176 results on '"Synthetic Biology and Bioengineering"'
Search Results
2. Comprehensive analysis of prime editing outcomes in human embryonic stem cells
- Author
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Omer Habib, Gizem Habib, Gue-Ho Hwang, and Sangsu Bae
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Gene Editing ,AcademicSubjects/SCI00010 ,alpha 1-Antitrypsin ,alpha 1-Antitrypsin Deficiency ,Human Embryonic Stem Cells ,Genetics ,Humans ,DNA ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering - Abstract
Prime editing is a versatile and precise genome editing technique that can directly copy desired genetic modifications into target DNA sites without the need for donor DNA. This technique holds great promise for the analysis of gene function, disease modeling, and the correction of pathogenic mutations in clinically relevant cells such as human pluripotent stem cells (hPSCs). Here, we comprehensively tested prime editing in hPSCs by generating a doxycycline-inducible prime editing platform. Prime editing successfully induced all types of nucleotide substitutions and small insertions and deletions, similar to observations in other human cell types. Moreover, we compared prime editing and base editing for correcting a disease-related mutation in induced pluripotent stem cells derived form a patient with α 1-antitrypsin (A1AT) deficiency. Finally, whole-genome sequencing showed that, unlike the cytidine deaminase domain of cytosine base editors, the reverse transcriptase domain of a prime editor does not lead to guide RNA-independent off-target mutations in the genome. Our results demonstrate that prime editing in hPSCs has great potential for complementing previously developed CRISPR genome editing tools.
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- 2022
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3. Modulating the chemo-mechanical response of structured DNA assemblies through binding molecules
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Jae Young Lee, Young Joo Kim, Chanseok Lee, Do-Nyun Kim, and Kyung Soo Kim
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Nanostructure ,AcademicSubjects/SCI00010 ,Finite Element Analysis ,Nanotechnology ,Biology ,Ligands ,Microscopy, Atomic Force ,chemistry.chemical_compound ,Ethidium ,DNA nanotechnology ,Genetics ,Molecule ,DNA origami ,Groove (engineering) ,Persistence length ,Benzoxazoles ,Quinolinium Compounds ,DNA ,Molecular machine ,Intercalating Agents ,Nanostructures ,chemistry ,Doxorubicin ,Spectrophotometry ,Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization ,Synthetic Biology and Bioengineering - Abstract
Recent advances in DNA nanotechnology led the fabrication and utilization of various DNA assemblies, but the development of a method to control their global shapes and mechanical flexibilities with high efficiency and repeatability is one of the remaining challenges for the realization of the molecular machines with on-demand functionalities. DNA-binding molecules with intercalation and groove binding modes are known to induce the perturbation on the geometrical and mechanical characteristics of DNA at the strand level, which might be effective in structured DNA assemblies as well. Here, we demonstrate that the chemo-mechanical response of DNA strands with binding ligands can change the global shape and stiffness of DNA origami nanostructures, thereby enabling the systematic modulation of them by selecting a proper ligand and its concentration. Multiple DNA-binding drugs and fluorophores were applied to straight and curved DNA origami bundles, which demonstrated a fast, recoverable, and controllable alteration of the bending persistence length and the radius of curvature of DNA nanostructures. This chemo-mechanical modulation of DNA nanostructures would provide a powerful tool for reconfigurable and dynamic actuation of DNA machineries.
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- 2021
4. Small-molecule compounds boost genome-editing efficiency of cytosine base editor
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Zongming Song, Qing Li, Chenchen Zhou, Xiaoyu Liu, Na Tang, Feng Gu, Haoyi Wang, Hongyan Liu, Junzhao Zhao, Jinsong Li, Tianxiang Tu, Xiujuan Lv, Yanbo Cheng, Changbao Liu, and Tianyuan Zhao
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Zygote ,AcademicSubjects/SCI00010 ,T-Lymphocytes ,Computational biology ,Biology ,Histone Deacetylase 6 ,Hydroxamic Acids ,medicine.disease_cause ,Small Molecule Libraries ,Cytosine ,Mice ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Genome editing ,Genetics ,medicine ,Animals ,Humans ,Stargardt Disease ,Gene ,030304 developmental biology ,Gene Editing ,0303 health sciences ,Mutation ,Pathogenic mutation ,Phenylurea Compounds ,Ricolinostat ,Base (topology) ,Small molecule ,HEK293 Cells ,Pyrimidines ,chemistry ,ATP-Binding Cassette Transporters ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery - Abstract
Cytosine base editor (CBE) enables targeted C-to-T conversions at single base-pair resolution and thus has potential therapeutic applications in humans. However, the low efficiency of the system limits practical use of this approach. We reported a high-throughput human cells-based reporter system that can be harnessed for quickly measuring editing activity of CBE. Screening of 1813 small-molecule compounds resulted in the identification of Ricolinostat (an HDAC6 inhibitor) that can enhance the efficiency of BE3 in human cells (2.45- to 9.21-fold improvement). Nexturastat A, another HDAC6 inhibitor, could also increase BE3-mediated gene editing by 2.18- to 9.95-fold. Ricolinostat and Nexturastat A also boost base editing activity of the other CBE variants (BE4max, YE1-BE4max, evoAPOBEC1-BE4max and SpRY-CBE4max, up to 8.32-fold). Meanwhile, combined application of BE3 and Ricolinostat led to >3-fold higher efficiency of correcting a pathogenic mutation in ABCA4 gene related to Stargardt disease in human cells. Moreover, we demonstrated that our strategy could be applied for efficient generation of mouse models through direct zygote injection and base editing in primary human T cells. Our study provides a new strategy to improve the activity and specificity of CBE in human cells. Ricolinostat and Nexturastat A augment the effectiveness and applicability of CBE.
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- 2021
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5. Efficient multiplexed gene regulation in Saccharomyces cerevisiae using dCas12a
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René Verwaal, Klaudia W Ciurkot, Thomas E. Gorochowski, and Johannes Andries Roubos
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AcademicSubjects/SCI00010 ,CRISPR-Associated Proteins ,Green Fluorescent Proteins ,Nuclear Localization Signals ,Saccharomyces cerevisiae ,Down-Regulation ,BrisSynBio ,Computational biology ,Biology ,03 medical and health sciences ,0302 clinical medicine ,Protein Domains ,Genetics ,NLS ,CRISPR ,Guide RNA ,Promoter Regions, Genetic ,Gene ,030304 developmental biology ,Trans-activating crRNA ,Regulation of gene expression ,0303 health sciences ,Reporter gene ,Endodeoxyribonucleases ,Bristol BioDesign Institute ,beta Carotene ,biology.organism_classification ,Gene Expression Regulation ,RNA ,RNA Polymerase II ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery - Abstract
CRISPR Cas12a is an RNA-programmable endonuclease particularly suitable for gene regulation. This is due to its preference for T-rich PAMs that allows it to more easily target AT-rich promoter sequences, and built-in RNase activity which can process a single CRISPR RNA array encoding multiple spacers into individual guide RNAs (gRNAs), thereby simplifying multiplexed gene regulation. Here, we develop a flexible dCas12a-based CRISPRi system for Saccharomyces cerevisiae and systematically evaluate its design features. This includes the role of the NLS position, use of repression domains, and the position of the gRNA target. Our optimal system is comprised of dCas12a E925A with a single C-terminal NLS and a Mxi1 or a MIG1 repression domain, which enables up to 97% downregulation of a reporter gene. We also extend this system to allow for inducible regulation via an RNAP II-controlled promoter, demonstrate position-dependent effects in crRNA arrays, and use multiplexed regulation to stringently control a heterologous β-carotene pathway. Together these findings offer valuable insights into the design constraints of dCas12a-based CRISPRi and enable new avenues for flexible and efficient gene regulation in S. cerevisiae.
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- 2021
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6. Optimizing protein V untranslated region sequence in M13 phage for increased production of single-stranded DNA for origami
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Min Kyu Oh, Seungwoo Lee, Bo Young Lee, Dong June Ahn, and Jaewon Lee
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Untranslated region ,AcademicSubjects/SCI00010 ,DNA, Single-Stranded ,02 engineering and technology ,Biology ,Virus Replication ,010402 general chemistry ,medicine.disease_cause ,01 natural sciences ,Viral Proteins ,chemistry.chemical_compound ,Escherichia coli ,Genetics ,medicine ,DNA origami ,Inducer ,Mutation ,M13 bacteriophage ,021001 nanoscience & nanotechnology ,biology.organism_classification ,0104 chemical sciences ,Cell biology ,DNA-Binding Proteins ,chemistry ,Rolling circle replication ,Fermentation ,Synthetic Biology and Bioengineering ,5' Untranslated Regions ,0210 nano-technology ,DNA ,Bacteriophage M13 - Abstract
DNA origami requires long scaffold DNA to be aligned with the guidance of short staple DNA strands. Scaffold DNA is produced in Escherichia coli as a form of the M13 bacteriophage by rolling circle amplification (RCA). This study shows that RCA can be reconfigured by reducing phage protein V (pV) expression, improving the production throughput of scaffold DNA by at least 5.66-fold. The change in pV expression was executed by modifying the untranslated region sequence and monitored using a reporter green fluorescence protein fused to pV. In a separate experiment, pV expression was controlled by an inducer. In both experiments, reduced pV expression was correlated with improved M13 bacteriophage production. High-cell-density cultivation was attempted for mass scaffold DNA production, and the produced scaffold DNA was successfully folded into a barrel shape without compromising structural quality. This result suggested that scaffold DNA production throughput can be significantly improved by reprogramming the RCA in E. coli.
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- 2021
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7. Topologies of synthetic gene circuit for optimal fold change activation
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Ramez Daniel, Ximing Li, Natalia Barger, and Phyana Litovco
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AcademicSubjects/SCI00010 ,Repressor ,Computational biology ,Biology ,03 medical and health sciences ,SOS Response (Genetics) ,0302 clinical medicine ,Transcription (biology) ,Narese/1 ,Escherichia coli ,Genes, Synthetic ,Genetics ,Gene Regulatory Networks ,SOS response ,Promoter Regions, Genetic ,Gene ,030304 developmental biology ,Feedback, Physiological ,0303 health sciences ,Feed forward ,Promoter ,Fold change ,Gene Expression Regulation ,Synthetic Biology ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery - Abstract
Computations widely exist in biological systems for functional regulations. Recently, incoherent feedforward loop and integral feedback controller have been implemented into Escherichia coli to achieve a robust adaptation. Here, we demonstrate that an indirect coherent feedforward loop and mutual inhibition designs can experimentally improve the fold change of promoters, by reducing the basal level while keeping the maximum activity high. We applied both designs to six different promoters in E. coli, starting with synthetic inducible promoters as a proof-of-principle. Then, we examined native promoters that are either functionally specific or systemically involved in complex pathways such as oxidative stress and SOS response. Both designs include a cascade having a repressor and a construct of either transcriptional interference or antisense transcription. In all six promoters, an improvement of up to ten times in the fold change activation was observed. Theoretically, our unitless models show that when regulation strength matches promoter basal level, an optimal fold change can be achieved. We expect that this methodology can be applied in various biological systems for biotechnology and therapeutic applications.
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- 2021
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8. Rational engineering of a modular bacterial CRISPR–Cas activation platform with expanded target range
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Maria Claudia Villegas Kcam, Annette J Tsong, and James Chappell
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Gene Editing ,Transcriptional Activation ,Flexibility (engineering) ,Bacteria ,AcademicSubjects/SCI00010 ,business.industry ,Modularity (biology) ,Computational biology ,Protein engineering ,Biology ,Modular design ,Protein Engineering ,Protein Domains ,Component (UML) ,Genetics ,CRISPR ,Clustered Regularly Interspaced Short Palindromic Repeats ,CRISPR-Cas Systems ,Transcription (software) ,Synthetic Biology and Bioengineering ,business ,Phylogeny ,Function (biology) ,Protein Binding ,RNA, Guide, Kinetoplastida - Abstract
CRISPR–Cas activator (CRISPRa) systems that selectively turn on transcription of a target gene are a potentially transformative technology for programming cellular function. While in eukaryotes versatile CRISPRa systems exist, in bacteria these systems suffer from a limited ability to activate different genes due to strict distance-dependent requirements of functional target binding sites, and require greater customization to optimize performance in different genetic and cellular contexts. To address this, we apply a rational protein engineering approach to create a new CRISPRa platform that is highly modular to allow for easy customization and has increased targeting flexibility through harnessing engineered Cas proteins. We first demonstrate that transcription activation domains can be recruited by CRISPR–Cas through noncovalent protein-protein interactions, which allows each component to be encoded on separate and easily interchangeable plasmid elements. We then exploit this modularity to rapidly screen a library of different activation domains, creating new systems with distinct regulatory properties. Furthermore, we demonstrate that by harnessing a library of circularly permuted Cas proteins, we can create CRISPRa systems that have different target binding site requirements, which together, allow for expanded target range.
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- 2021
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9. Small-molecule inhibitors of histone deacetylase improve CRISPR-based adenine base editing
- Author
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Ji-Eun See, Gayoung Jang, Yongsub Kim, Gi-Jun Sung, Kyung-Chul Choi, Jin-Soo Kim, Inki Kim, Heon Seok Kim, Ha Rim Shin, Jiyeon Kweon, An-Hee Jang, and Sojung Park
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AcademicSubjects/SCI00010 ,Green Fluorescent Proteins ,Computational biology ,Biology ,Genome engineering ,Romidepsin ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Depsipeptides ,Genetics ,medicine ,Humans ,CRISPR ,Nucleotide ,030304 developmental biology ,Gene Editing ,chemistry.chemical_classification ,0303 health sciences ,Luminescent Agents ,Adenine ,Small molecule ,Histone Deacetylase Inhibitors ,HEK293 Cells ,chemistry ,Doxycycline ,Protein Biosynthesis ,RNA ,Histone deacetylase ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,Cytosine ,DNA ,HeLa Cells ,medicine.drug - Abstract
CRISPR-based base editors (BEs) are widely used to induce nucleotide substitutions in living cells and organisms without causing the damaging DNA double-strand breaks and DNA donor templates. Cytosine BEs that induce C:G to T:A conversion and adenine BEs that induce A:T to G:C conversion have been developed. Various attempts have been made to increase the efficiency of both BEs; however, their activities need to be improved for further applications. Here, we describe a fluorescent reporter-based drug screening platform to identify novel chemicals with the goal of improving adenine base editing efficiency. The reporter system revealed that histone deacetylase inhibitors, particularly romidepsin, enhanced base editing efficiencies by up to 4.9-fold by increasing the expression levels of proteins and target accessibility. The results support the use of romidepsin as a viable option to improve base editing efficiency in biomedical research and therapeutic genome engineering.
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- 2021
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10. A supernumerary designer chromosome for modular in vivo pathway assembly in Saccharomyces cerevisiae
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Pascale Daran-Lapujade, Sofia Dashko, Jean-Marc Daran, Marcel van den Broek, Eline D. Postma, Shannara K. Taylor Parkins, and Lars van Breemen
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AcademicSubjects/SCI00010 ,Computer science ,In silico ,Cell ,Saccharomyces cerevisiae ,Computational biology ,Genome ,Chromosomes ,Genome engineering ,03 medical and health sciences ,chemistry.chemical_compound ,Narese/1 ,medicine ,Genetics ,Cell Engineering ,030304 developmental biology ,0303 health sciences ,biology ,030306 microbiology ,business.industry ,Chromosome ,Modular design ,biology.organism_classification ,Transformation (genetics) ,ComputingMethodologies_PATTERNRECOGNITION ,medicine.anatomical_structure ,chemistry ,Synthetic Biology and Bioengineering ,business ,Homologous recombination ,Glycolysis ,DNA - Abstract
The construction of microbial cell factories for sustainable production of chemicals and pharmaceuticals requires extensive genome engineering. UsingSaccharomyces cerevisiae, this study proposes Synthetic Chromosomes (SynChs) as orthogonal expression platforms for rewiring native cellular processes and implementing new functionalities. Capitalizing the powerful homologous recombination capability ofS. cerevisiae, modular SynChs of 50 and 100 Kb were fully assembledde novofrom up to 44 transcriptional-unit-sized fragments in a single transformation. These assemblies were remarkably efficient and faithful to theirin silicodesign. SynChs made of non-coding DNA were stably replicated and segregated irrespective of their size without affecting the physiology of their host. These non-coding SynChs were successfully used as landing pad and as exclusive expression platform for the essential glycolytic pathway. This work pushes the limit of DNA assembly inS. cerevisiaeand paves the way forde novodesigner chromosomes as modular genome engineering platforms inS. cerevisiae.
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- 2021
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11. Precise and broad scope genome editing based on high-specificity Cas9 nickases
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Jin Liu, Manuel A F V Gonçalves, Richard L. Frock, Marie Le Bouteiller, Qian Wang, and Josephine M. Janssen
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Genotyping Techniques ,Base pair ,AcademicSubjects/SCI00010 ,Streptococcus pyogenes ,Induced Pluripotent Stem Cells ,Computational biology ,Transfection ,Genome ,Substrate Specificity ,03 medical and health sciences ,Gene Knockout Techniques ,0302 clinical medicine ,Genome editing ,Bacterial Proteins ,Genes, Reporter ,CRISPR-Associated Protein 9 ,Heterochromatin ,Genetics ,CRISPR ,Deoxyribonuclease I ,Humans ,Gene Knock-In Techniques ,Gene ,030304 developmental biology ,Gene Editing ,0303 health sciences ,Nuclease ,Polymorphism, Genetic ,biology ,Base Sequence ,Cas9 ,High-Throughput Nucleotide Sequencing ,Recombinant Proteins ,Clone Cells ,HEK293 Cells ,biology.protein ,Narese/29 ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,HeLa Cells ,RNA, Guide, Kinetoplastida - Abstract
RNA-guided nucleases (RGNs) based on CRISPR systems permit installing short and large edits within eukaryotic genomes. However, precise genome editing is often hindered due to nuclease off-target activities and the multiple-copy character of the vast majority of chromosomal sequences. Dual nicking RGNs and high-specificity RGNs both exhibit low off-target activities. Here, we report that high-specificity Cas9 nucleases are convertible into nicking Cas9D10A variants whose precision is superior to that of the commonly used Cas9D10A nickase. Dual nicking RGNs based on a selected group of these Cas9D10A variants can yield gene knockouts and gene knock-ins at frequencies similar to or higher than those achieved by their conventional counterparts. Moreover, high-specificity dual nicking RGNs are capable of distinguishing highly similar sequences by ‘tiptoeing’ over pre-existing single base-pair polymorphisms. Finally, high-specificity RNA-guided nicking complexes generally preserve genomic integrity, as demonstrated by unbiased genome-wide high-throughput sequencing assays. Thus, in addition to substantially enlarging the Cas9 nickase toolkit, we demonstrate the feasibility in expanding the range and precision of DNA knockout and knock-in procedures. The herein introduced tools and multi-tier high-specificity genome editing strategies might be particularly beneficial whenever predictability and/or safety of genetic manipulations are paramount.
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- 2021
12. Programmable gene regulation for metabolic engineering using decoy transcription factor binding sites
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Mary J. Dunlop, Nathan Tague, Tiebin Wang, and Stephen A. Whelan
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0106 biological sciences ,AcademicSubjects/SCI00010 ,Gene Dosage ,medicine.disease_cause ,01 natural sciences ,environment and public health ,chemistry.chemical_compound ,Gene expression ,Genes, Synthetic ,Lac Repressors ,skin and connective tissue diseases ,Promoter Regions, Genetic ,Bicyclic Monoterpenes ,Regulation of gene expression ,0303 health sciences ,Mutation ,Chemistry ,Escherichia coli Proteins ,Cell biology ,Metabolic Engineering ,Decoy ,Synthetic Biology and Bioengineering ,Protein Binding ,Biology ,Arginine ,Binding, Competitive ,03 medical and health sciences ,Bacterial Proteins ,010608 biotechnology ,Drug Resistance, Bacterial ,Genetics ,medicine ,Escherichia coli ,Binding site ,Gene ,Transcription factor ,030304 developmental biology ,Binding Sites ,Base Sequence ,Molecular Mimicry ,biological factors ,DNA binding site ,Repressor Proteins ,Gene Expression Regulation ,Mutagenesis ,Drug Design ,health occupations ,Trans-Activators ,DNA ,Transcription Factors - Abstract
Transcription factor decoy binding sites are short DNA sequences that can serve as “sponges” to titrate a transcription factor away from its natural binding site, therefore regulating gene expression. In this study, we harness decoy sites to develop synthetic transcription factor sponge systems to regulate gene expression for metabolic pathways in Escherichia coli. We show that transcription factor sponges can effectively regulate expression of native and heterologous genes. Tunability of the sponge can be engineered via changes in copy number or modifications to the DNA decoy site sequence. Using arginine biosynthesis as a showcase, we observe a 16-fold increase in arginine production when we introduce the sponge system to steer metabolic flux towards increased arginine biosynthesis, with negligible growth differences compared to the wild type strain. The sponge-based production strain shows high genetic stability; in contrast to a gene knock-out approach where mutations were common, we detected no mutations in the production system using the sponge-based strain. We further show that transcription factor sponges are amenable to multiplexed library screening by demonstrating enhanced tolerance to pinene with a combinatorial sponge library. Our study shows that transcription factor sponges are a powerful and compact tool for metabolic engineering.
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- 2020
13. Stretching DNA origami: effect of nicks and Holliday junctions on the axial stiffness
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Stavros Gaitanaros, Enze Chen, Remi Veneziano, Wei-Hung Jung, and Yun Chen
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Polynucleotide 5'-Hydroxyl-Kinase ,AcademicSubjects/SCI00010 ,DNA, Single-Stranded ,02 engineering and technology ,Biology ,Molecular physics ,03 medical and health sciences ,chemistry.chemical_compound ,Genetics ,Holliday junction ,Fluid dynamics ,medicine ,DNA origami ,Elasticity (economics) ,030304 developmental biology ,0303 health sciences ,DNA, Cruciform ,Stiffness ,021001 nanoscience & nanotechnology ,Elasticity ,Biomechanical Phenomena ,Nanostructures ,chemistry ,DNA, Viral ,Thermodynamics ,Elastic rods ,medicine.symptom ,0210 nano-technology ,Synthetic Biology and Bioengineering ,Order of magnitude ,DNA ,Bacteriophage M13 - Abstract
The axial stiffness of DNA origami is determined as a function of key nanostructural characteristics. Different constructs of two-helix nanobeams with specified densities of nicks and Holliday junctions are synthesized and stretched by fluid flow. Implementing single particle tracking to extract force–displacement curves enables the measurement of DNA origami stiffness values at the enthalpic elasticity regime, i.e. for forces larger than 15 pN. Comparisons between ligated and nicked helices show that the latter exhibit nearly a two-fold decrease in axial stiffness. Numerical models that treat the DNA helices as elastic rods are used to evaluate the local loss of stiffness at the locations of nicks and Holliday junctions. It is shown that the models reproduce the experimental data accurately, indicating that both of these design characteristics yield a local stiffness two orders of magnitude smaller than the corresponding value of the intact double-helix. This local degradation in turn leads to a macroscopic loss of stiffness that is evaluated numerically for multi-helix DNA bundles.
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- 2020
14. The immunorecognition, subcellular compartmentalization, and physicochemical properties of nucleic acid nanoparticles can be controlled by composition modification
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Daniel K. Miller, Joseph S Cooper, Emil F. Khisamutdinov, Morgan Brittany Johnson, Justin R. Halman, Ian Marriott, and Kirill A. Afonin
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AcademicSubjects/SCI00010 ,Cell ,Oligonucleotides ,02 engineering and technology ,Biology ,Proinflammatory cytokine ,Cell Line ,03 medical and health sciences ,chemistry.chemical_compound ,Immune system ,Genetics ,medicine ,Humans ,030304 developmental biology ,0303 health sciences ,Innate immune system ,NF-kappa B ,RNA ,Biological Transport ,TLR7 ,DNA ,021001 nanoscience & nanotechnology ,Cell biology ,medicine.anatomical_structure ,chemistry ,Interferon Regulatory Factors ,Nucleic acid ,Cytokines ,Nanoparticles ,Thermodynamics ,0210 nano-technology ,Synthetic Biology and Bioengineering - Abstract
Nucleic acid nanoparticles (NANPs) have become powerful new platforms as therapeutic and diagnostic tools due to the innate biological ability of nucleic acids to identify target molecules or silence genes involved in disease pathways. However, the clinical application of NANPs has been limited by factors such as chemical instability, inefficient intracellular delivery, and the triggering of detrimental inflammatory responses following innate immune recognition of nucleic acids. Here, we have studied the effects of altering the chemical composition of a circumscribed panel of NANPs that share the same connectivity, shape, size, charge and sequences. We show that replacing RNA strands with either DNA or chemical analogs increases the enzymatic and thermodynamic stability of NANPs. Furthermore, we have found that such composition changes affect delivery efficiency and determine subcellular localization, effects that could permit the targeted delivery of NANP-based therapeutics and diagnostics. Importantly, we have determined that altering NANP composition can dictate the degree and mechanisms by which cell immune responses are initiated. While RNA NANPs trigger both TLR7 and RIG-I mediated cytokine and interferon production, DNA NANPs stimulate minimal immune activation. Importantly, incorporation of 2′F modifications abrogates RNA NANP activation of TLR7 but permits RIG-I dependent immune responses. Furthermore, 2′F modifications of DNA NANPs significantly enhances RIG-I mediated production of both proinflammatory cytokines and interferons. Collectively this indicates that off-target effects may be reduced and/or desirable immune responses evoked based upon NANPs modifications. Together, our studies show that NANP composition provides a simple way of controlling the immunostimulatory potential, and physicochemical and delivery characteristics, of such platforms.
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- 2020
15. Engineered signal-coupled inducible promoters: measuring the apparent RNA-polymerase resource budget
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James A. Davey and Corey J. Wilson
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Isopropyl Thiogalactoside ,AcademicSubjects/SCI00010 ,Green Fluorescent Proteins ,Computational biology ,Lac repressor ,Biology ,Metabolic engineering ,03 medical and health sciences ,chemistry.chemical_compound ,Synthetic biology ,RNA polymerase ,Escherichia coli ,Lac Repressors ,Genetics ,Protein biosynthesis ,Promoter Regions, Genetic ,Transcription factor ,030304 developmental biology ,0303 health sciences ,030302 biochemistry & molecular biology ,Promoter ,DNA-Directed RNA Polymerases ,Living systems ,chemistry ,Genetic Engineering ,Synthetic Biology and Bioengineering - Abstract
Inducible promoters are a central regulatory component in synthetic biology, metabolic engineering, and protein production for laboratory and commercial uses. Many of these applications utilize two or more exogenous promoters, imposing a currently unquantifiable metabolic burden on the living system. Here, we engineered a collection of inducible promoters (regulated by LacI-based transcription factors) that maximize the free-state of endogenous RNA polymerase (RNAP). We leveraged this collection of inducible promotors to construct simple two-channel logical controls that enabled us to measure metabolic burden – as it relates to RNAP resource partitioning. The two-channel genetic circuits utilized sets of signal-coupled transcription factors that regulate cognate inducible promoters in a coordinated logical fashion. With this fundamental genetic architecture, we evaluated the performance of each inducible promoter as discrete operations, and as coupled systems to evaluate and quantify the effects of resource partitioning. Obtaining the ability to systematically and accurately measure the apparent RNA-polymerase resource budget will enable researchers to design more robust genetic circuits, with significantly higher fidelity. Moreover, this study presents a workflow that can be used to better understand how living systems adapt RNAP resources, via the complementary pairing of constitutive and regulated promoters that vary in strength.
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- 2020
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16. Unbiased investigation of specificities of prime editing systems in human cells
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Daesik Kim, Do Yon Kim, Yong Sam Kim, Su Bin Moon, and Jeong Heon Ko
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AcademicSubjects/SCI00010 ,Computational biology ,Biology ,medicine.disease_cause ,Genome ,03 medical and health sciences ,0302 clinical medicine ,Plasmid ,Genome editing ,CRISPR-Associated Protein 9 ,Genetics ,medicine ,CRISPR ,Humans ,DNA Breaks, Single-Stranded ,030304 developmental biology ,Whole genome sequencing ,Gene Editing ,0303 health sciences ,Mutation ,Whole Genome Sequencing ,Cas9 ,Genome, Human ,Human genetics ,Narese/29 ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery - Abstract
Prime editors (PEs) enable targeted precise editing, including the generation of substitutions, insertions and deletions, in eukaryotic genomes. However, their genome-wide specificity has not been explored. Here, we developed Nickase-based Digenome-seq (nDigenome-seq), an in vitro assay that uses whole-genome sequencing to identify single-strand breaks induced by CRISPR (clustered regularly interspaced short palindromic repeats)-Cas9 (CRISPR-associated protein 9) nickase. We used nDigenome-seq to screen for potential genome-wide off-target sites of Cas9 H840A nickase, a PE component, targeted to nine human genomic sites. Then, using targeted amplicon sequencing of off-target candidates identified by nDigenome-seq, we showed that only five off-target sites showed detectable PE-induced modifications in cells, at frequencies ranging from 0.1 to 1.9%, suggesting that PEs provide a highly specific method of precise genome editing. We also found that PE specificity in human cells could be further improved by incorporating mutations from engineered Cas9 variants, particularly eSpCas9 and Sniper Cas9, into PE.
- Published
- 2020
17. Programmable cross-ribosome-binding sites to fine-tune the dynamic range of transcription factor-based biosensor
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Zhenqi Yuan, Yu Deng, Shenghu Zhou, Jing Chen, Xiaojuan Zhang, and Nana Ding
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Regulation of gene expression ,Binding Sites ,business.industry ,Dynamic range ,AcademicSubjects/SCI00010 ,Deep learning ,Translation (biology) ,Biosensing Techniques ,Gene Expression Regulation, Bacterial ,Biology ,Regulatory Sequences, Nucleic Acid ,Convolutional neural network ,Fold change ,Genetics ,Escherichia coli ,Protein folding ,Artificial intelligence ,Biological system ,business ,Synthetic Biology and Bioengineering ,Promoter Regions, Genetic ,Biosensor ,Ribosomes ,Transcription Factors - Abstract
Currently, predictive translation tuning of regulatory elements to the desired output of transcription factor (TF)-based biosensors remains a challenge. The gene expression of a biosensor system must exhibit appropriate translation intensity, which is controlled by the ribosome-binding site (RBS), to achieve fine-tuning of its dynamic range (i.e. fold change in gene expression between the presence and absence of inducer) by adjusting the translation level of the TF and reporter. However, existing TF-based biosensors generally suffer from unpredictable dynamic range. Here, we elucidated the connections and partial mechanisms between RBS, translation level, protein folding and dynamic range, and presented a design platform that predictably tuned the dynamic range of biosensors based on deep learning of large datasets cross-RBSs (cRBSs). In doing so, a library containing 7053 designed cRBSs was divided into five sub-libraries through fluorescence-activated cell sorting to establish a classification model based on convolutional neural network in deep learning. Finally, the present work exhibited a powerful platform to enable predictable translation tuning of RBS to the dynamic range of biosensors.
- Published
- 2020
18. Near-infrared-traceable DNA nano-hydrolase: specific eradication of telomeric G-overhang in vivo
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Xiaogang Qu, Yuhuan Sun, Hongshuang Qin, Jinsong Ren, Chuanqi Zhao, Jingsheng Niu, and Tingting Cui
- Subjects
AcademicSubjects/SCI00010 ,genetic processes ,Cell ,Antineoplastic Agents ,Biology ,010402 general chemistry ,G-quadruplex ,01 natural sciences ,Dexamethasone ,Mice ,03 medical and health sciences ,chemistry.chemical_compound ,Complementary DNA ,Hydrolase ,Organometallic Compounds ,Genetics ,medicine ,Animals ,Humans ,030304 developmental biology ,0303 health sciences ,Hydrolysis ,Cerium ,Neoplasms, Experimental ,Telomere ,0104 chemical sciences ,Cell biology ,G-Quadruplexes ,enzymes and coenzymes (carbohydrates) ,Cell nucleus ,medicine.anatomical_structure ,chemistry ,Cancer cell ,MCF-7 Cells ,Nanoparticles ,Synthetic Biology and Bioengineering ,Cell aging ,DNA - Abstract
Telomeric DNA, whose length homeostasis is closely correlated with immortality of cancer cells, is regarded as a molecular clock for cellular lifespan. Regarding the capacity in forming G-quadruplex, G-rich 3′-overhang (G-overhang) has been considered as an attractive anticancer target. However, it is still challenging to precisely target telomeric G-overhang with current ligands because of the polymorphism of G-quadruplexes in cells. Herein, we construct a telomeric G-overhang-specific near-infrared-traceable DNA nano-hydrolase, which is composed of four parts: (i) dexamethasone for targeting cell nuclei; (ii) complementary DNA for hybridizing with G-overhang; (iii) multinuclear Ce(IV) complexes for hydrolyzing G-overhang; and (iv) upconversion nanoparticles for real-time tracking. The multivalent targeted DNA nano-hydrolase can be traced to precisely digest telomeric G-overhang, which contributes to telomeric DNA shortening and thereby causes cell aging and apoptosis. The anticancer treatment is further proved by in vivo studies. In this way, this design provides a telomeric G-overhang-specific eradication strategy based on a non-G-quadruplex targeting manner.
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- 2020
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19. Developing an endogenous quorum-sensing based CRISPRi circuit for autonomous and tunable dynamic regulation of multiple targets in Streptomyces
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Yinhua Lu, Gaohua Yang, Yang Gu, Xinqiang Sun, Jinzhong Tian, and Weihong Jiang
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Sirolimus ,0106 biological sciences ,Regulation of gene expression ,0303 health sciences ,AcademicSubjects/SCI00010 ,Quorum Sensing ,Endogeny ,Gene Expression Regulation, Bacterial ,Computational biology ,Biology ,biology.organism_classification ,01 natural sciences ,Streptomyces ,Industrial Microbiology ,03 medical and health sciences ,Quorum sensing ,Narese/1 ,010608 biotechnology ,Growth arrest ,Genetics ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,Flux (metabolism) ,030304 developmental biology - Abstract
Quorum-sensing (QS) mediated dynamic regulation has emerged as an effective strategy for optimizing product titers in microbes. However, these QS-based circuits are often created on heterologous systems and require careful tuning via a tedious testing/optimization process. This hampers their application in industrial microbes. Here, we design a novel QS circuit by directly integrating an endogenous QS system with CRISPRi (named EQCi) in the industrial rapamycin-producing strain Streptomyces rapamycinicus. EQCi combines the advantages of both the QS system and CRISPRi to enable tunable, autonomous, and dynamic regulation of multiple targets simultaneously. Using EQCi, we separately downregulate three key nodes in essential pathways to divert metabolic flux towards rapamycin biosynthesis and significantly increase its titers. Further application of EQCi to simultaneously regulate these three key nodes with fine-tuned repression strength boosts the rapamycin titer by ∼660%, achieving the highest reported titer (1836 ± 191 mg/l). Notably, compared to static engineering strategies, which result in growth arrest and suboptimal rapamycin titers, EQCi-based regulation substantially promotes rapamycin titers without affecting cell growth, indicating that it can achieve a trade-off between essential pathways and product synthesis. Collectively, this study provides a convenient and effective strategy for strain improvement and shows potential for application in other industrial microorganisms.
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- 2020
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20. Highly efficient ‘hit-and-run’ genome editing with unconcentrated lentivectors carrying Vpr.Prot.Cas9 protein produced from RRE-containing transcripts
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Ivana Indikova and Stanislav Indik
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AcademicSubjects/SCI00010 ,THP-1 Cells ,viruses ,Transgene ,Genetic Vectors ,Green Fluorescent Proteins ,Biology ,Response Elements ,Transduction (genetics) ,Endonuclease ,Genome editing ,Transduction, Genetic ,CRISPR-Associated Protein 9 ,Genetics ,Humans ,Gene ,Gene Editing ,Lentivirus ,HEK 293 cells ,Fusion protein ,Cell biology ,HEK293 Cells ,Cell culture ,Narese/29 ,biology.protein ,Nanoparticles ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering - Abstract
The application of gene-editing technology is currently limited by the lack of safe and efficient methods to deliver RNA-guided endonucleases to target cells. We engineered lentivirus-based nanoparticles to co-package the U6-sgRNA template and the CRISPR-associated protein 9 (Cas9) fused with a virion-targeted protein Vpr (Vpr.Prot.Cas9), for simultaneous delivery to cells. Equal spatiotemporal control of the vpr.prot.cas9 and gag/pol gene expression (the presence of Rev responsive element, RRE) greatly enhanced the encapsidation of the fusion protein and resulted in the production of highly efficient lentivector nanoparticles. Transduction of the unconcentrated, Vpr.Prot.Cas9-containing vectors led to >98% disruption of the EGFP gene in reporter HEK293-EGFP cells with minimal cytotoxicity. Furthermore, we detected indels in the targeted endogenous loci at frequencies of up to 100% in cell lines derived from lymphocytes and monocytes and up to 15% in primary CD4+ T cells by high-throughput sequencing. This approach may provide a platform for the efficient, dose-controlled and tissue-specific delivery of genome editing enzymes to cells and it may be suitable for simultaneous endogenous gene disruption and a transgene delivery.
- Published
- 2020
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21. Toward a translationally independent RNA-based synthetic oscillator using deactivated CRISPR-Cas
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James Kuo, Ruoshi Yuan, Johan Paulsson, Pamela A. Silver, and Carlos Sánchez
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Periodicity ,AcademicSubjects/SCI00010 ,CRISPR-Associated Proteins ,Microfluidics ,Biology ,03 medical and health sciences ,0302 clinical medicine ,Bacterial Proteins ,Transcription (biology) ,CRISPR-Associated Protein 9 ,Escherichia coli ,Genetics ,Transcriptional regulation ,CRISPR ,Guide RNA ,030304 developmental biology ,Electronic circuit ,0303 health sciences ,Endodeoxyribonucleases ,Cas9 ,RNA ,Logic gate ,CRISPR-Cas Systems ,Single-Cell Analysis ,Synthetic Biology and Bioengineering ,Biological system ,030217 neurology & neurosurgery ,RNA, Guide, Kinetoplastida - Abstract
In synthetic circuits, CRISPR-Cas systems have been used effectively for endpoint changes from an initial state to a final state, such as in logic gates. Here, we use deactivated Cas9 (dCas9) and deactivated Cas12a (dCas12a) to construct dynamic RNA ring oscillators that cycle continuously between states over time in bacterial cells. While our dCas9 circuits using 103-nt guide RNAs showed irregular fluctuations with a wide distribution of peak-to-peak period lengths averaging approximately nine generations, a dCas12a oscillator design with 40-nt CRISPR RNAs performed much better, having a strongly repressed off-state, distinct autocorrelation function peaks, and an average peak-to-peak period length of ∼7.5 generations. Along with free-running oscillator circuits, we measure repression response times in open-loop systems with inducible RNA steps to compare with oscillator period times. We track thousands of cells for 24+ h at the single-cell level using a microfluidic device. In creating a circuit with nearly translationally independent behavior, as the RNAs control each others’ transcription, we present the possibility for a synthetic oscillator generalizable across many organisms and readily linkable for transcriptional control.
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- 2020
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22. CRISPR–Cas12a system in fission yeast for multiplex genomic editing and CRISPR interference
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Yu Zhao and Jef D. Boeke
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Gene Editing ,Trans-activating crRNA ,CRISPR interference ,Deoxyribonucleases ,AcademicSubjects/SCI00010 ,CRISPR-Associated Proteins ,Computational biology ,Biology ,biology.organism_classification ,Genome ,Ribonucleases ,Genome editing ,Schizosaccharomyces ,Schizosaccharomyces pombe ,Narese/29 ,Genetics ,RNA ,CRISPR ,RNA Polymerase II ,Guide RNA ,CRISPR-Cas Systems ,Francisella ,Synthetic Biology and Bioengineering ,Promoter Regions, Genetic ,Gene - Abstract
The CRISPR–Cas12a is a class II, type V clustered regularly interspaced short palindromic repeat (CRISPR) system with both RNase and DNase activity. Compared to the CRISPR–Cas9 system, it recognizes T-rich PAM sequences and has the advantage of multiplex genomic editing. Here, in fission yeast Schizosaccharomyces pombe, we successfully implemented the CRISPR–Cas12a system for versatile genomic editing and manipulation. In addition to the rrk1 promoter, we used new pol II promoters from endogenous coding genes to express crRNA for Cas12a and obtained a much higher editing efficiency. This new design expands the promoter choices for potential applications in fission yeast and other organisms. In addition, we expressed a gRNA array using a strong constitutive pol II promoter. The array transcript is processed by Cas12a itself to release multiple mature crRNAs. With this construct, multiplex genomic editing of up to three loci was achieved from a single yeast transformation. We also built a CRISPR interference system using a DNase-dead Cas12a to significantly repress endogenous gene expression. Our study provides the first CRISPR-Cas12a toolkit for efficient and rapid genomic gene editing and regulation in fission yeast.
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- 2020
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23. Spatial organization-dependent EphA2 transcriptional responses revealed by ligand nanocalipers
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Verheyen, Toon, Fang, Trixy, Lindenhofer, Dominik, Wang, Yang, Akopyan, Karen, Lindqvist, Arne, Högberg, Björn, and Teixeira, Ana I
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Transcription, Genetic ,AcademicSubjects/SCI00010 ,Cell Line, Tumor ,Receptor, EphA2 ,Humans ,DNA ,RNA-Seq ,Phosphorylation ,Synthetic Biology and Bioengineering ,Ligands ,Ephrin-A5 ,Nanostructures - Abstract
Ligand binding induces extensive spatial reorganization and clustering of the EphA2 receptor at the cell membrane. It has previously been shown that the nanoscale spatial distribution of ligands modulates EphA2 receptor reorganization, activation and the invasive properties of cancer cells. However, intracellular signaling downstream of EphA2 receptor activation by nanoscale spatially distributed ligands has not been elucidated. Here, we used DNA origami nanostructures to control the positions of ephrin-A5 ligands at the nanoscale and investigated EphA2 activation and transcriptional responses following ligand binding. Using RNA-seq, we determined the transcriptional profiles of human glioblastoma cells treated with DNA nanocalipers presenting a single ephrin-A5 dimer or two dimers spaced 14, 40 or 100 nm apart. These cells displayed divergent transcriptional responses to the differing ephrin-A5 nano-organization. Specifically, ephrin-A5 dimers spaced 40 or 100 nm apart showed the highest levels of differential expressed genes compared to treatment with nanocalipers that do not present ephrin-A5. These findings show that the nanoscale organization of ephrin-A5 modulates transcriptional responses to EphA2 activation.
- Published
- 2020
24. Enabling large-scale genome editing at repetitive elements by reducing DNA nicking
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Raphael Ferreira, Marc Güell, Chun-Ting Wu, Khaled Said, Parastoo Khoshakhlagh, Verena Volf, Hannu Myllykallio, Cory Smith, Shilpa Garg, Amanda Hornick, Alex Hay-Man Ng, George M. Church, Oscar Castanon, Harvard School of Public Health, Laboratoire d'Optique et Biosciences (LOB), École polytechnique (X)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), Laboratoire de genetique, Biodiversité et Environnement (UR 09/30), Institut Supérieur de Biotechnologie de Monastir (ISBM), Université de Monastir - University of Monastir (UM)-Université de Monastir - University of Monastir (UM), Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM)-École polytechnique (X), Department of Genetics [Boston], Harvard Medical School [Boston] (HMS), Wyss Institute for Biologically Inspired Engineering [Harvard University], Harvard University [Cambridge], Harvard John A. Paulson School of Engineering and Applied Sciences (SEAS), Department of Biology and Biological Engineering, Chalmers University of Technology, Chalmers University of Technology [Gothenburg, Sweden], and Barcelona Biomedical Research Park (PRBB)
- Subjects
[SDV.BIO]Life Sciences [q-bio]/Biotechnology ,Retroelements ,AcademicSubjects/SCI00010 ,Cell Survival ,Cell ,CRISPR-Associated Proteins ,Induced Pluripotent Stem Cells ,Computational biology ,Biology ,medicine.disease_cause ,Genome ,Genome engineering ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Plasmid ,Genome editing ,Genetics ,medicine ,Humans ,[SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology ,Cell survival ,ComputingMilieux_MISCELLANEOUS ,030304 developmental biology ,Gene Editing ,0303 health sciences ,Mutation ,Endodeoxyribonucleases ,[SDV.BBM.BM]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Molecular biology ,medicine.anatomical_structure ,HEK293 Cells ,chemistry ,Narese/29 ,RNA ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,DNA - Abstract
To extend the frontier of genome editing and enable editing of repetitive elements of mammalian genomes, we made use of a set of dead-Cas9 base editor (dBE) variants that allow editing at tens of thousands of loci per cell by overcoming the cell death associated with DNA double-strand breaks and single-strand breaks. We used a set of gRNAs targeting repetitive elements—ranging in target copy number from about 32 to 161 000 per cell. dBEs enabled survival after large-scale base editing, allowing targeted mutations at up to ∼13 200 and ∼12 200 loci in 293T and human induced pluripotent stem cells (hiPSCs), respectively, three orders of magnitude greater than previously recorded. These dBEs can overcome current on-target mutation and toxicity barriers that prevent cell survival after large-scale genome engineering.
- Published
- 2020
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25. Mutational characterization and mapping of the 70S ribosome active site
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Antje Krüger, Tasfia Azim, Adam J. Hockenberry, Anne E. d’Aquino, Michael C. Jewett, and Nikolay A. Aleksashin
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Models, Molecular ,Peptidyl transferase ,Mutant ,Computational biology ,Biology ,010402 general chemistry ,medicine.disease_cause ,01 natural sciences ,Ribosome ,03 medical and health sciences ,Synthetic biology ,Catalytic Domain ,Escherichia coli ,Genetics ,Protein biosynthesis ,medicine ,Codon ,030304 developmental biology ,0303 health sciences ,Mutation ,Point mutation ,RNA ,0104 chemical sciences ,RNA, Ribosomal ,Polyribosomes ,Protein Biosynthesis ,Peptidyl Transferases ,biology.protein ,Synthetic Biology and Bioengineering ,Ribosomes - Abstract
The synthetic capability of the Escherichia coli ribosome has attracted efforts to repurpose it for novel functions, such as the synthesis of polymers containing non-natural building blocks. However, efforts to repurpose ribosomes are limited by the lack of complete peptidyl transferase center (PTC) active site mutational analyses to inform design. To address this limitation, we leverage an in vitro ribosome synthesis platform to build and test every possible single nucleotide mutation within the PTC-ring, A-loop and P-loop, 180 total point mutations. These mutant ribosomes were characterized by assessing bulk protein synthesis kinetics, readthrough, assembly, and structure mapping. Despite the highly-conserved nature of the PTC, we found that >85% of the PTC nucleotides possess mutational flexibility. Our work represents a comprehensive single-point mutant characterization and mapping of the 70S ribosome's active site. We anticipate that it will facilitate structure-function relationships within the ribosome and make possible new synthetic biology applications.
- Published
- 2020
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26. Secondary nucleotide messenger c-di-GMP exerts a global control on natural product biosynthesis in streptomycetes
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Roman Makitrynskyy, Olga Tsypik, Thomas Paululat, Desirèe Nuzzo, David L. Zechel, and Andreas Bechthold
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Streptomycetaceae ,Mutant ,Biology ,Second Messenger Systems ,Streptomyces ,03 medical and health sciences ,chemistry.chemical_compound ,Bacterial Proteins ,Guanosine monophosphate ,Genetics ,Synthetic bioengineering ,Cyclic GMP ,Gene ,Synthetic biology ,030304 developmental biology ,Regulator gene ,Regulation of gene expression ,Biological Products ,0303 health sciences ,Peptidoglycan glycosyltransferase ,Nucleotides ,030306 microbiology ,Escherichia coli Proteins ,Gene Expression Regulation, Bacterial ,biology.organism_classification ,Cell biology ,DNA-Binding Proteins ,Bambermycins ,chemistry ,biology.protein ,Diguanylate cyclase ,Peptidoglycan Glycosyltransferase ,Phosphorus-Oxygen Lyases ,Synthetic Biology and Bioengineering ,Gene Deletion ,Transcription Factors - Abstract
Cyclic dimeric 3′-5′ guanosine monophosphate, c-di-GMP, is a ubiquitous second messenger controlling diverse cellular processes in bacteria. In streptomycetes, c-di-GMP plays a crucial role in a complex morphological differentiation by modulating an activity of the pleiotropic regulator BldD. Here we report that c-di-GMP plays a key role in regulating secondary metabolite production in streptomycetes by altering the expression levels of bldD. Deletion of cdgB encoding a diguanylate cyclase in Streptomycesghanaensis reduced c-di-GMP levels and the production of the peptidoglycan glycosyltransferase inhibitor moenomycin A. In contrast to the cdgB mutant, inactivation of rmdB, encoding a phosphodiesterase for the c-di-GMP hydrolysis, positively correlated with the c-di-GMP and moenomycin A accumulation. Deletion of bldD adversely affected the synthesis of secondary metabolites in S. ghanaensis, including the production of moenomycin A. The bldD-deficient phenotype is partly mediated by an increase in expression of the pleiotropic regulatory gene wblA. Genetic and biochemical analyses demonstrate that a complex of c-di-GMP and BldD effectively represses transcription of wblA, thus preventing sporogenesis and sustaining antibiotic synthesis. These results show that manipulation of the expression of genes controlling c-di-GMP pool has the potential to improve antibiotic production as well as activate the expression of silent gene clusters.
- Published
- 2020
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27. Nucleic Acids Research
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Anne C Barbosa, Zhengyao Xu, Kazhal Karari, Wendi Williams, Silke Hauf, and William R A Brown
- Subjects
construction ,Base Sequence ,AcademicSubjects/SCI00010 ,neocentromeres ,requirement ,Centromere ,heterochromatin ,association ,rates ,cenp-a ,Chromatin ,complementation ,Narese/1 ,artificial chromosomes ,Schizosaccharomyces ,evolution ,Genetics ,DNA, Fungal ,Synthetic Biology and Bioengineering ,Repetitive Sequences, Nucleic Acid - Abstract
We have used chromosome engineering to replace native centromeric DNA with different test sequences at native centromeres in two different strains of the fission yeast Schizosaccharomyces pombe and have discovered that A + T rich DNA, whether synthetic or of bacterial origin, will function as a centromere in this species. Using genome size as a surrogate for the inverse of effective population size (N-e) we also show that the relative A + T content of centromeric DNA scales with N-e across 43 animal, fungal and yeast (Opisthokonta) species. This suggests that in most of these species the A + T content of the centromeric DNA is determined by a balance between selection and mutation. Combining the experimental results and the evolutionary analyses allows us to conclude that A + T rich DNA of almost any sequence will function as a centromere in most Opisthokonta species. The fact that many G/C to A/T substitutions are unlikely to be selected against may contribute to the rapid evolution of centromeric DNA. We also show that a neo-centromere sequence is not simply a weak version of native centromeric DNA and suggest that neo-centromeres require factors either for their propagation or establishment in addition to those required by native centromeres. BBSRC [BB/K003356/1]; Brazilian 'NottinghamBirmingham' PhD scheme by CAPES, Brazil; Kurdistan Regional Government, Human Capacity Development Program; National Institute of General Medical Sciences of the National Institutes of Health [R35GM119723]; University of Nottingham; OUP Published version Nottingham was supported by BBSRC [BB/K003356/1]; A.C.B. was funded by the Brazilian `NottinghamBirmingham' PhD scheme organised by CAPES, Brazil; K.K. was funded by the Kurdistan Regional Government, Human Capacity Development Program; S.H. and W.W. were supported by the National Institute of General Medical Sciences of the National Institutes of Health R35GM119723]. Funding for open access charge: University of Nottingham transformative agreement with OUP.
- Published
- 2022
28. Rational design and construction of multi-copy biomanufacturing islands in mammalian cells
- Author
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Raffaele Altamura, Jiten Doshi, and Yaakov Benenson
- Subjects
Mice ,Cricetulus ,AcademicSubjects/SCI00010 ,Narese/1 ,Gene Targeting ,Genetic Vectors ,Genetics ,Animals ,Humans ,CHO Cells ,Transgenes ,Synthetic Biology and Bioengineering ,Recombinant Proteins - Abstract
Cell line development is a critical step in the establishment of a biopharmaceutical manufacturing process. Current protocols rely on random transgene integration and amplification. Due to considerable variability in transgene integration profiles, this workflow results in laborious screening campaigns before stable producers can be identified. Alternative approaches for transgene dosage increase and integration are therefore highly desirable. In this study, we present a novel strategy for the rapid design, construction, and genomic integration of engineered multiple-copy gene constructs consisting of up to 10 gene expression cassettes. Key to this strategy is the diversification, at the sequence level, of the individual gene cassettes without altering their protein products. We show a computational workflow for coding and regulatory sequence diversification and optimization followed by experimental assembly of up to nine gene copies and a sentinel reporter on a contiguous scaffold. Transient transfections in CHO cells indicates that protein expression increases with the gene copy number on the scaffold. Further, we stably integrate these cassettes into a pre-validated genomic locus. Altogether, our findings point to the feasibility of engineering a fully mapped multi-copy recombinant protein ‘production island’ in a mammalian cell line with greatly reduced screening effort, improved stability, and predictable product titers., Nucleic Acids Research, 50 (1), ISSN:1362-4962, ISSN:0301-5610
- Published
- 2022
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29. Design of a programmable biosensor-CRISPRi genetic circuits for dynamic and autonomous dual-control of metabolic flux in Bacillus subtilis
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Yaokang Wu, Rongzhen Tian, Jian Chen, Xueqin Lv, Jianghua Li, Guocheng Du, Long Liu, Yanfeng Liu, Chen Taichi, and Rodrigo Ledesma-Amaro
- Subjects
0106 biological sciences ,05 Environmental Sciences ,Glucose-6-Phosphate ,Bacillus subtilis ,Biosensing Techniques ,Biology ,01 natural sciences ,Acetylglucosamine ,03 medical and health sciences ,chemistry.chemical_compound ,010608 biotechnology ,Genetics ,Bioreactor ,Inducer ,Clustered Regularly Interspaced Short Palindromic Repeats ,Gene Regulatory Networks ,030304 developmental biology ,0303 health sciences ,Glucosamine ,Acetoin ,Robustness (evolution) ,06 Biological Sciences ,biology.organism_classification ,Metabolic pathway ,Glucose ,chemistry ,Metabolic Engineering ,08 Information and Computing Sciences ,Biological system ,Synthetic Biology and Bioengineering ,Biosensor ,Flux (metabolism) ,Metabolic Networks and Pathways ,Developmental Biology - Abstract
Dynamic regulation is an effective strategy for fine-tuning metabolic pathways in order to maximize target product synthesis. However, achieving dynamic and autonomous up- and down-regulation of the metabolic modules of interest simultaneously, still remains a great challenge. In this work, we created an autonomous dual-control (ADC) system, by combining CRISPRi-based NOT gates with novel biosensors of a key metabolite in the pathway of interest. By sensing the levels of the intermediate glucosamine-6-phosphate (GlcN6P) and self-adjusting the expression levels of the target genes accordingly with the GlcN6P biosensor and ADC system enabled feedback circuits, the metabolic flux towards the production of the high value nutraceutical N-acetylglucosamine (GlcNAc) could be balanced and optimized in Bacillus subtilis. As a result, the GlcNAc titer in a 15-l fed-batch bioreactor increased from 59.9 g/l to 97.1 g/l with acetoin production and 81.7 g/l to 131.6 g/l without acetoin production, indicating the robustness and stability of the synthetic circuits in a large bioreactor system. Remarkably, this self-regulatory methodology does not require any external level of control such as the use of inducer molecules or switching fermentation/environmental conditions. Moreover, the proposed programmable genetic circuits may be expanded to engineer other microbial cells and metabolic pathways.
- Published
- 2019
30. Multiplexed activation in mammalian cells using a split-intein CRISPR/Cas12a based synthetic transcription factor
- Author
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James W Bryson, Jamie Y Auxillos, and Susan J Rosser
- Subjects
Gene Editing ,Endodeoxyribonucleases ,HEK293 Cells ,Bacterial Proteins ,AcademicSubjects/SCI00010 ,CRISPR-Associated Proteins ,Genetics ,Humans ,Protein Splicing ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering - Abstract
The adoption of CRISPR systems for the generation of synthetic transcription factors has greatly simplified the process for upregulating endogenous gene expression, with a plethora of applications in cell biology, bioproduction and cell reprogramming. The recently discovered CRISPR/Cas12a (Cas12a) systems offer extended potential, as Cas12a is capable of processing its own crRNA array, to provide multiple individual crRNAs for subsequent targeting from a single transcript. Here we show the application of dFnCas12a-VPR in mammalian cells, with the Francisella novicida Cas12a (FnCas12a) possessing a shorter PAM sequence than Acidaminococcus sp. (As) or Lachnospiraceae bacterium (Lb) variants, enabling denser targeting of genomic loci, while performing just as well or even better than the other variants. We observe that synergistic activation and multiplexing can be achieved using crRNA arrays but also show that crRNAs expressed towards the 5′ of 6-crRNA arrays show evidence of enhanced activity. This not only represents a more flexible tool for transcriptional modulation but further expands our understanding of the design capabilities and limitations when considering longer crRNA arrays for multiplexed targeting.
- Published
- 2021
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31. Pairing of single mutations yields obligate Cre-type site-specific recombinases
- Author
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Jenna Hoersten, Gloria Ruiz-Gómez, Felix Lansing, Teresa Rojo-Romanos, Lukas Theo Schmitt, Jan Sonntag, M Teresa Pisabarro, and Frank Buchholz
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Gene Editing ,Recombination, Genetic ,0303 health sciences ,AcademicSubjects/SCI00010 ,food and beverages ,03 medical and health sciences ,0302 clinical medicine ,HEK293 Cells ,DNA Nucleotidyltransferases ,Genetics ,Humans ,Genetic Engineering ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,030304 developmental biology - Abstract
Tyrosine site-specific recombinases (SSRs) represent a versatile genome editing tool with considerable therapeutic potential. Recent developments to engineer and evolve SSRs into heterotetramers to improve target site flexibility signified a critical step towards their broad utility in genome editing. However, SSR monomers can form combinations of different homo- and heterotetramers in cells, increasing their off-target potential. Here, we discover that two paired mutations targeting residues implicated in catalysis lead to simple obligate tyrosine SSR systems, where the presence of all distinct subunits to bind as a heterotetramer is obligatory for catalysis. Therefore, only when the paired mutations are applied as single mutations on each recombinase subunit, the engineered SSRs can efficiently recombine the intended target sequence, while the subunits carrying the point mutations expressed in isolation are inactive. We demonstrate the utility of the obligate SSR system to improve recombination specificity of a designer-recombinase for a therapeutic target in human cells. Furthermore, we show that the mutations render the naturally occurring SSRs, Cre and Vika, obligately heteromeric for catalytic proficiency, providing a straight-forward approach to improve their applied properties. These results facilitate the development of safe and effective therapeutic designer-recombinases and advance our mechanistic understanding of SSR catalysis.
- Published
- 2021
32. Efficient target cleavage by Type V Cas12a effectors programmed with split CRISPR RNA
- Author
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Regina Shebanova, Natalia Nikitchina, Nikita Shebanov, Vladimir Mekler, Konstantin Kuznedelov, Egor Ulashchik, Ruslan Vasilev, Olga Sharko, Vadim Shmanai, Ivan Tarassov, Konstantin Severinov, Nina Entelis, Ilya Mazunin, Génétique moléculaire, génomique, microbiologie (GMGM), and Centre National de la Recherche Scientifique (CNRS)-Université de Strasbourg (UNISTRA)
- Subjects
Gene Editing ,0303 health sciences ,Endodeoxyribonucleases ,AcademicSubjects/SCI00010 ,[SDV]Life Sciences [q-bio] ,CRISPR-Associated Proteins ,DNA ,03 medical and health sciences ,0302 clinical medicine ,Bacterial Proteins ,Genetics ,Acidaminococcus ,CRISPR-Cas Systems ,DNA Cleavage ,Francisella ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,030304 developmental biology - Abstract
CRISPR RNAs (crRNAs) that direct target DNA cleavage by Type V Cas12a nucleases consist of constant repeat-derived 5′-scaffold moiety and variable 3′-spacer moieties. Here, we demonstrate that removal of most of the 20-nucleotide scaffold has only a slight effect on in vitro target DNA cleavage by a Cas12a ortholog from Acidaminococcus sp. (AsCas12a). In fact, residual cleavage was observed even in the presence of a 20-nucleotide crRNA spacer moiety only. crRNAs split into separate scaffold and spacer RNAs catalyzed highly specific and efficient cleavage of target DNA by AsCas12a in vitro and in lysates of human cells. In addition to dsDNA target cleavage, AsCas12a programmed with split crRNAs also catalyzed specific ssDNA target cleavage and non-specific ssDNA degradation (collateral activity). V-A effector nucleases from Francisella novicida (FnCas12a) and Lachnospiraceae bacterium (LbCas12a) were also functional with split crRNAs. Thus, the ability of V-A effectors to use split crRNAs appears to be a general property. Though higher concentrations of split crRNA components are needed to achieve efficient target cleavage, split crRNAs open new lines of inquiry into the mechanisms of target recognition and cleavage and may stimulate further development of single-tube multiplex and/or parallel diagnostic tests based on Cas12a nucleases.
- Published
- 2021
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33. Broadening the reach and investigating the potential of prime editors through fully viral gene-deleted adenoviral vector delivery
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Qian Wang, Jin Liu, Manuel A F V Gonçalves, Hailiang Mei, Francesca Tasca, and Josephine M. Janssen
- Subjects
AcademicSubjects/SCI00010 ,Genetic Vectors ,Context (language use) ,Computational biology ,Biology ,Gene delivery ,Genome ,Prime (order theory) ,Viral vector ,Adenoviridae ,03 medical and health sciences ,0302 clinical medicine ,Genome editing ,Genetics ,Humans ,Gene ,030304 developmental biology ,Gene Editing ,0303 health sciences ,Gene Transfer Techniques ,Replication (computing) ,HEK293 Cells ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,Gene Deletion ,HeLa Cells - Abstract
Prime editing is a recent precision genome editing modality whose versatility offers the prospect for a wide range of applications, including the development of targeted genetic therapies. Yet, an outstanding bottleneck for its optimization and use concerns the difficulty in delivering large prime editing complexes into cells. Here, we demonstrate that packaging prime editing constructs in adenoviral capsids overcomes this constrain resulting in robust genome editing in both transformed and non-transformed human cells with up to 90% efficiencies. Using this cell cycle-independent delivery platform, we found a direct correlation between prime editing activity and cellular replication and disclose that the proportions between accurate prime editing events and unwanted byproducts can be influenced by the target-cell context. Hence, adenovector particles permit the efficacious delivery and testing of prime editing reagents in human cells independently of their transformation and replication statuses. The herein integrated gene delivery and gene editing technologies are expected to aid investigating the potential and limitations of prime editing in numerous experimental settings and, eventually, in ex vivo or in vivo therapeutic contexts.
- Published
- 2021
34. Optimized nickase- and nuclease-based prime editing in human and mouse cells
- Author
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Paul Q. Thomas, Daniel Reti, Fatwa Adikusuma, Luke Gierus, Jayshen Arudkumar, Ashleigh Geiger, Yu C.J. Chey, Sandra Piltz, Denis C. Bauer, Caleb Lushington, Gelshan I. Godahewa, Yatish Jain, and Laurence O.W. Wilson
- Subjects
Zygote ,AcademicSubjects/SCI00010 ,Biology ,Genome ,Prime (order theory) ,HeLa ,Mice ,CRISPR-Associated Protein 9 ,Genetics ,Animals ,Humans ,Cells, Cultured ,Embryonic Stem Cells ,Gene Editing ,Nuclease ,HEK 293 cells ,biology.organism_classification ,Embryonic stem cell ,Cell biology ,HEK293 Cells ,Cell culture ,biology.protein ,Narese/29 ,K562 Cells ,Synthetic Biology and Bioengineering ,K562 cells ,HeLa Cells ,Plasmids - Abstract
Precise genomic modification using prime editing (PE) holds enormous potential for research and clinical applications. In this study, we generated all-in-one prime editing (PEA1) constructs that carry all the components required for PE, along with a selection marker. We tested these constructs (with selection) in HEK293T, K562, HeLa and mouse embryonic stem (ES) cells. We discovered that PE efficiency in HEK293T cells was much higher than previously observed, reaching up to 95% (mean 67%). The efficiency in K562 and HeLa cells, however, remained low. To improve PE efficiency in K562 and HeLa, we generated a nuclease prime editor and tested this system in these cell lines as well as mouse ES cells. PE-nuclease greatly increased prime editing initiation, however, installation of the intended edits was often accompanied by extra insertions derived from the repair template. Finally, we show that zygotic injection of the nuclease prime editor can generate correct modifications in mouse fetuses with up to 100% efficiency.
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- 2021
35. Orthogonal CRISPR-associated transposases for parallel and multiplexed chromosomal integration
- Author
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Yu Jiang, Sheng Yang, Junjie Yang, Yiwen Zhang, Jieze Zhang, Jiaqi Xu, Jiao Zhang, and Siqi Yang
- Subjects
AcademicSubjects/SCI00010 ,CRISPR-Associated Proteins ,Transposases ,Locus (genetics) ,Computational biology ,Biology ,Genome ,Transposition (music) ,Synthetic biology ,Protospacer adjacent motif ,Pseudoalteromonas ,RNA, Bacterial ,Plasmid ,Genetics ,Escherichia coli ,CRISPR ,Synthetic Biology ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,Cell Engineering ,Vibrio cholerae ,Transposase - Abstract
Cell engineering is commonly limited to the serial manipulation of a single gene or locus. The recently discovered CRISPR-associated transposases (CASTs) could manipulate multiple sets of genes to achieve predetermined cell diversity, with orthogonal CASTs being able to manipulate them in parallel. Here, a novel CAST from Pseudoalteromonas translucida KMM520 (PtrCAST) was characterized without a protospacer adjacent motif (PAM) preference which can achieve a high insertion efficiency for larger cargo and multiplexed transposition and tolerate mismatches out of 4-nucleotide seed sequence. More importantly, PtrCAST operates orthogonally with CAST from Vibrio cholerae Tn6677 (VchCAST), though both belonging to type I-F3. The two CASTs were exclusively active on their respective mini-Tn substrate with their respective crRNAs that target the corresponding 5 and 2 loci in one Escherichia coli cell. The multiplexed orthogonal MUCICAT (MUlticopy Chromosomal Integration using CRISPR-Associated Transposases) is a powerful tool for cell programming and appears promising with applications in synthetic biology.
- Published
- 2021
36. A nanoscale DNA force spectrometer capable of applying tension and compression on biomolecules
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Jenny V. Le, Kyle Crocker, Michael G. Poirier, Ralf Bundschuh, Cassie Croy, Dengke Zhao, Yuchen Wang, Michael A. Darcy, Nick Andrioff, Patrick D. Halley, and Carlos E. Castro
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chemistry.chemical_classification ,Spectrometer ,Tension (physics) ,AcademicSubjects/SCI00010 ,Biomolecule ,Spectrum Analysis ,Force spectroscopy ,Hinge ,Energy landscape ,Nanotechnology ,Bioengineering ,DNA ,Biology ,Compression (physics) ,Biomechanical Phenomena ,Nanostructures ,Nucleosomes ,chemistry ,Genetics ,DNA origami ,Synthetic Biology and Bioengineering - Abstract
Single molecule force spectroscopy is a powerful approach to probe the structure, conformational changes, and kinetic properties of biological and synthetic macromolecules. However, common approaches to apply forces to biomolecules require expensive and cumbersome equipment and relatively large probes such as beads or cantilevers, which limits their use for many environments and makes integrating with other methods challenging. Furthermore, existing methods have key limitations such as an inability to apply compressive forces on single molecules. We report a nanoscale DNA force spectrometer (nDFS), which is based on a DNA origami hinge with tunable mechanical and dynamic properties. The angular free energy landscape of the nDFS can be engineered across a wide range through substitution of less than 5% of the strand components. We further incorporate a removable strut that enables reversible toggling of the nDFS between open and closed states to allow for actuated application of tensile and compressive forces. We demonstrate the ability to apply compressive forces by inducing a large bend in a 249bp DNA molecule, and tensile forces by inducing DNA unwrapping of a nucleosome sample. These results establish a versatile tool for force spectroscopy and robust methods for designing nanoscale mechanical devices with tunable force application.
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- 2021
37. Development of a base editor for protein evolution via in situ mutation in vivo
- Author
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Zhongyi Cheng, Cui Wenjing, Han Laichuang, Zhou Li, Zhemin Zhou, Wenliang Hao, Feiya Suo, and Liu Zhongmei
- Subjects
AcademicSubjects/SCI00010 ,Mutant ,Cytidine ,Biology ,medicine.disease_cause ,Genomic Instability ,Evolution, Molecular ,Mutant protein ,Cytidine Deaminase ,Genetics ,medicine ,CRISPR ,Gene ,Gene Editing ,Mutation ,Proteins ,Cytidine deaminase ,Cell biology ,Heterologous expression ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,Systematic evolution of ligands by exponential enrichment ,Genome, Bacterial ,Bacillus subtilis ,Thymidine - Abstract
Protein evolution has significantly enhanced the development of life science. However, it is difficult to achieve in vitro evolution of some special proteins because of difficulties with heterologous expression, purification, and function detection. To achieve protein evolution via in situ mutation in vivo, we developed a base editor by fusing nCas with a cytidine deaminase in Bacillus subtilis through genome integration. The base editor introduced a cytidine-to-thymidine mutation of approximately 100% across a 5 nt editable window, which was much higher than those of other base editors. The editable window was expanded to 8 nt by extending the length of sgRNA, and conversion efficiency could be regulated by changing culture conditions, which was suitable for constructing a mutant protein library efficiently in vivo. As proof-of-concept, the Sec-translocase complex and bacitracin-resistance-related protein BceB were successfully evolved in vivo using the base editor. A Sec mutant with 3.6-fold translocation efficiency and the BceB mutants with different sensitivity to bacitracin were obtained. As the construction of the base editor does not rely on any additional or host-dependent factors, such base editors (BEs) may be readily constructed and applicable to a wide range of bacteria for protein evolution via in situ mutation., Graphical Abstract Graphical AbstractThe diagram for the construction of the base editor and its working process for protein evolution.
- Published
- 2021
38. A small-molecule chemical interface for molecular programs
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Camille Lescanne, Vasily A Shenshin, Guillaume Gines, and Yannick Rondelez
- Subjects
0301 basic medicine ,AcademicSubjects/SCI00010 ,Interface (computing) ,Bioengineering ,02 engineering and technology ,DNA-Directed DNA Polymerase ,Biology ,03 medical and health sciences ,Allosteric Regulation ,Genetics ,Tryptophan Synthase ,Sensitivity (control systems) ,Layer (object-oriented design) ,Electronic circuit ,Fluorescent Dyes ,Signal processing ,business.industry ,DNA ,Modular design ,021001 nanoscience & nanotechnology ,Small molecule ,DNA-Binding Proteins ,030104 developmental biology ,Exodeoxyribonucleases ,Pattern recognition (psychology) ,0210 nano-technology ,Biological system ,business ,Synthetic Biology and Bioengineering - Abstract
In vitro molecular circuits, based on DNA-programmable chemistries, can perform an increasing range of high-level functions, such as molecular level computation, image or chemical pattern recognition and pattern generation. Most reported demonstrations, however, can only accept nucleic acids as input signals. Real-world applications of these programmable chemistries critically depend on strategies to interface them with a variety of non-DNA inputs, in particular small biologically relevant chemicals. We introduce here a general strategy to interface DNA-based circuits with non-DNA signals, based on input-translating modules. These translating modules contain a DNA response part and an allosteric protein sensing part, and use a simple design that renders them fully tunable and modular. They can be repurposed to either transmit or invert the response associated with the presence of a given input. By combining these translating-modules with robust and leak-free amplification motifs, we build sensing circuits that provide a fluorescent quantitative time-response to the concentration of their small-molecule input, with good specificity and sensitivity. The programmability of the DNA layer can be leveraged to perform DNA based signal processing operations, which we demonstrate here with logical inversion, signal modulation and a classification task on two inputs. The DNA circuits are also compatible with standard biochemical conditions, and we show the one-pot detection of an enzyme through its native metabolic activity. We anticipate that this sensitive small-molecule-to-DNA conversion strategy will play a critical role in the future applications of molecular-level circuitry.
- Published
- 2021
39. Phylogenetic debugging of a complete human biosynthetic pathway transplanted into yeast
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Jef D. Boeke, Paolo Mita, Neta Agmon, Itai Yanai, Maayan Baron, Tobias Schraink, Zuojian Tang, James A. Martin, Jun Chen, Jasmine Temple, David Fenyö, and Benjamin P. Tu
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Carboxy-Lyases ,Saccharomyces cerevisiae ,Biology ,Chromosomes, Artificial, Human ,chemistry.chemical_compound ,Genetics ,Humans ,Amino Acid Sequence ,Peptide Synthases ,Gene ,Phylogeny ,Sequence Homology, Amino Acid ,Adenine ,Genetic Complementation Test ,biology.organism_classification ,Yeast ,DNA shuffling ,Biosynthetic Pathways ,Transplantation ,Isoenzymes ,Metabolic pathway ,chemistry ,Biochemistry ,Amidophosphoribosyltransferase ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,Genetic Engineering ,Sequence Alignment ,DNA ,Plasmids - Abstract
Cross-species pathway transplantation enables insight into a biological process not possible through traditional approaches. We replaced the enzymes catalyzing the entire Saccharomyces cerevisiae adenine de novo biosynthesis pathway with the human pathway. While the ‘humanized’ yeast grew in the absence of adenine, it did so poorly. Dissection of the phenotype revealed that PPAT, the human ortholog of ADE4, showed only partial function whereas all other genes complemented fully. Suppressor analysis revealed other pathways that play a role in adenine de-novo pathway regulation. Phylogenetic analysis pointed to adaptations of enzyme regulation to endogenous metabolite level ‘setpoints’ in diverse organisms. Using DNA shuffling, we isolated specific amino acids combinations that stabilize the human protein in yeast. Thus, using adenine de novo biosynthesis as a proof of concept, we suggest that the engineering methods used in this study as well as the debugging strategies can be utilized to transplant metabolic pathway from any origin into yeast.
- Published
- 2019
40. Control of ϕC31 integrase-mediated site-specific recombination by protein trans-splicing
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Jane E. Paget, Femi J. Olorunniji, Susan J. Rosser, Arlene L. McPherson, W. Marshall Stark, and Makeba Lawson-Williams
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Computational biology ,Protein Engineering ,RS ,Genome engineering ,Inteins ,Substrate Specificity ,Trans-Splicing ,QH301 ,03 medical and health sciences ,Protein splicing ,Genetics ,Escherichia coli ,Serine ,Protein Splicing ,Site-specific recombination ,Amino Acid Sequence ,Cloning, Molecular ,QH426 ,030304 developmental biology ,Recombination, Genetic ,0303 health sciences ,biology ,Integrases ,Organisms, Genetically Modified ,030302 biochemistry & molecular biology ,Protein engineering ,Integrase ,RNA splicing ,Exteins ,biology.protein ,Intein ,Synthetic Biology and Bioengineering - Abstract
Serine integrases are emerging as core tools in synthetic biology and have applications in biotechnology and genome engineering. We have designed a split-intein serine integrase-based system with potential for regulation of site-specific recombination events at the protein level in vivo. The ϕC31 integrase was split into two extein domains, and intein sequences (Npu DnaEN and Ssp DnaEC) were attached to the two termini to be fused. Expression of these two components followed by post-translational protein trans-splicing in Escherichia coli generated a fully functional ϕC31 integrase. We showed that protein splicing is necessary for recombination activity; deletion of intein domains or mutation of key intein residues inactivated recombination. We used an invertible promoter reporter system to demonstrate a potential application of the split intein-regulated site-specific recombination system in building reversible genetic switches. We used the same split inteins to control the reconstitution of a split Integrase-Recombination Directionality Factor fusion (Integrase-RDF) that efficiently catalysed the reverse attR x attL recombination. This demonstrates the potential for split-intein regulation of the forward and reverse reactions using the integrase and the integrase-RDF fusion, respectively. The split-intein integrase is a potentially versatile, regulatable component for building synthetic genetic circuits and devices.
- Published
- 2019
- Full Text
- View/download PDF
41. Cell-free expression of RNA encoded genes using MS2 replicase
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Hannes Mutschler, Laura I. Weise, Viktoria Mayr, and Michael Heymann
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Genes, Viral ,Transcription, Genetic ,viruses ,RNA-dependent RNA polymerase ,Computational biology ,010402 general chemistry ,01 natural sciences ,03 medical and health sciences ,chemistry.chemical_compound ,Transcription (biology) ,RNA polymerase ,Gene expression ,Genetics ,Gene ,Polymerase ,Levivirus ,030304 developmental biology ,0303 health sciences ,Cell-Free System ,biology ,RNA ,RNA-Dependent RNA Polymerase ,0104 chemical sciences ,Protein Subunits ,chemistry ,Protein Biosynthesis ,biology.protein ,RNA, Viral ,Emulsions ,Q beta Replicase ,Synthetic Biology and Bioengineering - Abstract
RNA replicases catalyse transcription and replication of viral RNA genomes. Of particular interest for in vitro studies are phage replicases due to their small number of host factors required for activity and their ability to initiate replication in the absence of any primers. However, the requirements for template recognition by most phage replicases are still only poorly understood. Here, we show that the active replicase of the archetypical RNA phage MS2 can be produced in a recombinant cell-free expression system. We find that the 3′ terminal fusion of antisense RNAs with a domain derived from the reverse complement of the wild type MS2 genome generates efficient templates for transcription by the MS2 replicase. The new system enables DNA-independent gene expression both in batch reactions and in microcompartments. Finally, we demonstrate that MS2-based RNA-dependent transcription-translation reactions can be used to control DNA-dependent gene expression by encoding a viral DNA-dependent RNA polymerase on a MS2 RNA template. Our study sheds light on the template requirements of the MS2 replicase and paves the way for new in vitro applications including the design of genetic circuits combining both DNA- and RNA-encoded systems.
- Published
- 2019
- Full Text
- View/download PDF
42. Fail-safe genetic codes designed to intrinsically contain engineered organisms
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Isaac Justice, Jonathan Calles, Drew Endy, Alexa Garcia, and Detravious Brinkley
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Mutation ,Point mutation ,Translation (biology) ,Computational biology ,Biology ,Genetic code ,medicine.disease_cause ,Phenotype ,Sense Codon ,Transfer RNA ,Genetics ,medicine ,Synthetic Biology and Bioengineering ,Organism - Abstract
One challenge in engineering organisms is taking responsibility for their behavior over many generations. Spontaneous mutations arising before or during use can impact heterologous genetic functions, disrupt system integration, or change organism phenotype. Here, we propose restructuring the genetic code itself such that point mutations in protein-coding sequences are selected against. Synthetic genetic systems so-encoded should fail more safely in response to most spontaneous mutations. We designed fail-safe codes and simulated their expected effects on the evolution of so-encoded proteins. We predict fail-safe codes supporting expression of 20 or 15 amino acids could slow protein evolution to ∼30% or 0% the rate of standard-encoded proteins, respectively. We also designed quadruplet-codon codes that should ensure all single point mutations in protein-coding sequences are selected against while maintaining expression of 20 or more amino acids. We demonstrate experimentally that a reduced set of 21 tRNAs is capable of expressing a protein encoded by only 20 sense codons, whereas a standard 64-codon encoding is not expressed. Our work suggests that biological systems using rationally depleted but otherwise natural translation systems should evolve more slowly and that such hypoevolvable organisms may be less likely to invade new niches or outcompete native populations.
- Published
- 2019
43. Engineering DNA recognition and allosteric response properties of TetR family proteins by using a module-swapping strategy
- Author
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Dustin P. Patterson, Xian-Li Jiang, Joseph S. Glavy, Clement T Y Chan, Benjamin R Jordan, Rey P Dimas, Catherine Martini, and Faruck Morcos
- Subjects
Models, Molecular ,Protein Conformation, alpha-Helical ,Recombinant Fusion Proteins ,Genetic Vectors ,Regulator ,Gene Expression ,Computational biology ,Lac repressor ,Biology ,Crystallography, X-Ray ,Protein Engineering ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Protein structure ,Allosteric Regulation ,Genetics ,Escherichia coli ,TetR ,Protein Interaction Domains and Motifs ,Cloning, Molecular ,030304 developmental biology ,0303 health sciences ,Binding Sites ,Base Sequence ,business.industry ,Escherichia coli Proteins ,Rational design ,Protein engineering ,DNA ,Modular design ,biochemical phenomena, metabolism, and nutrition ,Repressor Proteins ,Kinetics ,chemistry ,Mutation ,Nucleic Acid Conformation ,UniProt ,business ,Synthetic Biology and Bioengineering ,Sequence Alignment ,030217 neurology & neurosurgery ,Protein Binding ,Transcription Factors - Abstract
The development of synthetic biological systems requires modular biomolecular components to flexibly alter response pathways. In previous studies, we have established a module-swapping design principle to engineer allosteric response and DNA recognition properties among regulators in the LacI family, in which the engineered regulators served as effective components for implementing new cellular behavior. Here we introduced this protein engineering strategy to two regulators in the TetR family: TetR (UniProt Accession ID: P04483) and MphR (Q9EVJ6). The TetR DNA-binding module and the MphR ligand-binding module were used to create the TetR-MphR. This resulting hybrid regulator possesses DNA-binding properties of TetR and ligand response properties of MphR, which is able to control gene expression in response to a molecular signal in cells. Furthermore, we studied molecular interactions between the TetR DNA-binding module and MphR ligand-binding module by using mutant analysis. Together, we demonstrated that TetR family regulators contain discrete and functional modules that can be used to build biological components with novel properties. This work highlights the utility of rational design as a means of creating modular parts for cell engineering and introduces new possibilities in rewiring cellular response pathways.
- Published
- 2019
44. Noise-reducing optogenetic negative-feedback gene circuits in human cells
- Author
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Michael Tyler Guinn and Gábor Balázsi
- Subjects
Light ,In silico ,Optogenetics ,Biology ,Proto-Oncogene Proteins p21(ras) ,03 medical and health sciences ,chemistry.chemical_compound ,Synthetic biology ,0302 clinical medicine ,Gene expression ,Genetics ,Animals ,Humans ,Gene Regulatory Networks ,TetR ,Gene ,Cells, Cultured ,030304 developmental biology ,Feedback, Physiological ,0303 health sciences ,Models, Genetic ,Activator (genetics) ,HEK 293 cells ,Reproducibility of Results ,Cell biology ,HEK293 Cells ,Gene Expression Regulation ,chemistry ,Synthetic Biology ,Synthetic Biology and Bioengineering ,Algorithms ,030217 neurology & neurosurgery - Abstract
Gene autorepression is widely present in nature and is also employed in synthetic biology, partly to reduce gene expression noise in cells. Optogenetic systems have recently been developed for controlling gene expression levels in mammalian cells, but most have utilized activator-based proteins, neglecting negative feedback except for in silico control. Here, we engineer optogenetic gene circuits into mammalian cells to achieve noise-reduction for precise gene expression control by genetic, in vitro negative feedback. We build a toolset of these noise-reducing Light-Inducible Tuner (LITer) gene circuits using the TetR repressor fused with a Tet-inhibiting peptide (TIP) or a degradation tag through the light-sensitive LOV2 protein domain. These LITers provide a range of nearly 4-fold gene expression control and up to 5-fold noise reduction from existing optogenetic systems. Moreover, we use the LITer gene circuit architecture to control gene expression of the cancer oncogene KRAS(G12V) and study its downstream effects through phospho-ERK levels and cellular proliferation. Overall, these novel LITer optogenetic platforms should enable precise spatiotemporal perturbations for studying multicellular phenotypes in developmental biology, oncology and other biomedical fields of research.
- Published
- 2019
- Full Text
- View/download PDF
45. Rational design of an XNA ligase through docking of unbound nucleic acids to toroidal proteins
- Author
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Stephen D. Weeks, Piet Herdewijn, Vitor B. Pinheiro, Jamoliddin Razzokov, Annemie Bogaerts, Jef Rozenski, Guy Schepers, Mathy Froeyen, Michiel Vanmeert, Eveline Lescrinier, and Muhammad Usman Mirza
- Subjects
DNA Ligases ,Protein Conformation ,Computational biology ,Molecular Docking Simulation ,Substrate Specificity ,Structure-Activity Relationship ,Viral Proteins ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Genetics ,Computer Simulation ,Biology ,Nucleic acid analogue ,Polymerase ,030304 developmental biology ,chemistry.chemical_classification ,0303 health sciences ,DNA ligase ,Deoxyribonuclease BamHI ,biology ,DNA Viruses ,Rational design ,Templates, Genetic ,Chemistry ,Models, Chemical ,chemistry ,Docking (molecular) ,DNA, Viral ,Mutagenesis, Site-Directed ,biology.protein ,Nucleic acid ,Nucleic Acid Conformation ,Human medicine ,Corrigendum ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,DNA ,Protein Binding - Abstract
Xenobiotic nucleic acids (XNA) are nucleic acid analogues not present in nature that can be used for the storage of genetic information. In vivo XNA applications could be developed into novel biocontainment strategies, but are currently limited by the challenge of developing XNA processing enzymes such as polymerases, ligases and nucleases. Here, we present a structure-guided modelling-based strategy for the rational design of those enzymes essential for the development of XNA molecular biology. Docking of protein domains to unbound double-stranded nucleic acids is used to generate a first approximation of the extensive interaction of nucleic acid processing enzymes with their substrate. Molecular dynamics is used to optimise that prediction allowing, for the first time, the accurate prediction of how proteins that form toroidal complexes with nucleic acids interact with their substrate. Using the Chlorella virus DNA ligase as a proof of principle, we recapitulate the ligase's substrate specificity and successfully predict how to convert it into an XNA-templated XNA ligase. ispartof: NUCLEIC ACIDS RESEARCH vol:47 issue:13 pages:1-12 ispartof: location:England status: published
- Published
- 2019
46. Targeted amplification of a sequence of interest in artificial chromosome in mammalian cells
- Author
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Natsuko Tada, Manami Asoshina, Genki Myo, Noriaki Shimizu, and Koji Tajino
- Subjects
DNA Replication ,Replication Origin ,CHO Cells ,Biology ,Mice ,03 medical and health sciences ,Cricetulus ,0302 clinical medicine ,Plasmid ,Tandem repeat ,Cricetinae ,Extrachromosomal DNA ,Genetics ,Animals ,CRISPR ,Chromosomes, Artificial ,Clustered Regularly Interspaced Short Palindromic Repeats ,Homologous Recombination ,Scaffold/matrix attachment region ,Gene ,030304 developmental biology ,0303 health sciences ,Gene Amplification ,Endonucleases ,Matrix Attachment Regions ,Fusion protein ,Cell biology ,CRISPR-Cas Systems ,Synthetic Biology and Bioengineering ,Homologous recombination ,030217 neurology & neurosurgery ,Plasmids - Abstract
A plasmid with a replication initiation region (IR) and a matrix attachment region (MAR) initiates gene amplification in mammalian cells at a random chromosomal location. A mouse artificial chromosome (MAC) vector can stably carry a large genomic region. In this study we combined these two technologies with the clustered regularly interspaced short palindromic repeats (CRISPR)/CRISPR-associated nuclease (Cas)9 strategy to achieve targeted amplification of a sequence of interest. We previously showed that the IR/MAR plasmid was amplified up to the extrachromosomal tandem repeat; here we demonstrate that cleavage of these tandem plasmids and MAC by Cas9 facilitates homologous recombination between them. The plasmid array on the MAC could be further extended to form a ladder structure with high gene expression by a breakage–fusion–bridge cycle involving breakage at mouse major satellites. Amplification of genes on the MAC has the advantage that the MAC can be transferred between cells. We visualized the MAC in live cells by amplifying the lactose operator array on the MAC in cells expressing lactose repressor-green fluorescent protein fusion protein. This targeted amplification strategy is in theory be applicable to any sequence at any chromosomal site, and provides a novel tool for animal cell technology.
- Published
- 2019
- Full Text
- View/download PDF
47. Self-powered RNA nanomachine driven by metastable structure
- Author
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Yoko Nomura, Yohei Yokobayashi, and Shungo Kobori
- Subjects
Aptamer ,Biology ,Ligands ,Catalysis ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,Transcription (biology) ,RNA polymerase ,Metastability ,microRNA ,Genetics ,Nanotechnology ,Nucleotide ,030304 developmental biology ,chemistry.chemical_classification ,0303 health sciences ,RNA ,DNA ,DNA-Directed RNA Polymerases ,Aptamers, Nucleotide ,Kinetics ,chemistry ,RNA Sequence ,Biophysics ,Nucleic Acid Conformation ,Thermodynamics ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery - Abstract
Many non-coding and regulatory RNA elements have evolved to exploit transient or metastable structures that emerge during transcription to control complex folding pathways or to encode dynamic functions. However, efforts to engineer synthetic RNA devices have mostly focused on the thermodynamically stable structures. Consequently, significant challenges and opportunities exist in engineering functional RNAs that explicitly take advantage of cotranscriptionally generated transient or metastable structures. In this work, we designed a short RNA sequence that adopts a robust metastable structure when transcribed by an RNA polymerase. Although the metastable structure persists for hours at low temperature, it refolds almost completely into the thermodynamically stable structure upon heat denaturation followed by cooling. The synthetic RNA was also equipped with the Broccoli aptamer so that it can bind its ligand and become fluorescent only in the thermodynamically stable structure. We further demonstrated that the relaxation to the thermodynamically stable and fluorescent structure can be catalyzed by a short trigger RNA in a sequence-specific manner. Finally, the RNA architecture was redesigned to sense and respond to microRNA sequences. In summary, we designed RNA nanomachines that can detect an RNA sequence, amplify signal and produce an optical output, all encoded in a single RNA transcript, self-powered by a metastable structure.
- Published
- 2019
48. Next-level riboswitch development—implementation of Capture-SELEX facilitates identification of a new synthetic riboswitch
- Author
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Adrien Boussebayle, Kay Hamacher, Daniel Torka, Sandra Ollivaud, Max Dombrowski, Beatrix Suess, Cristina Bofill-Bosch, Florian Groher, and Johannes Braun
- Subjects
Riboswitch ,Paromomycin ,Aptamer ,Economic shortage ,Computational biology ,Biology ,Ligands ,Small Molecule Libraries ,03 medical and health sciences ,Structure-Activity Relationship ,0302 clinical medicine ,Theophylline ,Genetics ,Protein secondary structure ,030304 developmental biology ,0303 health sciences ,SELEX Aptamer Technique ,RNA ,Neomycin ,Aptamers, Nucleotide ,Identification (information) ,Nucleic Acid Conformation ,Synthetic Biology and Bioengineering ,030217 neurology & neurosurgery ,Systematic evolution of ligands by exponential enrichment - Abstract
The development of synthetic riboswitches has always been a challenge. Although a number of interesting proof-of-concept studies have been published, almost all of these were performed with the theophylline aptamer. There is no shortage of small molecule-binding aptamers; however, only a small fraction of them are suitable for RNA engineering since a classical SELEX protocol selects only for high-affinity binding but not for conformational switching. We now implemented RNA Capture-SELEX in our riboswitch developmental pipeline to integrate the required selection for high-affinity binding with the equally necessary RNA conformational switching. Thus, we successfully developed a new paromomycin-binding synthetic riboswitch. It binds paromomycin with a KD of 20 nM and can discriminate between closely related molecules both in vitro and in vivo. A detailed structure–function analysis confirmed the predicted secondary structure and identified nucleotides involved in ligand binding. The riboswitch was further engineered in combination with the neomycin riboswitch for the assembly of an orthogonal Boolean NOR logic gate. In sum, our work not only broadens the spectrum of existing RNA regulators, but also signifies a breakthrough in riboswitch development, as the effort required for the design of sensor domains for RNA-based devices will in many cases be much reduced.
- Published
- 2019
49. Engineering repressors with coevolutionary cues facilitates toggle switches with a master reset
- Author
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Jose Alberto de la Paz, Rey P Dimas, Faruck Morcos, Clement T Y Chan, and Xian-Li Jiang
- Subjects
Distributed computing ,Biology ,Network topology ,Ligands ,Protein Engineering ,03 medical and health sciences ,0302 clinical medicine ,Protein Domains ,Genetics ,Gene Regulatory Networks ,Set (psychology) ,030304 developmental biology ,0303 health sciences ,Signal processing ,Stochastic Processes ,Models, Statistical ,Bacteria ,Models, Genetic ,business.industry ,SIGNAL (programming language) ,Computational Biology ,Signal Processing, Computer-Assisted ,Modular design ,Kinetics ,ROC Curve ,Environmental sensing ,Synthetic Biology ,State (computer science) ,business ,Synthetic Biology and Bioengineering ,Reset (computing) ,030217 neurology & neurosurgery ,Algorithms ,Allosteric Site ,Plasmids ,Protein Binding ,Signal Transduction ,Transcription Factors - Abstract
Engineering allosteric transcriptional repressors containing an environmental sensing module (ESM) and a DNA recognition module (DRM) has the potential to unlock a combinatorial set of rationally designed biological responses. We demonstrated that constructing hybrid repressors by fusing distinct ESMs and DRMs provides a means to flexibly rewire genetic networks for complex signal processing. We have used coevolutionary traits among LacI homologs to develop a model for predicting compatibility between ESMs and DRMs. Our predictions accurately agree with the performance of 40 engineered repressors. We have harnessed this framework to develop a system of multiple toggle switches with a master OFF signal that produces a unique behavior: each engineered biological activity is switched to a stable ON state by different chemicals and returned to OFF in response to a common signal. One promising application of this design is to develop living diagnostics for monitoring multiple parameters in complex physiological environments and it represents one of many circuit topologies that can be explored with modular repressors designed with coevolutionary information.
- Published
- 2019
50. A plasmid toolbox for controlled gene expression across the Proteobacteria
- Author
-
Christopher R. Reisch and Layla Schuster
- Subjects
Cloning ,0303 health sciences ,biology ,030306 microbiology ,AcademicSubjects/SCI00010 ,Promoter ,Bioengineering ,Computational biology ,Origin of replication ,biology.organism_classification ,Fold change ,03 medical and health sciences ,Plasmid ,Gene Expression Regulation ,Gene expression ,Proteobacteria ,Genetics ,Promoter Regions, Genetic ,Synthetic Biology and Bioengineering ,Gene ,030304 developmental biology ,Plasmids - Abstract
Controlled gene expression is fundamental for the study of gene function and our ability to engineer bacteria. However, there is currently no easy-to-use genetics toolbox that enables controlled gene expression in a wide range of diverse species. To facilitate the development of genetics systems in a fast, easy, and standardized manner, we constructed and tested a plasmid assembly toolbox that will enable the identification of well-regulated promoters in many Proteobacteria and potentially beyond. Each plasmid is composed of four categories of genetic parts (i) the origin of replication, (ii) resistance marker, (iii) promoter-regulator and (iv) reporter. The plasmids can be efficiently assembled using ligation-independent cloning, and any gene of interest can be easily inserted in place of the reporter. We tested this toolbox in nine different Proteobacteria and identified regulated promoters with over fifty-fold induction range in eight of these bacteria. We also constructed variant libraries that enabled the identification of promoter-regulators with varied expression levels and increased inducible fold change relative to the original promoter. A selection of over 50 plasmids, which contain all of the toolbox's genetic parts, are available for community use and will enable easy construction and testing of genetics systems in both model and non-model bacteria.
- Published
- 2021
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