed.

Polymerase cycling assembly (PCA) uses a series of oligonucleotides (or oligos), approximately 40 to 60 nucleotides long, that altogether constitute both strands of the DNA being synthesized. These oligos are designed such that a single oligo from one strand contains a length of approximately 20 nucleotides at each end that is complementary to sequences of two different oligos on the opposite strand, thereby creating regions of overlap. The entire set is processed through cycles of: (a) hybridization at 60 °C; (b) elongation via Taq polymerase and a standard ligase; and (c) denaturation at 95 °C, forming progressively longer contiguous strands and ultimately resulting in the final genome.[3] PCA was used to generate the first synthetic genome in history, that of the Phi X 174 virus.[4]

Gibson Assembly Method

Gibson Assembly Method. The blue arrows represent DNA cassettes, which could be any size, 6 kb each for example. The orange segments represent areas of identical DNA sequences. This process can be carried out with multiple initial cassettes.

The Gibson Assembly Method, designed by Daniel Gibson during his time at the J. Craig Venter Institute, requires a set of double-stranded DNA cassettes that constitute the entire genome being synthesized. Note that cassettes differ from contigs by definition, in that these sequences contain regions of homology to other cassettes for the purposes of recombination. In contrast to Polymerase Cycling Assembly, Gibson Assembly is a single-step, isothermal reaction with larger sequence-length capacity; ergo, it is used in place of Polymerase Cycling Assembly for genomes larger than 6 kb.

A T5 exonuclease performs a chew-back reaction at the terminal segments, working in the 5' to 3' direction, thereby producing complimentary overhangs. The overhangs hybridize to each other, a Phusion DNA polymerase fills in any missing nucleotides and the nicks are sealed with a ligase. However, the genomes capable of being synthesized using this method alone is limited because as DNA cassettes increase in length, they require propagation in vitro in order to continue hybridizing; accordingly, Gibson assembly is often used in conjunction with Transformation-Associated Recombination (see below) to synthesize genomes several hundred kilobases in size.[5]

Transformation-Associated Recombination

Gap Repair Cloning. The blue arrows represent DNA contigs. Segments of the same colour represent complimentary or identical sequences. Specialized primers with extensions are used in a polymerase chain reaction to generate regions of homology at the terminal ends of the DNA contigs.

The goal of Transformation-Associated Recombination (TAR) technology in synthetic genomics is to combine DNA contigs by means of homologous recombination performed by the Yeast Artificial Chromosome (YAC). Of importance is the CEN element within the YAC vector, which corresponds to the yeast centromere. This sequence gives the vector the ability to behave in a chromosomal manner, thereby allowing it to perform homologous recombination.[6]

Transformation-Associated Recombination. Cross over events occur between regions of homology across the cassettes and YAC vector, thereby connecting the smaller DNA sequences into one larger contig.

First, Gap Repair Cloning is performed to generate regions of homology flanking the DNA contigs. Gap Repair Cloning is a particular form of the Polymerase Chain Reaction in which specialized primers with extensions beyond the sequence of the DNA target are utilized.[7] Then, the DNA cassettes are exposed to the YAC vector, which drives the process of homologous recombination, thereby connecting the DNA cassettes. Polymerase Cycling Assembly and TAR technology were used together to construct the 600 kb Mycoplasma genitalium genome in 2008, the first synthetic organism ever created.[8] Similar steps were taken in synthesizing the larger Mycoplasma mycoides genome a few years later.[9]

See also

References

  1. Montague, Michael G; Lartigue, Carole; Vashee, Sanjay. "Synthetic genomics: potential and limitations". Current Opinion in Biotechnology. 23 (5): 659–665. doi:10.1016/j.copbio.2012.01.014.
  2. Gibson, Daniel (2011). Synthetic Biology, Part B: Computer Aided Design and DNA Assembly; Chapter Fifteen - Enzymatic Assembly of Overlapping DNA Fragments. Academic Press. pp. 349–361. ISBN 978-0-12-385120-8.
  3. Stemmer, Willem P. C.; Crameri, Andreas; Ha, Kim D.; Brennan, Thomas M.; Heyneker, Herbert L. (1995-10-16). "Single-step assembly of a gene and entire plasmid from large numbers of oligodeoxyribonucleotides". Gene. 164 (1): 49–53. doi:10.1016/0378-1119(95)00511-4.
  4. Smith, Hamilton O.; Hutchison, Clyde A.; Pfannkoch, Cynthia; Venter, J. Craig (2003-12-23). "Generating a synthetic genome by whole genome assembly: φX174 bacteriophage from synthetic oligonucleotides". Proceedings of the National Academy of Sciences. 100 (26): 15440–15445. doi:10.1073/pnas.2237126100. ISSN 0027-8424. PMC 307586Freely accessible. PMID 14657399.
  5. Gibson, Daniel G; Young, Lei; Chuang, Ray-Yuan; Venter, J Craig; Hutchison, Clyde A; Smith, Hamilton O (2009-04-12). "Enzymatic assembly of DNA molecules up to several hundred kilobases". Nature Methods. 6 (5): 343–345. doi:10.1038/nmeth.1318.
  6. Kouprina, Natalay; Larionov, Vladimir (2003-12-01). "Exploiting the yeast Saccharomyces cerevisiae for the study of the organization and evolution of complex genomes". FEMS Microbiology Reviews. 27 (5): 629–649. doi:10.1016/S0168-6445(03)00070-6. ISSN 1574-6976. PMID 14638416.
  7. Marsischky, Gerald; LaBaer, Joshua (2004-10-15). "Many Paths to Many Clones: A Comparative Look at High-Throughput Cloning Methods". Genome Research. 14 (10b): 2020–2028. doi:10.1101/gr.2528804. ISSN 1088-9051. PMID 15489321.
  8. Gibson, Daniel G.; Benders, Gwynedd A.; Andrews-Pfannkoch, Cynthia; Denisova, Evgeniya A.; Baden-Tillson, Holly; Zaveri, Jayshree; Stockwell, Timothy B.; Brownley, Anushka; Thomas, David W. (2008-02-29). "Complete Chemical Synthesis, Assembly, and Cloning of a Mycoplasma genitalium Genome". Science. 319 (5867): 1215–1220. doi:10.1126/science.1151721. ISSN 0036-8075. PMID 18218864.
  9. Gibson, Daniel G.; Glass, John I.; Lartigue, Carole; Noskov, Vladimir N.; Chuang, Ray-Yuan; Algire, Mikkel A.; Benders, Gwynedd A.; Montague, Michael G.; Ma, Li (2010-07-02). "Creation of a Bacterial Cell Controlled by a Chemically Synthesized Genome". Science. 329 (5987): 52–56. doi:10.1126/science.1190719. ISSN 0036-8075. PMID 20488990.
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