Your search keyword '"Golden Gate cloning"' showing total 55 results

1. Combining Oligo Pools and Golden Gate Cloning to Create Protein Variant Libraries or Guide RNA Libraries for CRISPR Applications.

Author

Valero AM, Prins RC, de Vroet T, and Billerbeck S

Subjects

Oligonucleotides genetics, Gene Editing methods, Proteins genetics, Cloning, Molecular methods, RNA, Guide, CRISPR-Cas Systems genetics, CRISPR-Cas Systems, Gene Library

Abstract

Oligo pools are array-synthesized, user-defined mixtures of single-stranded oligonucleotides that can be used as a source of synthetic DNA for library cloning. While currently offering the most affordable source of synthetic DNA, oligo pools also come with limitations such as a maximum synthesis length (approximately 350 bases), a higher error rate compared to alternative synthesis methods, and the presence of truncated molecules in the pool due to incomplete synthesis. Here, we provide users with a comprehensive protocol that details how oligo pools can be used in combination with Golden Gate cloning to create user-defined protein mutant libraries, as well as single-guide RNA libraries for CRISPR applications. Our methods are optimized to work within the Yeast Toolkit Golden Gate scheme, but are in principle compatible with any other Golden Gate-based modular cloning toolkit and extendable to other restriction enzyme-based cloning methods beyond Golden Gate. Our methods yield high-quality, affordable, in-house variant libraries., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

2. Automation and Miniaturization of Golden Gate DNA Assembly Reactions Using Acoustic Dispensers.

Author

Köbel TS and Schindler D

Subjects

Synthetic Biology methods, Automation, Robotics methods, DNA genetics, DNA chemistry, Miniaturization, Acoustics, Cloning, Molecular methods

Abstract

Golden Gate cloning has become one of the most popular DNA assembly techniques. Its modular and hierarchical structure allows the construction of complex DNA fragments. Over time, Golden Gate cloning allows for the creation of a repository of reusable parts, reducing the cost of frequent sequence validation. However, as the number of reactions and fragments increases, so does the cost of consumables and the potential for human error. Typically, Golden Gate reactions are performed in volumes of 10-25 μL. Recent technological advances have led to the development of liquid handling robots that use sound to transfer liquids in the nL range from a source plate to a target plate. These acoustic dispensers have become particularly popular in the field of synthetic biology. The use of this technology allows miniaturization and parallelization of molecular reactions in a tip-free manner, making it sustainable by reducing plastic waste and reagent usage. Here, we provide a step-by-step protocol for performing and parallelizing Golden Gate cloning reactions in 1 μL total volume., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

3. Assembling DNA Plasmids with the Multi-Kingdom (MK) Cloning System.

Author

Scoville S and Chiasson DM

Subjects

DNA genetics, DNA Ligases metabolism, DNA Ligases genetics, Genetic Vectors genetics, Cloning, Molecular methods, Plasmids genetics

Abstract

The Golden Gate cloning technique is used to assemble DNA parts into higher-order assemblies. Individual parts containing compatible overhangs generated by type IIS restriction enzymes are joined together using DNA ligase. The technique enables users to assemble custom transcription units (TUs) for a wide array of experimental assays. Several Golden Gate cloning systems have been developed; however, they are typically used with a narrow range of organisms. Here we describe the Multi-Kingdom (MK) cloning system that allows users to generate DNA plasmids for use in a broad range of organisms., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

4. Simplifying Recombinant Protein Production: Combining Golden Gate Cloning with a Standardized Protein Purification Scheme.

Author

Zweng S, Mendoza-Rojas G, Lepak A, and Altegoer F

Subjects

Chromatography, Gel methods, Solubility, Genetic Vectors genetics, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Recombinant Fusion Proteins biosynthesis, Plasmids genetics, Gene Expression, Histidine genetics, Histidine metabolism, Endopeptidases, Cloning, Molecular methods, Escherichia coli genetics, Escherichia coli metabolism, Chromatography, Affinity methods, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism

Abstract

Recombinant protein production is pivotal in molecular biology, enabling profound insights into cellular processes through biophysical, biochemical, and structural analyses of the purified samples. The demand for substantial biomolecule quantities often presents challenges, particularly for eukaryotic proteins. Escherichia coli expression systems have evolved to address these issues, offering advanced features such as solubility tags, posttranslational modification capabilities, and modular plasmid libraries. Nevertheless, existing tools are often complex, which limits their accessibility and necessitate streamlined systems for rapid screening under standardized conditions. Based on the Golden Gate cloning method, we have developed a simple "one-pot" approach for the generation of expression constructs using strategically chosen protein purification tags like hexahistidine, SUMO, MBP, GST, and GB1 to enhance solubility and expression. The system allows visual candidate screening through mScarlet fluorescence and solubility tags are removable via TEV protease cleavage. We provide a comprehensive protocol encompassing oligonucleotide design, cloning, expression, His-tag affinity chromatography, and size-exclusion chromatography. This method, therefore, streamlines prokaryotic and eukaryotic protein production, rendering it accessible to standard molecular biology laboratories with basic protein biochemical equipment., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

5. Advancements in Golden Gate Cloning: A Comprehensive Review.

Author

Laborda-Mansilla J and García-Ruiz E

Subjects

DNA genetics, Genetic Vectors genetics, Cloning, Molecular methods

Abstract

Researchers have dedicated efforts to refining genetic part assembly techniques, responding to the demand for complex DNA constructs. The optimization efforts, targeting enhanced efficiency, fidelity, and modularity, have yielded streamlined protocols. Among these, Golden Gate cloning has gained prominence, offering a modular and hierarchical approach for constructing complex DNA fragments. This method is instrumental in establishing a repository of reusable parts, effectively reducing the costs and proving highly valuable for high-throughput DNA assembly projects. In this review, we delve into the main protocol of Golden Gate cloning, providing refined insights to enhance protocols and address potential challenges. Additionally, we perform a thorough evaluation of the primary modular cloning toolkits adopted by the scientific community. The discussion includes an exploration of recent advances and challenges in the field, providing a comprehensive overview of the current state of Golden Gate cloning., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

6. Generating Site Saturation Mutagenesis Libraries and Transferring Them to Broad Host-Range Plasmids Using Golden Gate Cloning.

Author

Oehlmann NN and Rebelein JG

Subjects

Rhodobacter capsulatus genetics, Host Specificity genetics, Mutagenesis genetics, Mutagenesis, Site-Directed methods, Multigene Family, Directed Molecular Evolution methods, Plasmids genetics, Cloning, Molecular methods, Gene Library

Abstract

Protein engineering is an established method for tailoring enzymatic reactivity. A commonly used method is directed evolution, where the mutagenesis and natural selection process is mimicked and accelerated in the laboratory. Here, we describe a reliable method for generating saturation mutagenesis libraries by Golden Gate cloning in a broad host range plasmid containing the pBBR1 replicon. The applicability is demonstrated by generating a mutant library of the iron nitrogenase gene cluster (anfHDGK) of Rhodobacter capsulatus, which is subsequently screened for the improved formation of molecular hydrogen., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

7. Golden Gate Cloning of Synthetic CRISPR RNA Spacer Sequences.

Author

Rust S and Randau L

Subjects

Clustered Regularly Interspaced Short Palindromic Repeats genetics, Escherichia coli genetics, RNA genetics, Cloning, Molecular methods, CRISPR-Cas Systems, Plasmids genetics

Abstract

Prokaryotes use CRISPR-Cas systems to interfere with viruses and other mobile genetic elements. CRISPR arrays comprise repeated DNA elements and spacer sequences that can be engineered for custom target sites. These arrays are transcribed into precursor CRISPR RNAs (pre-crRNAs) that undergo maturation steps to form individual CRISPR RNAs (crRNAs). Each crRNA contains a single spacer that identifies the target cleavage site for a large variety of Cas protein effectors. Precise manipulation of spacer sequences within CRISPR arrays is crucial for advancing the functionality of CRISPR-based technologies. Here, we describe a protocol for the design and creation of a minimal, plasmid-based CRISPR array to enable the expression of specific, synthetic crRNAs. Plasmids contain entry spacer sequences with two type IIS restriction sites and Golden Gate cloning enables the efficient exchange of these spacer sequences. Factors that influence the compatibility of the CRISPR arrays with native or recombinant Cas proteins are discussed., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

8. A Modular Cloning Toolkit Including CRISPRi for the Engineering of the Human Fungal Pathogen and Biotechnology Host Candida glabrata .

Author

Billerbeck S, Prins RC, and Marquardt M

Subjects

Humans, Biotechnology, Plasmids genetics, Saccharomyces cerevisiae genetics, Clustered Regularly Interspaced Short Palindromic Repeats, Genetic Engineering, Candida glabrata genetics, Cloning, Molecular methods

Abstract

The yeast Candida glabrata is an emerging, often drug-resistant opportunistic human pathogen that can cause severe systemic infections in immunocompromised individuals. At the same time, it is a valuable biotechnology host that naturally accumulates high levels of pyruvate─a valuable chemical precursor. Tools for the facile engineering of this yeast could greatly accelerate studies on its pathogenicity and its optimization for biotechnology. While a few tools for plasmid-based expression and genome engineering have been developed, there is no well-characterized cloning toolkit that would allow the modular assembly of pathways or genetic circuits. Here, by characterizing the Saccharomyces cerevisiae -based yeast molecular cloning toolkit (YTK) in C. glabrata and by adding missing components, we build a well-characterized CgTK ( C. glabrata toolkit). We used the CgTK to build a CRISPR interference system for C. glabrata that can be used to generate selectable phenotypes via single-gRNA targeting such as is required for genome-wide library screens.

Published

2023

9. Golden Gate vectors for efficient gene fusion and gene deletion in diverse filamentous fungi.

Author

Dahlmann TA, Terfehr D, Becker K, and Teichert I

Subjects

Fungi genetics, Genetic Vectors, Plasmids genetics, Sordariales genetics, Cloning, Molecular methods, Gene Deletion, Gene Fusion genetics, Genetic Engineering

Abstract

The cloning of plasmids can be time-consuming or expensive. Yet, cloning is a prerequisite for many standard experiments for the functional analysis of genes, including the generation of deletion mutants and the localization of gene products. Here, we provide Golden Gate vectors for fast and easy cloning of gene fusion as well as gene deletion vectors applicable to diverse fungi. In Golden Gate cloning, restriction and ligation occur simultaneously in a one-pot reaction. Our vector set contains recognition sites for the commonly used type IIS restriction endonuclease BsaI. We generated plasmids for C- as well as N-terminal tagging with GFP, mRFP and 3xFLAG. For gene deletion, we provide five different donor vectors for selection marker cassettes. These include standard cassettes for hygromycin B, nourseothricin and phleomycin resistance genes as well as FLP/FRT-based marker recycling cassettes for hygromycin B and nourseothricin resistance genes. To make cloning most feasible, we provide robust protocols, namely (1) an overview of cloning procedures described in this paper, (2) specific Golden Gate reaction protocols and (3) standard primers for cloning and sequencing of plasmids and generation of deletion cassettes by PCR and split-marker PCR. We show that our vector set is applicable for the biotechnologically relevant Penicillium chrysogenum and the developmental model system Sordaria macrospora. We thus expect these vectors to be beneficial for other fungi as well. Finally, the vectors can easily be adapted to organisms beyond the kingdom fungi.

Published

2021

10. GoldenBac: a simple, highly efficient, and widely applicable system for construction of multi-gene expression vectors for use with the baculovirus expression vector system.

Author

Neuhold J, Radakovics K, Lehner A, Weissmann F, Garcia MQ, Romero MC, Berrow NS, and Stolt-Bergner P

Subjects

Animals, DNA Restriction Enzymes genetics, Escherichia coli genetics, Gene Knockout Techniques, Genetic Vectors, Heat-Shock Proteins, Homologous Recombination, Polymerase Chain Reaction, Sf9 Cells, Baculoviridae genetics, Cloning, Molecular methods, Gene Expression, Recombinant Proteins genetics

Abstract

Background: Recombinant protein production and purification of large protein complexes in eukaryotes requires efficient methods to generate multi-gene expression constructs, where each individual gene is under the control of its own promoter and terminator. Current methods are based either on serial rounds of combination of several vectors containing loxP sites via the Cre-lox technology, or on multiple rounds of gene combination via PCR or other methods. These methods are multi-step, have lower efficiencies than single gene cloning, and may require laborious processes to verify that all genes of interest are present in the final product. Here, we describe a rapid and simple Golden Gate-based system for the generation of multi-gene expression constructs compatible with baculovirus expression vector systems (BEVS) using either Tn7 transposition or KO1629-based homologous recombination, which we refer to as "GoldenBac"., Results: This method is based on the construction of a series of vectors containing a promoter-gene of interest-terminator cassette flanked by cleavage sites of the BsaI type IIS restriction enzyme. This series of vectors can be cut by BsaI to excise cassettes with unique overhangs. In the same reaction, the cassettes are then ligated in the correct sequence in a final destination vector to generate multi-gene expression constructs containing 2-15 genes. Individual expression constructs can therefore be combined into a single vector in a single reaction, with over 90% efficiency when combining up to 14 expression cassettes. We demonstrate successful construction and expression of three different co-expression systems, the proteosomal lid complex, the anaphase promoting complex/cyclosome (APC/C), and a series of constructs used to test the effect of chaperone co-expression on the solubility of the HOIP protein., Conclusions: This robust, single-step cloning system provides an easy-to-use method for generation of multi-gene expression constructs for both transposition and homologous recombination-based baculovirus systems, making this technology available across all laboratories using baculovirus expression systems. This highly efficient and simple method allows for rapid incorporation of multi-gene expression cloning into the standardized service portfolio of protein production facilities and can also easily be adopted by any laboratory for routine generation of multi-gene baculovirus constructs.

Published

2020

11. Synthetic DNA Assembly Using Golden Gate Cloning and the Hierarchical Modular Cloning Pipeline.

Author

Marillonnet S and Grützner R

Subjects

Base Sequence, DNA Restriction Enzymes metabolism, Genetic Vectors, Plasmids genetics, Promoter Regions, Genetic, Transcription, Genetic, Cloning, Molecular methods, DNA genetics, Escherichia coli genetics, Genetic Engineering methods

Abstract

Methods that enable the construction of recombinant DNA molecules are essential tools for biological research and biotechnology. Golden Gate cloning is used for assembly of multiple DNA fragments in a defined linear order in a recipient vector using a one-pot assembly procedure. Golden Gate cloning is based on the use of a type IIS restriction enzyme for digestion of the DNA fragments and vector. Because restriction sites for the type IIS enzyme used for assembly must be present at the ends of the DNA fragments and vector but absent from all internal sequences, special care must be taken to prepare DNA fragments and the recipient vector with a structure suitable for assembly by Golden Gate cloning. In this article, protocols are presented for preparation of DNA fragments, modules, and vectors suitable for Golden Gate assembly cloning. Additional protocols are presented for assembly of defined parts in a transcription unit, as well as the stitching together of multiple transcription units into multigene constructs by the modular cloning (MoClo) pipeline. © 2020 The Authors. Basic Protocol 1: Performing a typical Golden Gate cloning reaction Basic Protocol 2: Accommodating a vector to Golden Gate cloning Basic Protocol 3: Accommodating an insert to Golden Gate cloning Basic Protocol 4: Generating small standardized parts compatible with hierarchical modular cloning (MoClo) using level 0 vectors Alternate Protocol: Generating large standardized parts compatible with hierarchical modular cloning (MoClo) using level -1 vectors Basic Protocol 5: Assembling transcription units and multigene constructs using level 1, M, and P MoClo vectors., (© 2020 The Authors.)

Published

2020

12. Joint Universal Modular Plasmids: A Flexible Platform for Golden Gate Assembly in Any Microbial Host.

Author

Valenzuela-Ortega M and French CE

Subjects

DNA genetics, Genetic Engineering methods, Genetic Vectors genetics, Synthetic Biology methods, Cloning, Molecular methods, Plasmids genetics

Abstract

Modular cloning standards based on Golden Gate DNA assembly allow for construction of complex DNA constructs over several rounds of assembly. Despite being reliable and automation-friendly, each standard uses a specific set of vectors, requiring researchers to generate new tool kits for novel hosts and cloning applications. JUMP vectors (Valenzuela-Ortega and French, bioRxiv 799585, 2019) combine the robustness of modular cloning standards with the Standard European Vector Architecture and a flexible design that allows researchers to easily modify the vector backbone via secondary cloning sites. This flexibility allows for JUMP vectors to be used in a wide variety of applications and hosts.

Published

2020

13. Good News for Nuclear Transgene Expression in Chlamydomonas .

Author

Schroda M

Subjects

Cell Nucleus genetics, Gene Expression Regulation, Plant, Gene Silencing, Genes, Plant genetics, Genome, Plant genetics, Chlamydomonas reinhardtii genetics, Cloning, Molecular methods, Transformation, Genetic genetics, Transgenes genetics

Abstract

Chlamydomonas reinhardtii is a well-established model system for basic research questions ranging from photosynthesis and organelle biogenesis, to the biology of cilia and basal bodies, to channelrhodopsins and photoreceptors. More recently, Chlamydomonas has also been recognized as a suitable host for the production of high-value chemicals and high-value recombinant proteins. However, basic and applied research have suffered from the inefficient expression of nuclear transgenes. The combined efforts of the Chlamydomonas community over the past decades have provided insights into the mechanisms underlying this phenomenon and have resulted in mutant strains defective in some silencing mechanisms. Moreover, many insights have been gained into the parameters that affect nuclear transgene expression, like promoters, introns, codon usage, or terminators. Here I critically review these insights and try to integrate them into design suggestions for the construction of nuclear transgenes that are to be expressed at high levels., Competing Interests: The author declares no conflict of interest.

Published

2019

14. The Use of an Automated Platform to Assemble Multigenic Constructs for Plant Transformation.

Author

Mann DGJ, Bevan SA, Harvey AJ, and Leffert-Sorenson RA

Subjects

Escherichia coli genetics, Plasmids genetics, Plasmids isolation & purification, Synthetic Biology instrumentation, Synthetic Biology methods, Transformation, Bacterial genetics, Cloning, Molecular methods, Genetic Vectors genetics, Multigene Family genetics, Plants, Genetically Modified genetics

Abstract

Compared to traditional means, modern DNA assembly methods allow cloning of large, multigenic vectors for plant transformation in rapid fashion. These methods are often robust and efficient and can assemble multiple DNA fragments into a single vector in one reaction. Here we describe the use of an automated DNA assembly platform for the generation of complex, multigenic T-DNA binary vectors using a hierarchical Golden Gate cloning strategy. These DNA constructs contained diverse DNA elements for the expression of multiple genes for trait stacking in the crop of interest. This platform streamlines the DNA assembly and validation process through high-efficiency cloning methods, integrated automation equipment, and increased throughput. The implementation of this platform removes bottlenecks for routine molecular biology and opens new possibilities for downstream experimental idea testing.

Published

2019

15. A novel one-step approach for the construction of yeast surface display Fab antibody libraries.

Author

Rosowski S, Becker S, Toleikis L, Valldorf B, Grzeschik J, Demir D, Willenbücher I, Gaa R, Kolmar H, Zielonka S, and Krah S

Subjects

Antibodies metabolism, Antibody Affinity, Flow Cytometry, Immunoglobulin Fab Fragments immunology, Peptide Library, Promoter Regions, Genetic, Surface Properties, Cloning, Molecular methods, Immunoglobulin Fab Fragments isolation & purification, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism

Abstract

Background: Yeast surface display (YSD) has proven to be a versatile platform technology for antibody discovery. However, the construction of antibody Fab libraries typically is a tedious three-step process that involves the generation of heavy chain as well as light chain display plasmids in different haploid yeast strains followed by yeast mating., Results: Within this study, we aimed at implementing a focused Golden Gate Cloning approach for the generation of YSD libraries. For this, antibodies heavy and light chains were encoded on one single plasmid. Fab display on yeast cells was either mediated by a two-directional promoter system (2dir) or by ribosomal skipping (bicis). The general applicability of this methodology was proven by the functional display of a therapeutic antibody. Subsequently, we constructed large antibody libraries with heavy chain diversities derived from CEACAM5 immunized animals in combination with a common light chain. Target-specific antibodies from both display systems were readily obtained after three rounds of fluorescence activated cell sorting. Isolated variants exhibited high affinities in the nanomolar and subnanomolar range as well as appropriate biophysical properties., Conclusion: We demonstrated that Golden Gate Cloning appears to be a valid tool for the generation of large yeast surface display antibody Fab libraries. This procedure simplifies the hit discovery process of antibodies from immune repertoires.

Published

2018

16. Standardized cloning vectors for protein production and generation of large gene libraries in Escherichia coli.

Author

Rohweder B, Semmelmann F, Endres C, and Sterner R

Subjects

Base Sequence, DNA Restriction Enzymes metabolism, Escherichia coli metabolism, Genetic Vectors metabolism, Plasmids genetics, Plasmids metabolism, Promoter Regions, Genetic, Cloning, Molecular methods, Escherichia coli genetics, Gene Library, Genetic Vectors genetics

Abstract

Here, we modified the multiple cloning sites from commonly used expression vectors to create a new suite of cloning plasmids that simplify and speed up cloning procedures in Escherichia coli. Each of our standardized plasmids contains two BsaI restriction sites, allowing for highly efficient cloning of genes and bringing their expression under control of either a T7 (pET21a_BsaI, pET28a_BsaI, and pMAL-c5T_BsaI) or T5 promoter (pUR22 and pUR23). Another plasmid in our suite (pTNA_BsaI) allows for generation of large gene libraries containing >108 variants, which can be constitutively expressed in selection experiments using metabolic complementation of auxotrophic E. coli strains. Coupling restriction and ligation with the BsaI restriction enzyme minimizes hands-on time, while the need for only three different primers to clone a target gene into the six different vectors keeps overall cloning costs low.

Published

2018

17. Construction of High-Quality Camel Immune Antibody Libraries.

Author

Romão E, Poignavent V, Vincke C, Ritzenthaler C, Muyldermans S, and Monsion B

Subjects

Animals, Camelus immunology, Single-Chain Antibodies immunology, Camelus genetics, Cloning, Molecular methods, Gene Library, Genetic Vectors, Peptide Library, Single-Chain Antibodies genetics

Abstract

Single-domain antibodies libraries of heavy-chain only immunoglobulins from camelids or shark are enriched for high-affinity antigen-specific binders by a short in vivo immunization. Thus, potent binders are readily retrieved from relatively small-sized libraries of 10 7 -10 8 individual transformants, mostly after phage display and panning on a purified target. However, the remaining drawback of this strategy arises from the need to generate a dedicated library, for nearly every envisaged target. Therefore, all the procedures that shorten and facilitate the construction of an immune library of best possible quality are definitely a step forward. In this chapter, we provide the protocol to generate a high-quality immune VHH library using the Golden Gate Cloning strategy employing an adapted phage display vector where a lethal ccdB gene has to be substituted by the VHH gene. With this procedure, the construction of the library can be shortened to less than a week starting from bleeding the animal. Our libraries exceed 10 8 individual transformants and close to 100% of the clones harbor a phage display vector having an insert with the length of a VHH gene. These libraries are also more economic to make than previous standard approaches using classical restriction enzymes and ligations. The quality of the Nanobodies that are retrieved from immune libraries obtained by Golden Gate Cloning is identical to those from immune libraries made according to the classical procedure.

Published

2018

18. Recursive DNA Assembly Using Protected Oligonucleotide Duplex Assisted Cloning (PODAC).

Author

Van Hove B, Guidi C, De Wannemaeker L, Maertens J, and De Mey M

Subjects

CRISPR-Cas Systems genetics, DNA genetics, DNA Methylation genetics, Genetic Engineering, Metabolic Networks and Pathways genetics, RNA chemistry, RNA genetics, RNA metabolism, Cloning, Molecular methods, DNA chemistry, DNA metabolism, Synthetic Biology methods

Abstract

A problem rarely tackled by current DNA assembly methods is the issue of cloning additional parts into an already assembled construct. Costly PCR workflows are often hindered by repeated sequences, and restriction based strategies impose design constraints for each enzyme used. Here we present Protected Oligonucleotide Duplex Assisted Cloning (PODAC), a novel technique that makes use of an oligonucleotide duplex for iterative Golden Gate cloning using only one restriction enzyme. Methylated bases confer protection from digestion during the assembly reaction and are removed during replication in vivo, unveiling a new cloning site in the process. We used this method to efficiently and accurately assemble a biosynthetic pathway and demonstrated its robustness toward sequence repeats by constructing artificial CRISPR arrays. As PODAC is readily amenable to standardization, it would make a useful addition to the synthetic biology toolkit.

Published

2017

19. Production of retroviral constructs for effective transfer and expression of T-cell receptor genes using Golden Gate cloning.

Author

Coren LV, Jain S, Trivett MT, Ohlen C, and Ott DE

Subjects

Animals, Gene Expression Regulation, Humans, Macaca mulatta genetics, Receptors, Antigen, T-Cell, alpha-beta biosynthesis, Transduction, Genetic, Cloning, Molecular, Genetic Vectors, Receptors, Antigen, T-Cell, alpha-beta genetics, T-Lymphocytes metabolism

Abstract

Here we present an improved strategy for producing T-cell receptor (TCR)-expressing retroviral vectors using a Golden Gate cloning strategy. This method takes advantage of the modular nature of TCR genes by directly amplifying TCR α and β variable regions from RNA or cDNA, then cloning and fusing them with their respective constant region genes resident in a retroviral TCR expression vector. Our one-step approach greatly streamlines the TCR vector production process in comparison to the traditional three-step procedure that typically involves cloning whole TCR genes, producing a TCR expression cassette, and constructing a retroviral construct. To date, we have generated TCR vectors that transferred seven functional human/rhesus macaque TCRs into primary T cells. The approach also holds promise for the assembly of other genes with defined variable regions, such as immunoglobulins.

Published

2015

20. Rapid and efficient assembly of transcription activator-like effector genes by USER cloning.

Author

Wang S, Li W, Wang S, and Hu B

Subjects

DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Gene Targeting, Genetic Loci, HEK293 Cells, Humans, Mixed Function Oxygenases, Protein Engineering, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins metabolism, Trans-Activators metabolism, Transcriptional Activation, Cloning, Molecular methods, Deoxyribonuclease (Pyrimidine Dimer) metabolism, Deoxyribonuclease I metabolism, Trans-Activators genetics, Uracil-DNA Glycosidase metabolism

Abstract

Transcription activator-like effectors (TALEs) that were related to bacteria immune system have lately been employed in a promising approach of precise gene targeting. Because of the repetitive characteristics of TALEs, existing TALE assembly methods are either very complicated, time-consuming, or too tricky to be handled in common labs. Here, we reported a rapid, efficient and easy method for TALE assembly. This method takes advantage of uracil-specific excision reagent (USER), an enzyme that can cleave DNA constructs and create long, unique single-strand DNA overhangs. Upon USER treatment, the overhangs on each individual TALE repeat unit can be rejoined hierarchically to form pentamers in a ligation-independent manner. Eventually, three pentamers are assembled into a full TALE construct by Golden Gate cloning. TALE nucleases (TALENs) generated with this method exhibit high genome-editing activity in human cells such as HEK293FT cells. Using this method, we have successfully synthesized three TALEN pairs targeting endogenous Tet1 locus, and proved that all can specifically target Tet1 gene, though in various degree. Comparing to other methods of TALEN assembly, this one is much less labor intensive and fairly faster, and positive clones can be obtained at high efficiency within only two days. We thus contribute to an easier approach for effective TALENs synthesis, which may highly facilitate the wide application of TALEN technology in genome editing, especially for human cells that require precise targeting., (Copyright © 2014. Published by Elsevier Ltd.)

Published

2014

21. Efficient construction of rAAV-based gene targeting vectors by Golden Gate cloning.

Author

Luo Y, Lin L, Bolund L, and Sørensen CB

Subjects

Cinnamates pharmacology, Drug Resistance, Microbial genetics, Gene Knockout Techniques, Genetic Engineering methods, Humans, Hygromycin B analogs & derivatives, Hygromycin B pharmacology, Neomycin pharmacology, Reproducibility of Results, tau Proteins genetics, Cloning, Molecular methods, Dependovirus genetics, Gene Targeting methods, Genetic Vectors

Abstract

The recombinant adeno-associated virus (rAAV) has proven to be an efficient and attractive tool for targeted genome engineering. Here we present a novel method employing the Golden Gate cloning strategy for fast and efficient construction of rAAV-based gene knockout or single-nucleotide knockin vectors. Two vectors, pGolden-Neo and pGolden-Hyg, were generated as common assembling modules to confer antibiotic resistance to the targeting vector. To validate the method, we then generated two rAAV-based targeting vectors: pAAV-pTP53-KO and pAAV-hTau(P301L)-KI. Furthermore, we generated a pGolden-AAV plasmid that allows one-step generation of an rAAV-based targeting vector. Our new methodology for rAAV targeting vector assembly is efficient, accurate, time-saving, and cost-effective.

Published

2014

22. Establishing a versatile Golden Gate cloning system for genetic engineering in fungi.

Author

Terfrüchte M, Joehnk B, Fajardo-Somera R, Braus GH, Riquelme M, Schipper K, and Feldbrügge M

Subjects

Aspergillus nidulans genetics, Gene Deletion, Genetic Engineering methods, Genetic Vectors, Homologous Recombination, Mutation, Cloning, Molecular methods, Ustilago genetics

Abstract

The corn pathogen Ustilago maydis is a well-studied fungal model organism. Along with a broad set of experimental tools, versatile strategies for the generation of gene replacement mutants by homologous recombination in U. maydis have been developed. Nevertheless, the production of corresponding linear DNA constructs still constitutes a time-limiting step. To overcome this bottleneck, various resistance cassette modules were adopted for use with the so-called Golden Gate cloning strategy. These modules allow not only simple gene deletions but also more sophisticated genetic manipulations like inserting sequences for C-terminal protein tagging. The type IIs restriction enzyme BsaI was selected for this novel approach as its recognition sites are comparatively rare in the U. maydis genome. To test the efficiency of the new strategy it was used to test the influence of varying flank lengths as well as the effect of non-homologous flank ends on homologous recombination. Importantly, to proof a broad applicability in other fungi the same strategy was used to generate mutants in the filamentous ascomycete Aspergillus nidulans. Hence, we present a highly efficient and economic cloning strategy that speeds up reverse genetic approaches in fungi., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2014

23. A molecular toolkit for the green seaweedUlva mutabilis

Author

Olivier De Clerck, Thomas Jacobs, Xiaojie Liu, and Jonas Blomme

Subjects

Crops, Agricultural, 0106 biological sciences, Physiology, Golden Gate Cloning, Transgene, Plant Science, Computational biology, Molecular cloning, Biology, Genes, Plant, 01 natural sciences, Ulva, 03 medical and health sciences, Chlorophyta, Genetics, Cloning, Molecular, Atlantic Ocean, Gene, 030304 developmental biology, 0303 health sciences, Reporter gene, Expression vector, Portugal, Seaweed, Regulatory sequence, Breakthrough Technologies, Tools, and Resources, Functional genomics, 010606 plant biology & botany

Abstract

The green seaweed Ulva mutabilis is an ecologically important marine primary producer as well as a promising cash crop cultivated for multiple uses. Despite its importance, several molecular tools are still needed to better understand seaweed biology. Here, we report the development of a flexible and modular molecular cloning toolkit for the green seaweed U. mutabilis based on a Golden Gate cloning system. The toolkit presently contains 125 entry vectors, 26 destination vectors, and 107 functionally validated expression vectors. We demonstrate the importance of endogenous regulatory sequences for transgene expression and characterize three endogenous promoters suitable to drive transgene expression. We describe two vector architectures to express transgenes via two expression cassettes or a bicistronic approach. The majority of selected transformants (50%–80%) consistently give clear visual transgene expression. Furthermore, we made different marker lines for intracellular compartments after evaluating 13 transit peptides and 11 tagged endogenous Ulva genes. Our molecular toolkit enables the study of Ulva gain-of-function lines and paves the way for gene characterization and large-scale functional genomics studies in a green seaweed.

Published

2021

24. A Golden-Gate Based Cloning Toolkit to Build Violacein Pathway Libraries in Yarrowia lipolytica

Author

Peng Xu, Liang Zhang, Jingwen Zhou, and Yingjia Tong

Subjects

0106 biological sciences, Yarrowia lipolytica, Indoles, Golden Gate Cloning, Biomedical Engineering, Yarrowia, Golden-Gate cloning, 01 natural sciences, Biochemistry, Genetics and Molecular Biology (miscellaneous), Calcium Carbonate, Fungal Proteins, 03 medical and health sciences, chemistry.chemical_compound, violacein, Biosynthesis, 010608 biotechnology, fermentation optimization, Cloning, Molecular, Promoter Regions, Genetic, Gene, 030304 developmental biology, Gene Library, Cloning, 0303 health sciences, Natural product, biology, library construction, General Medicine, Hydrogen-Ion Concentration, biology.organism_classification, Yeast, chemistry, Biochemistry, Metabolic Engineering, Batch Cell Culture Techniques, promoter engineering, Transformation efficiency, Research Article

Abstract

Violacein is a naturally occurring anticancer therapeutic compound with deep purple color. In this work, we harnessed the modular and combinatorial feature of a Golden Gate assembly method to construct a library of violacein producing strains in the oleaginous yeast Yarrowia lipolytica, where each gene in the violacein pathway was controlled by three different promoters with varying transcriptional strength. After optimizing the linker sequence and the Golden Gate reaction, we achieved high transformation efficiency and obtained a panel of representative Y. lipolytica recombinant strains. By evaluating the gene expression profile of 21 yeast strains, we obtained three colorful compounds in the violacein pathway: green (proviolacein), purple (violacein), and pink (deoxyviolacein). Our results indicated that strong expression of VioB, VioC, and VioD favors violacein production with minimal byproduct deoxyvioalcein in Y. lipolytica, and high deoxyviolacein production was found strongly associated with the weak expression of VioD. By further optimizing the carbon to nitrogen ratio and cultivation pH, the maximum violacein reached 70.04 mg/L with 5.28 mg/L of deoxyviolacein in shake flasks. Taken together, the development of Golden Gate cloning protocols to build combinatorial pathway libraries, and the optimization of culture conditions set a new stage for accessing the violacein pathway intermediates and engineering violacein production in Y. lipolytica. This work further expands the toolbox to engineering Y. lipolytica as an industrially relevant host for plant or marine natural product biosynthesis.

Published

2021

25. Simple and efficient modification of Golden Gate design standards and parts using oligo stitching

Author

Jonas De Saeger, Mattias Vermeersch, Christophe Gaillochet, and Thomas B. Jacobs

Subjects

oligo stitching, Genetic Vectors, Biomedical Engineering, Biology and Life Sciences, saturation mutagenesis, pegRNA, General Medicine, DNA, Biochemistry, Genetics and Molecular Biology (miscellaneous), Polymerase Chain Reaction, Golden Gate cloning, SYNTHETIC BIOLOGY, Mutagenesis, Gibson assembly, Synthetic Biology, Cloning, Molecular, Plasmids

Abstract

The assembly of DNA parts is a critical aspect of contemporary biological research. Gibson assembly and Golden Gate cloning are two popular options. Here, we explore the use of single stranded DNA oligos with Gibson assembly to augment Golden Gate cloning workflows in a process called “oligo stitching”. Our results show that oligo stitching can efficiently convert Golden Gate parts between different assembly standards and directly assemble incompatible Golden Gate parts without PCR amplification. Building on previous reports, we show that it can also be used to assemble de novo sequences. As a final application, we show that restriction enzyme recognition sites can be removed from plasmids and utilize the same concept to perform saturation mutagenesis. Given oligo stitching’s versatility and high efficiency, we expect that it will be a useful addition to the molecular biologist’s toolbox.Abstract Graphic

Published

2022

26. Rapid Assembly of Multi-Gene Constructs using Modular Golden Gate Cloning

Author

Minakshi Mukherjee, Zhen Wang, and Emily Caroll

Subjects

DNA Replication, Transcription, Genetic, Computer science, General Chemical Engineering, Golden Gate Cloning, Genetic Vectors, Gene Expression, Computational biology, Saccharomyces cerevisiae, General Biochemistry, Genetics and Molecular Biology, Plasmid, Genome editing, Escherichia coli, CRISPR, Vector (molecular biology), Cloning, Molecular, DNA Primers, Cloning, General Immunology and Microbiology, business.industry, General Neuroscience, Modular design, Restriction enzyme, Genes, Synthetic Biology, CRISPR-Cas Systems, business, Genetic Engineering, Plasmids

Abstract

The Golden Gate cloning method enables the rapid assembly of multiple genes in any user-defined arrangement. It utilizes type IIS restriction enzymes that cut outside of their recognition sites and create a short overhang. This modular cloning (MoClo) system uses a hierarchical workflow in which different DNA parts, such as promoters, coding sequences (CDS), and terminators, are first cloned into an entry vector. Multiple entry vectors then assemble into transcription units. Several transcription units then connect into a multi-gene plasmid. The Golden Gate cloning strategy is of tremendous advantage because it allows scar-less, directional, and modular assembly in a one-pot reaction. The hierarchical workflow typically enables the facile cloning of a large variety of multi-gene constructs with no need for sequencing beyond entry vectors. The use of fluorescent protein dropouts enables easy visual screening. This work provides a detailed, step-by-step protocol for assembling multi-gene plasmids using the yeast modular cloning (MoClo) kit. We show optimal and suboptimal results of multi-gene plasmid assembly and provide a guide for screening for colonies. This cloning strategy is highly applicable for yeast metabolic engineering and other situations in which multi-gene plasmid cloning is required.

Published

2021

27. Golden Gate vectors for efficient gene fusion and gene deletion in diverse filamentous fungi

Author

Kordula Becker, Dominik Terfehr, Tim A. Dahlmann, and Ines Teichert

Subjects

Filamentous fungi, Golden Gate Cloning, Genetic Vectors, Sordariales, Computational biology, Biology, Fusion gene, 03 medical and health sciences, chemistry.chemical_compound, Golden Gate cloning, Plasmid, Genetics, Technical Note, Split marker approach, Vector (molecular biology), Cloning, Molecular, 030304 developmental biology, Cloning, 0303 health sciences, Gene deletion, 030306 microbiology, Marker recycling, Fungi, General Medicine, Restriction enzyme, ddc:580, chemistry, Nourseothricin, Gene Fusion, Genetic Engineering, Hygromycin B, Plasmids

Abstract

The cloning of plasmids can be time-consuming or expensive. Yet, cloning is a prerequisite for many standard experiments for the functional analysis of genes, including the generation of deletion mutants and the localization of gene products. Here, we provide Golden Gate vectors for fast and easy cloning of gene fusion as well as gene deletion vectors applicable to diverse fungi. In Golden Gate cloning, restriction and ligation occur simultaneously in a one-pot reaction. Our vector set contains recognition sites for the commonly used type IIS restriction endonuclease BsaI. We generated plasmids for C- as well as N-terminal tagging with GFP, mRFP and 3xFLAG. For gene deletion, we provide five different donor vectors for selection marker cassettes. These include standard cassettes for hygromycin B, nourseothricin and phleomycin resistance genes as well as FLP/FRT-based marker recycling cassettes for hygromycin B and nourseothricin resistance genes. To make cloning most feasible, we provide robust protocols, namely (1) an overview of cloning procedures described in this paper, (2) specific Golden Gate reaction protocols and (3) standard primers for cloning and sequencing of plasmids and generation of deletion cassettes by PCR and split-marker PCR. We show that our vector set is applicable for the biotechnologically relevant Penicillium chrysogenum and the developmental model system Sordaria macrospora. We thus expect these vectors to be beneficial for other fungi as well. Finally, the vectors can easily be adapted to organisms beyond the kingdom fungi.

Published

2020

28. Oligonucleotide abundance biases aid design of a type IIS synthetic genomics framework with plant virome capacity

Author

Fabio Pasin

Subjects

0106 biological sciences, Computer science, BIO/13 Biologia applicata, Golden Gate Cloning, Oligonucleotides, Computational biology, 01 natural sciences, Applied Microbiology and Biotechnology, Insert (molecular biology), chemistry.chemical_compound, Bias, 010608 biotechnology, BIO/11 Biologia molecolare, Human virome, Cloning, Molecular, AGR/12 Patologia vegetale, Oligonucleotide, Virome, 010401 analytical chemistry, Rational design, General Medicine, Genomics, 0104 chemical sciences, Synthetic genomics, Subcloning, chemistry, Molecular Medicine, Synthetic Biology, DNA

Abstract

Synthetic genomics-driven dematerialization of genetic resources facilitates flexible hypothesis testing and rapid product development. Biological sequences have compositional biases, which, I reasoned, could be exploited for engineering of enhanced synthetic genomics systems. In proof-of-concept assays reported herein, the abundance of random oligonucleotides in viral genomic components was analyzed and used for the rational design of a synthetic genomics framework with plant virome capacity (SynViP). Type IIS endonucleases with low abundance in the plant virome, as well as Golden Gate and No See’m principles were combined with DNA chemical synthesis for seamless viral clone assembly by one-step digestion-ligation. The framework described does not require subcloning steps, is insensitive to insert terminal sequences, and was used with linear and circular DNA molecules. Based on a digital template, DNA fragments were chemically synthesized and assembled by one-step cloning to yield a scar-free infectious clone of a plant virus suitable for Agrobacterium-mediated delivery. SynViP allowed rescue of a genuine virus without biological material, and has the potential to greatly accelerate biological characterization and engineering of plant viruses as well as derived biotechnological tools. Finally, computational identification of compositional biases in biological sequences might become a common standard to aid scalable biosystems design and engineering.

Published

2020

29. GoldenBac: a simple, highly efficient, and widely applicable system for construction of multi-gene expression vectors for use with the baculovirus expression vector system

Author

Anita Lehner, Mari Carmen Romero, Florian Weissmann, Maria Queralt Garcia, Katharina Radakovics, Jana Neuhold, Peggy Stolt-Bergner, and Nicholas S. Berrow

Subjects

Multi-gene expression, lcsh:Biotechnology, Golden Gate Cloning, Genetic Vectors, Gene Expression, Cre recombinase, Computational biology, Biology, Polymerase Chain Reaction, Golden Gate cloning, Gene Knockout Techniques, Baculovirus expression, lcsh:TP248.13-248.65, Escherichia coli, Sf9 Cells, Animals, Cloning, Molecular, Homologous Recombination, Gene, Heat-Shock Proteins, Expression vector, Methodology Article, Protein complex, DNA Restriction Enzymes, Co-expression, Recombinant Proteins, Restriction enzyme, Terminator (genetics), Expression cloning, Homologous recombination, Baculoviridae, Biotechnology

Abstract

Background Recombinant protein production and purification of large protein complexes in eukaryotes requires efficient methods to generate multi-gene expression constructs, where each individual gene is under the control of its own promoter and terminator. Current methods are based either on serial rounds of combination of several vectors containing loxP sites via the Cre-lox technology, or on multiple rounds of gene combination via PCR or other methods. These methods are multi-step, have lower efficiencies than single gene cloning, and may require laborious processes to verify that all genes of interest are present in the final product. Here, we describe a rapid and simple Golden Gate-based system for the generation of multi-gene expression constructs compatible with baculovirus expression vector systems (BEVS) using either Tn7 transposition or KO1629-based homologous recombination, which we refer to as “GoldenBac”. Results This method is based on the construction of a series of vectors containing a promoter-gene of interest-terminator cassette flanked by cleavage sites of the BsaI type IIS restriction enzyme. This series of vectors can be cut by BsaI to excise cassettes with unique overhangs. In the same reaction, the cassettes are then ligated in the correct sequence in a final destination vector to generate multi-gene expression constructs containing 2–15 genes. Individual expression constructs can therefore be combined into a single vector in a single reaction, with over 90% efficiency when combining up to 14 expression cassettes. We demonstrate successful construction and expression of three different co-expression systems, the proteosomal lid complex, the anaphase promoting complex/cyclosome (APC/C), and a series of constructs used to test the effect of chaperone co-expression on the solubility of the HOIP protein. Conclusions This robust, single-step cloning system provides an easy-to-use method for generation of multi-gene expression constructs for both transposition and homologous recombination-based baculovirus systems, making this technology available across all laboratories using baculovirus expression systems. This highly efficient and simple method allows for rapid incorporation of multi-gene expression cloning into the standardized service portfolio of protein production facilities and can also easily be adopted by any laboratory for routine generation of multi-gene baculovirus constructs.

Published

2020

30. Standardized cloning vectors for protein production and generation of large gene libraries in Escherichia coli

Author

Reinhard Sterner, Florian Semmelmann, Bettina Rohweder, and Christiane Endres

Subjects

0301 basic medicine, Cloning, Base Sequence, 030102 biochemistry & molecular biology, Golden Gate Cloning, Genetic Vectors, Cloning vector, DNA Restriction Enzymes, Computational biology, Biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Restriction enzyme, Restriction site, 030104 developmental biology, Plasmid, Escherichia coli, Multiple cloning site, Genomic library, Cloning, Molecular, Promoter Regions, Genetic, Gene Library, Plasmids, Biotechnology

Abstract

Here, we modified the multiple cloning sites from commonly used expression vectors to create a new suite of cloning plasmids that simplify and speed up cloning procedures in Escherichia coli. Each of our standardized plasmids contains two BsaI restriction sites, allowing for highly efficient cloning of genes and bringing their expression under control of either a T7 (pET21a_BsaI, pET28a_BsaI, and pMAL-c5T_BsaI) or T5 promoter (pUR22 and pUR23). Another plasmid in our suite (pTNA_BsaI) allows for generation of large gene libraries containing >108 variants, which can be constitutively expressed in selection experiments using metabolic complementation of auxotrophic E. coli strains. Coupling restriction and ligation with the BsaI restriction enzyme minimizes hands-on time, while the need for only three different primers to clone a target gene into the six different vectors keeps overall cloning costs low.

Published

2018

31. Good News for Nuclear Transgene Expression in Chlamydomonas

Author

Michael Schroda

Subjects

0106 biological sciences, 0301 basic medicine, Transgene, Mutant, Chlamydomonas reinhardtii, Channelrhodopsin, algal synthetic biology, Review, Genes, Plant, 01 natural sciences, 03 medical and health sciences, Golden Gate cloning, Transformation, Genetic, Gene Expression Regulation, Plant, Gene silencing, Gene Silencing, Transgenes, Cloning, Molecular, Cell Nucleus, biology, modular cloning, histone modifications, Chlamydomonas, General Medicine, algal biotechnology, biology.organism_classification, Cell biology, 030104 developmental biology, Codon usage bias, Organelle biogenesis, transcriptional gene silencing, Genome, Plant, 010606 plant biology & botany

Abstract

Chlamydomonas reinhardtii is a well-established model system for basic research questions ranging from photosynthesis and organelle biogenesis, to the biology of cilia and basal bodies, to channelrhodopsins and photoreceptors. More recently, Chlamydomonas has also been recognized as a suitable host for the production of high-value chemicals and high-value recombinant proteins. However, basic and applied research have suffered from the inefficient expression of nuclear transgenes. The combined efforts of the Chlamydomonas community over the past decades have provided insights into the mechanisms underlying this phenomenon and have resulted in mutant strains defective in some silencing mechanisms. Moreover, many insights have been gained into the parameters that affect nuclear transgene expression, like promoters, introns, codon usage, or terminators. Here I critically review these insights and try to integrate them into design suggestions for the construction of nuclear transgenes that are to be expressed at high levels.

Published

2019

32. A unified multi-kingdom Golden Gate cloning platform

Author

Heinrich Leonhardt, Joel Ryan, Victor Giménez-Oya, Martin Parniske, Martin Bircheneder, Petra Dietrich, Michael Boshart, David Chiasson, Tanja Studtrucker, Katharina Sollweck, and Sabine Bachmaier

Subjects

0301 basic medicine, Trypanosoma, Transcription, Genetic, Molecular biology, Expression systems, Computer science, Golden Gate Cloning, ved/biology.organism_classification_rank.species, lcsh:Medicine, Computational biology, Article, Xenopus laevis, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Plasmid, Genome editing, Transcription (biology), Yeasts, Genetics, Animals, Humans, Golden gate, Transgenes, Cloning, Molecular, lcsh:Science, Model organism, Gene Editing, Cloning, Multidisciplinary, Bacteria, Organisms, Genetically Modified, ved/biology, business.industry, lcsh:R, Proteins, Plants, Modular design, Recombinant Proteins, 030104 developmental biology, chemistry, Oocytes, Female, lcsh:Q, Genetic techniques, business, 030217 neurology & neurosurgery, DNA, Plasmids

Abstract

Assembling composite DNA modules from custom DNA parts has become routine due to recent technological breakthroughs such as Golden Gate modular cloning. Using Golden Gate, one can efficiently assemble custom transcription units and piece units together to generate higher-order assemblies. Although Golden Gate cloning systems have been developed to assemble DNA plasmids required for experimental work in model species, they are not typically applicable to organisms from other kingdoms. Consequently, a typical molecular biology laboratory working across kingdoms must use multiple cloning strategies to assemble DNA constructs for experimental assays. To simplify the DNA assembly process, we developed a multi-kingdom (MK) Golden Gate assembly platform for experimental work in species from the kingdoms Fungi, Eubacteria, Protista, Plantae, and Animalia. Plasmid backbone and part overhangs are consistent across the platform, saving both time and resources in the laboratory. We demonstrate the functionality of the system by performing a variety of experiments across kingdoms including genome editing, fluorescence microscopy, and protein interaction assays. The versatile MK system therefore streamlines the assembly of modular DNA constructs for biological assays across a range of model organisms.

Published

2019

33. Facile generation of antibody heavy and light chain diversities for yeast surface display by Golden Gate Cloning

Author

Julius Grzeschik, Stefan Becker, Michael Busch, Stefan Zielonka, Harald Kolmar, Lukas Roth, Lars Toleikis, Steffen C. Hinz, and Simon Krah

Subjects

0301 basic medicine, Phage display, Surface Properties, Golden Gate Cloning, Clinical Biochemistry, Computational biology, Saccharomyces cerevisiae, Yeast display, Immunoglobulin light chain, Protein Engineering, Biochemistry, 03 medical and health sciences, 0302 clinical medicine, Peptide Library, Animals, Humans, Cloning, Molecular, Molecular Biology, biology, Chemistry, Surface display, Yeast, 030104 developmental biology, Mating of yeast, 030220 oncology & carcinogenesis, biology.protein, Immunoglobulin Light Chains, Antibody, Immunoglobulin Heavy Chains, Chickens

Abstract

Antibodies can be successfully engineered and isolated by yeast or phage display of combinatorial libraries. Still, generation of libraries comprising heavy chain as well as light chain diversities is a cumbersome process involving multiple steps. Within this study, we set out to compare the output of yeast display screening of antibody Fab libraries from immunized rodents that were generated by Golden Gate Cloning (GGC) with the conventional three-step method of individual heavy- and light-chain sub-library construction followed by chain combination via yeast mating (YM). We demonstrate that the GGC-based one-step process delivers libraries and antibodies from heavy- and light-chain diversities with similar quality to the traditional method while being significantly less complex and faster. Additionally, we show that this method can also be used to successfully screen and isolate chimeric chicken/human antibodies following avian immunization.

Published

2018

34. MIDAS: A Modular DNA Assembly System for Synthetic Biology

Author

Rudranuj Bundela, Kyle C. Van de Bittner, Matthew J. Nicholson, Emily J. Parker, Sarah A. Kessans, Craig J. van Dolleweerd, Leyla Y. Bustamante, and Barry Scott

Subjects

0301 basic medicine, Indoles, Computer science, Golden Gate Cloning, Genetic Vectors, Biomedical Engineering, Computational biology, 010402 general chemistry, 01 natural sciences, Biochemistry, Genetics and Molecular Biology (miscellaneous), 03 medical and health sciences, Synthetic biology, chemistry.chemical_compound, Gene Knockout Techniques, Penicillium paxilli, Cloning, Molecular, Gene, Gene Library, Cloning, business.industry, Penicillium, General Medicine, DNA, Modular design, 0104 chemical sciences, Restriction enzyme, 030104 developmental biology, chemistry, Metabolic Engineering, Mutation, Synthetic Biology, Microorganisms, Genetically-Modified, business, Metabolic Networks and Pathways

Abstract

A modular and hierarchical DNA assembly platform for synthetic biology based on Golden Gate (Type IIS restriction enzyme) cloning is described. This enabling technology, termed MIDAS (for Modular Idempotent DNA Assembly System), can be used to precisely assemble multiple DNA fragments in a single reaction using a standardized assembly design. It can be used to build genes from libraries of sequence-verified, reusable parts and to assemble multiple genes in a single vector, with full user control over gene order and orientation, as well as control of the direction of growth (polarity) of the multigene assembly, a feature that allows genes to be nested between other genes or genetic elements. We describe the detailed design and use of MIDAS, exemplified by the reconstruction, in the filamentous fungus Penicillium paxilli, of the metabolic pathway for production of paspaline and paxilline, key intermediates in the biosynthesis of a range of indole diterpenes-a class of secondary metabolites produced by several species of filamentous fungi. MIDAS was used to efficiently assemble a 25.2 kb plasmid from 21 different modules (seven genes, each composed of three basic parts). By using a parts library-based system for construction of complex assemblies, and a unique set of vectors, MIDAS can provide a flexible route to assembling tailored combinations of genes and other genetic elements, thereby supporting synthetic biology applications in a wide range of expression hosts.

Published

2018

35. A novel one-step approach for the construction of yeast surface display Fab antibody libraries

Author

Harald Kolmar, Ramona Gaa, Deniz Demir, Simon Krah, Simon Rosowski, Stefan Becker, Bernhard Valldorf, Stefan Zielonka, Iris Willenbücher, Lars Toleikis, and Julius Grzeschik

Subjects

0106 biological sciences, 0301 basic medicine, Ribosomal skipping, Surface Properties, Golden Gate Cloning, lcsh:QR1-502, Antibody Affinity, Bioengineering, Computational biology, Saccharomyces cerevisiae, Immunoglobulin light chain, 01 natural sciences, Applied Microbiology and Biotechnology, lcsh:Microbiology, Antibodies, 03 medical and health sciences, Immunoglobulin Fab Fragments, Plasmid, Peptide Library, 010608 biotechnology, Cloning, Molecular, Promoter Regions, Genetic, biology, Chemistry, Research, Fab fragment, Flow Cytometry, Surface display, Yeast, 030104 developmental biology, Mating of yeast, biology.protein, Antibody, Yeast surface display, Biotechnology, Antibody discovery

Abstract

Background Yeast surface display (YSD) has proven to be a versatile platform technology for antibody discovery. However, the construction of antibody Fab libraries typically is a tedious three-step process that involves the generation of heavy chain as well as light chain display plasmids in different haploid yeast strains followed by yeast mating. Results Within this study, we aimed at implementing a focused Golden Gate Cloning approach for the generation of YSD libraries. For this, antibodies heavy and light chains were encoded on one single plasmid. Fab display on yeast cells was either mediated by a two-directional promoter system (2dir) or by ribosomal skipping (bicis). The general applicability of this methodology was proven by the functional display of a therapeutic antibody. Subsequently, we constructed large antibody libraries with heavy chain diversities derived from CEACAM5 immunized animals in combination with a common light chain. Target-specific antibodies from both display systems were readily obtained after three rounds of fluorescence activated cell sorting. Isolated variants exhibited high affinities in the nanomolar and subnanomolar range as well as appropriate biophysical properties. Conclusion We demonstrated that Golden Gate Cloning appears to be a valid tool for the generation of large yeast surface display antibody Fab libraries. This procedure simplifies the hit discovery process of antibodies from immune repertoires. Electronic supplementary material The online version of this article (10.1186/s12934-017-0853-z) contains supplementary material, which is available to authorized users.

Published

2018

36. Production of retroviral constructs for effective transfer and expression of T-cell receptor genes using Golden Gate cloning

Author

Lori V. Coren, David E. Ott, Claes Ohlen, Sumiti Jain, and Matthew T. Trivett

Subjects

Cloning, Genetics, Expression vector, Receptors, Antigen, T-Cell, alpha-beta, T-Lymphocytes, Golden Gate Cloning, Genetic Vectors, T-cell receptor, hemic and immune systems, chemical and pharmacologic phenomena, Computational biology, Biology, Macaca mulatta, Article, General Biochemistry, Genetics and Molecular Biology, Gene Expression Regulation, Transduction, Genetic, T-Cell Receptor Gene, Complementary DNA, Animals, Humans, Vector (molecular biology), Expression cassette, Cloning, Molecular, Biotechnology

Abstract

Here we present an improved strategy for producing T-cell receptor (TCR)-expressing retroviral vectors using a Golden Gate cloning strategy. This method takes advantage of the modular nature of TCR genes by directly amplifying TCR α and β variable regions from RNA or cDNA, then cloning and fusing them with their respective constant region genes resident in a retroviral TCR expression vector. Our one-step approach greatly streamlines the TCR vector production process in comparison to the traditional three-step procedure that typically involves cloning whole TCR genes, producing a TCR expression cassette, and constructing a retroviral construct. To date, we have generated TCR vectors that transferred seven functional human/rhesus macaque TCRs into primary T cells. The approach also holds promise for the assembly of other genes with defined variable regions, such as immunoglobulins.

Published

2015

37. Development of a GAL4-VP16/UAS trans-activation system for tissue specific expression in Medicago truncatula

Author

Andreas Niebel, Charles Rosenberg, Mélanie Sicard, Sandra Bensmihen, Amélie Sevin-Pujol, Clare Gough, Marie-Christine Auriac, Agnes Lepage, Laboratoire des interactions plantes micro-organismes (LIPM), Centre National de la Recherche Scientifique (CNRS)-Institut National de la Recherche Agronomique (INRA), Bensmihen, Sandra, Institut National de la Recherche Agronomique (INRA)-Centre National de la Recherche Scientifique (CNRS), and 'Laboratoire d'Excellence (LABEX)' TULIP : ANR-10-LABX-41

Subjects

0301 basic medicine, Golden Gate Cloning, Gene Expression, lcsh:Medicine, Plant Science, Biochemistry, Medicago, Arabidopsis thaliana, Cloning, Molecular, Promoter Regions, Genetic, lcsh:Science, Flowering Plants, ComputingMilieux_MISCELLANEOUS, Multidisciplinary, Vegetal Biology, Plant Anatomy, Eukaryota, food and beverages, Fabaceae, medicago truncatula, Plants, Legumes, Medicago truncatula, Experimental Organism Systems, Research Article, Transcriptional Activation, Brassica, Computational biology, Biology, Research and Analysis Methods, Genes, Plant, 03 medical and health sciences, Model Organisms, Plant and Algal Models, Gene Types, DNA-binding proteins, Genetics, [SDV.BV]Life Sciences [q-bio]/Vegetal Biology, Gene Regulation, Molecular Biology Techniques, Molecular Biology, Gene, Transcription factor, Cloning, Reporter gene, Endodermis, lcsh:R, fungi, arabidopsis thaliana, Organisms, Biology and Life Sciences, Proteins, Promoter, biology.organism_classification, Regulatory Proteins, 030104 developmental biology, Trans-Activators, lcsh:Q, Pericycle, Biologie végétale, Transcription Factors, Reporter Genes

Abstract

International audience; Promoters with tissue-specific activity are very useful to address cell-autonomous and non cell autonomous functions of candidate genes. Although this strategy is widely used in Arabidopsis thaliana, its use to study tissue-specific regulation of root symbiotic interactions in legumes has only started recently. Moreover, using tissue specific promoter activity to drive a GAL4-VP16 chimeric transcription factor that can bind short upstream activation sequences (UAS) is an efficient way to target and enhance the expression of any gene of interest. Here, we developed a collection of promoters with different root cell layers specific activities in Medicago truncatula and tested their abilities to drive the expression of a chimeric GAL4-VP16 transcription factor in a trans-activation UAS: P-Glucuronidase (GUS) reporter gene system. By developing a binary vector devoted to modular Golden Gate cloning together with a collection of adapted tissue specific promoters and coding sequences we could test the activity of four of these promoters in trans-activation GAL4/UAS systems and compare them to "classical" promoter GUS fusions. Roots showing high levels of tissue specific expression of the GUS activity could be obtained with this trans-activation system. We therefore provide the legume community with new tools for efficient modular Golden Gate cloning, tissue specific expression and a trans-activation system. This study provides the ground work for future development of stable transgenic lines in Medicago truncatula.

Published

2017

38. Construction of a high-efficiency cloning system using the Golden Gate method and I-SceI endonuclease for targeted gene replacement in Bacillus anthracis

Author

Yufei Lyu, Dongshu Wang, Tiantian Wang, Li Zhu, Hengliang Wang, Chunjie Liu, Erling Feng, Xiankai Liu, and Yanchun Wang

Subjects

0301 basic medicine, DNA Ligases, Golden Gate Cloning, Genetic Vectors, Bioengineering, Computational biology, Molecular cloning, Applied Microbiology and Biotechnology, 03 medical and health sciences, Plasmid, Cloning, Molecular, Deoxyribonucleases, Type II Site-Specific, Homologous Recombination, Cloning, Membrane Glycoproteins, 030102 biochemistry & molecular biology, biology, General Medicine, biology.organism_classification, Bacillus anthracis, Restriction enzyme, Restriction site, 030104 developmental biology, Homologous recombination, Biotechnology

Abstract

To investigate gene function in Bacillus anthracis, a high-efficiency cloning system is required with an increased rate of allelic exchange. Golden Gate cloning is a molecular cloning strategy allowing researchers to simultaneously and directionally assemble multiple DNA fragments to construct target plasmids using type IIs restriction enzymes and T4 DNA ligase in the same reaction system. Here, a B. anthracis S-layer protein EA1 allelic exchange vector was successfully constructed using the Golden Gate method. No new restriction sites were introduced into this knockout vector, and seamless assembly of the DNA fragments was achieved. To elevate the efficiency of homologous recombination between the allelic exchange vector and chromosomal DNA, we introduced an I-SceI site into the allelic exchange vector. The eag gene was successfully knocked out in B. anthracis using this vector. Simultaneously, the allelic exchange vector construction method was developed into a system for generating B. anthracis allelic exchange vectors. To verify the effectiveness of this system, some other allelic exchange vectors were constructed and gene replacements were performed in B. anthracis. It is speculated that this gene knockout vector construction system and high-efficiency targeted gene replacement using I-SceI endonuclease can be applied to other Bacillus spp.

Published

2017

39. Recursive DNA Assembly Using Protected Oligonucleotide Duplex Assisted Cloning (PODAC)

Author

Bob Van Hove, Chiara Guidi, Jo Maertens, Lien De Wannemaeker, and Marjan De Mey

Subjects

0301 basic medicine, Genetics, 030102 biochemistry & molecular biology, Golden Gate Cloning, Biomedical Engineering, Robustness (evolution), General Medicine, DNA, Molecular cloning, Biology, DNA Methylation, Biochemistry, Genetics and Molecular Biology (miscellaneous), 03 medical and health sciences, Synthetic biology, Restriction enzyme, 030104 developmental biology, Cloning Site, Multiple cloning site, CRISPR, RNA, Synthetic Biology, CRISPR-Cas Systems, Cloning, Molecular, Genetic Engineering, Metabolic Networks and Pathways

Abstract

A problem rarely tackled by current DNA assembly methods is the issue of cloning additional parts into an already assembled construct. Costly PCR workflows are often hindered by repeated sequences, and restriction based strategies impose design constraints for each enzyme used. Here we present Protected Oligonucleotide Duplex Assisted Cloning (PODAC), a novel technique that makes use of an oligonucleotide duplex for iterative Golden Gate cloning using only one restriction enzyme. Methylated bases confer protection from digestion during the assembly reaction and are removed during replication in vivo, unveiling a new cloning site in the process. We used this method to efficiently and accurately assemble a biosynthetic pathway and demonstrated its robustness toward sequence repeats by constructing artificial CRISPR arrays. As PODAC is readily amenable to standardization, it would make a useful addition to the synthetic biology toolkit.

Published

2017

40. A simple method for construction of artificial microRNA vector in plant

Author

Yang Li, Sunping Zhao, Sheng Zhong, Zhaohai Wang, Bo Ding, and Yangsheng Li

Subjects

DNA, Plant, Golden Gate Cloning, Genetic Vectors, Nicotiana benthamiana, Bioengineering, Computational biology, Biology, Applied Microbiology and Biotechnology, Gene Expression Regulation, Plant, Tobacco, microRNA, Drosophila Proteins, Gene Silencing, Vector (molecular biology), Cloning, Molecular, business.industry, food and beverages, Oryza, General Medicine, biology.organism_classification, Biotechnology, DNA-Binding Proteins, MicroRNAs, Plant species, business

Abstract

Artificial microRNA (amiRNA) is a powerful tool for silencing genes in many plant species. Here we provide an easy method to construct amiRNA vectors that reinvents the Golden Gate cloning approach and features a novel system called top speed amiRNA construction (TAC). This speedy approach accomplishes one restriction-ligation step in only 5 min, allowing easy and high-throughput vector construction. Three primers were annealed to be a specific adaptor, then digested and ligated on our novel vector pTAC. Importantly, this method allows the recombined amiRNA constructs to maintain the precursor of osa-miR528 with exception of the desired amiRNA/amiRNA* sequences. Using this method, our results showed the expected decrease of targeted genes in Nicotiana benthamiana and Oryza sativa.

Published

2014

41. Rapid and Efficient Assembly of Transcription Activator-Like Effector Genes by USER Cloning

Author

Shuo Wang, Wei Li, Song Wang, and Baoyang Hu

Subjects

Transcriptional Activation, Golden Gate Cloning, Computational biology, Biology, Protein Engineering, Mixed Function Oxygenases, Deoxyribonuclease (Pyrimidine Dimer), Genome editing, TAL effector, Transcription (biology), Proto-Oncogene Proteins, Genetics, Deoxyribonuclease I, Humans, Cloning, Molecular, Uracil-DNA Glycosidase, Molecular Biology, Gene, Transcription activator-like effector nuclease, Effector, Gene targeting, DNA-Binding Proteins, HEK293 Cells, Genetic Loci, Gene Targeting, Trans-Activators

Abstract

Transcription activator-like effectors (TALEs) that were related to bacteria immune system have lately been employed in a promising approach of precise gene targeting. Because of the repetitive characteristics of TALEs, existing TALE assembly methods are either very complicated, time-consuming, or too tricky to be handled in common labs. Here, we reported a rapid, efficient and easy method for TALE assembly. This method takes advantage of uracil-specific excision reagent (USER), an enzyme that can cleave DNA constructs and create long, unique single-strand DNA overhangs. Upon USER treatment, the overhangs on each individual TALE repeat unit can be rejoined hierarchically to form pentamers in a ligation-independent manner. Eventually, three pentamers are assembled into a full TALE construct by Golden Gate cloning. TALE nucleases (TALENs) generated with this method exhibit high genome-editing activity in human cells such as HEK293FT cells. Using this method, we have successfully synthesized three TALEN pairs targeting endogenous Tet1 locus, and proved that all can specifically target Tet1 gene, though in various degree. Comparing to other methods of TALEN assembly, this one is much less labor intensive and fairly faster, and positive clones can be obtained at high efficiency within only two days. We thus contribute to an easier approach for effective TALENs synthesis, which may highly facilitate the wide application of TALEN technology in genome editing, especially for human cells that require precise targeting.

Published

2014

42. Efficient construction of rAAV-based gene targeting vectors by Golden Gate cloning

Author

Charlotte Brandt Sørensen, Yonglun Luo, Lin Lin, and Lars Bolund

Subjects

viruses, Golden Gate Cloning, Genetic Vectors, Reproducibility of Results, Gene targeting, Drug Resistance, Microbial, Neomycin, tau Proteins, Computational biology, Dependovirus, Biology, General Biochemistry, Genetics and Molecular Biology, Virus, Genome engineering, law.invention, Gene Knockout Techniques, Cinnamates, law, Gene Targeting, Recombinant DNA, Humans, Cloning, Molecular, Hygromycin B, Genetic Engineering, Biotechnology

Abstract

The recombinant adeno-associated virus (rAAV) has proven to be an efficient and attractive tool for targeted genome engineering. Here we present a novel method employing the Golden Gate cloning strategy for fast and efficient construction of rAAV-based gene knockout or single-nucleotide knockin vectors. Two vectors, pGolden-Neo and pGolden-Hyg, were generated as common assembling modules to confer antibiotic resistance to the targeting vector. To validate the method, we then generated two rAAV-based targeting vectors: pAAV-pTP53-KO and pAAV-hTauP301L-KI. Furthermore, we generated a pGolden-AAV plasmid that allows one-step generation of an rAAV-based targeting vector. Our new methodology for rAAV targeting vector assembly is efficient, accurate, time-saving, and cost-effective.

Published

2014

43. A Golden Gate Modular Cloning Toolbox for Plants

Author

Sylvestre Marillonnet, Nicola J. Patron, Tim-Martin Ehnert, Jonathan D. G. Jones, Ramona Gruetzner, Stefan Werner, Mark Youles, and Carola Engler

Subjects

Golden Gate Cloning, Genetic Vectors, Biomedical Engineering, Cloning vector, Nicotiana benthamiana, Computational biology, Molecular cloning, Biology, Biochemistry, Genetics and Molecular Biology (miscellaneous), Synthetic biology, Tobacco, Cloning, Molecular, Selectable marker, Models, Genetic, Cloning (programming), business.industry, fungi, food and beverages, General Medicine, biology.organism_classification, Biotechnology, Transformation (genetics), Agrobacterium tumefaciens, Synthetic Biology, Genetic Engineering, business

Abstract

Plant Synthetic Biology requires robust and efficient methods for assembling multigene constructs. Golden Gate cloning provides a precision module-based cloning technique for facile assembly of multiple genes in one construct. We present here a versatile resource for plant biologists comprising a set of cloning vectors and 96 standardized parts to enable Golden Gate construction of multigene constructs for plant transformation. Parts include promoters, untranslated sequences, reporters, antigenic tags, localization signals, selectable markers, and terminators. The comparative performance of parts in the model plant Nicotiana benthamiana is discussed.

Published

2014

44. Rapid Creation of Forward-Genetics Tools for C. briggsae Using TALENs: Lessons for Nonmodel Organisms

Author

Yongquan Shen, Qing Wei, Ronald E. Ellis, Xiangmei Chen, and Yelena Shifman

Subjects

Caenorhabditis briggsae, nematode, Golden Gate Cloning, ved/biology.organism_classification_rank.species, Gene Knockout Techniques, 03 medical and health sciences, 0302 clinical medicine, Species Specificity, evolution, Genetic model, Methods, Genetics, Animals, C. briggsae, Cloning, Molecular, Model organism, model organism, Molecular Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, 0303 health sciences, Transcription activator-like effector nuclease, Base Sequence, biology, ved/biology, Computational Biology, Endonucleases, biology.organism_classification, Biological Evolution, Forward genetics, Reverse genetics, Caenorhabditis, TALENs, Mutation, Trans-Activators, 030217 neurology & neurosurgery

Abstract

Although evolutionary studies of gene function often rely on RNA interference, the ideal approach would use reverse genetics to create null mutations for cross-species comparisons and forward genetics to identify novel genes in each species. We have used transcription activator-like effector nucleases (TALENs) to facilitate both approaches in Caenorhabditis nematodes. First, by combining golden gate cloning and TALEN technology, we can induce frameshifting mutations in any gene. Second, by combining this approach with bioinformatics we can predict and create the resources needed for forward genetic analysis in species like Caenorhabditis briggsae. Although developing genetic model organisms used to require years to isolate marker mutations, balancers, and tools, with TALENs, these reagents can now be produced in months. Furthermore, the analysis of nonsense mutants in related model organisms allows a directed approach for making these markers and tools. When used together, these methods could simplify the adaptation of other organisms for forward and reverse genetics.

Published

2013

45. Fast track assembly of multigene constructs using Golden Gate cloning and the MoClo system

Author

Carola Engler, Stefan Werner, Sylvestre Marillonnet, Ramona Gruetzner, and Ernst Weber

Subjects

Genetics, Models, Genetic, Cloning (programming), Golden Gate Cloning, Eukaryotic transcription, Gene regulatory network, Bioengineering, General Medicine, Computational biology, Biology, Directed evolution, Applied Microbiology and Biotechnology, Genome, Metabolic engineering, Synthetic biology, Synthetic Biology, Cloning, Molecular, Genetic Engineering, Biotechnology

Abstract

Recent progress in the field of synthetic biology has led to the creation of cells containing synthetic genomes. Although these first synthetic organisms contained copies of natural genomes, future work will be directed toward engineering of organisms with modified genomes and novel phenotypes. Much work, however, remains to be done to be able to routinely engineer novel biological functions. As a tool that will be useful for such purpose, we have recently developed a modular cloning system (MoClo) that allows high throughput assembly of multiple genetic elements. We present here new features of this cloning system that allow to increase the speed of assembly of multigene constructs. As an example, 68 DNA fragments encoding basic genetic elements were assembled using three one-pot cloning steps, resulting in a 50 kb construct containing 17 eukaryotic transcription units. This cloning system should be useful for generating the multiple construct variants that will be required for developing gene networks encoding novel functions, and fine-tuning the expression levels of the various genes involved.

Published

2012

46. Versatile single-step-assembly CRISPR/Cas9 vectors for dual gRNA expression

Author

Paul Q. Thomas, Chandran Pfitzner, and Fatwa Adikusuma

Subjects

0301 basic medicine, Molecular biology, Computer science, Golden Gate Cloning, Oligonucleotides, Selection Markers, lcsh:Medicine, Artificial Gene Amplification and Extension, Restriction Fragment Mapping, Polymerase Chain Reaction, Biochemistry, Synthetic Genome Editing, Genome Engineering, law.invention, Mice, 0302 clinical medicine, Plasmid, law, CRISPR, Clustered Regularly Interspaced Short Palindromic Repeats, Multiplex, Guide RNA, Cloning, Molecular, lcsh:Science, Cells, Cultured, Polymerase chain reaction, Multidisciplinary, Nucleotides, Crispr, Transfection, Engineering and Technology, Synthetic Biology, Restriction fragment length polymorphism, Research Article, Biotechnology, Plasmids, RNA, Guide, Kinetoplastida, Restriction Fragment Length Polymorphism Analysis, Genetic Vectors, Bioengineering, Nucleofection, Locus (genetics), Computational biology, DNA construction, 03 medical and health sciences, Animals, Embryonic Stem Cells, Cloning, Biology and life sciences, Oligonucleotide, Cas9, Gene Mapping, lcsh:R, RNA, Marker Genes, Synthetic Genomics, Research and analysis methods, Molecular biology techniques, 030104 developmental biology, Synthetic Bioengineering, Plasmid Construction, lcsh:Q, 030217 neurology & neurosurgery

Abstract

CRISPR/Cas9 technology enables efficient, rapid and cost-effective targeted genomic modification in a wide variety of cellular contexts including cultured cells. Some applications such as generation of double knock-outs, large deletions and paired-nickase cleavage require simultaneous expression of two gRNAs. Although single plasmids that enable multiplex expression of gRNAs have been developed, these require multiple rounds of cloning and/or PCR for generation of the desired construct. Here, we describe a series of vectors that enable generation of customized dual-gRNA expression constructs via an easy one-step golden gate cloning reaction using two annealed oligonucleotide inserts with different overhangs. Through nucleofection of mouse embryonic stem cells, we demonstrate highly efficient cleavage of the target loci using the dual-guide plasmids, which are available as Cas9-nuclease or Cas9-nickase expression constructs, with or without selection markers. These vectors are a valuable addition to the CRISPR/Cas9 toolbox and will be made available to all interested researchers via the Addgene plasmid repository.

Published

2017

47. Establishing a versatile Golden Gate cloning system for genetic engineering in fungi

Author

Bastian Joehnk, Marius Terfrüchte, Michael Feldbrügge, Rosa A. Fajardo-Somera, Kerstin Schipper, Gerhard H. Braus, and Meritxell Riquelme

Subjects

Genetics, Cloning, 0303 health sciences, biology, 030306 microbiology, Ustilago, Golden Gate Cloning, Mutant, Genetic Vectors, biology.organism_classification, Microbiology, Genome, Aspergillus nidulans, 03 medical and health sciences, Restriction enzyme, Mutation, Cloning, Molecular, Homologous recombination, Genetic Engineering, Homologous Recombination, Gene Deletion, 030304 developmental biology

Abstract

The corn pathogen Ustilago maydis is a well-studied fungal model organism. Along with a broad set of experimental tools, versatile strategies for the generation of gene replacement mutants by homologous recombination in U. maydis have been developed. Nevertheless, the production of corresponding linear DNA constructs still constitutes a time-limiting step. To overcome this bottleneck, various resistance cassette modules were adopted for use with the so-called Golden Gate cloning strategy. These modules allow not only simple gene deletions but also more sophisticated genetic manipulations like inserting sequences for C-terminal protein tagging. The type IIs restriction enzyme BsaI was selected for this novel approach as its recognition sites are comparatively rare in the U. maydis genome. To test the efficiency of the new strategy it was used to test the influence of varying flank lengths as well as the effect of non-homologous flank ends on homologous recombination. Importantly, to proof a broad applicability in other fungi the same strategy was used to generate mutants in the filamentous ascomycete Aspergillus nidulans. Hence, we present a highly efficient and economic cloning strategy that speeds up reverse genetic approaches in fungi.

Published

2013

48. Modular construction of plasmids by parallel assembly of linear vector components

Author

Xiaoying Li, XinZheng Gao, Peng Zhou, Yuenan Li, Pu Yan, and Wentao Shen

Subjects

Genetics, chemistry.chemical_classification, DNA ligase, Expression vector, Base Sequence, Golden Gate Cloning, Biophysics, Cloning vector, Cell Biology, Computational biology, Biology, Biochemistry, Restriction enzyme, Plasmid, chemistry, Multiple cloning site, Cloning, Molecular, Molecular Biology, T-DNA Binary system, Plasmids

Abstract

Construction of plasmids is the basic and pivotal technology in molecular biology. The common method for constructing plasmids is to cut DNA fragments by restriction enzymes and then join the resulting fragments using ligase. We present here a modified Golden Gate cloning method for modular construction of plasmids. Unlike the original Golden Gate cloning system for cloning from entry vector to expression vector, this method can be used to construct plasmids immediately from linear DNA fragments. After polymerase chain reaction (PCR) amplification for flanking with BsaI sites, multiple linear DNA components (modules) can be parallel assembled into a circle plasmid by a single restriction-ligation reaction using the method. This method is flexible to construct different types of plasmids because the modules can be freely selected and assembled in any combination. This method was applied successfully to construct a prokaryotic expression plasmid from four modules and a plant expression plasmid from five modules (fragments). The results suggest that this method provides a simple and flexible platform for modular construction of plasmids.

Published

2012

49. Golden gate shuffling: a one-pot DNA shuffling method based on type IIs restriction enzymes

Author

Sylvestre Marillonnet, Romy Kandzia, Carola Engler, and Ramona Gruetzner

Subjects

Trypsinogen, Science, Golden Gate Cloning, Genetic Vectors, Molecular Sequence Data, DNA, Recombinant, Computational biology, Molecular cloning, law.invention, chemistry.chemical_compound, Plasmid, law, Animals, Humans, Cloning, Molecular, Deoxyribonucleases, Type II Site-Specific, Molecular Biology, Genetics, Multidisciplinary, Shuffling, Base Sequence, Models, Genetic, Chemistry, Genetic Variation, DNA Shuffling, Genetics and Genomics/Gene Expression, DNA shuffling, Restriction enzyme, Recombinant DNA, Medicine, Cattle, Biotechnology/Bioengineering, Research Article, Biotechnology

Abstract

We have developed a protocol to assemble in one step and one tube at least nine separate DNA fragments together into an acceptor vector, with 90% of recombinant clones obtained containing the desired construct. This protocol is based on the use of type IIs restriction enzymes and is performed by simply subjecting a mix of 10 undigested input plasmids (nine insert plasmids and the acceptor vector) to a restriction-ligation and transforming the resulting mix in competent cells. The efficiency of this protocol allows generating libraries of recombinant genes by combining in one reaction several fragment sets prepared from different parental templates. As an example, we have applied this strategy for shuffling of trypsinogen from three parental templates (bovine cationic trypsinogen, bovine anionic trypsinogen and human cationic trypsinogen) each divided in 9 separate modules. We show that one round of shuffling using the 27 trypsinogen entry plasmids can easily produce the 19,683 different possible combinations in one single restriction-ligation and that expression screening of a subset of the library allows identification of variants that can lead to higher expression levels of trypsin activity. This protocol, that we call 'Golden Gate shuffling', is robust, simple and efficient, can be performed with templates that have no homology, and can be combined with other shuffling protocols in order to introduce any variation in any part of a given gene.

Published

2009

50. A One Pot, One Step, Precision Cloning Method with High Throughput Capability

Author

Romy Kandzia, Sylvestre Marillonnet, and Carola Engler

Subjects

Time Factors, Golden Gate Cloning, Science, Genetic Vectors, Kanamycin Resistance, Molecular Sequence Data, Arabidopsis, Computational biology, Efficiency, Molecular cloning, Genes, Plant, Models, Biological, Sensitivity and Specificity, law.invention, Plasmid, Recognition sequence, law, Escherichia coli, Cloning, Molecular, Biotechnology/Plant Biotechnology, Molecular Biology, Genetics, Physics, Multidisciplinary, Base Sequence, DNA Restriction Enzymes, Plants, Genetically Modified, Restriction site, Restriction enzyme, Subcloning, Recombinant DNA, Medicine, Research Article, Biotechnology

Abstract

Current cloning technologies based on site-specific recombination are efficient, simple to use, and flexible, but have the drawback of leaving recombination site sequences in the final construct, adding an extra 8 to 13 amino acids to the expressed protein. We have devised a simple and rapid subcloning strategy to transfer any DNA fragment of interest from an entry clone into an expression vector, without this shortcoming. The strategy is based on the use of type IIs restriction enzymes, which cut outside of their recognition sequence. With proper design of the cleavage sites, two fragments cut by type IIs restriction enzymes can be ligated into a product lacking the original restriction site. Based on this property, a cloning strategy called ‘Golden Gate’ cloning was devised that allows to obtain in one tube and one step close to one hundred percent correct recombinant plasmids after just a 5 minute restriction-ligation. This method is therefore as efficient as currently used recombination-based cloning technologies but yields recombinant plasmids that do not contain unwanted sequences in the final construct, thus providing precision for this fundamental process of genetic manipulation.

Published

2008