Additional Background Information
- Genomically Recoded E. coli
Whole-genome recoding was reported for the first time in 2011 by a team including our advisor, Professor Farren Isaacs, when it described replacing all TAG codons in E. coli by TAA. 9 Both TAG and TAA are stop codons (amber and ochre), but their transcripts are bound by different release factors (RF1 binds UAG and UAA, whereas RF2 binds UAA and UGA), not only making this recoding nonlethal but also allowing the deletion of RF1 (ΔprfA) from the recoded strain, given RF2’s response to both remaining stop codons.
This genome-wide recoding was enabled by lambda-Red recombineering10 and multiplex automated genome engineering. 11 lambda-Red recombineering uses the lambda prophage’s protein Beta to mediate the homologous recombination of an exogenous single-stranded oligonucleotide, delivered into the cell by electroporation, with the host genome, by annealing that oligonucleotide to single-stranded genomic DNA exposed on the lagging strand of the replication fork. 12 A 30-bp region of homology at either end of a sequence is sufficient to drive recombination of the entire strand, including mismatched regions, and mismatches thus incorporated are passed to progeny at high efficiency (up to 30%) in strains lacking methyl-directed mismatch repair (ΔmutS).13
Multiplex automated genome engineering (MAGE) using lambda-Red recombineering can then make many directed mutations across the host genome, as was necessary to replace all 314 TAG codons in the strain EcNR2 (E. coli MG1655 ΔmutS::cat Δ(ybhB-bioAB)::[λcI857 Δ(cro-ea59)::tetR-bla]).9 To allow recombineering, the lambda prophage was introduced into the host genome by P1 transduction. Because the probability of each target sequence being mutated in a given cycle is at most 30%, attempting to introduce all 314 mutations using a single pool of 314 mutagenic oligonucleotides would much sooner generate any of ~2314 other partially recoded strains before the fully recoded strain, and running enough MAGE cycles to obtain that strain would allow time for spontaneous point mutations to accumulate unchecked by the knocked-out mismatch repair system. To construct the strain we will use 32 separate strains were generated, each with a different recoded sector, and those sectors were assembled by hierarchical conjugation. The recoded strain was validated by sequencing, and its RF1 was deleted to free the TAG codon for reassignment to an orthogonal translation system.14
- Orthogonal Translation Systems
An amino acid can be assigned to a particular codon by a two-part translation system: a tRNA with its anticodon loop complementary to the codon, and an aminoacyl synthetase (hereafter called a synthetase) able to charge this tRNA with the amino acid. This system is orthogonal to endogenous translation systems if and only if this synthetase aminoacylates only this tRNA and endogenous synthetases cannot aminoacylate this tRNA. Usually, an unnatural amino acid thus assigned should also be sufficiently dissimilar from naturally encoded amino acids that endogenous synthetases would not charge endogenous tRNAs with the unnatural amino acid, to avoid partially reassigning other codons and disrupting cell function.15
Many synthetases include a nonconserved loop specific to their associated tRNA’s anticodon, preventing them from binding a tRNA reassigned to CUA, but the archaeum Methanococcus jannaschii’s tyrosyl-tRNA synthetase (MjtRNAs) and its associated tRNA translation system still bind after the anticodon is mutated, and is an amber suppressor when transformed into E. coli.16 This MjtRNAs was still aminoacylated by endogenous synthetases, so its specificity for its synthetase was improved by random mutation at eleven positions not directly interacting with its synthetase, followed by negative selection against nonspecific acylation and positive selection for specific acylation. 17
This orthogonal system has since been engineered by directed evolution of its synthetase to incorporate nonstandard amino acids, in place of tyrosine. 18 Diverse synthetases were generated by site-directed mutagenesis of five residues in the amino acid-binding pocket, and screened by positive selection, for incorporation of the amino acid into a protein conferring antibiotic resistance, and a negative screen, against mutants resistant to the antibiotic even in the absence of the nonstandard amino acid (by treating colonies on a replica plate lacking the amino acid and then observing which were killed). Selected mutants were then recombined and subjected to further mutagenesis.
- An Improved T7 Expression System
Our first challenge in making Ampersand was to develop a system that limits basal expression of our peptide, due to its toxicity to the host. Several expression systems have been designed in the past, including the T7 promoter and T7 RNA Polymerase system, to suppress protein expression. The current BL21 (DE3) strain is leaky due to the weak suppressing promoter lacUV5 that drives T7 RNA polymerase in the DE3 strains. As a result, low levels of toxic protein are constitutively expressed, ultimately killing the host it was made in and in turn lowering the overall yield of the protein produced.
In order to reduce the expression of T7 RNA polymerase and create an efficient system for the expression of recombinant proteins in E. coli we chose to introduce two levels of regulation: -
Transcriptional Regulation: We will use pZE21 of the pZ system of vectors developed by Lutz and Buschard with the PLlacO promoter to inhibit the expression of T7 RNA polymerase.
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Translational Regulation: We will use the artificial riboregulatory elements devised by Isaacs et al.. to restrict translation of the mRNA sequence encoding T7 RNA Polymerase.19 The cis-repressing RNA (crRNA) sequence will be inserted downstream of the promoter driving T7 RNA Polymerase and upstream of the ribosomal binding site (RBS). The crRNA is complimentary to the RBS and forms a stem loop at the 5’ end of the mRNA segment, blocking ribosomal docking and translation. A second promoter, PLtetO will express the trans-activating RNA (taRNA) capable of undergoing a linear-loop interaction that will expose the RBS and allow for translation of T7 RNA Polymerase. The ribo-regulated T7 RNA Polymerase will be ultimately incorporated into the genome of strain capable of high protein production. A second pZ plasmid will contain the gene of interest expressed by a T7 promoter.
In summary, the benefits to this type of system are its robustness, portability, and efficiency in that it does not require the cell to expend more energy on the constitutive synthesis of another protein. We theorize that by utilizing these two levels of control we will be able to reduce the expression of T7 RNA polymerase and produce a system with zero basal expression of the gene of interest and permit stable cloning of toxic recombinant proteins.
Figure 3. This diagram illustrates the T7 riboregulation system developed to ensure low basal levels of protein expression.19
- Mussel Adhesion Proteins
The ability for mussels to survive the harsh conditions of the intertidal zone is directly related to their capability to bind to both organic and inorganic surfaces that they come in contact with. As a result, these mussels have evolved to secrete “adhesion proteins” that enable formation of powerful bonds in an otherwise deleterious aqueous environment. The quantity known as “work of adhesion (WA)” amongst interfaces in an aqueous environment is significantly less favorable due to the water-surface interactions that must be outcompeted by the adhesive if binding is to occur.10 Therefore, these mussel adhesion proteins offer a promising avenue towards enhanced bioadhesives that retain functionality in aqueous environments.
The structure responsible for the binding of mussels to these surfaces is known as the byssus, which is composed of a well-characterized assembly of approximately 25-30 proteins.20 The byssus manifests itself as an outgrowth from the mussel’s “foot” composed of threads, which terminate in plaques deposited on the surface. Thus far, a total of 5 proteins, known as mussel foot proteins (mfp’s), were shown to be unique to the plaque. Of these 5 plaque proteins, mfp-3 and mfp-5 have elicited the most investigation for adhesive applications, as both are localized at the interface between the plaque and surface. Additionally, it was shown that all such mfp’s have a uniquely high concentration of tyrosine, which is post-translationally modified to 3,4-dihydroxy-L-phenylalanine (L-Dopa). Atomic force microscopy studies focusing on a single dopa residue showed that its interaction with a metal oxide surface involves a remarkably high strength, reversible coordination bond.21 It has been shown that catechol oxidase enzymes present in mfp secretions are able to convert the catechol groups of L-dopa into reactive orthoquinone functionalities, which undergo irreversible covalent bonding with organic surfaces.21,22 Ultimately, the high degree of surface affinity such dopa-containing peptides possess makes them novel tools in the development of biomimetic adhesive peptides.
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References
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- Isaacs, F. J. (2012). Synthetic biology: Automated design of RNA devices. Nat Chem Biol, 8(5), 413-415.
- Isaacs, F. J., Carr, P. A., Wang, H. H., Lajoie, M. J., Sterling, B., Kraal, L., et al.. (2011). Precise manipulation of chromosomes in vivo enables genome-wide codon replacement. Science, 333(6040), 348-353.
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- Gao, Y., Zorman, S., Gundersen G., Xi, Z., Ma L., Sirinakis G., Rothman J.E., & Zhang Y. (2012) Single Reconstituted Neuronal SNARE Complexes Zipper in Three Distinct Stages. Science (New York, N.Y.) 337(6100):1340-1343
- Isaacs, Farren J., et al. "Precise manipulation of chromosomes in vivo enables genome-wide codon replacement." Science 333.6040 (2011): 348-353.
- Sharan, Shyam K., Lynn C. Thomason, and Sergey G. Kuznetsov. "Recombineering: a homologous recombination-based method of genetic engineering." Nature protocols 4.2 (2009): 206-223.
- Wang, Harris H., et al. "Programming cells by multiplex genome engineering and accelerated evolution." Nature 460.7257 (2009): 894-898.
- Ellis, Hilary M., Daiguan Yu, and Tina DiTizio. "High efficiency mutagenesis, repair, and engineering of chromosomal DNA using single-stranded oligonucleotides." Proceedings of the National Academy of Sciences 98.12 (2001): 6742-6746.
- Costantino, Nina. & Court, Donald L. “Enhanced levels of Red-mediated recombinants in mismatch repair mutants.” Proceedings of the National Academy of Sciences 100.26 (2003): 15748–15753.
- Lajoie, M. J., Rovner, A. J., Goodman, D. B., Aerni, H. R., Haimovich, A. D., Kuznetsov, G., et al. (2013). Genomically recoded organisms expand biological functions. Science, 342(6156), 357-360.
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- Wang, Lei, et al. "A new functional suppressor tRNA/aminoacyl-tRNA synthetase pair for the in vivo incorporation of unnatural amino acids into proteins." JOURNAL-AMERICAN CHEMICAL SOCIETY122.20 (2000): 5010-5011.
- Wang, Lei, and Peter G. Schultz. "A general approach for the generation of orthogonal tRNAs." amino acids 3 (2001): 4.
- Wang, Lei, et al. "Expanding the genetic code of Escherichia coli." Science 292.5516 (2001): 498-500.
- Isaacs, F. J., et al. (2004). "Engineered riboregulators enable post-transcriptional control of gene expression." Nature biotechnology 22(7): 841-847.
- BP Lee, PB Messersmith, JN Israelachvili, JH Waite. (2011) Mussel-Inspired Adhesives and Coatings. Annual Review of Materials Research; 41: 99-132.
- H Lee , NF Scherer, PB Messersmith. (2006) Single-Molecule Mechanics of Mussel Adhesion. Proc Natl Acad Sci; 103:12999-3003.
- M Yu, J Hwang, TJ Deming. (1999) Role of L-3,4-Dihydroxyphenylalanine in Mussel Adhesive Proteins. J. Am. Chem. Soc. 1999, 121, 5825-5826
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