Your search keyword '"Yeasts genetics"' showing total 160 results

1. Measurement of rRNA Synthesis and Degradation Rates by 3 H-Uracil Labeling in Yeast.

Author

García-Marcelo MJ, Singh G, Chávez S, and Pérez-Ortín JE

Subjects

RNA, Fungal metabolism, RNA, Fungal genetics, RNA Stability, Isotope Labeling methods, Blotting, Northern methods, Yeasts metabolism, Yeasts genetics, RNA, Ribosomal metabolism, RNA, Ribosomal genetics, Uracil metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae genetics

Abstract

In order to measure the actual synthesis and degradation rates (SR, DR) for rRNA in yeast, we developed a method based on the pulse labeling and quantification of newly synthesized large rRNA molecules by a known mass of cells. The SR is calculated as the ratio of new rRNA molecules (synthesized after a short [5,6- 3 H]-uracil pulse) to total rRNA (a proxy of cell mass), calculated by northern blotting after hybridization with a 32 P-labeled rRNA probe. Then to measure the DR we perform a chase of the existing 3 H-labeled rRNA for several hours during yeast culture growth. We have used this method in control experiments where the yeast cell volume varies as a way to check if the SR and DR are constant with the cell volume., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

2. PicoShells: Hollow Hydrogel Microparticles for High-Throughput Screening of Clonal Libraries.

Author

Williamson C, van Zee M, and Di Carlo D

Subjects

Flow Cytometry, Yeasts genetics, Yeasts growth & development, Yeasts metabolism, Clone Cells physiology, Hydrogels chemical synthesis, High-Throughput Screening Assays instrumentation, High-Throughput Screening Assays methods, Single-Cell Gene Expression Analysis instrumentation, Single-Cell Gene Expression Analysis methods, Microfluidics instrumentation, Microfluidics methods

Abstract

Microfluidics enables the creation of monodisperse, micron-scale aqueous droplets, or other compartments. These droplets serve as picolitre-volume reaction chambers which can be utilized for various chemical assays or reactions. Here we describe the use of a microfluidic droplet generator to encapsulate single cells within hollow hydrogel microparticles called PicoShells. The PicoShell fabrication utilizes a mild pH-based crosslinking modality of an aqueous two-phase prepolymer system, avoiding the cell death and unwanted genomic modifications that accompany more typical, ultraviolet light crosslinking techniques. The cells are grown inside of these PicoShells into monoclonal colonies in any number of environments, including scaled production environments using commercially relevant incubation methods. Colonies can be phenotypically analyzed and/or sorted using standard, high-throughput laboratory techniques, namely, fluorescence-activated cell sorting (FACS). Cell viability is maintained throughout particle fabrication and analysis, and cells exhibiting a desired phenotype can be selected and released for re-culturing and downstream analysis. Large-scale cytometry runs are of particular use when measuring the protein expression of heterogeneous cells in response to environmental stimuli, notably to identify targets early in the drug discovery process. The sorted cells can also be encapsulated multiple times to direct the evolution of a cell line to a desired phenotype., (© 2023. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

3. ChIP-SICAP: A New Tool to Explore Gene-Regulatory Networks in Candida albicans and Other Yeasts.

Author

van Wijlick L, Goyal A, Bachellier-Bassi S, and d'Enfert C

Subjects

Chromatin genetics, Chromatin Immunoprecipitation methods, Gene Regulatory Networks, Candida albicans genetics, Yeasts genetics

Abstract

Chromatin immunoprecipitation followed by mass spectrometry (ChIP-MS) is a powerful method to identify protein interactions, and has long been used to gain insights into regulatory networks in relevant fungal species as well as many other organisms. In this chapter, we discuss a similar technique called ChIP-SICAP (chromatin immunoprecipitation with selective isolation of chromatin-associated proteins) that overcomes many of the traditional limitations of ChIP-MS, and describe a protocol that allows ChIP-SICAP to be applied to Candida albicans and other yeasts. Notably, the technique design permits stringent washing to remove contaminating proteins and antibodies before subsequent mass spectrometry processing, allows for genome-wide mapping of the bait protein by ChIP-seq after ChIP-SICAP from the same sample through a DNA recovery process, and specifically purifies and identifies proteins associating with chromatin. In the future, ChIP-SICAP will provide the yeast genomics research community an additional method to explore the complex dynamics of the gene-regulatory networks modulating morphology, metabolism and response to stress., (© 2022. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2022

4. Automated Evolutionary Engineering of Yeasts.

Author

de Hulster E, Mooiman C, Timmermans R, and Mans R

Subjects

Bioreactors, Metabolic Engineering methods, Industrial Microbiology methods, Yeasts genetics

Abstract

Evolutionary engineering of microbes provides a powerful tool for untargeted optimization of (engineered) cell factories and identification of genetic targets for further research. Directed evolution is an intrinsically time-intensive effort, and automated methods can significantly reduce manual labor. Here, design considerations for various evolutionary engineering methods are described, and generic workflows for batch-, chemostat-, and accelerostat-based evolution in automated bioreactors are provided. These methods can be used to evolve yeast cultures for >1000 generations and are designed to require minimal manual intervention., (© 2022. Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2022

5. Yeast Nucleoplasmic Extracts and an Application to Visualize Chromatin Assembly on Single Molecules of DNA.

Author

Wang Y and Fu YV

Subjects

Data Analysis, Microscopy, Fluorescence methods, Chromatin Assembly and Disassembly, DNA, Fungal, Molecular Imaging methods, Nucleosomes metabolism, Single Molecule Imaging methods, Subcellular Fractions, Yeasts genetics, Yeasts metabolism

Abstract

In eukaryotic cells, the genomic DNA is packaged into chromatin, the basic unit of which is the nucleosome. Studying the mechanism of chromatin formation under physiological conditions is inherently difficult due to the limitations of research approaches. Here we describe how to prepare a biochemical system called yeast nucleoplasmic extracts (YNPE). YNPE is derived from yeast nuclei, and the in vitro system can mimic the physiological conditions of the yeast nucleus in vivo. In YNPE, the dynamic process of chromatin assembly has been observed in real time at the single-molecule level by total internal reflection fluorescence microscopy. YNPE provides a novel tool to investigate many aspects of chromatin assembly under physiological conditions and is competent for single-molecule approaches.

Published

2021

6. Use of a Lariat Capping Ribozyme to Study Cap Function In Vivo.

Author

Pietschmann M, Tempel G, Halladjian M, Krogh N, and Nielsen H

Subjects

Blotting, Northern, Dinucleoside Phosphates genetics, Electrophoresis, Polyacrylamide Gel, Exonucleases metabolism, Flow Cytometry, Internal Ribosome Entry Sites genetics, Models, Molecular, Nucleic Acid Conformation, RNA Caps metabolism, RNA, Messenger chemistry, Yeasts genetics, Dinucleoside Phosphates metabolism, RNA, Catalytic genetics, RNA, Catalytic metabolism, RNA, Messenger metabolism, Yeasts metabolism

Abstract

A lariat cap is a naturally occurring substitute of a conventional mRNA cap and is found in a particular genomic setting in a few eukaryotic microorganisms. It is installed by the lariat capping ribozyme acting in cis. In principle, any RNA molecule in any organism can be equipped with a lariat cap in vivo when expressed downstream of a lariat capping ribozyme. Lariat capping is thus a versatile tool for studying the importance of the 5' end structure of RNA molecules. In this chapter, we present protocols to validate the presence of the lariat cap and measure the efficiency of in vivo cleavage by the lariat capping ribozyme.

Published

2021

7. Monitoring 5'-End Resection at Site-Specific Double-Strand Breaks by Southern Blot Analysis.

Author

Peng H, Zhang S, and Chen X

Subjects

Genome, Fungal, Rad51 Recombinase metabolism, Yeasts genetics, Yeasts metabolism, Blotting, Southern methods, DNA Breaks, Double-Stranded, Recombinational DNA Repair

Abstract

DNA double-strand break (DSB) is one of the most deleterious types of DNA lesions threatening genome integrity. Cells have evolved several exquisite pathways to repair these breaks. Homologous recombination (HR) is an essential DSB repair mechanism that utilizes an intact homologous sequence as a template to repair DSBs with high fidelity. To initiate the HR repair, the 5'-ends of DSBs have to be nucleolytically cleaved by nucleases to generate 3'-single-strand DNA (ssDNA). Exposed 3'-ssDNA recruits the ssDNA binding protein complex RPA to activate the DNA damage checkpoint. RPA is subsequently replaced by Rad51 recombinase to form Rad51 nucleoprotein filament that catalyzes strand invasion and formation of the D-loop. Processing of 5'-ends (called resection) is a crucial step that determines the choice of repair pathways. Here we introduce an assay for monitoring the dynamics of resection at different locations from a site-specific DSB in yeast.

Published

2021

8. Use YeastFab to Construct Genetic Parts and Multicomponent Pathways for Metabolic Engineering.

Author

Jiang S, Luo Z, and Dai J

Subjects

Gene Expression, Gene Order, Open Reading Frames, Polymerase Chain Reaction, Saccharomycetales genetics, Saccharomycetales metabolism, Synthetic Biology methods, Transformation, Genetic, Cloning, Molecular methods, Genetic Vectors genetics, Metabolic Engineering methods, Yeasts genetics, Yeasts metabolism

Abstract

Budding yeast, as a eukaryotic model organism, has well-defined genetic information and a highly efficient recombination system, making it a good host to produce exogenous chemicals. Since most metabolic pathways require multiple genes to function in coordination, it is usually laborious and time-consuming to construct a working pathway. To facilitate the construction and optimization of multicomponent exogenous pathways in yeast, we recently developed a method called YeastFab Assembly, which includes three steps: (1) make standard and reusable genetic parts, (2) construct transcription units from characterized parts, and (3) assemble a complete pathway. Here we describe a detailed protocol of this method.

Published

2021

9. Chromosomal Rearrangements of Synthetic Yeast by SCRaMbLE.

Author

Luo Z, Jiang S, and Dai J

Subjects

Gene Expression Regulation, Fungal, Genetic Engineering methods, Genetic Loci, Genome, Fungal, Open Reading Frames, Phenotype, Chromosome Aberrations, Chromosomes, Fungal, Recombination, Genetic, Synthetic Biology methods, Yeasts genetics

Abstract

Diversified genomes derived from chromosomal rearrangements are valuable materials for evolution. Naturally, chromosomal rearrangements occur at extremely low frequency to ensure genome stability. In the synthetic yeast genome project (Sc2.0), an inducible chromosome rearrangement system named Synthetic Chromosome Rearrangement and Modification by LoxP-mediated Evolution (SCRaMbLE) is built to produce chromosomal rearrangements such as deletion, duplication, inversion, and translocation at high efficiency. Here, we detail the method to activate SCRaMbLE in a synthetic strain, to analyze the SCRaMbLEd genome, and to dissect the causative rearrangements for a desired phenotype after SCRaMbLEing.

Published

2021

10. CRISPR Nickase-Mediated Base Editing in Yeast.

Author

Kuroda K and Ueda M

Subjects

CRISPR-Cas Systems, DNA Repair, Gene Order, Genetic Vectors genetics, Mutagenesis, RNA, Guide, CRISPR-Cas Systems, Recombinational DNA Repair, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Clustered Regularly Interspaced Short Palindromic Repeats, Deoxyribonuclease I metabolism, Gene Editing, Yeasts genetics, Yeasts metabolism

Abstract

The clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9 system has enabled efficient, markerless genome editing in a wide range of organisms. However, there is an off-target effect and a limit to the area of precise editing. Bases that can be precisely edited are limited to within the 20-base pair gRNA-targeting site and protospacer adjacent motif (PAM) sequence. We have developed a CRISPR nickase system that can perform a precise genome-wide base editing in Saccharomyces cerevisiae using a single Cas9 nickase. This system can precisely edit a broader genomic region by the avoidance of double-strand break (DSB) and subsequent non-homologous end joining (NHEJ). Furthermore, unintended mutations were not found at off-target sites in this system. In combination with yeast gap repair cloning, precise genome editing of yeast cells can be performed in 5 days. Here, we describe the methods for precise and convenient genome editing using this novel CRISPR nickase system.

Published

2021

11. Use of Yeast Plasmids: Transformation and Inheritance Assays.

Author

Mereshchuk A, Chew JSK, and Dobson MJ

Subjects

Centromere genetics, Genes, Fungal, Genetic Markers, Genetic Testing, Genetic Vectors genetics, Genomic Instability, Inheritance Patterns, Transformation, Genetic, Plasmids genetics, Yeasts genetics

Abstract

The use of the budding yeast Saccharomyces cerevisiae as a model genetic organism has been facilitated by the availability of a wide range of yeast shuttle vectors, plasmids that can be propagated in Escherichia coli and also in yeast, where they are stably maintained at low- or high-copy number, depending on the plasmid system. Here we provide an introduction to the low-copy (ARS/CEN) and multi-copy (2-μm-based) plasmids, the marker genes commonly used for plasmid selection in yeast, methods for transforming yeast and monitoring plasmid inheritance, and tips for working with yeast transformants.

Published

2021

12. RNA Precipitation.

Author

Bourguignon-Igel V, Abel Y, and Rederstorff M

Subjects

Alcohols chemistry, Chemical Precipitation, RNA, Fungal chemistry, Salts chemistry, RNA, Transfer chemistry, RNA, Transfer isolation & purification, Yeasts genetics

Abstract

Precipitation is a critical step to recover RNA of high purity. This chapter describes the principles of alcoholic precipitation as well as a standard, basic protocol with key advices to observe, but numerous variations on the theme are discussed. Indeed, several important parameters, such as the choice of salt, alcohol, or carrier, have to be considered to improve the efficiency of precipitation and the yield of RNA recovery.

Published

2021

13. FLP-Mediated Site-Specific Gene Integration in Rice.

Author

Srivastava V

Subjects

DNA Nucleotidyltransferases genetics, Gene Targeting, Genetic Vectors genetics, Oryza growth & development, Oryza metabolism, Phenotype, Plants, Genetically Modified growth & development, Plants, Genetically Modified metabolism, Promoter Regions, Genetic, Oryza genetics, Plant Proteins genetics, Plants, Genetically Modified genetics, Recombination, Genetic, Yeasts genetics

Abstract

Enabling precise gene integration is important for installing traits in the plants. One of the practical methods of achieving precise gene integration is by using the yeast FLP-FRT recombination system that is efficient in directing DNA integration into the "engineered" genomic sites. The critical parameters of this method include the use of the thermostable version of FLP protein and the promoter trap design to select site-specific integration clones. The resulting transgenic plants display stable expression that is transmitted to the progeny. Therefore, FLP-mediated site-specific integration method could be used for trait engineering in the crop plants or testing gene functions in the model plants.

Published

2021

14. A Versatile Protocol to Generate Translocations in Yeast Genomes Using CRISPR/Cas9.

Author

Agier N, Fleiss A, Delmas S, and Fischer G

Subjects

Cloning, Molecular, DNA Shuffling, Gene Editing, Gene Order, Gene Rearrangement, Genetic Engineering methods, Genetic Vectors genetics, Plasmids genetics, RNA, Guide, CRISPR-Cas Systems, Recombination, Genetic, Transformation, Genetic, CRISPR-Cas Systems, Genome, Fungal, Translocation, Genetic, Yeasts genetics

Abstract

Genomic engineering methods represent powerful tools to examine chromosomal modifications and to subsequently study their impacts on cellular phenotypes. However, quantifying the fitness impact of translocations, independently from base substitutions or the insertion of genetic markers, remains a challenge. Here we report a rapid and straightforward protocol for engineering either targeted reciprocal translocations at the base pair level of resolution between two chromosomes or multiple simultaneous rearrangements in the yeast genome, without inserting any marker sequence in the chromosomes. Our CRISPR/Cas9-based method consists of inducing either (1) two double-strand breaks (DSBs) in two different chromosomes with two distinct guide RNAs (gRNAs) while providing specifically designed homologous donor DNA forcing the trans-repair of chromosomal extremities to generate a targeted reciprocal translocation or (2) multiple DSBs with a single gRNA targeting dispersed repeated sequences and leaving endogenous uncut copies of the repeat to be used as donor DNA, thereby generating multiple translocations, often associated with large segmental duplications (Fleiss, et al. PLoS Genet 15:e1008332, 2019).

Published

2021

15. Sparse Regression Models for Unraveling Group and Individual Associations in eQTL Mapping.

Author

Cheng W, Zhang X, and Wang W

Subjects

Algorithms, Computational Biology methods, Humans, ROC Curve, Reproducibility of Results, Yeasts genetics, Chromosome Mapping, Gene Expression, Genome-Wide Association Study methods, Quantitative Trait Loci, Regression Analysis

Abstract

As a promising tool for dissecting the genetic basis of common diseases, expression quantitative trait loci (eQTL) study has attracted increasing research interest. Traditional eQTL methods focus on testing the associations between individual single-nucleotide polymorphisms (SNPs) and gene expression traits. A major drawback of this approach is that it cannot model the joint effect of a set of SNPs on a set of genes, which may correspond to biological pathways. To alleviate this limitation, in this chapter, we propose geQTL, a sparse regression method that can detect both group-wise and individual associations between SNPs and expression traits. geQTL can also correct the effects of potential confounders. Our method employs computationally efficient technique, thus it is able to fulfill large scale studies. Moreover, our method can automatically infer the proper number of group-wise associations. We perform extensive experiments on both simulated datasets and yeast datasets to demonstrate the effectiveness and efficiency of the proposed method. The results show that geQTL can effectively detect both individual and group-wise signals and outperform the state-of-the-arts by a large margin. This book chapter well illustrates that decoupling individual and group-wise associations for association mapping is able to improve eQTL mapping accuracy, and inferring individual and group-wise associations.

Published

2020

16. Transportomics for the Characterization of Plant Apocarotenoid Transmembrane Transporters.

Author

Demurtas OC, de Brito Francisco R, Martinoia E, and Giuliano G

Subjects

Biological Transport, Chromatography, High Pressure Liquid, Chromatography, Liquid, Electroporation, Mass Spectrometry, Membrane Transport Proteins genetics, Microsomes metabolism, Plants genetics, Yeasts genetics, Yeasts metabolism, Carotenoids metabolism, Membrane Transport Proteins metabolism, Plants metabolism, Proteomics methods

Abstract

Apocarotenoids are carotenoid derivatives produced by the nonenzymatic or enzymatic cleavage of carotenoids, followed by different enzymatic modifications. In plants, apocarotenoids play different roles, such as attraction of pollinators and seeds dispersal, defense against pathogens and herbivores, protection against photo-oxidative stresses, stimulation and inhibition of plant growth and regulation of biological processes in the case of phytohormones abscisic acid and strigolactones. While carotenoids are in general plastid-localized metabolites, apocarotenoids can reach different final destinations inside or outside the cell. The mechanisms of apocarotenoid transport through biological membranes have been poorly studied. This chapter describes a method to characterize transmembrane transporters involved in the transport of polar and amphipathic apocarotenoids. This protocol was successfully used to in vitro characterize the transport activity of ATP-binding cassette (ABC) and multidrug and toxic extrusion (MATE) in microsomes isolated from Saccharomyces cerevisiae expressing these plant transporters.

Published

2020

17. Selection of the Optimal Yeast Host for the Synthesis of Recombinant Enzymes.

Author

Bischoff F, Giersberg M, Matthes F, Schwalenberg T, Worch S, and Kunze G

Subjects

Enzymes chemistry, Enzymes genetics, Fermentation, Genetic Vectors, Microorganisms, Genetically-Modified, Plasmids genetics, Polymerase Chain Reaction, Protein Folding, Protein Processing, Post-Translational, Recombinant Proteins metabolism, Transformation, Genetic, Yeasts metabolism, Enzymes metabolism, Molecular Biology methods, Protein Engineering methods, Recombinant Proteins genetics, Yeasts genetics

Abstract

Yeasts, like Arxula adeninivorans, Hansenula polymorpha, Pichia pastoris, Debaryomyces hansenii, Debaryomyces polymorphus, Schwanniomyces occidentalis, Yarrowia lipolytica, and Saccharomyces cerevisiae are frequently used producers of recombinant enzymes, particularly when posttranslational modifications are mandatory to obtain full functionality. The wide-range transformation/expression platform presented in this chapter can be used to select the optimal yeast host for high-level synthesis of the desired enzyme with favorable biochemical properties. This platform is composed of a selection marker and up to four expression modules in a linearized cassette. Here we describe the protocols for the assembly as well as the transformation of yeast strains with the respective cassettes, screening of transformants, the isolation and biochemical characterization of the enzymes, and finally a simple fermentation strategy to achieve maximal yields of the chosen recombinant enzyme.

Published

2019

18. Determining the Lipid-Binding Specificity of SMP Domains: An ERMES Subunit as a Case Study.

Author

AhYoung AP and Egea PF

Subjects

Bacteria genetics, Biological Transport, Carrier Proteins isolation & purification, Chromatography, Liquid, Chromatography, Thin Layer, Endoplasmic Reticulum metabolism, Gene Expression Regulation, Liposomes, Mitochondrial Proteins chemistry, Mitochondrial Proteins isolation & purification, Phospholipids chemistry, Phospholipids metabolism, Protein Subunits chemistry, Protein Subunits metabolism, Recombinant Proteins, Structure-Activity Relationship, Yeasts genetics, Carrier Proteins chemistry, Carrier Proteins metabolism, Mitochondrial Proteins metabolism, Protein Interaction Domains and Motifs

Abstract

Membrane contact sites between the endoplasmic reticulum (ER) and mitochondria function as a central hub for the exchange of phospholipids and calcium. The yeast Endoplasmic Reticulum-Mitochondrion Encounter Structure (ERMES) complex is composed of five subunits that tether the ER and mitochondria. Three ERMES subunits (i.e., Mdm12, Mmm1, and Mdm34) contain the synaptotagmin-like mitochondrial lipid-binding protein (SMP) domain. The SMP domain belongs to the tubular lipid-binding protein (TULIP) superfamily, which consists of ubiquitous lipid scavenging and transfer proteins. Herein, we describe the methods for expression and purification of recombinant Mdm12, a bona fide SMP-containing protein, together with the subsequent identification of its bound phospholipids by high-performance thin-layer chromatography (HPTLC) and the characterization of its lipid exchange and transfer functions using lipid displacement and liposome flotation in vitro assays with liposomes as model biological membranes. These methods can be applied to the study and characterization of novel lipid-binding and lipid-transfer proteins.

Published

2019

19. Analysis of the Chromosomal Localization of Yeast SMC Complexes by Chromatin Immunoprecipitation.

Author

Makrantoni V, Robertson D, and Marston AL

Subjects

Binding Sites genetics, Chromatin genetics, Chromosome Segregation genetics, Protein Binding genetics, Chromatin Immunoprecipitation methods, Chromosomes, Fungal genetics, Yeasts genetics

Abstract

A plethora of biological processes like gene transcription, DNA replication, DNA recombination, and chromosome segregation are mediated through protein-DNA interactions. A powerful method for investigating proteins within a native chromatin environment in the cell is chromatin immunoprecipitation (ChIP). Combined with the recent technological advancement in next generation sequencing, the ChIP assay can map the exact binding sites of a protein of interest across the entire genome. Here we describe a-step-by step protocol for ChIP followed by library preparation for ChIP-seq from yeast cells.

Published

2019

20. Novel Microbial Modification Tools to Convert Lipids into Other Value-Added Products.

Author

Kumari P, Yusuf F, and Gaur NA

Subjects

Cloning, Molecular methods, Genetic Vectors genetics, RNA, Guide, CRISPR-Cas Systems genetics, Transformation, Genetic, CRISPR-Cas Systems, Gene Editing methods, Lipids genetics, Yeasts genetics

Abstract

CRISPR-Cas9 Clustered Regularly Interspaced Short Palindromic Repeats (CRISPR) and CRISPR associated (Cas) is a microbial adaptive immune system that has revolutionized the field of molecular biology and genome engineering. The Type II CRISPR system consists of Cas9 nuclease of Streptococcus pyogenes and the RNA complex that guides Cas9 nuclease to a specific sequence of DNA in the genome. The CRISPR-Cas9 technology has reformed our ability to edit DNA and to regulate expression levels of genes of interest to high precision and accuracy. It is a powerful technology, which is used for genome engineering of a wide range of organisms for various applications. Here, we describe a method involving CRISPR-Cas9-mediated genome editing via nonhomologous end joining (NHEJ) or homology-directed repair (HDR) mechanisms for biotechnological applications in yeast. The complete procedure of genome editing including target sequence selection, cloning gRNA with a target sequence, transformation, and verification of the desired mutation/deletion or insertion can be achieved within 2-3 weeks in yeast.

Published

2019

21. Established and Upcoming Yeast Expression Systems.

Author

Gündüz Ergün B, Hüccetoğulları D, Öztürk S, Çelik E, and Çalık P

Subjects

Gene Expression Regulation, Fungal, Genetic Markers, Microorganisms, Genetically-Modified, Yeasts metabolism, Genetic Engineering methods, Genetic Vectors, Promoter Regions, Genetic, Yeasts genetics

Abstract

Yeast was the first microorganism used by mankind for biotransformation of feedstock that laid the foundations of industrial biotechnology. Long historical use, vast amount of data, and experience paved the way for Saccharomyces cerevisiae as a first yeast cell factory, and still it is an important expression platform as being the production host for several large volume products. Continuing special needs of each targeted product and different requirements of bioprocess operations have led to identification of different yeast expression systems. Modern bioprocess engineering and advances in omics technology, i.e., genomics, transcriptomics, proteomics, secretomics, and interactomics, allow the design of novel genetic tools with fine-tuned characteristics to be used for research and industrial applications. This chapter focuses on established and upcoming yeast expression platforms that have exceptional characteristics, such as the ability to utilize a broad range of carbon sources or remarkable resistance to various stress conditions. Besides the conventional yeast S. cerevisiae, established yeast expression systems including the methylotrophic yeasts Pichia pastoris and Hansenula polymorpha, the dimorphic yeasts Arxula adeninivorans and Yarrowia lipolytica, the lactose-utilizing yeast Kluyveromyces lactis, the fission yeast Schizosaccharomyces pombe, and upcoming yeast platforms, namely, Kluyveromyces marxianus, Candida utilis, and Zygosaccharomyces bailii, are compiled with special emphasis on their genetic toolbox for recombinant protein production.

Published

2019

22. Yeast-Based Screens to Target Alpha-Synuclein Toxicity.

Author

Brás IC, Popova B, Braus GH, and Outeiro TF

Subjects

Humans, Parkinson Disease genetics, Parkinson Disease metabolism, Parkinson Disease pathology, Reproducibility of Results, Yeasts metabolism, alpha-Synuclein metabolism, Drug Evaluation, Preclinical methods, High-Throughput Screening Assays, Yeasts genetics, alpha-Synuclein antagonists & inhibitors, alpha-Synuclein genetics

Abstract

The budding yeast Saccharomyces cerevisiae (S. cerevisiae) has been a remarkable experimental model for the discovery of fundamental biological processes. The high degree of conservation of cellular and molecular processes between the budding yeast and higher eukaryotes has made it a valuable system for the investigation of the molecular mechanisms behind various types of devastating human pathologies. Genetic screens in yeast provided important insight into the toxic mechanisms associated with the accumulation of misfolded proteins. Thus, using yeast genetics and high-throughput screens, novel molecular targets with therapeutic potential have been identified. Here, we describe a yeast screen protocol for the identification of genetic modifiers of alpha-synuclein (aSyn) toxicity, thereby accelerating the identification of novel potential targets for intervention in Parkinson's disease (PD) and other synucleinopathies.

Published

2019

23. A Genetic Screen for the Isolation of Mutants with Increased Flux in the Isoprenoid Pathway of Yeast.

Author

Wadhwa M and Bachhawat AK

Subjects

Carotenoids metabolism, Cloning, Molecular methods, Escherichia coli genetics, Escherichia coli metabolism, Metabolic Networks and Pathways, Mutagenesis, Plasmids genetics, Reproducibility of Results, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Transformation, Genetic, Genes, Fungal, Genetic Testing, Mutation, Terpenes metabolism, Yeasts genetics, Yeasts metabolism

Abstract

The yeast Saccharomyces cerevisiae is one of the preferred hosts for the production of terpenoids through metabolic engineering. A genetic screen to identify novel mutants that can increase the flux in the isoprenoid pathway has been lacking. We present here the method that has led to the development of a carotenoid based visual screen by exploiting the carotenogenic genes from the red yeast Rhodosporidium toruloides, an organism known to have high levels of carotenoids. We also discuss the methods to use this screen for the identification of mutants that can lead to higher isoprenoid flux. The carotenoid based screen was developed in S. cerevisiae using phytoene synthase RtPSY1 and a hyperactive mutant of the enzyme phytoene dehydrogenase, RtCRTI(A393T) from Rhodosporidium toruloides. As validation of the genetic screen is critical at all stages, we describe the method to validate the screen using a known flux increasing gene, a truncated HMG1 (tHMG1). To demonstrate how this screen can be exploited to isolate mutants, we described how targeted mutagenesis of candidate gene, SPT15 a TATA binding protein involved in the global transcription machinery can be carried out to yield novel mutants with increased metabolic flux. Since it is also important to ensure that the isolated mutants are enhancing general isoprenoid flux, we describe how this can be established using an alternate isoprenoid, α-farnesene.

Published

2019

24. Detection and Quantification of Pseudouridine in RNA.

Author

Adachi H, DeZoysa MD, and Yu YT

Subjects

Animals, Cell Line, Isotope Labeling, Plants genetics, RNA chemistry, RNA Cleavage, Yeasts genetics, Pseudouridine, RNA genetics, RNA Processing, Post-Transcriptional

Abstract

Pseudouridylation is the most abundant of all RNA modifications. Pseudouridylation is dynamic and widespread among many different types of RNAs in living organisms, thus drawing a lot of recent interest from the RNA and epigenetics communities. To successfully carry out an investigation into RNA pseudouridylation, it is desirable to have a convenient and effective method capable of detection and quantification of pseudouridylation. Here, we present two such methods: one relies on pseudouridine (Ψ)-specific CMCT modification followed by reverse transcription/primer-extension (semiquantitative), and the other is based on site-specific cleavage and radiolabeling followed by nuclease digestion and TLC (quantitative). Although only semiquantitative, the CMCT and reverse transcription-based method is capable of detecting multiple Ψs (present in the same RNA molecule) in one reaction. In contrast, the second method, based on site-specific cleavage/labeling, nuclease digestion, and TLC, is quantitative, but can be used to analyze only one site at a time. These two methods can be used independently or in combination.

Published

2019

25. Detection and Elimination of Cellular Bottlenecks in Protein-Producing Yeasts.

Author

Zahrl RJ, Gasser B, Mattanovich D, and Ferrer P

Subjects

Gene Expression Regulation, Fungal, Microorganisms, Genetically-Modified, Protein Biosynthesis, Protein Folding, Recombinant Proteins genetics, Recombinant Proteins metabolism, Transcription, Genetic, Yeasts cytology, Protein Engineering methods, Recombinant Proteins biosynthesis, Yeasts genetics, Yeasts metabolism

Abstract

Yeasts are efficient cell factories and are commonly used for the production of recombinant proteins for biopharmaceutical and industrial purposes. For such products high levels of correctly folded proteins are needed, which sometimes requires improvement and engineering of the expression system. The article summarizes major breakthroughs that led to the efficient use of yeasts as production platforms and reviews bottlenecks occurring during protein production. Special focus is given to the metabolic impact of protein production. Furthermore, strategies that were shown to enhance secretion of recombinant proteins in different yeast species are presented.

Published

2019

26. Efficient Depletion of Fission Yeast Condensin by Combined Transcriptional Repression and Auxin-Induced Degradation.

Author

Kakui Y and Uhlmann F

Subjects

Cell Cycle Proteins genetics, Chromatin genetics, Chromosomes, Fungal genetics, Interphase genetics, Mitosis genetics, Adenosine Triphosphatases genetics, DNA-Binding Proteins genetics, Indoleacetic Acids pharmacology, Multiprotein Complexes genetics, Proteolysis drug effects, Transcription, Genetic genetics, Yeasts drug effects, Yeasts genetics

Abstract

Structural maintenance of chromosomes (SMC) complexes play pivotal roles in controlling chromatin organization. Condensin is an essential SMC complex that compacts chromatin to form condensed chromosomes in mitosis. Complete condensin inactivation is necessary to reveal how condensin converts interphase chromatin into mitotic chromosomes. Here, we have developed a condensin depletion system in fission yeast that combines transcriptional repression with auxin-inducible protein degradation. This achieves efficient condensin depletion without need for a temperature shift. Our system is useful when studying how condensin contributes to chromosome architecture and is applicable to the study of other SMC complexes.

Published

2019

27. Assessing the Quality of Recombinant Products Made in Yeast.

Author

Vorauer-Uhl K and Lhota G

Subjects

Chromatography, Gel, Recombinant Proteins genetics, Yeasts genetics, Recombinant Proteins metabolism, Yeasts metabolism

Abstract

The product quality of recombinant proteins is of major importance for their intended purpose. The initial characterization of both simple and complex products should be performed as soon as practical. However, to comply with this high standard, appropriate selection of complementary methods is required. Therefore, conventional and sophisticated techniques are available, providing diverse information about the product quality.In this chapter methods are presented, which enable the determination of the overall protein quality, their aggregation and peptide composition. Methods applied for the determination of posttranslational modifications such as glycan analysis are not described. In this regard, chromatographic, high-resolution technologies for the integrity of proteins as well as Western blot with specific detection methods are introduced, and individual strengths and perceived limitations are highlighted.

Published

2019

28. Redesigning of Microbial Cell Surface and Its Application to Whole-Cell Biocatalysis and Biosensors.

Author

Han L, Zhao Y, Cui S, and Liang B

Subjects

Catalysis, Bacteria chemistry, Bacteria genetics, Bacteria metabolism, Bacterial Proteins genetics, Bacterial Proteins metabolism, Biosensing Techniques methods, Fungal Proteins chemistry, Fungal Proteins genetics, Fungal Proteins metabolism, Peptide Library, Yeasts chemistry, Yeasts genetics, Yeasts metabolism

Abstract

Microbial cell surface display technology can redesign cell surfaces with functional proteins and peptides to endow cells some unique features. Foreign peptides or proteins are transported out of cells and immobilized on cell surface by fusing with anchoring proteins, which is an effective solution to avoid substance transfer limitation, enzyme purification, and enzyme instability. As the most frequently used prokaryotic and eukaryotic protein surface display system, bacterial and yeast surface display systems have been widely applied in vaccine, biocatalysis, biosensor, bioadsorption, and polypeptide library screening. In this review of bacterial and yeast surface display systems, different cell surface display mechanisms and their applications in biocatalysis as well as biosensors are described with their strengths and shortcomings. In addition to single enzyme display systems, multi-enzyme co-display systems are presented here. Finally, future developments based on our and other previous reports are discussed.

Published

2018

29. A qPCR-Based Protocol to Quantify DSB Resection.

Author

Ferrari M, Twayana S, Marini F, and Pellicioli A

Subjects

Computational Biology methods, DNA, Fungal, Yeasts genetics, DNA Breaks, Double-Stranded, Real-Time Polymerase Chain Reaction methods

Abstract

The nucleolytic degradation of the 5'-ending strand of a Double-Strand DNA break (DSB) is necessary to initiate homologous recombination to correctly repair the break. This process is called DNA end resection and it is finely regulated to prevent genome rearrangements. Here, we describe a protocol to quantify DSB resection rate by qPCR, which could be applied to every organisms whenever the break site and its flanking region sequences are known.

Published

2018

30. Synthetic Biology to Engineer Bacteriophage Genomes.

Author

Rita Costa A, Milho C, Azeredo J, and Pires DP

Subjects

Electroporation, Recombination, Genetic, Yeasts genetics, Bacteriophages genetics, Genetic Engineering methods, Genome, Viral, Synthetic Biology methods

Abstract

Recent advances in the synthetic biology field have enabled the development of new molecular biology techniques used to build specialized bacteriophages with new functionalities. Bacteriophages have been engineered towards a wide range of applications including pathogen control and detection, targeted drug delivery, or even assembly of new materials.In this chapter, two strategies that have been successfully used to genetically engineer bacteriophage genomes are addressed: a yeast-based platform and bacteriophage recombineering of electroporated DNA.

Published

2018

31. Isolation and Characterization of Extrachromosomal Double-Stranded RNA Elements from Carotenogenic Yeasts.

Author

Baeza M, Fernández-Lobato M, Alcaíno J, and Cifuentes V

Subjects

Fungal Viruses, Nucleic Acid Hybridization, RNA, Fungal genetics, RNA, Fungal isolation & purification, Yeasts virology, Carotenoids biosynthesis, RNA, Double-Stranded, Yeasts genetics, Yeasts metabolism

Abstract

Double-stranded RNA (dsRNA) molecules are widely found in yeasts and filamentous fungi. It has been suggested that these molecules may play an important role in the evolution of eukaryote genomes and could be a valuable tool in yeast typing. The characterization of these extrachromosomal genetic elements is usually a laborious process, especially when trying to analyze a large number of samples. In this chapter, we describe a simple method to isolate dsRNA elements from yeasts using low amounts of starting material and their application to different Xanthophyllomyces dendrorhous strains and other psychrotolerant carotenogenic yeasts. Furthermore, the methodologies for enzymatic and hybridization characterizations and quantification of relative dsRNA abundance are detailed.

Published

2018

32. A Method to Monitor Protein Turnover by Flow Cytometry and to Screen for Factors that Control Degradation by Fluorescence-Activated Cell Sorting.

Author

Comyn SA and Mayor T

Subjects

Gene Expression, Genes, Reporter, Genotype, High-Throughput Screening Assays, Mutation, Proteasome Endopeptidase Complex, Protein Folding, Protein Stability, Yeasts genetics, Yeasts metabolism, Flow Cytometry methods, Proteins metabolism, Proteolysis

Abstract

The protein quality control network consists of multiple proteins or protein complexes that monitor proteome integrity by mediating protein folding and the removal of proteins that cannot be folded. An integral component of this network is the ubiquitin-proteasome system, which controls the degradation of thousands of cellular proteins. A number of questions remain unanswered regarding the degradation of misfolded proteins. For example, how are substrates recognized and triaged? What are the identities of the components involved? And finally, what substrates are targeted by any given component of the quality control network? Finding answers to these questions is what inspires our work in protein quality control. Further characterization of protein quality control mechanisms requires methods that can reliably quantify turnover rates of model substrates. One such method is based on flow cytometry. Here, we present protocols detailing how to assess protein stability with flow cytometry and how fluorescence-activated cell sorting (FACS) can be used to screen for factors important for protein quality control and protein turnover.

Published

2018

33. Chromatin Immunoprecipitation in Human and Yeast Cells.

Author

Lee JB and Keung AJ

Subjects

Chromatin chemistry, Chromatin genetics, Chromatin metabolism, Cross-Linking Reagents chemistry, DNA genetics, DNA metabolism, DNA Fragmentation, DNA, Fungal analysis, DNA, Fungal genetics, DNA, Fungal metabolism, DNA-Binding Proteins chemistry, DNA-Binding Proteins metabolism, Formaldehyde chemistry, Fungal Proteins chemistry, Fungal Proteins metabolism, High-Throughput Nucleotide Sequencing methods, Humans, Micrococcal Nuclease metabolism, Polymerase Chain Reaction methods, Sequence Analysis, DNA methods, Sonication, Yeasts chemistry, Yeasts genetics, Yeasts metabolism, Chromatin Immunoprecipitation methods, DNA analysis

Abstract

Chromatin immunoprecipitation (ChIP) is an invaluable method to characterize interactions between proteins and genomic DNA, such as the genomic localization of transcription factors and posttranslational modification of histones. DNA and proteins are reversibly and covalently crosslinked using formaldehyde. Then the cells are lysed to release the chromatin. The chromatin is fragmented into smaller sizes either by micrococcal nuclease (MNase) or sonication and then purified from other cellular components. The protein-DNA complexes are enriched by immunoprecipitation (IP) with antibodies that target the epitope of interest. The DNA is released from the proteins by heat and protease treatment, followed by degradation of contaminating RNAs with RNase. The resulting DNA is analyzed using various methods, including PCR, qPCR, or sequencing. This protocol outlines each of these steps for both yeast and human cells.

Published

2018

34. Monitoring of Iron Depletion-Induced Mitophagy in Pathogenic Yeast.

Author

Tanabe K and Nagi M

Subjects

Fungal Proteins genetics, Fungal Proteins metabolism, Genes, Reporter, Hydro-Lyases genetics, Hydro-Lyases metabolism, Microscopy, Fluorescence, Mitochondria genetics, Sequence Deletion, Vacuoles metabolism, Yeasts genetics, Iron metabolism, Mitochondria metabolism, Mitophagy, Yeasts metabolism

Abstract

Mitophagy, which is the degradation of mitochondria via selective autophagic machinery, is thought to be involved in regulating the mass and function of mitochondria. Methods for detection of mitophagy have been reported for several fungal cells including some budding yeast, methylotrophic yeast, and filamentous fungi. Mitophagy in Saccharomyces cerevisiae is activated under nitrogen-poor conditions; however, the regulatory mechanism of mitophagy in most fungi has not been elucidated. Here we describe methods to monitor mitophagy in the pathogenic yeast Candida glabrata under iron-depleted conditions but not under nitrogen starvation. This observation may provide some clues to elucidate the physiological roles of mitophagy in eukaryotes.

Published

2018

35. Short Overview.

Author

Furuya N

Subjects

Animals, Autophagy, Biomarkers, Humans, Mitochondria genetics, Mitochondria metabolism, Yeasts genetics, Yeasts metabolism, Mitophagy

Abstract

Mitochondrial autophagy (mitophagy) is a mitochondrial quality control mechanism that selectively removes damaged mitochondria via autophagic degradation. Autophagic adaptor/receptor proteins contribute to the selective degradation of damaged mitochondria by autophagy. A part of them containing both ubiquitin binding domains and Atg8 interacting motif (AIM)/LC3 interacting region (LIR) motifs, which bind to the autophagy-related protein 8 (Atg8) family (LC3 and GABARAP family), lead ubiquitylated (damaged) mitochondria to selective removal. On the other hand, some specific outer mitochondrial membrane-anchored proteins containing AIM/LIR motif function as another type of autophagy adaptor/receptor proteins. Here I briefly summarize mechanisms of mitophagy and its related proteins.

Published

2018

36. A Rapid Combinatorial Approach to Assembling Synthetic Prokaryotic and Eukaryotic Protein Expression Vectors.

Author

Mullinax R, Johns SE, Rhodes D, Zhang V, McKinney N, Felts KA, Carstens CP, and Sheffield P

Subjects

Animals, Bacteria genetics, Cloning, Molecular methods, DNA genetics, Mammals genetics, Plasmids genetics, Recombination, Genetic genetics, Synthetic Biology methods, Yeasts genetics, Eukaryota genetics, Eukaryotic Cells metabolism, Gene Expression genetics, Genetic Vectors genetics, Prokaryotic Cells metabolism, Proteins genetics

Abstract

Vector construction and gene cloning are ubiquitous techniques essential to all fields of biological and medical research. They are the first steps in many endeavors leading to expressing proteins to understand gene function and regulation. However, they can often be rate-limiting, particularly in multi-gene studies, due to the time and effort required to assemble gene constructs and to identify the optimal constructs for protein expression.The SureVector system was developed to address this by enabling the rapid and reliable assembly of multiple DNA modules into a recombinant plasmid containing a gene-of-interest (GOI). It harnesses the power of synthetic biology to combine DNA modules from standard parts into a customized vector that expresses proteins in bacterial, mammalian, or yeast cells. The key advantages of the innovative SureVector system include rapid custom vector generation, enhanced flexibility to assemble new vectors quickly as experimental requirements change, and the reliable and precise assembly of fully interchangeable standard DNA modules that retain their functionality. The SureVector system is the only next-generation plasmid assembly technology to guarantee assembly of multiple functional DNA modules.

Published

2018

37. Quantitative Bromodeoxyuridine Immunoprecipitation Analyzed by High-Throughput Sequencing (qBrdU-Seq or QBU).

Author

Haye-Bertolozzi JE and Aparicio OM

Subjects

DNA Barcoding, Taxonomic, DNA Replication, DNA, Fungal, Gene Library, Quality Control, Yeasts genetics, Bromodeoxyuridine, High-Throughput Nucleotide Sequencing methods, Immunoprecipitation methods

Abstract

Incorporation into DNA of nucleoside analogs like 5-bromo-2'-deoxyuridine (BrdU) is a powerful tool for in vivo studies of DNA synthesis during replication and repair. Immunoprecipitation of BrdU-labeled DNA analyzed by DNA sequencing (BrdU-IP-seq) allows for genome-wide, sequence-specific tracking of replication origin and replication fork dynamics under different conditions, such as DNA damage and replication stress, and in mutant strains. We have recently developed a quantitative method for BrdU-IP-seq (qBrdU-seq) involving DNA barcoding to enable quantitative analysis of multiple experimental samples subjected to BrdU-IP-seq. After initial barcoding of multiple, individually BrdU-labeled genomic DNA samples, a pooling strategy is used for all subsequent steps including immunoprecipitation, amplification, and sequencing, which eliminates sample-to-sample variability in these steps. Parallel processing of an aliquot of the pooled input sample provides a direct control for the normalization of the data and yields results that allow quantitative comparisons of the experimental samples. Though developed for the analysis of S. cerevisiae, this method should be directly adaptable to other model systems.

Published

2018

38. The A-Like Faker Assay for Measuring Yeast Chromosome III Stability.

Author

Novoa CA, Ang JS, and Stirling PC

Subjects

Genome, Fungal, Genomic Instability, Saccharomyces cerevisiae genetics, Chromosomal Instability, Chromosomes, Fungal, Genetic Testing methods, Yeasts genetics

Abstract

The ability to rapidly assess chromosome instability (CIN) has enabled profiling of most yeast genes for potential effects on genome stability. The A-like faker (ALF) assay is one of several qualitative and quantitative marker loss assays that indirectly measure loss or conversion of genetic material using a counterselection step. The ALF assay relies on the ability to count spurious mating events that occur upon loss of the MATα locus of haploid Saccharomyces cerevisiae strains. Here, we describe the deployment of the ALF assay for both rapid and simple qualitative, and more in-depth quantitative analysis allowing determination of absolute ALF frequencies.

Published

2018

39. Quantitative Analysis of the Rates for Repeat-Mediated Genome Instability in a Yeast Experimental System.

Author

Radchenko EA, McGinty RJ, Aksenova AY, Neil AJ, and Mirkin SM

Subjects

Mutagenesis, Mutation Rate, Saccharomyces cerevisiae genetics, Trinucleotide Repeat Expansion, Trinucleotide Repeats, Genome, Fungal, Genomic Instability, Repetitive Sequences, Nucleic Acid, Yeasts genetics

Abstract

Instability of repetitive DNA sequences causes numerous hereditary disorders in humans, the majority of which are associated with trinucleotide repeat expansions. Here, we describe a unique system to study instability of triplet repeats in a yeast experimental setting. Using fluctuation assay and the novel program FluCalc we are able to accurately estimate the rates of large-scale expansions, as well as repeat-mediated mutagenesis and gross chromosomal rearrangements for different repeat sequences.

Published

2018

40. Transformation of an Exotic Yeast Species into a Platform Organism: A Case Study for Engineering Glycolipid Production in the Yeast Starmerella bombicola.

Author

Lodens S, De Graeve M, Roelants SLKW, De Maeseneire SL, and Soetaert W

Subjects

Genetic Engineering methods, Promoter Regions, Genetic genetics, Terminator Regions, Genetic genetics, Glycolipids genetics, Yeasts genetics

Abstract

In this chapter, a step-by-step approach on how to transform non-conventional yeasts or fungi into platform organisms is described. The non-conventional glycolipid producing yeast Starmerella bombicola (and in some cases also Pseudohyphozyma bogoriensis) is used as a case study. And more specifically how to engineer it toward production of new-to-nature glycolipids like bola sophorolipids. When starting genetic engineering efforts for non-lab strains, one should start at the very basis: identifying selection markers and possibly developing auxotrophic strains. Once this is done, the quest for the development of an optimal transformation method can be started. After optimization thereof, knock-out and knock-in strains can be generated based upon the specific strategy/aim. Sometimes this can lead to unexpected, but yet very interesting findings. To fully and efficiently expand the potential as a production platform of these yeast strains, a range of additional molecular tools are required. A well-equipped molecular toolbox should contain a set of characterized promotors, terminators, and defined genomic landing paths. The availability of an episomal system greatly facilitates engineering and screening efforts, but also offers the possibility of developing more advanced engineering techniques such as Crispr-Cas. InBio.be is a world leading pioneer to do this for the yeast S. bombicola and combined, these efforts will result in the commercialization of new types of glycolipids in the next few years.

Published

2018

41. Integrated Proteogenomic Approach for Identifying Degradation Motifs in Eukaryotic Cells.

Author

Geffen Y, Appleboim A, Gardner RG, and Ravid T

Subjects

Data Interpretation, Statistical, Fungal Proteins chemistry, Fungal Proteins metabolism, Gene Library, Genetic Vectors genetics, High-Throughput Nucleotide Sequencing, Proteasome Endopeptidase Complex metabolism, Protein Binding, Protein Conformation, Ubiquitin genetics, Ubiquitin metabolism, Yeasts genetics, Yeasts metabolism, Amino Acid Motifs, Eukaryotic Cells metabolism, Protein Interaction Domains and Motifs, Proteogenomics methods

Abstract

Since its discovery nearly 40 years ago, many components of the ubiquitin-proteasome system (UPS) have been identified and characterized in detail. However, a key aspect of the UPS that remains largely obscure is the signals that initiate the interaction of a substrate with enzymes of the UPS machinery. Understanding these signals is of particular interest for studies that examine the mechanism of substrate recognition for proteins that have adopted a non-native structure, as part of the cellular protein quality control (PQC) defense mechanism. Such studies are quite salient as the entire proteome makes up the potential battery of PQC substrates, and yet only a limited number of ubiquitination pathways are known to handle misfolded proteins. Our current research aims at understanding how a small number of PQC ubiquitin-protein ligases specifically recognize and ubiquitinate the overwhelming assortment of misfolded proteins. Here, we present a new proteogenomic approach for identifying and characterizing recognition motifs within degradation elements (degrons) in a high-throughput manner. The method utilizes yeast growth under restrictive conditions for selecting protein fragments that confer instability. The corresponding cDNA fragments are analyzed by next-generation sequencing (NGS) that provides information about each fragment's identity, reading frame, and abundance over time. This method was used by us to identify PQC-specific and compartment-specific degrons. It can readily be modified to study protein degradation signals and pathways in other organisms and in various settings, such as different strain backgrounds and under various cell conditions, all of which can be sequenced and analyzed simultaneously.

Published

2018

42. High-Resolution Mapping of Modified DNA Nucleobases Using Excision Repair Enzymes.

Author

Ransom M, Bryan DS, and Hesselberth JR

Subjects

DNA drug effects, DNA radiation effects, DNA Damage drug effects, DNA Damage radiation effects, Escherichia coli genetics, Sequence Analysis, DNA, Ultraviolet Rays, Uracil pharmacology, Yeasts genetics, DNA genetics, DNA metabolism, DNA Repair, High-Throughput Nucleotide Sequencing

Abstract

Modification of DNA nucleobases has a profound effect on genome function. We developed a method that maps the positions of the modified DNA nucleobases throughout genomic DNA. This method couples in vitro nucleobase excision with massively parallel DNA sequencing to determine the location of modified DNA nucleobases with single base precision. This protocol was used to map uracil incorporation and UV photodimers in DNA, and a modification of the protocol has been used to map sparse modification events in cells. The Excision-seq protocol is broadly applicable to a variety of base modifications for which an excision enzyme is available.

Published

2018

43. Integrated Microarray-based Tools for Detection of Genomic DNA Damage and Repair Mechanisms.

Author

van Eijk P, Teng Y, Bennet MR, Evans KE, Powell JR, Webster RM, and Reed SH

Subjects

Antineoplastic Agents pharmacology, Cell Line, Computational Biology methods, DNA, Fungal, Genomic Instability, Humans, Mutagens, Ultraviolet Rays, Yeasts drug effects, Yeasts genetics, Yeasts radiation effects, DNA Damage, DNA Repair, Genome, Genomics methods, Oligonucleotide Array Sequence Analysis methods

Abstract

The genetic information contained within the DNA molecule is highly susceptible to chemical and physical insult, caused by both endogenous and exogenous sources that can generate in the order of thousands of lesions a day in each of our cells (Lindahl, Nature 362(6422):709-715, 1993). DNA damages interfere with DNA metabolic processes such as transcription and replication and can be potent inhibitors of cell division and gene expression. To combat these regular threats to genome stability, a host of DNA repair mechanisms have evolved. When DNA lesions are left unrepaired due to defects in the repair pathway, mutations can arise that may alter the genetic information of the cell. DNA repair is thus fundamental to genome stability and defects in all the major repair pathways can lead to cancer predisposition. Therefore, the ability to accurately measure DNA damage at a genomic scale and determine the level, position, and rates of removal by DNA repair can contribute greatly to our understanding of how DNA repair in chromatin is organized throughout the genome. For this reason, we developed the 3D-DIP-Chip protocol described in this chapter. Conducting such measurements has potential applications in a variety of other fields, such as genotoxicity testing and cancer treatment using DNA damage inducing chemotherapy. Being able to detect and measure genomic DNA damage and repair patterns in individuals following treatment with chemotherapy could enable personalized medicine by predicting response to therapy.

Published

2018

44. Trapping Chromatin Interacting Proteins with Genetically Encoded, UV-Activatable Crosslinkers In Vivo.

Author

Hoffmann C, Neumann H, and Neumann-Staubitz P

Subjects

Amino Acids chemistry, Amino Acids genetics, Cell Cycle genetics, Histones metabolism, Mitosis genetics, Protein Binding, Yeasts genetics, Yeasts metabolism, Chromatin genetics, Chromatin metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Genetic Code, Ultraviolet Rays

Abstract

The installation of unnatural amino acids into proteins of living cells is an enabling technology that facilitates an enormous number of applications. UV-activatable crosslinker amino acids allow the formation of a covalent bond between interaction partners in living cells with nearly perfect spatial and temporal control. Here, we describe how this method can be employed to map chromatin interactions and to follow these interactions across the cell cycle in synchronized yeast populations. This method thereby provides unprecedented insights into the molecular events controlling chromatin reorganization in mitosis. As similar tools are available for other organisms, it should be possible to derive similar strategies for these and for other synchronizable processes.

Published

2018

45. The Chromosome Transmission Fidelity Assay for Measuring Chromosome Loss in Yeast.

Author

Duffy S and Hieter P

Subjects

Chromosomal Instability, Genetic Association Studies, Genomic Instability, Phenotype, Chromosome Deletion, Chromosomes, Fungal, Yeasts genetics

Abstract

The budding yeast Saccharomyces cerevisiae has served as an excellent model system for studying highly conserved biological pathways including pathways involved in genome transmission and maintenance. The Chromosome Transmission Fidelity (CTF) colony color assay was developed to assess chromosome instability (CIN) in yeast, by monitoring the loss or gain during cell division of an artificial chromosome fragment carrying a visual marker. The CTF assay monitors changes in chromosome number, allowing the detection of mutants that exhibit increased rates of chromosome nondisjunction or chromosome loss. In this article, we describe the SUP11-marker-based CTF assay system, and the methodologies for both qualitative analysis of mutants affecting chromosome transmission, and quantitative analysis for determining the types and rates of errors in chromosome transmission using half-sector analysis.

Published

2018

46. Assays to Study Repair of Inducible DNA Double-Strand Breaks at Telomeres.

Author

Oshidari R and Mekhail K

Subjects

DNA End-Joining Repair, DNA, Fungal, Homologous Recombination, Humans, Yeasts genetics, Yeasts metabolism, DNA Breaks, Double-Stranded, DNA Repair, Telomere genetics

Abstract

The ends of linear chromosomes are constituted of repetitive DNA sequences called telomeres. Telomeres, nearby regions called subtelomeres, and their associated factors prevent chromosome erosion over cycles of DNA replication and prevent chromosome ends from being recognized as DNA double-strand breaks (DSBs). This raises the question of how cells repair DSBs that actually occur near chromosome ends. One approach is to edit the genome and engineer cells harboring inducible DSB sites within the subtelomeric region of different chromosome ends. This provides a reductionist and tractable genetic model system in which mechanisms mediating repair can be dissected via genetics, molecular biology, and microscopy tools.

Published

2018

47. Genome-Wide Quantitative Fitness Analysis (QFA) of Yeast Cultures.

Author

Holstein EM, Lawless C, Banks P, and Lydall D

Subjects

Diploidy, Gene Deletion, Genomics methods, Meiosis genetics, Mutation, Spores, Fungal, Genetic Fitness, Genome, Fungal, Genome-Wide Association Study methods, Yeasts genetics

Abstract

We provide a detailed protocol for robot-assisted, genome-wide measurement of fitness in the model yeast Saccharomyces cerevisiae using Quantitative Fitness Analysis (QFA). We first describe how we construct thousands of double or triple mutant yeast strains in parallel using Synthetic Genetic Array (SGA) procedures. Strains are inoculated onto solid agar surfaces by liquid spotting followed by repeated photography of agar plates. Growth curves are constructed and the fitness of each strain is estimated. Robot-assisted QFA, can be used to identify genetic interactions and chemical sensitivity/resistance in genome-wide experiments, but QFA can also be used in smaller scale, manual workflows.

Published

2018

48. High-Throughput Analysis of Mammalian Receptor Tyrosine Kinase Activation in Yeast Cells.

Author

Yoshimoto N and Kuroda S

Subjects

Animals, Cell Line, Tumor, Cell Surface Display Techniques, DNA, Complementary genetics, Enzyme Activation, Epidermal Growth Factor genetics, Epidermal Growth Factor metabolism, ErbB Receptors metabolism, Gene Expression, Humans, Ligands, Peptide Library, Peptides genetics, Peptides isolation & purification, Peptides metabolism, Phosphorylation, Protein Interaction Mapping, Receptor Protein-Tyrosine Kinases agonists, Receptor Protein-Tyrosine Kinases genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Single-Cell Analysis, Yeasts genetics, High-Throughput Screening Assays methods, Receptor Protein-Tyrosine Kinases metabolism, Yeasts metabolism

Abstract

Tyrosine phosphorylation is an essential posttranslational modification in intracellular signaling molecules. Since tyrosine phosphorylation occurs in less than 0.1 % of all phosphorylated amino acids in mammalian cells, it is difficult to detect the nascent phosphotyrosine at a high signal-to-noise ratio due to high intracellular backgrounds (i.e., unexpected crosstalks among endogenous signaling molecules). In order to address this issue, we reconstituted the mammalian signaling pathway involving an extracellular ligand and a receptor tyrosine kinase (RTK) in Saccharomyces cerevisiae, a lower eukaryote that lacks endogenous tyrosine kinases. In this chapter, we describe a method for high-throughput analysis of ligand-receptor interaction by combining the yeast cell-surface display technique with an automated single-cell analysis and isolation system. Yeast cells coexpressing the cell-wall-anchored form of the human epidermal growth factor (EGF) and the human EGF receptor (EGFR) fused with a signal peptide at the N terminus facilitated the interaction of EGF with EGFR in an autocrine manner, followed by EGFR oligomerization and subsequent autophosphorylation. Furthermore, yeast cells expressing cell-wall-anchored forms of a conformationally constrained random peptide library instead of EGF are treated with a fluorophore-labeled anti-phosphorylated EGFR antibody and then subjected to the automated single-cell analysis and isolation system. The yeast cells with the highest level of fluorescence were shown to display novel and efficient EGFR agonistic peptides. Thus, our yeast display technique serves as a quantitative measurement for RTK activation, which is applicable to high-throughput de novo screening of RTK agonistic peptides.

Published

2017

49. Analysis of Ethylene Receptors: Ethylene-Binding Assays.

Author

Binder BM and Schaller GE

Subjects

Cell Membrane metabolism, Isotope Labeling, Ligands, Protein Binding, Yeasts genetics, Yeasts metabolism, Biological Assay methods, Ethylenes metabolism, Plant Proteins metabolism, Receptors, Cell Surface metabolism

Abstract

Plant ethylene receptors bind ethylene with high affinity. Most of the characterization of ethylene binding to the receptors has been carried out using a radioligand-binding assay on functional receptors expressed in yeast. In this chapter, we describe methods for expressing ethylene receptors in yeast and conducting ethylene-binding assays on intact yeast and yeast membranes. The ethylene-binding assays can be modified to analyze ethylene binding to intact plants and other organisms as well as membranes isolated from any biological source.

Published

2017

50. Localizing mRNAs Encoding Mitochondrial Proteins in Yeast by Fluorescence Microscopy and Subcellular Fractionation.

Author

Zabezhinsky D, Sperber H, and Gerst JE

Subjects

In Situ Hybridization, Fluorescence methods, Mitochondrial Proteins metabolism, Mutation, Protein Biosynthesis, Single Molecule Imaging methods, Cell Fractionation, Microscopy, Fluorescence, Mitochondrial Proteins genetics, RNA Transport, RNA, Messenger metabolism, Yeasts genetics, Yeasts metabolism

Abstract

Mitochondria are thought to have evolved from ancestral proteobacteria and, as a result of symbiosis, became an indispensable organelle in all eukaryotic cells. Mitochondria perform essential functions that provide the cell with ATP, amino acids, phospholipids, and both heme and iron-sulfur clusters. However, only 1% of mitochondrial proteins are encoded by the mitochondrial genome, while the remaining 99% are encoded in the nucleus. This raises a logistical challenge to the cell, as these nuclear-encoded proteins have to be translated, delivered to the mitochondrial surface, and translocated to its various compartments. Over the past decade, it was shown that subsets of mRNAs encoding mitochondrial proteins (mMPs) are localized to the mitochondrial surface in both yeast and mammalian cells. Moreover, factors (e.g., RNA-binding proteins) have been discovered that facilitate mMP targeting, and their loss leads to RNA mislocalization and defects in mitochondrial function (e.g., deficient respiration). Therefore, there is a demand in the field of mitochondrial biology to accurately measure mMP localization to the mitochondrial surface. In this chapter, we describe two techniques that allow for the visualization of mMPs using single-molecule fluorescent in situ hybridization and preparation of a highly enriched mitochondrial fraction followed by quantitative real-time PCR. Together, these techniques constitute powerful tools to link changes in mMP trafficking to defects in mitochondrial physiology.

Published

2017