Your search keyword '"Terminator"' showing total 433 results

1. High-Level Production of a Recombinant Protein in Nicotiana benthamiana Leaves Through Transient Expression Using a Double Terminator.

Author

Lee, Jihyea, Lee, Kyeong-Ryeol, Kim, Nan-Sun, Lee, Juho, Lee, Seon-Kyeong, and Lee, Sichul

Subjects

*RECOMBINANT proteins, *GENE expression, *FOLIAR diagnosis, *PLANT proteins, *PLANT yields, *NICOTIANA benthamiana

Abstract

Various bio-based recombinant proteins have been produced for industrial, medical, and research purposes. Plants are potential platforms for recombinant protein production because of several advantages. Therefore, establishing a system with high target gene expression to compensate for the low protein yield of plant systems is crucial. In particular, selecting and combining strong terminators is essential because the expression of target genes can be substantially enhanced. Here, we aimed to quantify the enhancement in the fluorescence intensity of the turbo green fluorescence protein (tGFP) caused by the best double-terminator combinations compared to that of the control vector using agroinfiltration in Nicotiana benthamiana leaves. tGFP fluorescence increased by 4.1-fold in leaf samples infiltrated with a vector containing a double terminator and markedly increased by a maximum of 23.7-fold when co-infiltrated with the geminiviral vector and P19 compared to that in constructs containing an octopine synthase terminator. Polyadenylation site analysis in leaf tissues expressing single or dual terminators showed that the first terminator influenced the polyadenylation site determination of the second terminator, resulting in different polyadenylation sites compared with when the terminator is located first. The combination of the high-expression terminators and geminiviral vectors can increase the production of target proteins. [ABSTRACT FROM AUTHOR]

Published

2024

2. Desirability of Using AWS

Author

Kwik, Jonathan and Kwik, Jonathan

Published

2024

3. Ghosting: Abandonment in the Digital Era.

Author

Daraj, Lateefa Rashed, Buhejji, Mariam Rashid, Perlmutter, Gretta, Jahrami, Haitham, and Seeman, Mary V.

Subjects

*DIGITAL technology, *NARCISSISM, *ONLINE dating, *ONLINE dating mobile apps, *MACHIAVELLIANISM (Psychology), *PSYCHOPATHY

Abstract

Definition: This entry synthesizes the multidisciplinary literature on ghosting published through late 2023 across psychological and social science journals. Search terms include "ghosting" and "online dating". Both quantitative and qualitative studies are included. The rise in ghosting can be attributed to advancements in technology and the increased popularity of dating apps. It is defined as an abrupt one-sided ending, without explanation, of an established friendship/romantic or other communication connection. The prevalence of ghosting has increased, as reported by both ghosters (i.e., persons who stopped responding) and ghostees (i.e., persons who were "dumped"). Individuals characterized by dark triad traits (i.e., psychopathy, Machiavellianism, and narcissism) are more likely than others to be ghosters. These individuals have a history of using ghosting as their preferred method of ending relationships without concern for its negative impact on ghostees or, indeed, on themselves. The psychological effects of ghosting can influence mental health, although most individuals ultimately find ways of coping. [ABSTRACT FROM AUTHOR]

Published

2024

4. Widespread stop-codon recoding in bacteriophages may regulate translation of lytic genes

Author

Borges, Adair L, Lou, Yue Clare, Sachdeva, Rohan, Al-Shayeb, Basem, Penev, Petar I, Jaffe, Alexander L, Lei, Shufei, Santini, Joanne M, and Banfield, Jillian F

Subjects

Genetics, Aetiology, 2.2 Factors relating to the physical environment, Infection, Animals, Bacteria, Bacteriophages, Biological Evolution, Codon, Terminator, Proteins, Microbiology, Medical Microbiology

Abstract

Bacteriophages (phages) are obligate parasites that use host bacterial translation machinery to produce viral proteins. However, some phages have alternative genetic codes with reassigned stop codons that are predicted to be incompatible with bacterial translation systems. We analysed 9,422 phage genomes and found that stop-codon recoding has evolved in diverse clades of phages that infect bacteria present in both human and animal gut microbiota. Recoded stop codons are particularly over-represented in phage structural and lysis genes. We propose that recoded stop codons might function to prevent premature production of late-stage proteins. Stop-codon recoding has evolved several times in closely related lineages, which suggests that adaptive recoding can occur over very short evolutionary timescales.

Published

2022

5. A FAIR-compliant parts catalogue for genome engineering and expression control in Saccharomyces cerevisiae

Author

D'Ambrosio, Vasil, Hansen, Lea G, Zhang, Jie, Jensen, Emil D, Arsovska, Dushica, Laloux, Marcos, Jakočiūnas, Tadas, Hjort, Pernille, De Lucrezia, Davide, Marletta, Serena, Keasling, Jay D, and Jensen, Michael K

Subjects

Human Genome, Bioengineering, Genetics, gRNA, Promoter, Terminator, Yeast, Standardization

Abstract

The synthetic biology toolkit for baker's yeast, Saccharomyces cerevisiae, includes extensive genome engineering toolkits and parts repositories. However, with the increasing complexity of engineering tasks and versatile applications of this model eukaryote, there is a continued interest to expand and diversify the rational engineering capabilities in this chassis by FAIR (findable, accessible, interoperable, and reproducible) compliance. In this study, we designed and characterised 41 synthetic guide RNA sequences to expand the CRISPR-based genome engineering capabilities for easy and efficient replacement of genomically encoded elements. Moreover, we characterize in high temporal resolution 20 native promoters and 18 terminators using fluorescein and LUDOX CL-X as references for GFP expression and OD600 measurements, respectively. Additionally, all data and reported analysis is provided in a publicly accessible jupyter notebook providing a tool for researchers with low-coding skills to further explore the generated data as well as a template for researchers to write their own scripts. We expect the data, parts, and databases associated with this study to support a FAIR-compliant resource for further advancing the engineering of yeasts.

Published

2022

6. Optimization of mammalian expression vector by cis-regulatory element combinations.

Author

Zhou, Lu-Yu, Zhang, Shuang, Li, Li-Yun, Yang, Guo-Yu, and Zeng, Lei

Subjects

*GENE expression, *SARS-CoV-2, *GENETIC regulation, *AVIAN influenza, *COVID-19 pandemic, *ANGIOTENSIN II

Abstract

The regulation of gene expression in mammalian cells by combining various cis-regulatory features has rarely been discussed. In this study, we constructed expression vectors containing various combinations of regulatory elements to examine the regulation of gene expression by different combinations of cis-regulatory elements. The effects of four promoters (CMV promoter, PGK promoter, Polr2a promoter, and EF-1α core promoter), two enhancers (CMV enhancer and SV40 enhancer), two introns (EF-1α intron A and hybrid intron), two terminators (CYC1 terminator and TEF terminator), and their different combinations on downstream gene expression were compared in various mammalian cells using fluorescence microscopy to observe fluorescence, quantitative real-time PCR (qRT-PCR), and western blot. The receptor binding domain (RBD) sequence from severe acute respiratory syndrome coronavirus-2 (SARS-CoV-2) spike protein was used to replace the eGFP sequence in the expression vector and the RBD expression was detected by qRT-PCR and western blot. The results showed that protein expression can be regulated by optimizing the combination of cis-acting elements. The vector with the CMV enhancer, EF-1α core promoter, and TEF terminator was found to express approximately threefold higher eGFP than the unmodified vector in different animal cells, as well as 2.63-fold higher recombinant RBD protein than the original vector in HEK-293T cells. Moreover, we suggest that combinations of multiple regulatory elements capable of regulating gene expression do not necessarily exhibit synergistic effects to enhance expression further. Overall, our findings provide insights into biological applications that require the regulation of gene expression and will help to optimize expression vectors for biosynthesis and other fields. Additionally, we provide valuable insights into the production of RBD proteins, which may aid in developing reagents for diagnosis and treatment during the COVID-19 pandemic. [ABSTRACT FROM AUTHOR]

Published

2023

7. Premature termination codon readthrough upregulates progranulin expression and improves lysosomal function in preclinical models of GRN deficiency

Author

Frew, Jonathan, Baradaran-Heravi, Alireza, Balgi, Aruna D, Wu, Xiujuan, Yan, Tyler D, Arns, Steve, Shidmoossavee, Fahimeh S, Tan, Jason, Jaquith, James B, Jansen-West, Karen R, Lynn, Francis C, Gao, Fen-Biao, Petrucelli, Leonard, Feldman, Howard H, Mackenzie, Ian R, Roberge, Michel, and Nygaard, Haakon B

Subjects

Brain Disorders, Alzheimer's Disease including Alzheimer's Disease Related Dementias (AD/ADRD), Stem Cell Research, Genetics, Stem Cell Research - Induced Pluripotent Stem Cell, Neurosciences, Frontotemporal Dementia (FTD), Stem Cell Research - Induced Pluripotent Stem Cell - Human, Acquired Cognitive Impairment, Neurodegenerative, Dementia, Alzheimer's Disease Related Dementias (ADRD), 2.1 Biological and endogenous factors, Aetiology, Neurological, Animals, Cells, Cultured, Codon, Nonsense, Codon, Terminator, Frontotemporal Lobar Degeneration, Gene Expression, Gentamicins, HEK293 Cells, Humans, Lysosomes, Mice, Neurons, Progranulins, Up-Regulation, Progranulin, GRN, Frontotemporal lobar degeneration, Nonsense mutation, Premature termination codon, Readthrough, G418, Induced pluripotent stem cell, Clinical Sciences, Neurology & Neurosurgery

Abstract

BackgroundFrontotemporal lobar degeneration (FTLD) is a devastating and progressive disorder, and a common cause of early onset dementia. Progranulin (PGRN) haploinsufficiency due to autosomal dominant mutations in the progranulin gene (GRN) is an important cause of FTLD (FTLD-GRN), and nearly a quarter of these genetic cases are due to a nonsense mutation. Premature termination codons (PTC) can be therapeutically targeted by compounds allowing readthrough, and aminoglycoside antibiotics are known to be potent PTC readthrough drugs. Restoring endogenous PGRN through PTC readthrough has not previously been explored as a therapeutic intervention in FTLD.MethodsWe studied whether the aminoglycoside G418 could increase PGRN expression in HEK293 and human induced pluripotent stem cell (hiPSC)-derived neurons bearing the heterozygous S116X, R418X, and R493X pathogenic GRN nonsense mutations. We further tested a novel substituted phthalimide PTC readthrough enhancer in combination with G418 in our cellular models. We next generated a homozygous R493X knock-in hiPSC isogenic line (R493X-/- KI), assessing whether combination treatment in hiPSC-derived neurons and astrocytes could increase PGRN and ameliorate lysosomal dysfunction relevant to FTLD-GRN. To provide in vivo proof-of-concept of our approach, we measured brain PGRN after intracerebroventricular administration of G418 in mice expressing the V5-tagged GRN nonsense mutation R493X.ResultsThe R418X and R493X mutant GRN cell lines responded to PTC readthrough with G418, and treatments increased PGRN levels in R493X-/- KI hiPSC-derived neurons and astrocytes. Combining G418 with a PTC readthrough enhancer increased PGRN levels over G418 treatment alone in vitro. PGRN deficiency has been shown to impair lysosomal function, and the mature form of the lysosomal protease cathepsin D is overexpressed in R493X-/- KI neurons. Increasing PGRN through G418-mediated PTC readthrough normalized this abnormal lysosomal phenotype in R493X-/- KI neuronal cultures. A single intracerebroventricular injection of G418 induced GRN PTC readthrough in 6-week-old AAV-GRN-R493X-V5 mice.ConclusionsTaken together, our findings suggest that PTC readthrough may be a potential therapeutic strategy for FTLD caused by GRN nonsense mutations.

Published

2020

8. Transcription termination and antitermination of bacterial CRISPR arrays.

Author

Stringer, Anne M, Baniulyte, Gabriele, Lasek-Nesselquist, Erica, Seed, Kimberley D, and Wade, Joseph T

Subjects

Bacteria, Bacterial Proteins, RNA, Bacterial, Codon, Terminator, Transcription Termination, Genetic, Clustered Regularly Interspaced Short Palindromic Repeats, Antitermination, CRISPR, Rho termination, genetics, genomics, infectious disease, microbiology, Genetics, Biochemistry and Cell Biology

Abstract

A hallmark of CRISPR-Cas immunity systems is the CRISPR array, a genomic locus consisting of short, repeated sequences ('repeats') interspersed with short, variable sequences ('spacers'). CRISPR arrays are transcribed and processed into individual CRISPR RNAs that each include a single spacer, and direct Cas proteins to complementary sequences in invading nucleic acid. Most bacterial CRISPR array transcripts are unusually long for untranslated RNA, suggesting the existence of mechanisms to prevent premature transcription termination by Rho, a conserved bacterial transcription termination factor that rapidly terminates untranslated RNA. We show that Rho can prematurely terminate transcription of bacterial CRISPR arrays, and we identify a widespread antitermination mechanism that antagonizes Rho to facilitate complete transcription of CRISPR arrays. Thus, our data highlight the importance of transcription termination and antitermination in the evolution of bacterial CRISPR-Cas systems.

Published

2020

9. Pathway-guided analysis identifies Myc-dependent alternative pre-mRNA splicing in aggressive prostate cancers

Author

Phillips, John W, Pan, Yang, Tsai, Brandon L, Xie, Zhijie, Demirdjian, Levon, Xiao, Wen, Yang, Harry T, Zhang, Yida, Lin, Chia Ho, Cheng, Donghui, Hu, Qiang, Liu, Song, Black, Douglas L, Witte, Owen N, and Xing, Yi

Subjects

Genetics, Aging, Urologic Diseases, Human Genome, Prostate Cancer, Cancer, Adenocarcinoma, Breast Neoplasms, Cell Line, Tumor, Codon, Terminator, Computer Simulation, Datasets as Topic, Drug Resistance, Neoplasm, Exons, Female, Frameshift Mutation, Humans, Lung Neoplasms, Male, Prostatic Neoplasms, Proto-Oncogene Proteins c-myc, RNA Precursors, RNA Splicing, RNA-Seq, Signal Transduction, Software, alternative splicing, prostate cancer, Myc, rMATS, PEGASAS

Abstract

We sought to define the landscape of alternative pre-mRNA splicing in prostate cancers and the relationship of exon choice to known cancer driver alterations. To do so, we compiled a metadataset composed of 876 RNA-sequencing (RNA-Seq) samples from five publicly available sources representing a range of prostate phenotypes from normal tissue to drug-resistant metastases. We subjected these samples to exon-level analysis with rMATS-turbo, purpose-built software designed for large-scale analyses of splicing, and identified 13,149 high-confidence cassette exon events with variable incorporation across samples. We then developed a computational framework, pathway enrichment-guided activity study of alternative splicing (PEGASAS), to correlate transcriptional signatures of 50 different cancer driver pathways with these alternative splicing events. We discovered that Myc signaling was correlated with incorporation of a set of 1,039 cassette exons enriched in genes encoding RNA binding proteins. Using a human prostate epithelial transformation assay, we confirmed the Myc regulation of 147 of these exons, many of which introduced frameshifts or encoded premature stop codons. Our results connect changes in alternative pre-mRNA splicing to oncogenic alterations common in prostate and many other cancers. We also establish a role for Myc in regulating RNA splicing by controlling the incorporation of nonsense-mediated decay-determinant exons in genes encoding RNA binding proteins.

Published

2020

10. Prediction of Premature Termination Codon Suppressing Compounds for Treatment of Duchenne Muscular Dystrophy Using Machine Learning

Author

Wang, Kate, Romm, Eden L, Kouznetsova, Valentina L, and Tsigelny, Igor F

Subjects

Medicinal and Biomolecular Chemistry, Organic Chemistry, Chemical Sciences, Rare Diseases, Pediatric, Intellectual and Developmental Disabilities (IDD), Brain Disorders, Genetics, Muscular Dystrophy, Duchenne/ Becker Muscular Dystrophy, Neurosciences, Codon, Terminator, Databases, Chemical, Dystrophin, Humans, Machine Learning, Muscular Dystrophy, Duchenne, Duchenne muscular dystrophy, stop codon, machine learning, deep learning, pharmacophore, PTC-suppressing compounds, Theoretical and Computational Chemistry, Medicinal and biomolecular chemistry, Organic chemistry

Abstract

A significant percentage of Duchenne muscular dystrophy (DMD) cases are caused by premature termination codon (PTC) mutations in the dystrophin gene, leading to the production of a truncated, non-functional dystrophin polypeptide. PTC-suppressing compounds (PTCSC) have been developed in order to restore protein translation by allowing the incorporation of an amino acid in place of a stop codon. However, limitations exist in terms of efficacy and toxicity. To identify new compounds that have PTC-suppressing ability, we selected and clustered existing PTCSC, allowing for the construction of a common pharmacophore model. Machine learning (ML) and deep learning (DL) models were developed for prediction of new PTCSC based on known compounds. We conducted a search of the NCI compounds database using the pharmacophore-based model and a search of the DrugBank database using pharmacophore-based, ML and DL models. Sixteen drug compounds were selected as a consensus of pharmacophore-based, ML, and DL searches. Our results suggest notable correspondence of the pharmacophore-based, ML, and DL models in prediction of new PTC-suppressing compounds.

Published

2020

11. Promoter and Terminator Optimization for DNA Methylation Targeting in Arabidopsis

Author

Gardiner, Jason, Zhao, Jenny M, Chaffin, Kendall, and Jacobsen, Steven E

Subjects

Biological Sciences, Genetics, Biotechnology, Human Genome, epigenetics, DNA methylation, targeting, zinc finger, Arabidopsis, plant, transcription, promoter, terminator, RNA-directed DNA methylation, silencing

Abstract

DNA methylation is an important epigenetic mark involved in gene regulation and silencing of transposable elements. The presence or absence of DNA methylation at specific sites can influence nearby gene expression and cause phenotypic changes that remain stable over generations. Recently, development of new technologies has enabled the targeted addition or removal of DNA methylation at specific sites of the genome. Of these new technologies, the targeting of the catalytic domain of Nicotiana tabacum DOMAINS REARRANGED METHYLTRANSFERASE 2 (ntDRM2cd) offers a promising tool for the addition of DNA methylation as it can directly methylate DNA. However, the methylation targeting efficiency of constructs using ntDRM2cd thus far has been relatively low. Previous studies have shown that the use of different promoters or terminators can greatly improve genome-editing efficiencies. In this study, we systematically survey a variety of promoter and terminator combinations to identify optimal combinations to use when targeting the addition of DNA methylation in Arabidopsis thaliana.

Published

2020

12. Management of Disturbance Behavior

Author

Zacher, Serge and Zacher, Serge

Published

2022

13. Development of Terminator–Promoter Bifunctional Elements for Application in Saccharomyces cerevisiae Pathway Engineering.

Author

Ni, Xiaoxia, Liu, Zhengyang, Guo, Jintang, and Zhang, Genlin

Subjects

*SACCHAROMYCES cerevisiae, *LYCOPENE, *ENGINEERING, *SYNTHETIC biology, *GENETIC transcription regulation, *YEAST

Abstract

The construction of a genetic circuit requires the substitution and redesign of different promoters and terminators. The assembly efficiency of exogenous pathways will also decrease significantly when the number of regulatory elements and genes is increased. We speculated that a novel bifunctional element with promoter and terminator functions could be created via the fusion of a termination signal with a promoter sequence. In this study, the elements from a Saccharomyces cerevisiae promoter and terminator were employed to design a synthetic bifunctional element. The promoter strength of the synthetic element is apparently regulated through a spacer sequence and an upstream activating sequence (UAS) with a ~5-fold increase, and the terminator strength could be finely regulated by the efficiency element, with a ~5-fold increase. Furthermore, the use of a TATA box-like sequence resulted in the adequate execution of both functions of the TATA box and the efficiency element. By regulating the TATA box-like sequence, UAS, and spacer sequence, the strengths of the promoter-like and terminator-like bifunctional elements were optimally fine-tuned with ~8-fold and ~7-fold increases, respectively. The application of bifunctional elements in the lycopene biosynthetic pathway showed an improved pathway assembly efficiency and higher lycopene yield. The designed bifunctional elements effectively simplified pathway construction and can serve as a useful toolbox for yeast synthetic biology. [ABSTRACT FROM AUTHOR]

Published

2023

14. Plant terminators: the unsung heroes of gene expression.

Author

Felippes, Felipe F de and Waterhouse, Peter M

Subjects

*GENE expression, *GENETIC regulation, *NON-coding RNA, *PLANT genes

Abstract

To be properly expressed, genes need to be accompanied by a terminator, a region downstream of the coding sequence that contains the information necessary for the maturation of the mRNA 3ʹ end. The main event in this process is the addition of a poly(A) tail at the 3ʹ end of the new transcript, a critical step in mRNA biology that has important consequences for the expression of genes. Here, we review the mechanism leading to cleavage and polyadenylation of newly transcribed mRNAs and how this process can affect the final levels of gene expression. We give special attention to an aspect often overlooked, the effect that different terminators can have on the expression of genes. We also discuss some exciting findings connecting the choice of terminator to the biogenesis of small RNAs, which are a central part of one of the most important mechanisms of regulation of gene expression in plants. [ABSTRACT FROM AUTHOR]

Published

2023

15. Mutation update for the SATB2 gene.

Author

Zarate, Yuri, Bosanko, Katherine, Caffrey, Aisling, Bernstein, Jonathan, Martin, Donna, Williams, Marc, Berry-Kravis, Elizabeth, Mark, Paul, Manning, Melanie, Bhambhani, Vikas, Vargas, Marcelo, Seeley, Andrea, Estrada-Veras, Juvianee, van Dooren, Marieke, Schwab, Maria, Vanderver, Adeline, Melis, Daniela, Alsadah, Adnan, Sadler, Laurie, Van Esch, Hilde, Callewaert, Bert, Oostra, Ann, Maclean, Jane, Dentici, Maria, Orlando, Valeria, Lipson, Mark, Sparagana, Steven, Maarup, Timothy, Alsters, Suzanne, Brautbar, Ariel, Kovitch, Eliana, Naidu, Sakkubai, Lees, Melissa, Smith, Douglas, Turner, Lesley, Raggio, Víctor, Spangenberg, Lucía, Garcia-Miñaúr, Sixto, Roeder, Elizabeth, Littlejohn, Rebecca, Grange, Dorothy, Pfotenhauer, Jean, Jones, Marilyn, Balasubramanian, Meena, Martinez-Monseny, Antonio, Blok, Lot, Gavrilova, Ralitza, and Fish, Jennifer

Subjects

SATB2, SATB2-associated syndrome, genotype-phenotype correlation, pathogenic variants, whole exome sequencing, Adolescent, Animals, Child, Child, Preschool, Codon, Terminator, Disease Models, Animal, Female, Gene Rearrangement, Genetic Association Studies, Humans, Male, Matrix Attachment Region Binding Proteins, Mutation, Mutation, Missense, Neurodevelopmental Disorders, Polymorphism, Single Nucleotide, Transcription Factors

Abstract

SATB2-associated syndrome (SAS) is an autosomal dominant neurodevelopmental disorder caused by alterations in the SATB2 gene. Here we present a review of published pathogenic variants in the SATB2 gene to date and report 38 novel alterations found in 57 additional previously unreported individuals. Overall, we present a compilation of 120 unique variants identified in 155 unrelated families ranging from single nucleotide coding variants to genomic rearrangements distributed throughout the entire coding region of SATB2. Single nucleotide variants predicted to result in the occurrence of a premature stop codon were the most commonly seen (51/120 = 42.5%) followed by missense variants (31/120 = 25.8%). We review the rather limited functional characterization of pathogenic variants and discuss current understanding of the consequences of the different molecular alterations. We present an expansive phenotypic review along with novel genotype-phenotype correlations. Lastly, we discuss current knowledge of animal models and present future prospects. This review should help provide better guidance for the care of individuals diagnosed with SAS.

Published

2019

16. Feedback to the central dogma: cytoplasmic mRNA decay and transcription are interdependent processes

Author

Hartenian, Ella and Glaunsinger, Britt A

Subjects

Genetics, 1.1 Normal biological development and functioning, Underpinning research, Generic health relevance, Animals, Cell Nucleus, Codon, Terminator, Cytoplasm, Exoribonucleases, Gene Expression, Homeostasis, Humans, Infections, Microtubule-Associated Proteins, RNA Polymerase II, RNA Stability, RNA, Messenger, RNA-Binding Proteins, Transcription, Genetic, mRNA decay, transcription, Xrn1, host shutoff, genetic buffering, NITC, Biochemistry and Cell Biology, Biochemistry & Molecular Biology

Abstract

Transcription and RNA decay are key determinants of gene expression; these processes are typically considered as the uncoupled beginning and end of the messenger RNA (mRNA) lifecycle. Here we describe the growing number of studies demonstrating interplay between these spatially disparate processes in eukaryotes. Specifically, cells can maintain mRNA levels by buffering against changes in mRNA stability or transcription, and can also respond to virally induced accelerated decay by reducing RNA polymerase II gene expression. In addition to these global responses, there is also evidence that mRNAs containing a premature stop codon can cause transcriptional upregulation of homologous genes in a targeted fashion. In each of these systems, RNA binding proteins (RBPs), particularly those involved in mRNA degradation, are critical for cytoplasmic to nuclear communication. Although their specific mechanistic contributions are yet to be fully elucidated, differential trafficking of RBPs between subcellular compartments are likely to play a central role in regulating this gene expression feedback pathway.

Published

2019

17. Expression of a novel versican variant in dorsal root ganglia from spared nerve injury rats

Author

Bogen, Oliver, Bender, Olaf, Alvarez, Pedro, Kern, Marie, Tomiuk, Stefan, Hucho, Ferdinand, and Levine, Jon D

Subjects

Peripheral Neuropathy, Genetics, Neurodegenerative, Neurosciences, Animals, Codon, Terminator, Exons, Ganglia, Spinal, Male, Neuralgia, RNA Stability, RNA, Messenger, Rats, Rats, Sprague-Dawley, Versicans, Versican, nerve injury, neuropathic pain, nonsense mediated RNA decay, eIF2 alpha(PO4)(2-), Isolectin B4, eIF2α(PO), Biochemistry and Cell Biology, Neurology & Neurosurgery

Abstract

The size and modular structure of versican and its gene suggest the existence of multiple splice variants. We have identified, cloned, and sequenced a previously unknown exon located within the noncoding gene sequence downstream of exon 8. This exon, which we have named exon 8β, specifies two stop-codons. mRNAs of the versican gene with exon 8β are predicted to be constitutively degraded by nonsense-mediated RNA decay. Here, we tested the hypothesis that these transcripts become expressed in a model of neuropathic pain.

Published

2019

18. Drone fiction, empathy gap and the reader: Mohsin Hamid's short story Terminator: Attack of the Drone (2011).

Author

Liaqat, Qurratulaen

Subjects

*DRONE aircraft, *EMPATHY, *DRONE warfare, *THEORY of knowledge

Abstract

This article contends that the analysis of drone fiction from the perspective of Reader-Response Theory yields valuable insights into the configuration of this newly emerging genre and constitutes a neo Reader-Response theoretical paradigm. Drawing on insights from Reader-Response Theory and drone fiction critical approaches, this study delineates how Mohsin Hamid's short story Terminator: Attack of the Drone (2011) prompts readers to affectively engage in the process of reconstructing this text and empathise with the drone victims. By conducting a textual analysis of the narrative strategies and literary devices, this article demonstrates that how this narrative simultaneously exploits the notion of 'empathy gap', inherent in the drone fiction theory, and the propositions of Reader-Response theory related to 'gaps' to unpack the ongoing dehumanisation of certain races and communities in contemporary milieu. I contend that this short text evokes empathy of readers and encourages them to reconfigure the humanity of the drone victims. Hence, Hamid's drone fiction acts as an aesthetic conduit which invokes readers to become active participants in the process of deciphering the social, racial, political and humanitarian repercussions of unprecedented drone warfare and to recognise the socio-political epistemology of 'being human' under drone warfare. [ABSTRACT FROM AUTHOR]

Published

2023

19. A single mutation attenuates both the transcription termination and RNA-dependent RNA polymerase activity of T7 RNA polymerase.

Author

Wu, Hui, Wei, Ting, Yu, Bingbing, Cheng, Rui, Huang, Fengtao, Lu, Xuelin, Yan, Yan, Wang, Xionglue, Liu, Chenli, and Zhu, Bin

Subjects

RNA replicase, RNA polymerases, RNA synthesis, RNA analysis, CATALYTIC RNA, BINDING site assay

Abstract

Transcription termination is one of the least understood processes of gene expression. As the prototype model for transcription studies, the single-subunit T7 RNA polymerase (RNAP) is known to respond to two types of termination signals, but the mechanism underlying such termination, especially the specific elements of the polymerase involved, is still unclear, due to a lack of knowledge with respect to the structure of the termination complex. Here we applied phage-assisted continuous evolution to obtain variants of T7 RNAP that can bypass the typical class I T7 terminator with stem-loop structure. Through in vivo selection and in vitro characterization, we discovered a single mutation (S43Y) that significantly decreased the termination efficiency of T7 RNAP at all transcription terminators tested. Coincidently, the S43Y mutation almost eliminates the RNA-dependent RNAP (RdRp) activity of T7 RNAP without impeding the major DNA-dependent RNAP (DdRp) activity of the enzyme. S43 is located in a hinge region and regulates the transformation between transcription initiation and elongation of T7 RNAP. Steady-state kinetics analysis and an RNA binding assay indicate that the S43Y mutation increases the transcription efficiency while weakening RNA binding of the enzyme. As an enzymatic reagent for in vitro transcription, the T7 RNAP S43Y mutant reduces the undesired termination in run-off RNA synthesis and produces RNA with higher terminal homogeneity. [ABSTRACT FROM AUTHOR]

Published

2023

20. Dusty Plasmas in the Vicinity of the Moon: Current Research and New Vistas.

Author

Popel, S. I., Zakharov, A. V., and Zelenyi, L. M.

Subjects

*LUNAR surface, *MOON, *DUSTY plasmas, *PLASMA astrophysics, *MAGNETIC fields

Abstract

A brief review of recent studies on dusty plasma above the lunar surface at the Space Research Institute, Russian Academy of Sciences is presented. The research is related to the future Luna-25 and Luna-27 missions, which will study the properties of dust and dusty plasma above the lunar surface. The problems of formation of dusty plasma over the illuminated part of the Moon, in the region of the lunar terminator, the influence of magnetic fields on the circumlunar dusty plasma, and the influence on the results of measurements of the spacecraft landing module are considered. Unsolved problems concerning the study of the near-lunar dusty plasma are formulated. [ABSTRACT FROM AUTHOR]

Published

2023

21. DOKSZTAŁCANIE TERMINATORÓW W II RP NA PRZYKŁADZIE ZAWODOWEJ SZKOŁY DOKSZTAŁCAJĄCEJ W DĄBIU.

Author

RADZISZEWSKA, MARIA

Abstract

Copyright of Polonia Maior Orientalis is the property of Jagiellonian University Press and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2023

22. A FAIR-compliant parts catalogue for genome engineering and expression control in Saccharomyces cerevisiae

Author

Vasil D'Ambrosio, Lea G. Hansen, Jie Zhang, Emil D. Jensen, Dushica Arsovska, Marcos Laloux, Tadas Jakočiūnas, Pernille Hjort, Davide De Lucrezia, Serena Marletta, Jay D. Keasling, and Michael K. Jensen

Subjects

gRNA, Promoter, Terminator, Yeast, Standardization, Biotechnology, TP248.13-248.65, Biology (General), QH301-705.5

Abstract

The synthetic biology toolkit for baker's yeast, Saccharomyces cerevisiae, includes extensive genome engineering toolkits and parts repositories. However, with the increasing complexity of engineering tasks and versatile applications of this model eukaryote, there is a continued interest to expand and diversify the rational engineering capabilities in this chassis by FAIR (findable, accessible, interoperable, and reproducible) compliance. In this study, we designed and characterised 41 synthetic guide RNA sequences to expand the CRISPR-based genome engineering capabilities for easy and efficient replacement of genomically encoded elements. Moreover, we characterize in high temporal resolution 20 native promoters and 18 terminators using fluorescein and LUDOX CL-X as references for GFP expression and OD600 measurements, respectively. Additionally, all data and reported analysis is provided in a publicly accessible jupyter notebook providing a tool for researchers with low-coding skills to further explore the generated data as well as a template for researchers to write their own scripts. We expect the data, parts, and databases associated with this study to support a FAIR-compliant resource for further advancing the engineering of yeasts.

Published

2022

23. Terminator und Avatar

Author

Ulrich Kumher

Subjects

Science-Fiction, Film, James Cameron, Filmdidaktik, Filmanalyse, Terminator, Communication. Mass media, P87-96

Abstract

In diesem Beitrag werden zwei Figuren erhellt, die im Œuvre von James Cameron wichtige Rollen spielen: Terminator und Avatar. Nach einem Einblick in Camerons Werk, der mögliche Gründe für dessen Erfolg beleuchtet (1.), wird der Blick auf ein Strukturmerkmal seiner Filmgeschichten gelenkt, nämlich auf unterschiedliche Sphären, die in den jeweiligen Filmgeschichten vorkommen (2.). Diese Sphären spielen auch im Film Abyss eine wichtige Rolle, durch den sich bereits das jüngste Werk Camerons ankündigt (3.). Vor diesem Hintergrund wird auf zwei Figuren eingegangen, die Camerons Spielfilme stark prägen: Terminator (4.) und Avatar (5.). Was Terminator und Avatar als Allegorien undDenkfiguren bedeuten könnten, ist Thema des sechsten Abschnitts (6.). Der Artikel endet mit medienpädagogischen Anmerkungen (7.).

Published

2023

24. Nutrient depletion and TOR inhibition induce 18S and 25S ribosomal RNAs resistant to a 5′-phosphate-dependent exonuclease in Candida albicans and other yeasts

Author

Fleischmann, Jacob and Rocha, Miguel A

Subjects

Microbiology, Biological Sciences, Genetics, Alkaline Phosphatase, Candida albicans, Phosphodiesterase I, Protein Kinase Inhibitors, Pyrophosphatases, RNA, Fungal, RNA, Ribosomal, RNA, Ribosomal, 18S, Sirolimus, Stress, Physiological, TOR Serine-Threonine Kinases, RNA, Ribosomal, Terminator, Exonuclease, Biochemistry and Cell Biology, Medical Biochemistry and Metabolomics, Opthalmology and Optometry, Developmental Biology, Biochemistry and cell biology

Abstract

BackgroundMessenger RNA (mRNA) represents a small percentage of RNAs in a cell, with ribosomal RNA (rRNA) making up the bulk of it. To isolate mRNA from eukaryotes, typically poly-A selection is carried out. Recently, a 5´-phosphate-dependent, 5´→3´ processive exonuclease called Terminator has become available. It will digest only RNA that has a 5´-monophosphate end and therefore it is very useful to eliminate most of rRNAs in cell.ResultsWe have found that in the pathogenic yeast Candida albicans, while 18S and 25S components isolated from yeast in robust growth phase are easily eliminated by Terminator, those isolated from cells in the nutritionally diminished stationary phase, become resistant to digestion by this enzyme. Additional digestions with alkaline phosphatase, tobacco pyrophosphatase combined with Terminator point toward the 5'-prime end of 18S and 25S as the source of this resistance. Inhibition of TOR by rapamycin also induces resistance by these molecules. We also find that these molecules are incorporated into the ribosome and are not just produced incidentally. Finally, we show that three other yeasts show the same behavior.ConclusionsDigestion of RNA by Terminator has revealed 18S and 25S rRNA molecules different from the accepted processed ones seen in ribosome generation. The reason for these molecules and the underlying mechanism for their formation is unknown. The preservation of this behavior across these yeasts suggests a useful biological role for it, worthy of further inquiry.

Published

2018

25. Site-Specific Incorporation of Selenocysteine Using an Expanded Genetic Code and Palladium-Mediated Chemical Deprotection

Author

Liu, Jun, Zheng, Feng, Cheng, Rujin, Li, Shanshan, Rozovsky, Sharon, Wang, Qian, and Wang, Lei

Subjects

Codon, Terminator, Escherichia coli, Escherichia coli Proteins, Genetic Code, Glutathione Peroxidase, HeLa Cells, Humans, Models, Molecular, Palladium, Protein Biosynthesis, Protein Engineering, Selenocysteine, Selenoproteins, Thioredoxins, Glutathione Peroxidase GPX1, Hela Cells, Chemical Sciences, General Chemistry

Abstract

Selenoproteins containing the 21st amino acid selenocysteine (Sec) exist in all three kingdoms of life and play essential roles in human health and development. The distinct low p Ka, high reactivity, and redox property of Sec also afford unique routes to protein modification and engineering. However, natural Sec incorporation requires idiosyncratic translational machineries that are dedicated to Sec and species-dependent, which makes it challenging to recombinantly prepare selenoproteins with high Sec specificity. As a consequence, the function of half of human selenoproteins remains unclear, and Sec-based protein manipulation has been greatly hampered. Here we report a new general method enabling the site-specific incorporation of Sec into proteins in E. coli. An orthogonal tRNAPyl-ASecRS was evolved to specifically incorporate Se-allyl selenocysteine (ASec) in response to the amber codon, and the incorporated ASec was converted to Sec in high efficiency through palladium-mediated cleavage under mild conditions compatible with proteins and cells. This approach completely obviates the natural Sec-dedicated factors, thus allowing various selenoproteins, regardless of Sec position and species source, to be prepared with high Sec specificity and enzyme activity, as shown by the preparation of human thioredoxin and glutathione peroxidase 1. Sec-selective labeling in the presence of Cys was also demonstrated on the surface of live E. coli cells. The tRNAPyl-ASecRS pair was further used in mammalian cells to incorporate ASec, which was converted into Sec by palladium catalyst in cellulo. This robust and versatile method should greatly facilitate the study of diverse natural selenoproteins and the engineering of proteins in general via site-specific introduction of Sec.

Published

2018

26. Atomic mutagenesis of stop codon nucleotides reveals the chemical prerequisites for release factor-mediated peptide release

Author

Hoernes, Thomas Philipp, Clementi, Nina, Juen, Michael Andreas, Shi, Xinying, Faserl, Klaus, Willi, Jessica, Gasser, Catherina, Kreutz, Christoph, Joseph, Simpson, Lindner, Herbert, Hüttenhofer, Alexander, and Erlacher, Matthias David

Subjects

Genetics, Codon, Terminator, Escherichia coli, Escherichia coli Proteins, Mutagenesis, Site-Directed, Nucleotides, Peptide Chain Termination, Translational, Peptide Termination Factors, Protein Biosynthesis, ribosome, translation, peptide release, release factor, mRNA modification

Abstract

Termination of protein synthesis is triggered by the recognition of a stop codon at the ribosomal A site and is mediated by class I release factors (RFs). Whereas in bacteria, RF1 and RF2 promote termination at UAA/UAG and UAA/UGA stop codons, respectively, eukaryotes only depend on one RF (eRF1) to initiate peptide release at all three stop codons. Based on several structural as well as biochemical studies, interactions between mRNA, tRNA, and rRNA have been proposed to be required for stop codon recognition. In this study, the influence of these interactions was investigated by using chemically modified stop codons. Single functional groups within stop codon nucleotides were substituted to weaken or completely eliminate specific interactions between the respective mRNA and RFs. Our findings provide detailed insight into the recognition mode of bacterial and eukaryotic RFs, thereby revealing the chemical groups of nucleotides that define the identity of stop codons and provide the means to discriminate against noncognate stop codons or UGG sense codons.

Published

2018

27. Conceptions of Property and the Biotechnology Debate

Author

Thompson, Paul B., Korthals, Michiel, Series Editor, and Thompson, Paul B., Series Editor

Published

2020

28. Complex Transcriptional Profiles of the PPP1R12A Gene in Cells of the Circulatory System as Revealed by In Silico Analysis and Reverse Transcription PCR.

Author

Saldanha, Paulo André, Bolanle, Israel Olapeju, Palmer, Timothy Martin, Nikitenko, Leonid Leonidovich, and Rivero, Francisco

Subjects

*CARDIOVASCULAR system, *ALTERNATIVE RNA splicing, *SAPHENOUS vein, *MUSCLE cells, *UMBILICAL veins, *BLOOD platelet aggregation, *RNA splicing

Abstract

The myosin light chain phosphatase target subunit 1 (MYPT1), encoded by the PPP1R12A gene, is a key component of the myosin light chain phosphatase (MLCP) protein complex. MYPT1 isoforms have been described as products of the cassette-type alternative splicing of exons E13, E14, E22, and E24. Through in silico analysis of the publicly available EST and mRNA databases, we established that PPP1R12A contains 32 exons (6 more than the 26 previously reported), of which 29 are used in 11 protein-coding transcripts. An in silico analysis of publicly available RNAseq data combined with validation by reverse transcription (RT)-PCR allowed us to determine the relative abundance of each transcript in three cell types of the circulatory system where MYPT1 plays important roles: human umbilical vein endothelial cells (HUVEC), human saphenous vein smooth muscle cells (HSVSMC), and platelets. All three cell types express up to 10 transcripts at variable frequencies. HUVECs and HSVSMCs predominantly express the full-length variant (58.3% and 64.3%, respectively) followed by the variant skipping E13 (33.7% and 23.1%, respectively), whereas in platelets the predominant variants are those skipping E14 (51.4%) and E13 (19.9%), followed by the full-length variant (14.4%). Variants including E24 account for 5.4% of transcripts in platelets but are rare (<1%) in HUVECs and HSVSMCs. Complex transcriptional profiles were also found across organs using in silico analysis of RNAseq data from the GTEx project. Our findings provide a platform for future studies investigating the specific (patho)physiological roles of understudied MYPT1 isoforms. [ABSTRACT FROM AUTHOR]

Published

2022

29. Identification of a Transferrable Terminator Element That Inhibits Small RNA Production and Improves Transgene Expression Levels.

Author

de Felippes, Felipe Fenselau, Shand, Kylie, and Waterhouse, Peter M.

Subjects

NON-coding RNA, GENE expression, TRANSGENE expression

Abstract

The role of terminators is more commonly associated with the polyadenylation and 3′ end formation of new transcripts. Recent evidence, however, suggests that this regulatory region can have a dramatic impact on gene expression. Nonetheless, little is known about the molecular mechanisms leading to the improvements associated with terminator usage in plants and the different elements in a plant terminator. Here, we identified an element in the Arabidopsis HSP18.2 terminator (tHSP) to be essential for the high level of expression seen for transgenes under the regulation of this terminator. Our molecular analyses suggest that this newly identified sequence acts to improve transcription termination, leading to fewer read-through events and decreased amounts of small RNAs originating from the transgene. Besides protecting against silencing, the tHSP-derived sequence positively impacts splicing efficiency, helping to promote gene expression. Moreover, we show that this sequence can be used to generate chimeric terminators with enhanced efficiency, resulting in stronger transgene expression and significantly expanding the availability of efficient terminators that can be part of good expression systems. Thus, our data make an important contribution toward a better understanding of plant terminators, with the identification of a new element that has a direct impact on gene expression, and at the same time, creates new possibilities to modulate gene expression via the manipulation of 3′ regulatory regions. [ABSTRACT FROM AUTHOR]

Published

2022

30. Identification of a Transferrable Terminator Element That Inhibits Small RNA Production and Improves Transgene Expression Levels

Author

Felipe Fenselau de Felippes, Kylie Shand, and Peter M. Waterhouse

Subjects

PTGS, small RNAs, silencing, transcription termination, terminator, HSP terminator, Plant culture, SB1-1110

Abstract

The role of terminators is more commonly associated with the polyadenylation and 3′ end formation of new transcripts. Recent evidence, however, suggests that this regulatory region can have a dramatic impact on gene expression. Nonetheless, little is known about the molecular mechanisms leading to the improvements associated with terminator usage in plants and the different elements in a plant terminator. Here, we identified an element in the Arabidopsis HSP18.2 terminator (tHSP) to be essential for the high level of expression seen for transgenes under the regulation of this terminator. Our molecular analyses suggest that this newly identified sequence acts to improve transcription termination, leading to fewer read-through events and decreased amounts of small RNAs originating from the transgene. Besides protecting against silencing, the tHSP-derived sequence positively impacts splicing efficiency, helping to promote gene expression. Moreover, we show that this sequence can be used to generate chimeric terminators with enhanced efficiency, resulting in stronger transgene expression and significantly expanding the availability of efficient terminators that can be part of good expression systems. Thus, our data make an important contribution toward a better understanding of plant terminators, with the identification of a new element that has a direct impact on gene expression, and at the same time, creates new possibilities to modulate gene expression via the manipulation of 3′ regulatory regions.

Published

2022

31. Prevalent, Dynamic, and Conserved R-Loop Structures Associate with Specific Epigenomic Signatures in Mammals

Author

Sanz, Lionel A, Hartono, Stella R, Lim, Yoong Wearn, Steyaert, Sandra, Rajpurkar, Aparna, Ginno, Paul A, Xu, Xiaoqin, and Chédin, Frédéric

Subjects

Biochemistry and Cell Biology, Bioinformatics and Computational Biology, Biological Sciences, Human Genome, Genetics, Underpinning research, 1.1 Normal biological development and functioning, Animals, Base Sequence, Chromatin, Codon, Terminator, Computational Biology, Conserved Sequence, DNA, Databases, Genetic, Epigenesis, Genetic, Epigenomics, Humans, K562 Cells, Mice, NIH 3T3 Cells, Nucleic Acid Conformation, Promoter Regions, Genetic, RNA, Structure-Activity Relationship, Transcription, Genetic, Transcriptome, Medical and Health Sciences, Developmental Biology, Biological sciences, Biomedical and clinical sciences, Health sciences

Abstract

R-loops are three-stranded nucleic acid structures formed upon annealing of an RNA strand to one strand of duplex DNA. We profiled R-loops using a high-resolution, strand-specific methodology in human and mouse cell types. R-loops are prevalent, collectively occupying up to 5% of mammalian genomes. R-loop formation occurs over conserved genic hotspots such as promoter and terminator regions of poly(A)-dependent genes. In most cases, R-loops occur co-transcriptionally and undergo dynamic turnover. Detailed epigenomic profiling revealed that R-loops associate with specific chromatin signatures. At promoters, R-loops associate with a hyper-accessible state characteristic of unmethylated CpG island promoters. By contrast, terminal R-loops associate with an enhancer- and insulator-like state and define a broad class of transcription terminators. Together, this suggests that the retention of nascent RNA transcripts at their site of expression represents an abundant, dynamic, and programmed component of the mammalian chromatin that affects chromatin patterning and the control of gene expression.

Published

2016

32. The A31P missense mutation in cardiac myosin binding protein C alters protein structure but does not cause haploinsufficiency

Author

van Dijk, Sabine J, Kooiker, Kristina Bezold, Mazzalupo, Stacy, Yang, Yuanzhang, Kostyukova, Alla S, Mustacich, Debbie J, Hoye, Elaine R, Stern, Joshua A, Kittleson, Mark D, and Harris, Samantha P

Subjects

Biological Sciences, Bioinformatics and Computational Biology, Genetics, Rare Diseases, Pediatric Cardiomyopathy, Pediatric, Heart Disease, Cardiovascular, 2.1 Biological and endogenous factors, Alanine, Animals, Cardiomyopathy, Hypertrophic, Carrier Proteins, Cats, Circular Dichroism, Codon, Terminator, Haploinsufficiency, Heart, Immunohistochemistry, Muscle Cells, Mutation, Mutation, Missense, Myocardium, Proline, Protein Conformation, Protein Domains, Protein Structure, Secondary, Recombinant Proteins, Sarcomeres, cMyBP-C, Hypertrophic cardiomyopathy, Missense mutation, Animal models of cardiac disease, Biochemistry & Molecular Biology

Abstract

Mutations in MYBPC3, the gene encoding cardiac myosin binding protein C (cMyBP-C), are a major cause of hypertrophic cardiomyopathy (HCM). While most mutations encode premature stop codons, missense mutations causing single amino acid substitutions are also common. Here we investigated effects of a single proline for alanine substitution at amino acid 31 (A31P) in the C0 domain of cMyBP-C, which was identified as a natural cause of HCM in cats. Results using recombinant proteins showed that the mutation disrupted C0 structure, altered sensitivity to trypsin digestion, and reduced recognition by an antibody that preferentially recognizes N-terminal domains of cMyBP-C. Western blots detecting A31P cMyBP-C in myocardium of cats heterozygous for the mutation showed a reduced amount of A31P mutant protein relative to wild-type cMyBP-C, but the total amount of cMyBP-C was not different in myocardium from cats with or without the A31P mutation indicating altered rates of synthesis/degradation of A31P cMyBP-C. Also, the mutant A31P cMyBP-C was properly localized in cardiac sarcomeres. These results indicate that reduced protein expression (haploinsufficiency) cannot account for effects of the A31P cMyBP-C mutation and instead suggest that the A31P mutation causes HCM through a poison polypeptide mechanism that disrupts cMyBP-C or myocyte function.

Published

2016

33. Translation readthrough mitigation

Author

Arribere, Joshua A, Cenik, Elif S, Jain, Nimit, Hess, Gaelen T, Lee, Cameron H, Bassik, Michael C, and Fire, Andrew Z

Subjects

Genetics, Prevention, 1.1 Normal biological development and functioning, Underpinning research, Generic health relevance, 3' Untranslated Regions, Animals, Animals, Genetically Modified, CRISPR-Cas Systems, Caenorhabditis elegans, Codon, Terminator, Genes, Hemoglobins, Abnormal, Humans, Peptides, Protein Biosynthesis, Proteins, Ribosomes, General Science & Technology

Abstract

A fraction of ribosomes engaged in translation will fail to terminate when reaching a stop codon, yielding nascent proteins inappropriately extended on their C termini. Although such extended proteins can interfere with normal cellular processes, known mechanisms of translational surveillance are insufficient to protect cells from potential dominant consequences. Here, through a combination of transgenics and CRISPR–Cas9 gene editing in Caenorhabditis elegans, we demonstrate a consistent ability of cells to block accumulation of C-terminal-extended proteins that result from failure to terminate at stop codons. Sequences encoded by the 3′ untranslated region (UTR) were sufficient to lower protein levels. Measurements of mRNA levels and translation suggested a co- or post-translational mechanism of action for these sequences in C. elegans. Similar mechanisms evidently operate in human cells, in which we observed a comparable tendency for translated human 3′ UTR sequences to reduce mature protein expression in tissue culture assays, including 3′ UTR sequences from the hypomorphic ‘Constant Spring’ haemoglobin stop codon variant. We suggest that 3′ UTRs may encode peptide sequences that destabilize the attached protein, providing mitigation of unwelcome and varied translation errors.

Published

2016

34. Facile Recoding of Selenocysteine in Nature

Author

Mukai, Takahito, Englert, Markus, Tripp, H James, Miller, Corwin, Ivanova, Natalia N, Rubin, Edward M, Kyrpides, Nikos C, and Söll, Dieter

Subjects

Genetics, Bacteria, Base Sequence, Codon, Terminator, Evolution, Molecular, Genetic Code, Genome, Bacterial, Metagenome, Selenocysteine, genetic code, metagenome, selenocysteine, sense codon recoding, synthetic biology, Chemical Sciences, Organic Chemistry

Abstract

Selenocysteine (Sec or U) is encoded by UGA, a stop codon reassigned by a Sec-specific elongation factor and a distinctive RNA structure. To discover possible code variations in extant organisms we analyzed 6.4 trillion base pairs of metagenomic sequences and 24 903 microbial genomes for tRNA(Sec) species. As expected, UGA is the predominant Sec codon in use. We also found tRNA(Sec) species that recognize the stop codons UAG and UAA, and ten sense codons. Selenoprotein synthesis programmed by UAG in Geodermatophilus and Blastococcus, and by the Cys codon UGU in Aeromonas salmonicida was confirmed by metabolic labeling with (75) Se or mass spectrometry. Other tRNA(Sec) species with different anticodons enabled E. coli to synthesize active formate dehydrogenase H, a selenoenzyme. This illustrates the ease by which the genetic code may evolve new coding schemes, possibly aiding organisms to adapt to changing environments, and show the genetic code is much more flexible than previously thought.

Published

2016

35. BRCA2 Polymorphic Stop Codon K3326X and the Risk of Breast, Prostate, and Ovarian Cancers.

Author

Meeks, Huong D, Song, Honglin, Michailidou, Kyriaki, Bolla, Manjeet K, Dennis, Joe, Wang, Qin, Barrowdale, Daniel, Frost, Debra, EMBRACE, McGuffog, Lesley, Ellis, Steve, Feng, Bingjian, Buys, Saundra S, Hopper, John L, Southey, Melissa C, Tesoriero, Andrea, kConFab Investigators, James, Paul A, Bruinsma, Fiona, Campbell, Ian G, Australia Ovarian Cancer Study Group, Broeks, Annegien, Schmidt, Marjanka K, Hogervorst, Frans BL, HEBON, Beckman, Matthias W, Fasching, Peter A, Fletcher, Olivia, Johnson, Nichola, Sawyer, Elinor J, Riboli, Elio, Banerjee, Susana, Menon, Usha, Tomlinson, Ian, Burwinkel, Barbara, Hamann, Ute, Marme, Frederik, Rudolph, Anja, Janavicius, Ramunas, Tihomirova, Laima, Tung, Nadine, Garber, Judy, Cramer, Daniel, Terry, Kathryn L, Poole, Elizabeth M, Tworoger, Shelley S, Dorfling, Cecilia M, van Rensburg, Elizabeth J, Godwin, Andrew K, Guénel, Pascal, Truong, Thérèse, GEMO Study Collaborators, Stoppa-Lyonnet, Dominique, Damiola, Francesca, Mazoyer, Sylvie, Sinilnikova, Olga M, Isaacs, Claudine, Maugard, Christine, Bojesen, Stig E, Flyger, Henrik, Gerdes, Anne-Marie, Hansen, Thomas VO, Jensen, Allen, Kjaer, Susanne K, Hogdall, Claus, Hogdall, Estrid, Pedersen, Inge Sokilde, Thomassen, Mads, Benitez, Javier, González-Neira, Anna, Osorio, Ana, Hoya, Miguel de la, Segura, Pedro Perez, Diez, Orland, Lazaro, Conxi, Brunet, Joan, Anton-Culver, Hoda, Eunjung, Lee, John, Esther M, Neuhausen, Susan L, Ding, Yuan Chun, Castillo, Danielle, Weitzel, Jeffrey N, Ganz, Patricia A, Nussbaum, Robert L, Chan, Salina B, Karlan, Beth Y, Lester, Jenny, Wu, Anna, Gayther, Simon, Ramus, Susan J, Sieh, Weiva, Whittermore, Alice S, Monteiro, Alvaro NA, Phelan, Catherine M, Terry, Mary Beth, Piedmonte, Marion, Offit, Kenneth, Robson, Mark, and Levine, Douglas

Subjects

EMBRACE, kConFab Investigators, Australia Ovarian Cancer Study Group, HEBON, GEMO Study Collaborators, OCGN, PRostate cancer AssoCiation group To Investigate Cancer Associated aLterations in the genome, Humans, Breast Neoplasms, Ovarian Neoplasms, Prostatic Neoplasms, Neoplasm Invasiveness, Genetic Predisposition to Disease, Lysine, BRCA2 Protein, Codon, Terminator, Logistic Models, Odds Ratio, Risk Assessment, Risk Factors, Heterozygote, Polymorphism, Single Nucleotide, Adult, Aged, Middle Aged, Female, Male, Clinical Research, Prevention, Cancer, Prostate Cancer, Aging, Urologic Diseases, Breast Cancer, Ovarian Cancer, Rare Diseases, Aetiology, 2.1 Biological and endogenous factors, Oncology and Carcinogenesis, Oncology & Carcinogenesis

Abstract

The K3326X variant in BRCA2 (BRCA2*c.9976A>T; p.Lys3326*; rs11571833) has been found to be associated with small increased risks of breast cancer. However, it is not clear to what extent linkage disequilibrium with fully pathogenic mutations might account for this association. There is scant information about the effect of K3326X in other hormone-related cancers. Using weighted logistic regression, we analyzed data from the large iCOGS study including 76 637 cancer case patients and 83 796 control patients to estimate odds ratios (ORw) and 95% confidence intervals (CIs) for K3326X variant carriers in relation to breast, ovarian, and prostate cancer risks, with weights defined as probability of not having a pathogenic BRCA2 variant. Using Cox proportional hazards modeling, we also examined the associations of K3326X with breast and ovarian cancer risks among 7183 BRCA1 variant carriers. All statistical tests were two-sided. The K3326X variant was associated with breast (ORw = 1.28, 95% CI = 1.17 to 1.40, P = 5.9x10(-) (6)) and invasive ovarian cancer (ORw = 1.26, 95% CI = 1.10 to 1.43, P = 3.8x10(-3)). These associations were stronger for serous ovarian cancer and for estrogen receptor-negative breast cancer (ORw = 1.46, 95% CI = 1.2 to 1.70, P = 3.4x10(-5) and ORw = 1.50, 95% CI = 1.28 to 1.76, P = 4.1x10(-5), respectively). For BRCA1 mutation carriers, there was a statistically significant inverse association of the K3326X variant with risk of ovarian cancer (HR = 0.43, 95% CI = 0.22 to 0.84, P = .013) but no association with breast cancer. No association with prostate cancer was observed. Our study provides evidence that the K3326X variant is associated with risk of developing breast and ovarian cancers independent of other pathogenic variants in BRCA2. Further studies are needed to determine the biological mechanism of action responsible for these associations.

Published

2016

36. Prolepsis in the Terminator Series.

Author

Hall, Kenneth E.

Subjects

SCIENCE fiction films

Abstract

THe article discusses the treatment prolepsis in the "Terminator" films and the spinoff television series "Terminator: The Sarah Connor Chronicles." Topics covered include the appearance of narratological prolepsis, which treats future events as if they have already occurred, within the Terminator storyline, the dependence of the overall storyline on the manipulation of temporal tropes, and how the film "Terminator: Dark Fate" presented time structure while preserving proleptic elements.

Published

2022

37. A single mutation attenuates both the transcription termination and RNA-dependent RNA polymerase activity of T7 RNA polymerase.

Author

Wu, Hui, Wei, Ting, Yu, Bingbing, Cheng, Rui, Huang, Fengtao, Lu, Xuelin, Yan, Yan, Wang, Xionglue, Liu, Chenli, and Zhu, Bin

Subjects

RNA replicase, RNA polymerases, RNA synthesis, CATALYTIC RNA, BINDING site assay, RNA analysis

Abstract

Transcription termination is one of the least understood processes of gene expression. As the prototype model for transcription studies, the single-subunit T7 RNA polymerase (RNAP) is known to respond to two types of termination signals, but the mechanism underlying such termination, especially the specific elements of the polymerase involved, is still unclear, due to a lack of knowledge with respect to the structure of the termination complex. Here we applied phage-assisted continuous evolution to obtain variants of T7 RNAP that can bypass the typical class I T7 terminator with stem-loop structure. Through in vivo selection and in vitro characterization, we discovered a single mutation (S43Y) that significantly decreased the termination efficiency of T7 RNAP at all transcription terminators tested. Coincidently, the S43Y mutation almost eliminates the RNA-dependent RNAP (RdRp) activity of T7 RNAP without impeding the major DNA-dependent RNAP (DdRp) activity of the enzyme. S43 is located in a hinge region and regulates the transformation between transcription initiation and elongation of T7 RNAP. Steady-state kinetics analysis and an RNA binding assay indicate that the S43Y mutation increases the transcription efficiency while weakening RNA binding of the enzyme. As an enzymatic reagent for in vitro transcription, the T7 RNAP S43Y mutant reduces the undesired termination in run-off RNA synthesis and produces RNA with higher terminal homogeneity. [ABSTRACT FROM AUTHOR]

Published

2021

38. 解脂耶氏酵母作为微生物细胞工厂的 应用研究进展.

Author

赵 禹, 刘士琦, 李 建, 李圣龙, 赵雅坤, 肖冬光, and 于爱群

Subjects

BIOLOGICAL systems, INDUSTRIAL goods, MICROBIAL cells, INFORMATION design, GENOME editing, BIOMASS energy, GENE clusters

Abstract

Copyright of Shipin Kexue/ Food Science is the property of Food Science Editorial Department and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2021

39. Increased Susceptibility to Skin Carcinogenesis Associated with a Spontaneous Mouse Mutation in the Palmitoyl Transferase Zdhhc13 Gene.

Author

Perez, Carlos J, Mecklenburg, Lars, Jaubert, Jean, Martinez-Santamaria, Lucia, Iritani, Brian M, Espejo, Alexsandra, Napoli, Eleonora, Song, Gyu, Del Río, Marcela, DiGiovanni, John, Giulivi, Cecilia, Bedford, Mark T, Dent, Sharon YR, Wood, Richard D, Kusewitt, Donna F, Guénet, Jean-Louis, Conti, Claudio J, and Benavides, Fernando

Subjects

NIH 3T3 Cells, Keratinocytes, Animals, Mice, Skin Neoplasms, Genetic Predisposition to Disease, Leukocyte Elastase, Acyltransferases, NF-kappa B, Codon, Terminator, Bromodeoxyuridine, Neutrophil Infiltration, Phenotype, Mutation, Epidermal Cells, Codon, Terminator, Clinical Sciences, Oncology and Carcinogenesis, Dermatology & Venereal Diseases

Abstract

Here we describe a spontaneous mutation in the Zdhhc13 (zinc finger, DHHC domain containing 13) gene (also called Hip14l), one of 24 genes encoding palmitoyl acyltransferase (PAT) enzymes in the mouse. This mutation (Zdhhc13luc) was identified as a nonsense base substitution, which results in a premature stop codon that generates a truncated form of the ZDHHC13 protein, representing a potential loss-of-function allele. Homozygous Zdhhc13luc/Zdhhc13luc mice developed generalized hypotrichosis, associated with abnormal hair cycle, epidermal and sebaceous gland hyperplasia, hyperkeratosis, and increased epidermal thickness. Increased keratinocyte proliferation and accelerated transit from basal to more differentiated layers were observed in mutant compared with wild-type (WT) epidermis in untreated skin and after short-term 12-O-tetradecanoyl-phorbol-13-acetate treatment and acute UVB exposure. Interestingly, this epidermal phenotype was associated with constitutive activation of NF-κB (RelA) and increased neutrophil recruitment and elastase activity. Furthermore, tumor multiplicity and malignant progression of papillomas after chemical skin carcinogenesis were significantly higher in mutant mice than WT littermates. To our knowledge, this is the first report of a protective role for PAT in skin carcinogenesis.

Published

2015

40. Genome-wide burden of deleterious coding variants increased in schizophrenia.

Author

Loohuis, Loes M Olde, Vorstman, Jacob AS, Ori, Anil P, Staats, Kim A, Wang, Tina, Richards, Alexander L, Leonenko, Ganna, Walters, James T, DeYoung, Joseph, GROUP consortium, Cantor, Rita M, and Ophoff, Roel A

Subjects

GROUP consortium, Humans, Genetic Predisposition to Disease, Codon, Terminator, RNA Splice Sites, Case-Control Studies, Schizophrenia, Gene Frequency, Genotype, Multifactorial Inheritance, Polymorphism, Single Nucleotide, Alleles, European Continental Ancestry Group, Female, Male, Genetic Variation, Genome-Wide Association Study, Codon, Terminator, Polymorphism, Single Nucleotide

Abstract

Schizophrenia is a common complex disorder with polygenic inheritance. Here we show that by using an approach that compares the individual loads of rare variants in 1,042 schizophrenia cases and 961 controls, schizophrenia cases carry an increased burden of deleterious mutations. At a genome-wide level, our results implicate non-synonymous, splice site as well as stop-altering single-nucleotide variations occurring at minor allele frequency of ≥ 0.01% in the population. In an independent replication sample of 5,585 schizophrenia cases and 8,103 controls of European ancestry we confirm an enrichment in cases of the alleles identified in our study. In addition, the genes implicated by the increased burden of rare coding variants highlight the involvement of neurodevelopment in the aetiology of schizophrenia.

Published

2015

41. Synthetic Gene Regulation in Cyanobacteria

Author

Immethun, Cheryl M., Moon, Tae Seok, COHEN, IRUN R., Series Editor, LAJTHA, ABEL, Series Editor, LAMBRIS, JOHN D., Series Editor, PAOLETTI, RODOLFO, Series Editor, REZAEI, NIMA, Series Editor, Zhang, Weiwen, editor, and Song, Xinyu, editor

Published

2018

42. Response and Adaptation of Escherichia coli to Suppression of the Amber Stop Codon

Author

Wang, Qian, Sun, Tingting, Xu, Jianfeng, Shen, Zhouxin, Briggs, Steven P, Zhou, Demin, and Wang, Lei

Subjects

Genetics, Amino Acids, Codon, Terminator, Escherichia coli, Genetic Code, Ligases, Protein Engineering, Proteomics, RNA, Transfer, amber codon suppression, amino acids, expansion of the genetic code, mutagenesis, synthetic biology, Medicinal and Biomolecular Chemistry, Biochemistry and Cell Biology, Organic Chemistry

Abstract

Some extant organisms reassign the amber stop codon to a sense codon through evolution, and suppression of the amber codon with engineered tRNAs has been exploited to expand the genetic code for incorporating non-canonical amino acids (ncAAs) in live systems. However, it is unclear how the host cells respond and adapt to such amber suppression. Herein we suppressed the amber codon in Escherichia coli with an orthogonal tRNA/synthetase pair and cultured the cells under such a pressure for about 500 generations. We discovered that E. coli quickly counteracted the suppression with transposon insertion to inactivate the orthogonal synthetase. Persistent amber suppression evading transposon inactivation led to global proteomic changes with a notable up-regulation of a previously uncharacterized protein (YdiI) for which we identified an unexpected function of expelling plasmids. These results should be valuable for understanding codon reassignment in genetic code evolution and for improving the efficiency of ncAA incorporation.

Published

2014

43. Thermodynamic and kinetic insights into stop codon recognition by release factor 1.

Author

Trappl, Krista, Mathew, Merrill A, and Joseph, Simpson

Subjects

Ribosomes, Escherichia coli, Escherichia coli Proteins, Peptide Termination Factors, Codon, Terminator, Hydrolysis, Kinetics, Mutation, Thermodynamics, Models, Molecular, Codon, Terminator, Models, Molecular, General Science & Technology

Abstract

Stop codon recognition is a crucial event during translation termination and is performed by class I release factors (RF1 and RF2 in bacterial cells). Recent crystal structures showed that stop codon recognition is achieved mainly through a network of hydrogen bonds and stacking interactions between the stop codon and conserved residues in domain II of RF1/RF2. Additionally, previous studies suggested that recognition of stop codons is coupled to proper positioning of RF1 on the ribosome, which is essential for triggering peptide release. In this study we mutated four conserved residues in Escherichia coli RF1 (Gln185, Arg186, Thr190, and Thr198) that are proposed to be critical for discriminating stop codons from sense codons. Our thermodynamic and kinetic analysis of these RF1 mutants showed that the mutations inhibited the binding of RF1 to the ribosome. However, the mutations in RF1 did not affect the rate of peptide release, showing that imperfect recognition of the stop codon does not affect the proper positioning of RF1 on the ribosome.

Published

2014

44. Complex Transcriptional Profiles of the PPP1R12A Gene in Cells of the Circulatory System as Revealed by In Silico Analysis and Reverse Transcription PCR

Author

Paulo André Saldanha, Israel Olapeju Bolanle, Timothy Martin Palmer, Leonid Leonidovich Nikitenko, and Francisco Rivero

Subjects

MYPT1, PPP1R12A, alternative splicing, promoter, terminator, HUVEC, Cytology, QH573-671

Abstract

The myosin light chain phosphatase target subunit 1 (MYPT1), encoded by the PPP1R12A gene, is a key component of the myosin light chain phosphatase (MLCP) protein complex. MYPT1 isoforms have been described as products of the cassette-type alternative splicing of exons E13, E14, E22, and E24. Through in silico analysis of the publicly available EST and mRNA databases, we established that PPP1R12A contains 32 exons (6 more than the 26 previously reported), of which 29 are used in 11 protein-coding transcripts. An in silico analysis of publicly available RNAseq data combined with validation by reverse transcription (RT)-PCR allowed us to determine the relative abundance of each transcript in three cell types of the circulatory system where MYPT1 plays important roles: human umbilical vein endothelial cells (HUVEC), human saphenous vein smooth muscle cells (HSVSMC), and platelets. All three cell types express up to 10 transcripts at variable frequencies. HUVECs and HSVSMCs predominantly express the full-length variant (58.3% and 64.3%, respectively) followed by the variant skipping E13 (33.7% and 23.1%, respectively), whereas in platelets the predominant variants are those skipping E14 (51.4%) and E13 (19.9%), followed by the full-length variant (14.4%). Variants including E24 account for 5.4% of transcripts in platelets but are rare (

Published

2022

45. The identification of novel promoters and terminators for protein expression and metabolic engineering applications in Kluyveromyces marxianus

Author

Pradeep Kumar, Debendra Kumar Sahoo, and Deepak Sharma

Subjects

Kluyveromyces marxianus, Protein expression, Metabolic engineering, Promoter, Terminator, β-Galactosidase, Biotechnology, TP248.13-248.65, Biology (General), QH301-705.5

Abstract

The K. marxianus has emerged as a potential yeast strain for various biotechnological applications. However, the limited number of available genetic tools has hindered the widespread usage of this yeast. In the current study we have expanded the molecular tool box by identifying novel sets of promoters and terminators for increased recombinant protein expression in K. marxianus. The previously available transcriptomic data were analyzed to identify top 10 promoters of highest gene expression activity. We further characterized and compared strength of these identified promoters using eGFP as a reporter protein, at different temperatures and carbon sources. To examine the regulatory region driving protein expression, serially truncated shorter versions of two selected strong promoters were designed, and examined for their ability to drive eGFP protein expression. The activities of these two promoters were further enhanced using different combinations of native transcription terminators of K. marxianus. We further utilized the identified DNA cassette encoding strong promoter in metabolic engineering of K. marxianus for enhanced β-galactosidase activity. The present study thus provides novel sets of promoters and terminators as well as engineered K. marxianus strain for its wider utility in applications requiring lactose degradation such as in cheese whey and milk.

Published

2021

46. Construction of a reporter system for bifidobacteria using chloramphenicol acetyltransferase and its application for evaluation of promoters and terminators.

Author

Tomoya KOZAKAI, Yoko SHIMOFUSA, Izumi NOMURA, and Tohru SUZUKI

Subjects

BIFIDOBACTERIUM, ACTINOMYCETACEAE, CHLORAMPHENICOL, ANTIBACTERIAL agents, ACETYLTRANSFERASES, NITROBENZOIC acid

Abstract

A reporter assay system is an essential tool for investigating gene expression mechanisms. In the case of bifidobacteria, several convenient and sensitive reporter systems have been developed. Here, we developed a new reporter system for bifidobacteria using the chloramphenicol acetyltransferase gene (cat) from Staphylococcus aureus. This enzyme stoichiometrically produced free CoA-SH, which was analyzed quantitatively with Ellman's test using 2-nitrobenzoic acid (DTNB). The 2-nitro-5-thiobenzoate (TNB2-) produced showed a strong yellowish color with maximum absorbance at 412 nm. We also constructed a new pBCMAT plasmid series for CAT assays in bifidobacteria to evaluate promoters and terminators. Analyses using promoters from Bifidobacterium longum NCC2705 indicated that the CAT assay using these promoters is quantitative, has a wide measurement range, and is stable. In addition, this assay was useful for several bifidobacterial species, including B. longum, Bifidobacterium breve, and Bifidobacterium adolescentis. Compared with evoglow-Bs2, a fluorescent protein used under anaerobic conditions, the CAT assay showed about 0.25% background activity. In analyses using this CAT assay, we identified 11 promoters and 12 terminators of B. longum NCC2705. The genes encoding ribosomal proteins, elongation factors, and transfer RNAs possessed strong promoters, and terminators that include strong stem-loops and poly-U tails structures tended to show high activities. Although the abovementioned promoters made stronger contributions to expression activities than the terminators, the maximum fold difference in the activities among the tested terminators was approximately 17-fold. Modification of the -10 box and 5'-UTR in the promoters and the structure around the stem-loop in the terminators affected expression levels. These results suggest that the CAT assay is useful for various analyses of bifidobacterial gene expression. [ABSTRACT FROM AUTHOR]

Published

2021

47. A New Series of Small Molecular Weight Compounds Induce Read Through of All Three Types of Nonsense Mutations in the ATM Gene

Author

Du, Liutao, Jung, Michael E, Damoiseaux, Robert, Completo, Gladys, Fike, Francesca, Ku, Jin-Mo, Nahas, Shareef, Piao, Cijing, Hu, Hailiang, and Gatti, Richard A

Subjects

Medical Biotechnology, Biomedical and Clinical Sciences, Clinical Sciences, Neurosciences, Prevention, Genetics, Orphan Drug, Rare Diseases, 5.1 Pharmaceuticals, Development of treatments and therapeutic interventions, Acetanilides, Ataxia Telangiectasia, Ataxia Telangiectasia Mutated Proteins, Benzodioxoles, Cells, Cultured, Codon, Nonsense, Codon, Terminator, DNA-Binding Proteins, High-Throughput Screening Assays, Humans, Molecular Targeted Therapy, Molecular Weight, Small Molecule Libraries, Structure-Activity Relationship, Thiourea, Triazoles, Biological Sciences, Technology, Medical and Health Sciences, Biotechnology, Clinical sciences, Medical biotechnology

Abstract

Chemical-induced read through of premature stop codons might be exploited as a potential treatment strategy for genetic disorders caused by nonsense mutations. Despite the promise of this approach, only a few read-through compounds (RTCs) have been discovered to date. These include aminoglycosides (e.g., gentamicin and G418) and nonaminoglycosides (e.g., PTC124 and RTC13). The therapeutic benefits of these RTCs remain to be determined. In an effort to find new RTCs, we screened an additional ~36,000 small molecular weight compounds using a high-throughput screening (HTS) assay that we had previously developed and identified two novel RTCs, GJ071, and GJ072. The activity of these two compounds was confirmed in cells derived from ataxia telangiectasia (A-T) patients with three different types of nonsense mutation in the ATM gene. Both compounds showed activity comparable to stop codons (TGA, TAG, and TAA) PTC124 and RTC13. Early structure-activity relationship studies generated eight active analogs of GJ072. Most of those analogs were effective on all three stop codons. GJ071 and GJ072, and some of the GJ072 analogs, appeared to be well tolerated by A-T cells. We also identified another two active RTCs in the primary screen, RTC204 and RTC219, which share a key structural feature with GJ072 and its analogs.

Published

2013

48. Development and optimization of a pepino mosaic virus-based vector for rapid expression of heterologous proteins in plants.

Author

Abrahamian, Peter, Hammond, John, and Hammond, Rosemarie W.

Subjects

*PLANT proteins, *GREEN fluorescent protein, *PROTEIN expression, *MOSAIC viruses, *GENETIC vectors, *VIRAL proteins

Abstract

Plant-virus–derived vectors are versatile tools with multiple applications in agricultural and medical biotechnology. In this study, we developed pepino mosaic virus (PepMV) (family Alphaflexiviridae; genus Potexvirus) into a vector for heterologous protein expression in plants. PepMV was initially cloned in a step-wise manner, fully sequenced and the full-length infectious clone was tested for infectivity in Nicotiana benthamiana. Initial infectious clones resulted in poor replication of PepMV and lack of systemic movement. Mutations in the viral sequence affected systemic infection. Two suspected mutations were altered to restore systemic infectivity. PepMV infection was apparent as early as 4 days post agroinfiltration (dpa) inoculation in N. benthamiana. A multiple cloning site was inserted into the PepMV genome for introduction and expression of foreign genes. Several modifications to the wild-type vector were made, such as a replacing the native subgenomic promoter (SGP) with a heterologous SGP, and introduction of translational enhancers and terminators, to improve heterologous expression of the foreign gene-of-interest. GFP was used as a reporter for monitoring virus infection and protein production. Strong GFP expression was observed as early as 4 dpa with a translational enhancer. The PepMV-based vector produces rapid expression of the foreign gene in comparison to two other potexvirus-based vectors. GFP production was monitored over time and optimal protein production was recorded between 5 and 7 dpa. GFP protein levels reached up to 4% and decreased to 0.5% total soluble protein at 7 and 14 dpa, respectively. Future studies will evaluate this virus-based vector for large-scale production of pharmaceutical compounds. Key points: • A pepino mosaic virus isolate was developed into a plant-based expression vector. • Expression levels of the heterologous protein were comparable or exceeded previously developed viral vectors. • Protein levels in plants were highest between 5 and 7 days and decreased gradually. [ABSTRACT FROM AUTHOR]

Published

2021

49. 2-Oxazolina: Polimerización y síntesis de macromonómeros.

Author

Azael Ludeña-Huaman, Michael

Subjects

*GRAFT copolymers, *LIVING polymerization, *MACROMONOMERS, *DENDRIMERS, *CHEMICAL properties, *STAR-branched polymers, *THERMORESPONSIVE polymers

Abstract

The chemistry of poly(2-oxazoline) has resurfaced in the last two decades due to their easy synthesis, as well as the ability to modulate their chemical structure and properties. Furthermore, poly(2-oxazoline)s are biocompatible and many have thermoresponsive properties. 2-Oxazoline macromonomers are usually used as a starting material to perform the synthesis of graft copolymers, star copolymers and also dendrimers. But also macromonomers can be introduced in the synthesis of materials with more complex structures as hydrogels or nanogeles. For this reason, this manuscript describes fundamental and important chemical aspects about the polymerization and preparation of macromonomers by the initiator and terminator method of the living polymerization of 2-oxazoline. The importance of the initiator, terminator as well as the substituent on 2-oxazoline is discussed. [ABSTRACT FROM AUTHOR]

Published

2021

50. Genetic basis of hidden phenotypic variation revealed by increased translational readthrough in yeast.

Author

Torabi, Noorossadat and Kruglyak, Leonid

Subjects

Saccharomyces cerevisiae, Hydrogen Peroxide, Diamide, Endodeoxyribonucleases, Exodeoxyribonucleases, Protein-Serine-Threonine Kinases, Saccharomyces cerevisiae Proteins, Prions, Peptide Termination Factors, Codon, Terminator, Chromosome Mapping, Protein Biosynthesis, RNA Stability, Peptide Chain Termination, Translational, Phenotype, Mutation, Alleles, Quantitative Trait Loci, Codon, Terminator, Peptide Chain Termination, Translational, Genetics, Developmental Biology

Abstract

Eukaryotic release factors 1 and 3, encoded by SUP45 and SUP35, respectively, in Saccharomyces cerevisiae, are required for translation termination. Recent studies have shown that, besides these two key factors, several genetic and epigenetic mechanisms modulate the efficiency of translation termination. These mechanisms, through modifying translation termination fidelity, were shown to affect various cellular processes, such as mRNA degradation, and in some cases could confer a beneficial phenotype to the cell. The most studied example of such a mechanism is [PSI+], the prion conformation of Sup35p, which can have pleiotropic effects on growth that vary among different yeast strains. However, genetic loci underlying such readthrough-dependent, background-specific phenotypes have yet to be identified. Here, we used sup35(C653R), a partial loss-of-function allele of the SUP35 previously shown to increase readthrough of stop codons and recapitulate some [PSI+]-dependent phenotypes, to study the genetic basis of phenotypes revealed by increased translational readthrough in two divergent yeast strains: BY4724 (a laboratory strain) and RM11_1a (a wine strain). We first identified growth conditions in which increased readthrough of stop codons by sup35(C653R) resulted in different growth responses between these two strains. We then used a recently developed linkage mapping technique, extreme QTL mapping (X-QTL), to identify readthrough-dependent loci for the observed growth differences. We further showed that variation in SKY1, an SR protein kinase, underlies a readthrough-dependent locus observed for growth on diamide and hydrogen peroxide. We found that the allelic state of SKY1 interacts with readthrough level and the genetic background to determine growth rate in these two conditions.

Published

2012