Your search keyword '"Cistron"' showing total 1,263 results

1. Cistron

Author

Gargaud, Muriel, editor, Irvine, William M., editor, Amils, Ricardo, editor, Claeys, Philippe, editor, Cleaves, Henderson James, editor, Gerin, Maryvonne, editor, Rouan, Daniel, editor, Spohn, Tilman, editor, Tirard, Stéphane, editor, and Viso, Michel, editor

Published

2023

2. Cistron

Author

Vonk, Jennifer, editor and Shackelford, Todd K., editor

Published

2022

3. Differential bicistronic gene translation mediated by the internal ribosome entry site element of encephalomyocarditis virus

Author

Chao-Lin Liu, Chia-Rui Shen, Ya-Shan Chen, Hsi-Jien Chen, and Yih-Shiou Hwang

Subjects

Reporter gene, Translational efficiency, viruses, Upstream and downstream (transduction), fungi, Translation (biology), General Medicine, Internal Ribosome Entry Sites, Biology, Cell biology, Mice, Internal ribosome entry site, Cistron, Genes, Reporter, Gene expression, Protein biosynthesis, Animals, Encephalomyocarditis virus, Peptide Chain Initiation, Translational, Ribosomes

Abstract

Background Internal ribosome entry sites (IRESs) allow the translation of a transcript independent of its cap structure. They are distributed in some viruses and cellular RNA. The element is applied in dual gene expression in a single vector. Although it appears the lower efficiency of IRES-mediated translation than that of cap-dependent translation, it is with the crucial needs to know the precise differences in translational efficacy between upstream cistrons (cap-dependent) and downstream cistrons (IRES-mediate, cap-independent) before applying the bicistronic vector in biomedical applications. Material and methods This study aimed to provide real examples and showed the precise differences for translational efficiency dependent upon target gene locations. We generated various bicistronic constructs with quantifiable reporter genes as upstream and downstream cistrons of the encephalomyocarditis virus (EMCV) IRES to precisely evaluate the efficacy of IRES-mediated translation in mammalian cells. Results There was no significant difference in protein production when the reporter gene was cloned as an upstream cistron. However, lower levels of protein production were obtained when the reporter gene was located downstream of the IRES. Moreover, in the presence of an upstream cistron, a markedly reduced level of protein production was observed. Conclusion Our findings demonstrate the version of the EMCV IRES that is provided in many commercial vectors is relatively less efficient than cap-dependent translation and provide valuable information regarding the utilization of IRES to facilitate the expression of more than one protein from a transcript.

Published

2021

4. Cloning and application of the complete nuclear ribosomal DNA (nrDNA) cistron sequence of Pyropia haitanensis (Bangiales, Rhodophyta).

Author

Yuan He, Songdong Shen, and Zonggen Shen

Subjects

*RIBOSOMAL DNA, *CLONING, *RED algae, *GENES, *CULTIVARS

Abstract

Pyropia haitanensis (Bangiales, Rhodophyta) ((T.J. Chang et B.F. Zheng) N. Kikuchi et M. Miyata) is a unique cultivar in China and the main problem with its cultivation lies in a lack of effective technology to distinguish intraspecific strains. In this study, we firstly obtained the complete sequence of rDNA of Pyropia haitanensis in China, which can help identify intraspecific variation within this species. The whole unit is composed of a small-subunit (SSU) rRNA gene with a full length of 2953 base pairs (bp) with two classes of introns and an exon sequence of 1837 bp; moreover, the complete sequence of the large-subunit (LSU) rRNA gene (length 4444 bp) also contains two introns; the length of the 5.8S rRNA gene is 158 bp; the length of internal transcribed spacers 1 (ITS1) is 334 bp and that of ITS2 is 678 bp; and the complete sequence of intergenic spacer (IGS) is 6969 bp. Some portions of the IGS sequences were used to analyze the similarities among five strains of Pyropia haitanensis; the sequence ranged from 4264 bp to 4273 bp and the G + C content was 53%. We also found 118 variable sites in the IGS which account for approximately 2.8% of the whole length. In conclusion, the nuclear ribosomal DNA sequence turned out to be an effective molecular marker for the taxonomic identification of Pyropia haitanensis. [ABSTRACT FROM AUTHOR]

Published

2017

5. Chromosome 19 microRNA cluster enhances cell reprogramming by inhibiting epithelial-to-mesenchymal transition

Author

Thomas Tuschl, Kemal M. Akat, John H. Lockhart, Ying Yang, Ezinne Francess Mong, Jeffrey VanWye, Charles J. Lockwood, Hana Totary-Jain, Frederick Schatz, John C.M. Tsibris, John Canfield, and Umit A. Kayisli

Subjects

Transcriptional Activation, Epithelial-Mesenchymal Transition, Placenta, Induced Pluripotent Stem Cells, lcsh:Medicine, Biology, Article, 03 medical and health sciences, 0302 clinical medicine, Cistron, Pregnancy, microRNA, Humans, Epithelial–mesenchymal transition, Induced pluripotent stem cell, lcsh:Science, reproductive and urinary physiology, 030304 developmental biology, Regulation of gene expression, 0303 health sciences, Multidisciplinary, lcsh:R, Reprogramming, Cell Differentiation, Cellular Reprogramming, Embryonic stem cell, Cell Hypoxia, Trophoblasts, Cell biology, MicroRNAs, HEK293 Cells, Gene Expression Regulation, Differentiation, Multigene Family, 030220 oncology & carcinogenesis, embryonic structures, Female, lcsh:Q, Cytotrophoblasts, Chromosomes, Human, Pair 19, Biomarkers

Abstract

During implantation, cytotrophoblasts undergo epithelial-to-mesenchymal transition (EMT) as they differentiate into invasive extravillous trophoblasts (EVTs). The primate-specific microRNA cluster on chromosome 19 (C19MC) is exclusively expressed in the placenta, embryonic stem cells and certain cancers however, its role in EMT gene regulation is unknown. In situ hybridization for miR-517a/c, a C19MC cistron microRNA, in first trimester human placentas displayed strong expression in villous trophoblasts and a gradual decrease from proximal to distal cell columns as cytotrophoblasts differentiate into invasive EVTs. To investigate the role of C19MC in the regulation of EMT genes, we employed the CRISPR/dCas9 Synergistic Activation Mediator (SAM) system, which induced robust transcriptional activation of the entire C19MC cistron and resulted in suppression of EMT associated genes. Exposure of human iPSCs to hypoxia or differentiation of iPSCs into either cytotrophoblast-stem-like cells or EVT-like cells under hypoxia reduced C19MC expression and increased EMT genes. Furthermore, transcriptional activation of the C19MC cistron induced the expression of OCT4 and FGF4 and accelerated cellular reprogramming. This study establishes the CRISPR/dCas9 SAM as a powerful tool that enables activation of the entire C19MC cistron and uncovers its novel role in suppressing EMT genes critical for maintaining the epithelial cytotrophoblasts stem cell phenotype.

Published

2020

6. Precise Exchange of the Helper-Component Proteinase Cistron Between Soybean mosaic virus and Clover yellow vein virus: Impact on Virus Viability and Host Range Specificity

Author

Y Wang, W Xu, M. R. Hajimorad, Junya Abe, and Kenji S. Nakahara

Subjects

0106 biological sciences, 0301 basic medicine, biology, Potyviridae, Inoculation, Host (biology), viruses, Potyvirus, food and beverages, Soybean mosaic virus, Plant Science, biology.organism_classification, 01 natural sciences, Virology, Vicia faba, 03 medical and health sciences, 030104 developmental biology, Cistron, Genotype, Agronomy and Crop Science, 010606 plant biology & botany

Abstract

Soybean mosaic virus and Clover yellow vein virus are two definite species of the genus Potyvirus within the family Potyviridae. Soybean mosaic virus-N (SMV-N) is well adapted to cultivated soybean (Glycine max) genotypes and wild soybean (G. soja), whereas it remains undetectable in inoculated broad bean (Vicia faba). In contrast, clover yellow vein virus No. 30 (ClYVV-No. 30) is capable of systemic infection in broad bean and wild soybean; however, it infects cultivated soybean genotypes only locally. In this study, SMV-N was shown to also infect broad bean locally; hence, broad bean is a host for SMV-N. Based on these observations, it was hypothesized that lack of systemic infection by SMV-N in broad bean and by ClYVV-No. 30 in cultivated soybean is attributable to the incompatibility of multifunctional helper-component proteinase (HC-Pro) in these hosts. The logic of selecting the HC-Pro cistron as a target is based on its established function in systemic movement and being a relevant factor in host range specificity of potyviruses. To test this hypothesis, chimeras were constructed with precise exchanges of HC-Pro cistrons between SMV-N and ClYVV-No. 30. Upon inoculation, both chimeras were viable in infection, but host range specificity of the recombinant viruses did not differ from those of the parental viruses. These observations suggest that (i) HC-Pro cistrons from SMV-N and ClYVV-No. 30 are functionally compatible in infection despite 55.6 and 48.9% nucleotide and amino acid sequence identity, respectively, and (ii) HC-Pro cistrons from SMV-N and ClYVV-No. 30 are not the determinants of host specificity on cultivated soybean or broad beans, respectively.

Published

2020

7. Specificity of Resistance and Tolerance to Cucumber Vein Yellowing Virus in Melon Accessions and Resistance Breaking with a Single Mutation in VPg

Author

Hervé Lecoq, Juan José López-Moya, Maria Luisa Domingo Calap, Cécile Desbiez, Catherine Wipf-Scheibel, Gregory Girardot, Inmaculada Ferriol, and Michel Pitrat

Subjects

0106 biological sciences, Infectious clone, Evolution, Melon, Ecology and epidemiology, Plant Science, Plant disease resistance, 01 natural sciences, Virus, 03 medical and health sciences, Ipomovirus, Cistron, Virology, Fitness, Allele, Gene, Disease control and pest management, 030304 developmental biology, Plant Diseases, VPg, Genetics, Disease resistance, 0303 health sciences, biology, Potyviridae, biology.organism_classification, Reverse genetics, Cucurbitaceae, Plant Breeding, Resistance-breaking, Mutation, Cucumis sativus, Tolerance, Agronomy and Crop Science, 010606 plant biology & botany

Abstract

Cucumber vein yellowing virus (CVYV) is an emerging virus on cucurbits in the Mediterranean Basin, against which few resistance sources are available, particularly in melon. The melon accession PI 164323 displays complete resistance to isolate CVYV-Esp, and accession HSD 2458 presents a tolerance, i.e., very mild symptoms despite virus accumulation in inoculated plants. The resistance is controlled by a dominant allele Cvy-11, while the tolerance is controlled by a recessive allele cvy-2, independent from Cvy-11. Before introducing the resistance or tolerance in commercial cultivars through a long breeding process, it is important to estimate their specificity and durability. Upon inoculation with eight molecularly diverse CVYV isolates, the resistance was found to be isolate-specific because many CVYV isolates induced necrosis on PI 164323, whereas the tolerance presented a broader range. A resistance-breaking isolate inducing severe mosaic on PI 164323 was obtained. This isolate differed from the parental strain by a single amino acid change in the VPg coding region. An infectious CVYV cDNA clone was obtained, and the effect of the mutation in the VPg cistron on resistance to PI 164323 was confirmed by reverse genetics. This represents the first determinant for resistance-breaking in an ipomovirus. Our results indicate that the use of the Cvy-11 allele alone will not provide durable resistance to CVYV and that, if used in the field, it should be combined with other control methods such as cultural practices and pyramiding of resistance genes to achieve long-lasting resistance against CVYV.

Published

2021

8. sRNA-mediated regulation of gal mRNA in E. coli: Involvement of transcript cleavage by RNase E together with Rho-dependent transcription termination

Author

Monford Paul Abishek N, Heung Jin Jeon, Heon M. Lim, Yonho Lee, Xun Wang, and Dhruba K. Chattoraj

Subjects

Cancer Research, Transcription, Genetic, Operon, Hydrolases, Gene Expression, QH426-470, Biochemistry, Cistron, Transcriptional Termination, Genetics (clinical), Regulation of gene expression, Nucleotides, Organic Compounds, Messenger RNA, Escherichia coli Proteins, Monosaccharides, Translation (biology), Cell biology, Enzymes, Nucleic acids, Chemistry, RNA, Bacterial, Transfer RNA, Physical Sciences, Research Article, Substitution Mutation, RNase P, Nucleases, DNA transcription, Carbohydrates, Biology, Ribonucleases, DNA-binding proteins, Endoribonucleases, Escherichia coli, Genetics, Gene Regulation, RNA, Messenger, Operons, Molecular Biology, Gene, Ecology, Evolution, Behavior and Systematics, Biology and life sciences, Organic Chemistry, Chemical Compounds, Proteins, Galactose, DNA, Gene Expression Regulation, Bacterial, Transcription Termination, Genetic, Mutation, Enzymology, RNA, RNA, Small Untranslated

Abstract

In bacteria, small non-coding RNAs (sRNAs) bind to target mRNAs and regulate their translation and/or stability. In the polycistronic galETKM operon of Escherichia coli, binding of the Spot 42 sRNA to the operon transcript leads to the generation of galET mRNA. The mechanism of this regulation has remained unclear. We show that sRNA-mRNA base pairing at the beginning of the galK gene leads to both transcription termination and transcript cleavage within galK, and generates galET mRNAs with two different 3’-OH ends. Transcription termination requires Rho, and transcript cleavage requires the endonuclease RNase E. The sRNA-mRNA base-paired segments required for generating the two galET species are different, indicating different sequence requirements for the two events. The use of two targets in an mRNA, each of which causes a different outcome, appears to be a novel mode of action for a sRNA. Considering the prevalence of potential sRNA targets at cistron junctions, the generation of new mRNA species by the mechanisms reported here might be a widespread mode of bacterial gene regulation., Author summary sRNAs are regulators of gene expression in all forms of life. In bacteria such as E. coli, sRNAs base-pair with mRNA, which can have many consequences such as premature transcription termination by Rho and degradation of mRNA by the endoribonuclease RNase E. Here we show that the two processes can occur on the same sRNA-mRNA pair and produce shorter but stable mRNA that can be of functional significance. Thus, in sRNA regulation of mRNA, transcript cleavage can be an additional mechanism to well-known transcription termination to generate new mRNA species. The choice between the mechanisms is dictated by where on the mRNA the base pairing with sRNA takes place.

Published

2021

9. High-risk human papillomavirus-18 uses an mRNA sequence to synthesize oncoprotein E6 in tumors

Author

Alejandro García-Carrancá, Giovanna Maldonado, Nahum Sonenberg, Greco Hernández, David Cantú, Yuri V. Svitkin, Jose L. González, and Alejandra García

Subjects

Untranslated region, Gene Expression Regulation, Viral, Codon, Initiator, Uterine Cervical Neoplasms, Biology, Eukaryotic translation, Start codon, Cistron, Cell Line, Tumor, medicine, HaCaT Cells, Humans, RNA, Messenger, Peptide Chain Initiation, Translational, Messenger RNA, Multidisciplinary, Human papillomavirus 18, TOR Serine-Threonine Kinases, EIF4E, Cancer, Translation (biology), Oncogene Proteins, Viral, Biological Sciences, medicine.disease, DNA-Binding Proteins, Eukaryotic Initiation Factor-4E, HEK293 Cells, Eukaryotic Initiation Factor-4A, Cancer research, RNA, Viral, Female, Tumor Suppressor Protein p53, 5' Untranslated Regions, HeLa Cells

Abstract

Cervical cancer is the fourth most common cause of cancer in women worldwide in terms of both incidence and mortality. Persistent infection with high-risk types of human papillomavirus (HPV), namely 16, 18, 31, 33, 35, 39, 45, 51, 52, 56, 58, 59, and 68, constitute a necessary cause for the development of cervical cancer. Viral oncoproteins E6 and E7 play central roles in the carcinogenic process by virtue of their interactions with cell master proteins such as p53, retinoblastoma (Rb), mammalian target of rapamycin (mTOR), and c-MYC. For the synthesis of E6 and E7, HPVs use a bicistronic messenger RNA (mRNA) that has been studied in cultured cells. Here, we report that in cervical tumors, HPV-18, -39, and -45 transcribe E6/E7 mRNAs with extremely short 5' untranslated regions (UTRs) or even lacking a 5' UTR (i.e., zero to three nucleotides long) to express E6. We show that the translation of HPV-18 E6 cistron is regulated by the motif ACCaugGCGCG(C/A)UUU surrounding the AUG start codon, which we term Translation Initiation of Leaderless mRNAs (TILM). This motif is conserved in all HPV types of the phylogenetically coherent group forming genus alpha, species 7, which infect mucosal epithelia. We further show that the translation of HPV-18 E6 largely relies on the cap structure and eIF4E and eIF4AI, two key translation initiation factors linking translation and cancer but does not involve scanning. Our results support the notion that E6 forms the center of the positive oncogenic feedback loop node involving eIF4E, the mTOR cascade, and p53.

Published

2021

10. Cistron

Author

Gargaud, Muriel, editor, Irvine, William M., editor, Amils, Ricardo, editor, Cleaves, Henderson James (Jim), II, editor, Pinti, Daniele L., editor, Quintanilla, José Cernicharo, editor, Rouan, Daniel, editor, Spohn, Tilman, editor, Tirard, Stéphane, editor, and Viso, Michel, editor

Published

2015

11. Three new species of Lachemilla (Rosaceae) from South America

Author

Diego F. Morales-Briones, Katya Romoleroux, and David C. Tank

Subjects

0106 biological sciences, Indumentum, páramo, Rosaceae, Andes, Plant Science, Colombia, 010603 evolutionary biology, 01 natural sciences, Magnoliopsida, 03 medical and health sciences, Cistron, lcsh:Botany, Peru, Botany, Rosales, Plastid, Plantae, Lachemilla, Identification Key, Phylogeny, Ecology, Evolution, Behavior and Systematics, Taxonomy, 030304 developmental biology, new species, 0303 health sciences, biology, Phylogenetic tree, Allopolyploidy, South America, Ribosomal RNA, biology.organism_classification, lcsh:QK1-989, Tracheophyta, Taxon, Research Article

Abstract

Three new species ofLachemilla(Rosaceae), two from Colombia and one from Peru, are described and illustrated.Lachemillarothmalerianais characterized by its stout stems, sericeous-villous indumentum, and wide ascending sheaths with trilobate lateral lobes.Lachemillaargenteapresents a unique combination of tripartite basal leaves with an adaxial silvery villous indumentum, and decumbent branches with verticillate lobed sheaths. Finally,Lachemillacyaneahas distinctly basal reniform leaves with a blue-green color and hirsute pubescence. Phylogenetic analyses of the nuclear ribosomal cistron and multiple regions of the plastid genome revealed the allopolyploid origin of the three new taxa.

Published

2019

12. The complete genome sequence of wild tomato mosaic virus isolated from Solanum nigrum reveals recombination in the P1 cistron

Author

Jia Qi, Min Zhang, Jing Shang, Lei Zhang, Wenyu Yang, and Guoshu Gong

Subjects

China, Genome, Viral, Solanum nigrum, Genome, Open Reading Frames, 03 medical and health sciences, Cistron, Phylogenetics, Virology, Tobacco, Phylogeny, Plant Diseases, 030304 developmental biology, Sequence (medicine), Recombination, Genetic, Whole genome sequencing, 0303 health sciences, Base Sequence, Whole Genome Sequencing, biology, 030306 microbiology, Tobamovirus, Potyvirus, General Medicine, biology.organism_classification, Recombination

Abstract

The complete genome sequence of a wild tomato mosaic virus (WTMV) isolate (named WTMV-Sn) was determined and identified in Solanum nigrum in China. The complete genome of WTMV-Sn is 9,659 nucleotides in length, excluding the poly(A) tail and encodes a polyprotein of 3,074 amino acids. This is the first report of WTMV infecting S. nigrum. Despite the high degree of sequence similarity between the WTMV-Sn and WTMV-XC-1 isolates, the 349 nucleotides at the 5' terminus of WTMV-Sn appear to have originated by recombination with another isolate. The recombination parent remains unknown, but the recombination region shares 74.57% sequence identity with isolate WTMV-Laichau, which is below the species demarcation threshold for the genus Potyvirus. A pathogenicity test showed that WTMV-Sn can infect tobacco. This suggests that variation in the P1 cistron of WTMV-Sn may contribute to its ability to infect S. nigrum.

Published

2019

13. microRNA response in potato virus Y infected tobacco shows strain-specificity depending on host and symptom severity

Author

Fuliang Xie, Magdalena Pawełkowicz, Baohong Zhang, Zhimin Yin, Renata Lebecka, Zofia Murawska, and Krystyna Michalak

Subjects

0303 health sciences, Cancer Research, biology, 030306 microbiology, Gene Expression Profiling, Cellular differentiation, Potyvirus, RNA, biology.organism_classification, Virology, MicroRNAs, 03 medical and health sciences, Infectious Diseases, Potato virus Y, Cistron, Gene Expression Regulation, Plant, Transcription (biology), Host-Pathogen Interactions, Tobacco, microRNA, Tobacco mosaic virus, Gene, Plant Diseases, 030304 developmental biology

Abstract

The present study demonstrates how different potato virus Y (PVY) strains affect the miRNA balance in tobacco cv. Samsun. The two prevalent strains PVYNTN and PVYN−Wi caused severe and mild veinal necrosis (VN) respectively, and the unique PVYZ-NTN strain induced milder vein clearing (VCl) in the upper non-inoculated leaves. A single amino acid polymorphisms (SAPs) I252V and a Q412 to R412 substitution in the HC-Pro cistron of the PVYZ-NTN strain might relate to the loss of VN in tobacco. The abundance of 18 out of the 26 tested miRNAs was increased upon infection by the severe strains PVYNTN and PVYN−Wi. Expression of a group of defense related transcripts were increased accordingly. Two miRNAs, nta-miR6020a-5p and nta-miR6164a/b, which target the TIR-NBS-LRR type resistant TMV N genes involving in signal transduction, might correlate with the PVYNTN and PVYN-Wi induced VN. The down-regulated mRNAs, e.g., RAP2-7 and TOE3, PXC3, LRR-RLK, ATHB-14 and TCP4 targeted by nta-miR172, nta-miR390, nta-miR482, nta-miR166 and nta-miR319/159 respectively, were related to regulation of transcription, protein phosphorylation and cell differentiation. The observed strain-specific alteration of miRNAs and their targets are host dependent and corresponds to the symptom severity and the viral HC-Pro RNA levels.

Published

2019

14. Protein Dosage of the lldPRD Operon Is Correlated with RNase E-Dependent mRNA Processing

Author

Ohsuk Kwon, Ismael Hernández-Lucas, Dimitris Georgellis, Liliana Medina-Aparicio, Enrique Merino, Adrián F. Alvarez, and Lidia E. Angel-Lerma

Subjects

0303 health sciences, Messenger RNA, 030306 microbiology, Permease, Operon, RNase P, Biology, Microbiology, Cell biology, 03 medical and health sciences, Cistron, Gene expression, Transcriptional regulation, Molecular Biology, Gene, 030304 developmental biology, Research Article

Abstract

The ability of Escherichia coli to grow on l-lactate as a sole carbon source depends on the expression of the lldPRD operon. A striking feature of this operon is that the gene encoding the transcriptional regulator (LldR) is located between the genes encoding the permease (LldP) and the dehydrogenase (LldD). In this study, we report that the dosages of the LldP, LldR, and LldD proteins are not modulated on the transcriptional level. Instead, modulation of the protein dosage is correlated primarily with RNase E-dependent mRNA-processing events that take place within the lldR mRNA, leading to the immediate inactivation of lldR, to differential segmental stabilities of the resulting cleavage products, and to differences in the translation efficiencies of the three cistrons. A model for the processing events controlling the molar quantities of the proteins in the lldPRD operon is presented and discussed. IMPORTANCE Adjustment of gene expression is critical for proper cell function. In the case of polycistronic transcripts, posttranscriptional regulatory mechanisms can be used to fine-tune the expression of individual cistrons. Here, we elucidate how the protein dosage of the Escherichia coli lldPRD operon, which presents the paradox of having the gene encoding a regulator protein located between genes that code for a permease and an enzyme, is regulated. Our results demonstrate that the key event in this regulatory mechanism involves the RNase E-dependent cleavage of the primary lldPRD transcript at an internal site(s) located within the lldR cistron, resulting in a drastic decrease in the amount of intact lldR mRNA, in differential segmental stabilities of the resulting cleavage products, and in differences in the translation efficiencies of the three cistrons.

Published

2021

15. Complete Genome Sequence of the Naegleria fowleri (Strain LEE) Closed Circular Extrachromosomal Ribosomal DNA Element

Author

Kristen M. Drescher, Nora M. Chapman, John C. Mullican, and Steven Tracy

Subjects

Genetics, Whole genome sequencing, 0303 health sciences, Naegleria fowleri, 030306 microbiology, Genome Sequences, Biology, biology.organism_classification, 03 medical and health sciences, Open reading frame, Immunology and Microbiology (miscellaneous), Cistron, Extrachromosomal DNA, parasitic diseases, Direct repeat, Molecular Biology, Ribosomal DNA, 030304 developmental biology, Sequence (medicine)

Abstract

The circular extrachromosomal ribosomal DNA (rDNA) element of Naegleria fowleri strain LEE was molecularly cloned and fully sequenced. The element comprises 15,786 bp and encodes a single copy of the organism’s rDNA cistron. The nonribosomal sequence contains five potential open reading frames, two large direct repeat sequences, and numerous smaller repeated-sequence regions., The circular extrachromosomal ribosomal DNA (rDNA) element of Naegleria fowleri strain LEE was molecularly cloned and fully sequenced. The element comprises 15,786 bp and contains a single copy of the organism’s rDNA cistron. The nonribosomal sequence contains five potential open reading frames, two large direct repeat sequences, and numerous smaller repeated-sequence regions.

Published

2020

16. Translation Initiation Control of RNase E-Mediated Decay of Polycistronic gal mRNA

Author

Yonho Lee, Xun Wang, Monford Paul Abishek N, Changjo Kang, Heon M. Lim, Dhruba K. Chattoraj, and Heung Jin Jeon

Subjects

0301 basic medicine, RNase P, RNase E, viruses, Cleavage (embryo), Biochemistry, Genetics and Molecular Biology (miscellaneous), Biochemistry, Ribosome, translation initiation, 03 medical and health sciences, 0302 clinical medicine, Eukaryotic translation, Cistron, mRNA decay, Gene expression, gal operon, Molecular Biosciences, mRNA stability, lcsh:QH301-705.5, Molecular Biology, Original Research, Messenger RNA, Chemistry, Cell biology, 030104 developmental biology, lcsh:Biology (General), polycistronic gal mRNA, 030220 oncology & carcinogenesis

Abstract

In bacteria, mRNA decay is a major mechanism for regulating gene expression. In Escherichia coli, mRNA decay initiates with endonucleolytic cleavage by RNase E. Translating ribosomes impede RNase E cleavage, thus providing stability to mRNA. In transcripts containing multiple cistrons, the translation of each cistron initiates separately. The effect of internal translation initiations on the decay of polycistronic transcripts remains unknown, which we have investigated here using the four-cistron galETKM transcript. We find that RNase E cleaves a few nucleotides (14–36) upstream of the translation initiation site of each cistron, generating decay intermediates galTKM, galKM, and galM mRNA with fewer but full cistrons. Blocking translation initiation reduced stability, particularly of the mutated cistrons and when they were the 5′-most cistrons. This indicates that, together with translation failure, the location of the cistron is important for its elimination. The instability of the 5′-most cistron did not propagate to the downstream cistrons, possibly due to translation initiation there. Cistron elimination from the 5′ end was not always sequential, indicating that RNase E can also directly access a ribosome-free internal cistron. The finding in gal operon of mRNA decay by cistron elimination appears common in E. coli and Salmonella.

Published

2020

17. Temperature Restriction in Entomopathogenic Bacteria

Author

Joseph R. J. Healey, Nicholas R. Waterfield, Geraldine Mulley, and Alexia Hapeshi

Subjects

Microbiology (medical), Operon, Mutant, lcsh:QR1-502, Locus (genetics), Biology, Microbiology, lcsh:Microbiology, 03 medical and health sciences, Cistron, Photorhabdus luminescens, evolution, pathogenicity, Allele, Gene, 030304 developmental biology, Original Research, mutants, Genetics, Whole genome sequencing, 0303 health sciences, 030306 microbiology, biology.organism_classification, temperature restriction, Photorhabdus

Abstract

Temperature plays an important role in bacteria-host interactions and can be a determining factor for host switching. In this study we sought to investigate the reasons behind growth temperature restriction in the entomopathogenic enterobacterium Photorhabdus. Photorhabdus has a complex dual symbiotic and pathogenic life cycle. The genus consists of 19 species but only one subgroup, previously all classed together as P. asymbiotica, have been shown to cause human disease. These clinical isolates necessarily need to be able to grow at 37 °C, whilst the remaining species are largely restricted to growth temperatures below 34 °C and are therefore unable to infect mammalian hosts. Here, we have isolated spontaneous mutant lines of P. laumondii DJC that were able to grow up to 36 °C-37 °C. Following whole genome sequencing of 29 of these mutants we identified a single gene, encoding a protein with a RecG-like helicase domain, that for the majority of isolates contained single nucleotide polymorphisms. Importantly, provision of the wild-type allele of this gene in trans restored the temperature restriction, confirming the mutations are recessive, and the dominant effect of the protein product of this gene. The gene appears to be part of a short three cistron operon, which we have termed the Temperature Restricting Locus (TRL). Transcription reporter strains revealed that this operon is induced upon the switch from 30 °C to 37 °C, leading to replication arrest of the bacteria. TRL is absent from all of the human pathogenic species so far examined, although its presence is not uniform in different strains of the P. luminescens subgroup. In a wider context, the presence of this gene is not limited to Photorhabdus, being found in phylogenetically diverse proteobacteria. We therefore suggest that this system may play a more fundamental role in temperature restriction in diverse species, relating to as yet cryptic aspects of their ecological niches and life cycle requirements.

Published

2020

18. Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia

Author

Huseyin Mehmet, Wajahatullah Khan, Futwan Al-Mohanna, Zainularifeen Abduljaleel, Simon N. Waddington, Michael Themis, Charles Coutelle, Zuhair N. Al-Hassnan, S Apostolidou, Brian W. Bigger, Mohiuddin M. Taher, Mohammad Athar, Abdellatif Bouazzaoui, Mukaddes Colakogullari, Mohammed N. Al-Ahdal, and Faisal A. Al-Allaf

Subjects

0301 basic medicine, lcsh:QH426-470, Base pair, Internal ribosome entry site, Familial hypercholesterolemia, Biochemistry, Article, 03 medical and health sciences, 0302 clinical medicine, Gene therapy, Cistron, IRES, Gene expression, Genetics, Inter-cistronic sequences, Molecular Biology, Gene, Messenger RNA, Chemistry, Biochemistry (medical), Translation (biology), MD simulation, Transfection, Cell biology, lcsh:Genetics, 030104 developmental biology, 030220 oncology & carcinogenesis, Protein structure modeling

Abstract

Internal ribosome entry site (IRES) sequences have become a valuable tool in the construction of gene transfer and therapeutic vectors for multi-cistronic gene expression from a single mRNA transcript. The optimal conditions for effective use of this sequence to construct a functional expression vector are not precisely defined but it is generally assumed that the internal ribosome entry site dependent expression of the second gene in such as cassette is less efficient than the cap-dependent expression of the first gene. Mainly tailoring inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector further in construction of optimised cassette for gene therapy of familial hypercholesterolemia. We tailored the size of the inter-cistronic spacer sequence at the 5′ region of the internal ribosome entry site sequence using sequential deletions and demonstrated that the expression of the 3′ gene can be significantly increased to similar levels as the cap-dependent expression of the 5’ gene. Maximum expression efficiency of the downstream gene was obtained when the spacer is composed of 18–141 base pairs. In this case a single mRNA transcriptional unit containing both the first and the second Cistron was detected. Whilst constructs with spacer sequences of 216 bp or longer generate a single transcriptional unit containing only the first Cistron. This suggests that long spacers may affect transcription termination. When the spacer is 188 bp, both transcripts were produced simultaneously in most transfected cells, while a fraction of them expressed only the first but not the second gene. Expression analyses of vectors containing optimised cassettes clearly confirm that efficiency of gene transfer and biological activity of the expressed transgenic proteins in the transduced cells can be achieved. Furthermore, Computational analysis was carried out by molecular dynamics (MD) simulation to determine the most emerges as viable containing specific binding site and bridging of 5′ and 3′ ends involving direct RNA-RNA contacts and RNA-protein interactions. These results provide a mechanistic basis for translation stimulation and RNA resembling for the synergistic stimulation of cap-dependent translation. Keywords: Internal ribosome entry site, IRES, Gene therapy, Inter-cistronic sequences, MD simulation, Protein structure modeling, Familial hypercholesterolemia

Published

2018

19. Intercistronic expression elements (IEE) from the chloroplast of Chlamydomonas reinhardtii can be used for the expression of foreign genes in synthetic operons

Author

Karla S. Macedo-Osorio, Jesús A. Badillo-Corona, Claudio Garibay-Orijel, Noé V. Durán-Figueroa, Victor Hugo Pérez-España, and Daniel Guzmán-Zapata

Subjects

0106 biological sciences, 0301 basic medicine, Chloroplasts, Operon, Green Fluorescent Proteins, Chlamydomonas reinhardtii, Plant Science, Genes, Plant, 01 natural sciences, Genome, 03 medical and health sciences, Cistron, Gene Expression Regulation, Plant, Genetics, Gene, Kanamycin Kinase, biology, Chlamydomonas, General Medicine, Plants, Genetically Modified, biology.organism_classification, Chloroplast, 030104 developmental biology, Metabolic Engineering, DNA, Intergenic, Genetic Engineering, Agronomy and Crop Science, 010606 plant biology & botany, Transplastomic plant

Abstract

Two intercistronic regions were identified as functional intercistronic expression elements (IEE) for the simultaneous expression of aphA-6 and gfp in a synthetic operon in the chloroplast of C. reinhardtii. Chlamydomonas reinhardtii, a biflagellate photosynthetic microalga, has been widely used in basic and applied science. Already three decades ago, Chlamydomonas had its chloroplast genome transformed and to this day constitutes the only alga routinely used in transplastomic technology. Despite the fact that over a 100 foreign genes have been expressed from the chloroplast genome, little has been done to address the challenge of expressing multiple genes in the form of operons, a development that is needed and crucial to push forward metabolic engineering and synthetic biology in this organism. Here, we studied five intercistronic regions and investigated if they can be used as intercistronic expression elements (IEE) in synthetic operons to drive the expression of foreign genes in the chloroplast of C. reinhardtii. The intercistronic regions were those from the psbB-psbT, psbN-psbH, psaC-petL, petL-trnN and tscA-chlN chloroplast operons, and the foreign genes were the aminoglycoside 3'-phosphotransferase (aphA-6), which confers resistance to kanamycin, and the green fluorescent protein gene (gfp). While all the intercistronic regions yielded lines that were resistant to kanamycin, only two (obtained with intercistronic regions from psbN-psbH and tscA-chlN) were identified as functional IEEs, yielding lines in which the second cistron (gfp) was translated and generated GFP. The IEEs we have identified could be useful for the stacking of genes for metabolic engineering or synthetic biology circuits in the chloroplast of C. reinhardtii.

Published

2018

20. The conserved 3' UTR-derived small RNA NarS mediates mRNA crossregulation during nitrate respiration

Author

Jörg Vogel, Yanjie Chao, Gianluca Matera, Qian Gao, Chuan Wang, and HIRI, Helmholtz-Institut für RNA-basierte Infektionsforschung, Josef-Shneider Strasse 2, 97080 Würzburg, Germany.

Subjects

Untranslated region, Small RNA, Operon, RNase P, RNA Stability, Anion Transport Proteins, Biology, Host Factor 1 Protein, Cistron, Endoribonucleases, Genetics, RNA and RNA-protein complexes, Escherichia coli, RNA, Messenger, RNA Processing, Post-Transcriptional, 3' Untranslated Regions, Messenger RNA, Nitrates, Escherichia coli Proteins, Respiration, RNA, RNA-Binding Proteins, Salmonella enterica, Nitrate Transporters, Gene Expression Regulation, Bacterial, Methyltransferases, Cell biology, Transfer RNA, RNA, Small Untranslated

Abstract

Small noncoding RNAs (sRNAs) from mRNA 3′ UTRs seem to present a previously unrecognized layer of bacterial post-transcriptional control whereby mRNAs influence each other's expression, independently of transcriptional control. Studies in Escherichia coli and Salmonella enterica showed that such sRNAs are natural products of RNase E-mediated mRNA decay and associate with major RNA-binding proteins (RBPs) such as Hfq and ProQ. If so, there must be additional sRNAs from mRNAs that accumulate only under specific physiological conditions. We test this prediction by characterizing candidate NarS that represents the 3′ UTR of nitrate transporter NarK whose gene is silent during standard aerobic growth. We find that NarS acts by Hfq-dependent base pairing to repress the synthesis of the nitrite transporter, NirC, resulting in mRNA cross-regulation of nitrate and nitrite transporter genes. Interestingly, the NarS-mediated repression selectively targets the nirC cistron of the long nirBDC-cysG operon, an observation that we rationalize as a mechanism to protect the bacterial cytoplasm from excessive nitrite toxicity during anaerobic respiration with abundant nitrate. Our successful functional assignment of a 3′ UTR sRNA from a non-standard growth condition supports the notion that mRNA crossregulation is more pervasive than currently appreciated.

Published

2019

21. Innovative RNAi Strategies and Tactics to Tackle Plum Pox Virus (PPV) Genome in Prunus domestica-Plum

Author

Ralph Scorza, Pascal Briard, Michel Ravelonandro, Biologie du fruit et pathologie (BFP), Université Sciences et Technologies - Bordeaux 1-Université Bordeaux Segalen - Bordeaux 2-Institut National de la Recherche Agronomique (INRA), USDA-ARS : Agricultural Research Service, and Ravelonandro, Michel

Subjects

0106 biological sciences, 0301 basic medicine, Phytopathology and phytopharmacy, Virologie, Context (language use), Plant Science, Biology, 01 natural sciences, Genome, resistance, 03 medical and health sciences, Prunus, recovery, Cistron, RNA interference, Virology, santé des plantes, Plant virus, Prunus domestica, RNAi, plum pox virus stability, silencing, pathologie végétale, Gene, Ecology, Evolution, Behavior and Systematics, Genetics, virus phytopathogène, Ecology, Phytopathologie et phytopharmacie, Phenotype, [SDV.BV.PEP]Life Sciences [q-bio]/Vegetal Biology/Phytopathology and phytopharmacy, arbre fruitier à noyau, 030104 developmental biology, [SDV.MP.VIR]Life Sciences [q-bio]/Microbiology and Parasitology/Virology, fruit à noyau, 010606 plant biology & botany

Abstract

UMR BFP - Equipe Virologie; International audience; We developed an innovative RNAi concept based on two gene constructs built from the capsid gene (CP) cistron of the Plum pox virus (PPV) genome. First, designated as amiCPRNA, a potential molecule interfering with PPV genome translation and the second one is the ami-siCPRNA to target viral genome translation and PPV RNA replication. Following the previous engineering of these constructs in an experimental herbaceous host, they were introduced into Prunus domestica (plum tree) genome. Previously propagated onto a susceptible rootstock, these clones were graft-inoculated with PPV. After four dormancy cycles, and consistent with our experience of PPV infection, some clones showed a common phenomenon of silencing that can differ between the detailed plant phenotypes. Three different phenotypes were developed by the amisiCPRNA clones. First, the high resistance character shown by the amisiCPRNA plum-7 that was similar to the resistance expressed by HoneySweet plum. Secondly, a recovery reaction was developed by the two other amisiCPRNA plum-3 and plum-4 that differed from the rest, characterized as susceptible clones, among these were the amiCPRNA plums. Having assessed the behavior of these plums versus the herbaceous host accumulating the similar form of RNAi: ami-, si-, and ami-siRNA, challenging assays in perennials consistently reflect the natural context of viral genome targeting

Published

2019

22. Conditional effects of the epigenetic regulator JUMONJI 14 in Arabidopsis root growth

Author

Petra Marhava, Pietro Cattaneo, Moritz Graeff, and Christian S. Hardtke

Subjects

0106 biological sciences, 0303 health sciences, Mutation, biology, Mutant, food and beverages, Meristem, biology.organism_classification, medicine.disease_cause, 01 natural sciences, Cell biology, 03 medical and health sciences, Histone, Cistron, Arabidopsis, medicine, biology.protein, Arabidopsis thaliana, Epigenetics, Molecular Biology, 030304 developmental biology, 010606 plant biology & botany, Developmental Biology

Abstract

Methylation of lysine 4 in histone 3 (H3K4) is a post-translational modification that promotes gene expression. H3K4 methylation can be reversed by specific demethylases with an enzymatic Jumonji C domain. In Arabidopsis thaliana, H3K4-specific JUMONJI (JMJ) proteins distinguish themselves by the association with an F/Y-rich (FYR) domain. Here, we report that jmj14 mutations partially suppress reduced root meristem size and growth vigor of brevis radix (brx) mutants. Similar to its close homologs, JMJ15, JMJ16 and JMJ18, the JMJ14 promoter confers expression in mature root vasculature. Yet, unlike jmj14, neither jmj16 nor jmj18 mutation markedly suppresses brx phenotypes. Domain-swapping experiments suggest that the specificity of JMJ14 function resides in the FYR domain. Despite JMJ14 promoter activity in the mature vasculature, jmj14 mutation affects root meristem size. However, JMJ14 protein is observed throughout the meristem, suggesting that the JMJ14 transcript region contributes substantially to the spatial aspect of JMJ14 expression. In summary, our data reveal a role for JMJ14 in root growth in sensitized genetic backgrounds that depends on its FYR domain and regulatory input from the JMJ14 cistron.

Published

2019

23. Translation of dipeptide repeat proteins from the C9ORF72 expanded repeat is associated with cellular stress

Author

Elaine Fuchs, Yoshifumi Sonobe, Raymond P. Roos, Katsuhisa Masaki, Ataman Sendoel, and Ghanashyam D. Ghadge

Subjects

0301 basic medicine, Unconventional translation, Kozak consensus sequence, Repeat associated non-AUG (RAN) translation, Reading frame, C9ORF72, Hexanucleotide repeat expansions (HREs), Chick Embryo, Biology, Dipeptide protein repeats (DPRs), Article, lcsh:RC321-571, 03 medical and health sciences, Mice, Eukaryotic translation, Cistron, C9orf72, Integrated stress response, Animals, Humans, lcsh:Neurosciences. Biological psychiatry. Neuropsychiatry, Genetics, Mice, Knockout, C9orf72 Protein, Cell Death, Translation (biology), Dipeptides, Internal ribosome entry site (IRES), Antisense RNA, 030104 developmental biology, HEK293 Cells, Neurology, Protein Biosynthesis

Abstract

Expansion of a hexanucleotide repeat (HRE), GGGGCC, in the C9ORF72 gene is recognized as the most common cause of familial amyotrophic lateral sclerosis (FALS), frontotemporal dementia (FTD) and ALS-FTD, as well as 5–10% of sporadic ALS. Despite the location of the HRE in the non-coding region (with respect to the main C9ORF72 gene product), dipeptide repeat proteins (DPRs) that are thought to be toxic are translated from the HRE in all three reading frames from both the sense and antisense transcript. Here, we identified a CUG that has a good Kozak consensus sequence as the translation initiation codon. Mutation of this CTG significantly suppressed polyglycine-alanine (GA) translation. GA was translated when the G(4)C(2) construct was placed as the second cistron in a bicistronic construct. CRISPR/Cas9-induced knockout of a non-canonical translation initiation factor, eIF2A, impaired GA translation. Transfection of G(4)C(2) constructs induced an integrated stress response (ISR), while triggering the ISR led to a continuation of translation of GA with a decline in conventional cap-dependent translation. These in vitro observations were confirmed in chick embryo neural cells. The findings suggest that DPRs translated from an HRE in C9ORF72 aggregate and lead to an ISR that then leads to continuing DPR production and aggregation, thereby creating a continuing pathogenic cycle.

Published

2018

24. Development of bicistronic expression system for the enhanced and reliable production of recombinant proteins in Leuconostoc citreum

Author

Ki Jun Jeong, Seung Hoon Jang, Nam Soo Han, and Ji Won Cha

Subjects

0301 basic medicine, Signal peptide, animal structures, 030106 microbiology, Green Fluorescent Proteins, lcsh:Medicine, medicine.disease_cause, law.invention, Green fluorescent protein, 03 medical and health sciences, Cistron, Leuconostoc citreum, law, Gene expression, medicine, lcsh:Science, Escherichia coli, Glutathione Transferase, Multidisciplinary, biology, Chemistry, Human Growth Hormone, Lactococcus lactis, lcsh:R, biology.organism_classification, Recombinant Proteins, Biochemistry, Recombinant DNA, lcsh:Q, alpha-Amylases, Leuconostoc

Abstract

The lactic acid bacteria (LAB) Leuconostoc citreum are non-sporulating hetero-fermentative bacteria that play an important role in the fermented food industry. In this study, for the enhanced and reliable production of recombinant proteins in L. citreum, we developed a bicistronic design (BCD) expression system which includes a short leader peptide (1st cistron) followed by target genes (2nd cistron) under the control of a single promoter. Using superfolder green fluorescent protein (sfGFP) as a reporter, the functionality of BCD in L. citreum was verified. Further, to improve the expression in BCD, we tried to engineer a Shine-Dalgarno sequence (SD2) for the 2nd cistron and a promoter by FACS screening of random libraries, and both strong SD2 (eSD2) and promoter (P710V4) were successfully isolated. The usefulness of the engineered BCD with P710V4 and eSD2 was further validated using three model proteins—glutathione-s-transferase, human growth hormone, and α-amylase. All examined proteins were successfully produced with levels highly increased compared with those in the original BCD as well as the monocistronic design (MCD) expression system.

Published

2018

25. Soybean mosaic virus: a successful potyvirus with a wide distribution but restricted natural host range

Author

M. R. Hajimorad, Sue A. Tolin, Steven A. Whitham, M. A. Saghai Maroof, and Leslie L. Domier

Subjects

0106 biological sciences, 0301 basic medicine, Genetics, biology, Potyviridae, Potyvirus, food and beverages, Soil Science, Soybean mosaic virus, RNA, Plant Science, biology.organism_classification, 01 natural sciences, 03 medical and health sciences, Open reading frame, Pathosystem, 030104 developmental biology, Cistron, Botany, Agronomy and Crop Science, Molecular Biology, Gene, 010606 plant biology & botany

Abstract

SUMMARY Taxonomy. Soybean mosaic virus (SMV) is a species within the genus Potyvirus, family Potyviridae that includes almost a quarter of all known plant RNA viruses affecting agriculturally important plants. The Potyvirus genus is the largest of all genera of plant RNA viruses with 160 species. Particle. The filamentous particles of SMV, typical of potyviruses, are about 7,500 A long and 120 A in diameter with a central hole of about 15 A in diameter. Coat protein residues are arranged in helice of about 34 A pitch having slightly less than 9 subunits per turn. Genome. The SMV genome consists of a single-stranded positive-sense polyadenylated RNA of approximately 9.6 kb with a virus-encoded protein (VPg) linked at the 5' terminus. The genomic RNA contains a single large open reading frame (ORF). The polypeptide produced from the large ORF is processed proteolytically by three viral-encoded proteinases to yield about 10 functional proteins. A small ORF, partially overlapping the P3 cistron, pipo, is encoded as a fusion protein in the N-terminus of P3 (P3N+PIPO). Biological properties. SMV's host range is restricted mostly to two plant species of a single genus; Glycine max (cultivated soybean) and G. soja (wild soybean). SMV is transmitted by aphids non-persistently and by seeds. Variability of SMV is recognized by reactions on cultivars with dominant resistance (R) genes. Recessive resistance genes are not known. Geographical distribution and economic importance. As a consequence of its seed transmissibility, SMV is present in all soybean growing areas of the world. SMV infections can reduce significantly seed quantity and quality (e.g., mottled seed coats, reduced seed size and viability, and altered chemical composition). Control. The most effective means of managing losses from SMV are planting virus-free seeds and cultivars containing single or multiple R genes. Key attractions. The interactions of SMV with soybean genotypes containing different dominant R genes and understanding functional role(s) of SMV-encoded proteins in virulence, transmission and pathogenicity have been intensively investigated. The SMV-soybean pathosystem has become an excellent model for examining the genetics and genomics of uniquely complex gene-for-gene resistance model in a crop of worldwide importance. This article is protected by copyright. All rights reserved.

Published

2018

26. Cistron

Author

Gargaud, Muriel, editor, Amils, Ricardo, editor, Quintanilla, José Cernicharo, editor, Cleaves, Henderson James (Jim), II, editor, Irvine, William M., editor, Pinti, Daniele L., editor, and Viso, Michel, editor

Published

2011

27. Cistron

Author

Gooch, Jan W. and Gooch, Jan W., editor

Published

2011

28. Cistron

Author

Rédei, George P.

Published

2008

29. Looking back to the future: From the development of the gene concept to toxicogenomics.

Author

Choudhuri, Supratim

Subjects

*TOXICOGENOMICS, *GENES, *GENOMES, *GENOMICS, *PHARMACOGENOMICS, *MOLECULAR biology

Abstract

Initial progress in the science of ‘genetics’ in the first half of the 20th century was mainly driven by studies utilizing mutations and consequent changes in phenotype. The structural and functional nature of the gene was far from being understood. That state of understanding started changing from the 1940s. In the following decades, with the discovery of the double helix followed by the discoveries on gene structure and expression, there was a period when the structural and functional aspects of the gene could be conceived in terms of one entity, the cistron. However, the discovery of intervening sequences caused this unified concept to fall apart, making the gene concept a subject of philosophical debate again. Meanwhile, over time, technological progress in molecular biology had the field forge ahead rapidly, ultimately leading to the sequencing of the human genome and genomes of other species, and giving birth to the science of genomics. Developments in genomics have given rise to certain applied sub-disciplines like pharmacogenomics and toxicogenomics. While the full potential of pharmaco- and toxicogenomics is yet to be harnessed, they nevertheless have had an impact in drug development and safety assessment, such that the future promise of genomics seems achievable. At present, it is a good opportunity to revisit the path from the development of the initial gene concept and the philosophical debate surrounding the meaning of the term ‘gene’ to the current state of understanding of genes and genomes and their role in health and disease. [ABSTRACT FROM AUTHOR]

Published

2009

30. Termination codon-dependent translation of partially overlapping ndhC-ndhK transcripts in chloroplasts.

Author

Yukawa, Maki and Suguira, Masahiro

Subjects

*NAD(P)H dehydrogenases, *CHLOROPLASTS, *PLANT mitochondria, *CHLOROPLAST DNA, *MESSENGER RNA, *GENETIC translation, *TOBACCO, *STOICHIOMETRY

Abstract

The chloroplast NAD(P)H dehydrogenase complex, a homologue of mitochondrial complex I, consists of >15 subunits, of which 11 are encoded by the chloroplast genome (ndhA-K). The ndhC and ndhK genes are partially overlapped and cotranscribed in many land plants. The downstream ndhK mRNA possesses 4 possible AUG initiation codons in many dicot plants. By using an efficient in vitro translation system from tobacco chloroplasts, we defined that the major initiation site of tobacco ndhK mRNA5 is the third AUG that is located 4 nt upstream from the ndhCstop codon. Mutation of the ndhC stop codon (UAG) arrested translation of the ndhK cistron. Frameshift of the ndhC coding strand inhibited also translation of the distal cistron. The results indicated that ndhK translation depends on termination of the preceding cistron, namely transla- tional coupling. Surprisingly, removal of the ndhC 5'-UTR and its AUG still supported substantial translation of the ndhK cistron. This translation was abolished again by removing the ndhC stop codon. Although translation of the downstream cistron of an overlapping mRNA is generally very low, we found that the ndhCIK mRNA produces NdhK and NdhC in similar amounts. Based on subunit compositions of the bacterial complex I, the stoichiometry of NdhK and NdhC is suggested to be 1:1 in chloroplasts. To meet this stoichiometry, the ndhC/K mRNA is translated not only by a translational coupling event but also by a termination codon- dependent pathway. [ABSTRACT FROM AUTHOR]

Published

2008

31. The Cistron Systematic Model of Corporate Gene and Its Application in Corporate Transformation.

Author

Xu Xiaoming and Dai Jianhua

Abstract

Through summarizing the evolution of corporate gene theory,the paper finds out that in the current research full attention has not yet been paid to the significance of the dividable feature of gene. Then, by using the cistron theory of gene, we build a new cistron systematic model of corporate gene, which is a three-level systematic structure including an internal fine structure of corporate gene (i. e. the belief-awareness base pair controlling corporate spirit and the resource-capacity base pair controlling the corporate body), a corporate routine as a corporate gene itself, and corporate values explicit mechanism as a corporate genetic carrier. The completion and systematization of the said systematic structure offer obvious instructive meaning to the process of firm growth and transformation. The application of the model in corporate transformation involves the cistron genetic systematic model of corporate transformation based on the cistron systematic model of corporate gene and the cistron genetic strategy and operation in two major forms of corporate transformation. In this way of application, we demonstrate the practical significance and theoretical value of the new cistron systematic model of corporate gene. [ABSTRACT FROM AUTHOR]

Published

2008

32. An analysis of the effect of the internal ribosome entry site of the encephalomyocarditis virus on the expression of the second gene in the bicistronic matrix in neurons of primary hippocampal cultures

Author

Pavel M. Balaban, Mikhail A. Ostrovsky, A. Yu. Malyshev, Lada E. Petrovskaya, and V. S. Shtefanyuk

Subjects

0301 basic medicine, Expression vector, fungi, Mutant, Translation (biology), Biology, Biochemistry, Cell biology, 03 medical and health sciences, Cellular and Molecular Neuroscience, Internal ribosome entry site, 030104 developmental biology, 0302 clinical medicine, Plasmid, Cistron, mCherry, Molecular Biology, Gene, 030217 neurology & neurosurgery

Abstract

Molecular biological experiments sometimes require expression of two or more genes in a single cell with an accurate ratio between their expression levels. One of the methods to provide this control is the use of the internal ribosome entry site (IRES) from the encephalomyocarditis virus as a separating insert between two target genes in the expression vector. Previously, it was shown that the efficacy of translation of the gene after IRES varies considerably in a range from 6 to 100% depending on the cell type. In neurons, the exact ratio between the expression levels of genes that are located before and after the IRES in the expression vector is unknown. Here, we analyzed the ratio between the amounts of products of the first and second genes located before and after the IRES in a plasmid that was used to transfect neurons in a primary hippocampal culture. We created two plasmid vectors that contain genes of the yellow (Venus) and red (mCherry) fluorescent proteins in different orders, which are separated by the IRES. We found that the unmodified IRES sequence of the encephalomyocarditis virus decreases the expression in the second cistron by a factor of 2.7 in a primary culture of hippocampal neurons. These data will help us to use currently available libraries of mutant IRES sequences for accurate control of the relationships between the expression of different target genes in neurons.

Published

2017

33. A bicistronic vector with destabilized mRNA secondary structure yields scalable higher titer expression of human neurturin in E. coli

Author

Varnika Roy, Mark Berge, Srilatha Kuntumalla, Robert G. Roth, Albert E. Schmelzer, Rajesh Chitta, Ron Schoner, and Sucheta Vajrala

Subjects

0301 basic medicine, Messenger RNA, 030102 biochemistry & molecular biology, Neurturin, Cystine knot, Bioengineering, Biology, Applied Microbiology and Biotechnology, Ribosome, Molecular biology, 03 medical and health sciences, 030104 developmental biology, Eukaryotic translation, Cistron, Coding region, Protein secondary structure, Biotechnology

Abstract

Human neurturin (NTN) is a cystine knot growth factor with potential therapeutic use in diseases such as Parkinson's and diabetes. Scalable high titer production of native NTN is particularly challenging because of the cystine knot structure which consists of an embedded ring comprised of at least three disulfide bonds. We sought to pursue enhanced scalable production of NTN in Escherichia coli. Our initial efforts focused on codon optimization of the first two codons following AUG but these studies resulted in only a marginal increase in NTN expression. Therefore, we pursued an alternative strategy of using a bicistronic vector for NTN expression designed to reduce mRNA secondary structure to achieve increased ribosome binding and re-initiation. The first cistron was designed to prevent sequestration of the translation initiation region in a secondary conformation. The second cistron, which contained the NTN coding sequence itself, was engineered to disrupt double bonded base pairs and destabilize the secondary structure for ribosome re-initiation. The ensemble approach of reducing NTN's mRNA secondary structure and using the bicistronic vector had an additive effect resulting in significantly increased NTN expression. Our stain selection studies were conducted in a miniaturized bioreactor. An optimized strain was selected and scaled up to a 100 liter fermentor which yielded an inclusion body titer of 2 g/L. The inclusion bodies were refolded to yield active NTN. We believe that our strategy is applicable to other candidate proteins that are difficult-to-express due to stable mRNA secondary structures. This article is protected by copyright. All rights reserved

Published

2017

34. Functional replacement of Wheat streak mosaic virus HC-Pro with the corresponding cistron from a diverse array of viruses in the family Potyviridae

Author

Stenger, Drake C. and French, Roy

Subjects

*WHEATGRASSES, *WHEAT, *TURNIP mosaic virus, *VIRUSES

Abstract

Helper component-proteinase (HC-Pro) of Wheat streak mosaic virus strain Sidney 81 (WSMV-Sidney 81) was systematically replaced with the corresponding cistron derived from four strains of WSMV (Type, TK1, CZ, and El Batán 3), the tritimovirus Oat necrotic mottle virus (ONMV), the rymoviruses Agropyron mosaic virus (AgMV) and Hordeum mosaic virus (HoMV), or the potyviruses Tobacco etch virus (TEV) and Turnip mosaic virus (TuMV). These HC-Pro proteins varied in amino acid sequence identity shared with HC-Pro of WSMV-Sidney 81 from high (strains of WSMV at ∼86–99%) to moderate (ONMV at 70%) to low (rymoviruses and potyviruses at ∼15–17%). Surprisingly, all chimeric viral genomes examined were capable of systemic infection of wheat upon inoculation with RNA transcripts produced in vitro. HC-Pro replacements derived from tritimoviruses did not alter host range relative to WSMV-Sidney 81, as each of these chimeric viruses was able to systemically infect wheat, oat, and corn line SDp2. These results indicate that differences in host range among tritimoviruses, including the inability of ONMV to infect wheat or the inability of WSMV strains Type and El Batán 3 to infect SDp2 corn, are not determined by HC-Pro. In contrast, all chimeric viruses bearing HC-Pro replacements derived from rymoviruses or potyviruses were unable to infect SDp2 corn and oat. Collectively, these results indicate that HC-Pro from distantly related virus species of the family Potyviridae are competent to provide WSMV-Sidney 81 with all functions necessary for infection of a permissive host (wheat) and that virus–host interactions required for systemic infection of oat and SDp2 corn are more stringent. Changes in symptom severity or mechanical transmission efficiency observed for some chimeric viruses further suggest that HC-Pro affects virulence in WSMV. [Copyright &y& Elsevier]

Published

2004

35. Cistron

Published

2006

36. Use of Potyvirus Vectors to Produce Carotenoids in Plants

Author

José-Antonio Daròs

Subjects

0106 biological sciences, 0301 basic medicine, Genetics, Expression vector, biology, Tobacco etch virus, viruses, fungi, Potyvirus, food and beverages, Nicotiana benthamiana, Agrobacterium tumefaciens, biology.organism_classification, Recombinant virus, 01 natural sciences, Viral vector, 03 medical and health sciences, 030104 developmental biology, Cistron, 010606 plant biology & botany

Abstract

Potyviruses are plus-strand RNA viruses that can be easily transformed into expression vectors to quickly express one carotenogenic enzyme or transcription factor, or more, in plant tissues. Unlike the technically challenging and time-consuming process of plant transformation, manipulation of a roughly 10,000 nt-long viral genome is rather straightforward via common molecular biology techniques. Here I describe how to insert the cDNAs of the proteins of interest into two particular positions of the cDNA of a Tobacco etch virus (TEV) mutant that lacks the viral NIb cistron and only infects the plants in which this protein is expressed. This deletion increases the space to harbor foreign sequences. The selection of the expression site must be made according to subcellular localization requirements. The recombinant virus is then inoculated into Nicotiana benthamiana plants by means of Agrobacterium tumefaciens. The expression of the viral genome entails the production of carotenogenic proteins in the plant tissues with a consequent effect on the plant carotenoid pathway.

Published

2019

37. Lost in Translation: population genomics and long-read sequencing reveals relaxation of concerted evolution of the ribosomal DNA cistron

Author

Laura M. Suz, Bryn T. M. Dentinger, and Keaton Tremble

Subjects

0106 biological sciences, 0301 basic medicine, Locus (genetics), Biology, DNA, Ribosomal, 010603 evolutionary biology, 01 natural sciences, DNA barcoding, Evolution, Molecular, Population genomics, 03 medical and health sciences, Gene Frequency, Cistron, Phylogenetics, DNA, Ribosomal Spacer, Genetics, Gene conversion, Molecular Biology, Gene, Ribosomal DNA, Phylogeny, Ecology, Evolution, Behavior and Systematics, Likelihood Functions, Concerted evolution, Genetic Variation, Genomics, Sequence Analysis, DNA, Nanopore Sequencing, Genetics, Population, 030104 developmental biology, Haplotypes, Genetic Loci, Evolutionary biology, Metagenomics, Genome, Fungal, Agaricales

Abstract

Concerted evolution of the ribosomal DNA array has been studied in numerous eukaryotic taxa, yet is still poorly understood. rDNA genes are repeated dozens to hundreds of times in the eukaryotic genome (Eickbush and Eickbush, 2007) and it is believed that these arrays are homogenized through concerted evolution (Zimmer et al., 1980; Dover, 1993) preventing the accumulation of intragenomic, and intraspecific, variation. However, numerous studies have reported rampant intragenomic and intraspecific variation in the rDNA array (Ganley and Kobayashi, 2011; Naidoo et al., 2013; Hughes and Petersen, 2001; Lindner and Banik, 2011; Li et al., 2013; Lindner et al., 2013; Hughes et al., 2018), contradicting our current understanding of concerted evolution. The internal transcribed spacers (ITS) of the rDNA cistron are the most commonly used DNA barcoding region in Fungi (Schoch et al., 2012), and rely on concerted evolution to homogenize the rDNA array leading to a "barcode gap" (Puillandre et al., 2012). Here we show that in Boletus edulis Bull., ITS intragenomic variation persists at low allele frequencies throughout the rDNA array, this variation does not correlate with genomic relatedness between populations, and rDNA genes may not evolve in a strictly concerted fashion despite the presence of unequal recombination and gene conversion. Under normal assumptions, heterozygous positions found in ITS sequences represent hybridization between populations, yet through allelic mapping of the rDNA array we found numerous heterozygous alleles to be stochastically introgressed throughout, presenting a dishonest signal of gene flow. Moreover, despite the signal of gene flow in ITS, our organisms were highly inbred, indicating a disconnect between true gene flow and barcoding signals. In addition, we show that while the mechanisms of concerted evolution are ongoing in pseudo-heterozygous individuals, they are not fully homogenizing the ITS array. Concerted evolution of the rDNA array may insufficiently homogenize the ITS gene, allowing for misleading signals of gene flow to persist, vastly complicating the use of the ITS locus for DNA barcoding in Fungi.

Published

2019

38. Immunization of rabbits with recombinant Clostridium perfringens alpha toxins CPA-C and CTB-CPA-C in a bicistronic design expression system confers strong protection against challenge

Author

Jiang Yuwen, Lifang Feng, Lingying Dong, Peng Xiaobing, Li Xuni, and Peng Guorui

Subjects

0106 biological sciences, Cholera Toxin, Clostridium perfringens, Bacterial Toxins, Clostridium perfringens alpha toxin, medicine.disease_cause, 01 natural sciences, law.invention, Microbiology, 03 medical and health sciences, Mice, Cistron, law, 010608 biotechnology, medicine, Escherichia coli, Animals, heterocyclic compounds, Cloning, Molecular, 030304 developmental biology, 0303 health sciences, Chemistry, Lethal dose, Cholera toxin, Calcium-Binding Proteins, Vaccination, Toxoid, Antibody titer, Antibodies, Bacterial, Recombinant Proteins, Type C Phospholipases, Bacterial Vaccines, cardiovascular system, Recombinant DNA, Rabbits, Biotechnology

Abstract

The Clostridium perfringens alpha toxin (CPA), encoded by the plc gene, is the causative pathogen of gas gangrene, which is a lethal infection. In this study, we used an E. coli system for the efficient production of recombinant proteins and developed a bicistronic design (BCD) expression construct consisting of two copies of the C-terminal (247–370) domain of the alpha toxin (CPA-C) in the first cistron, followed by Cholera Toxin B (CTB) linked with another two copies of CPA-C in the second cistron that is controlled by a single promoter. Rabbits were immunized twice with purified proteins (rCPA-C rCTB-CPA-C) produced in the BCD expression system, with an inactivated recombinant E. coli vaccine (RE), C. perfringens formaldehyde-inactivated alpha toxoid (FA-CPA) and C. perfringens l -lysine/formaldehyde alpha toxoid (LF-CPA) vaccines. Following the second vaccination, 0.1 mL of pooled sera of the RE-vaccinated rabbits could neutralize 12× mouse LD100 (100% lethal dose) of CPA, while that of the rCPA-C rCTB-CPA-C-vaccinated rabbits could neutralize 6× mouse LD100 of CPA. Antibody titers against CPA were also assessed by ELISA, reaching titers as high as 1:2048000 in the RE group; this was significantly higher compared to the C. perfringens alpha toxoid vaccinated groups (FA-CPA and LF-CPA). Rabbits from all vaccinated groups were completely protected from a 2× rabbit LD100 of CPA challenge. These results demonstrate that the recombinant proteins are able to induce a strong immune responses, indicating that they may be potentially utilized as targets for novel vaccines specifically against the C. perfringens alpha toxin.

Published

2019

39. How dynamic could be the 45S rDNA cistron? An intriguing variability in a grasshopper species revealed by integration of chromosomal and genomic data

Author

Cesar Martins, Francisco J. Ruiz-Ruano, Erica Ramos, Vilma Loreto, Dardo Andrea Marti, Diogo Cavalcanti Cabral-de-Mello, Ana B. S. M. Ferretti, Diogo Milani, Universidade Estadual Paulista (Unesp), Facultad de Ciencias, Evolutionary Biology Centre, Universidade Federal de Pernambuco (UFPE), and IBS - UNaM - CONICET

Subjects

Transposable element, Male, viruses, Pseudogene, Genome, Insect, rDNA, Grasshoppers, DNA, Ribosomal, Ciencias Biológicas, 03 medical and health sciences, Genética y Herencia, 0302 clinical medicine, Cistron, FISH, Genetics, Animals, Silver impregnation, Ectopic recombination, Abracris flavolineata, Evolutionary dynamics, Grasshopper, Genetics (clinical), 030304 developmental biology, 0303 health sciences, biology, biology.organism_classification, Chromosomes, Insect, Evolutionary biology, RNA, Ribosomal, %22">Fish , Multigene family, Developmental biology, 030217 neurology & neurosurgery, CIENCIAS NATURALES Y EXACTAS

Abstract

To better understand the structure and variability of the 45S rDNA cistron and its evolutionary dynamics in grasshoppers, we performed a detailed analysis combining classical and molecular cytogenetic data with whole-genome sequencing in Abracris flavolienata, which shows extraordinary variability in the chromosomal distribution for this element. We found astonishing variability in the number and size of rDNA clusters at intra- and inter-population levels. Interestingly, FISH using distinct parts of 45S rDNA cistron (18S rDNA, 28S rDNA, and ITS1) as probes revealed a distinct number of clusters, suggesting independent mobility and amplification of the 45S rDNA components. This hypothesis is consistent with the higher genomic coverage of almost the entire cistron of 45S rDNA observed in A. flavolineata compared to other grasshoppers, besides coverage variability along the 45S rDNA cistron in the species. In addition, these differences in coverage for distinct components of the 45S rDNA cistron indicate emergence of pseudogenes evidenced by existence of truncated sequences, demonstrating the rDNA dynamics in the species. Although the chromosomal distribution of 18S rDNA was highly variable, the chromosomes 1, 3, 6, and 9 harbored rDNA clusters in all individuals with the occurrence of NOR activity in pair 9, suggesting ancestry or selective pressures to prevent pseudogenization of rDNA sequences in this chromosome pair. Additionally, small NORs and cryptic rDNA loci were observed. Finally, there was no evidence of enrichment and association of transposable elements, at least, inside or nearby rDNA cistron. These findings broaden our knowledge of rDNA dynamics, revealing an independent movement and amplification of segments of 45S rDNA cistron, which in A. flavolineata could be attributed to ectopic recombination. Fil: Ferretti, Ana B. S. M.. Universidade Estadual Paulista Julio de Mesquita Filho. Faculdade de Engenharia.; Brasil Fil: Ruiz Ruano, Francisco J.. Uppsala University; Suecia. Universidad de Granada; España Fil: Milani, Diogo. Universidade Estadual Paulista Julio de Mesquita Filho. Faculdade de Engenharia.; Brasil Fil: Loreto, Vilma. Universidade Federal de Pernambuco; Brasil Fil: Marti, Dardo Andrea. Consejo Nacional de Investigaciones Científicas y Técnicas. Centro Científico Tecnológico Conicet - Nordeste. Instituto de Biología Subtropical. Instituto de Biología Subtropical - Nodo Posadas | Universidad Nacional de Misiones. Instituto de Biología Subtropical. Instituto de Biología Subtropical - Nodo Posadas; Argentina Fil: Ramos, Érica Daniela. Universidade Estadual Paulista Julio de Mesquita Filho; Brasil Fil: Martins, Cesar. Universidade Estadual Paulista Julio de Mesquita Filho; Brasil Fil: Cabral de Mello, Diogo C.. Universidade Estadual Paulista Julio de Mesquita Filho; Brasil

Published

2019

40. High-efficiency expression and secretion of human FGF21 in Bacillus subtilis by intercalation of a mini-cistron cassette and combinatorial optimization of cell regulatory components

Author

Zhaoxia Jin, Dawei Zhang, Dandan Li, Gang Fu, and Ran Tu

Subjects

Signal peptide, 0106 biological sciences, Proteases, lcsh:QR1-502, Heterologous, Bioengineering, Chaperone, Bacillus subtilis, Protein Sorting Signals, 01 natural sciences, Applied Microbiology and Biotechnology, lcsh:Microbiology, Heterologous protein expression, 03 medical and health sciences, FGF21, Cistron, 010608 biotechnology, Humans, Mini-cistron, Secretion, Codon, Promoter Regions, Genetic, 0303 health sciences, Expression vector, biology, 030306 microbiology, Chemistry, Research, biology.organism_classification, Recombinant Proteins, Fibroblast Growth Factors, Biochemistry, Chaperone (protein), Fermentation, biology.protein, Molecular Chaperones, Biotechnology

Abstract

Background Recombinant human Fibroblast growth factor 21 (rhFGF21) is an endocrine hormone that has profound effects on treatment of metabolic diseases. However, rhFGF21 is prone to form inclusion body when expressed in bacteria, which results in, the downstream process of purification of bioactive rhFGF21 is time-consuming and labor intensive. The aim of this work is to explore a new method for improving the soluble expression and secretion level of rhFGF21 in B. subtilis. Results A codon optimized rhFGF21 gene was expressed under the control of a strong inducible promoter PmalA in B. subtilis. A mini-cistron cassette (from gsiB) was located upstream of rhFGF21 in expression vector (pMATEFc5), which could reduce the locally stabilized mRNA secondary structure of transcripts and enhance the efficiency of translation initiation. Then various chaperones were further overexpressed to improve the expression efficiency of rhFGF21. Results showed that overexpression of the chaperone DnaK contributed to the increase of solubility of rhFGF21. Moreover, an extracellular proteases deficient strain B. subtilis Kno6cf was used to accumulate the secreted rhFGF21 solidly. In addition, eleven signal peptides from B. subtilis were evaluated and the SPdacB appeared the highest secretion yield of rhFGF21 in B. subtilis. Finally, the combinatorial optimized strain achieved an about ninefold increase of the soluble rhFGF21 production after 24 h of flask fermentation in comparison with the initial production strain. Conclusion This work provided a comprehensive strategy for secretory expressing the heterologous protein rhFGF21 in B. subtilis. To our knowledge, this is the first report of the highly efficient production of rhFGF21 in B. subtilis and this approach may provide some suggestions for heterologous proteins production in B. subtilis. Electronic supplementary material The online version of this article (10.1186/s12934-019-1066-4) contains supplementary material, which is available to authorized users.

Published

2019

41. Characterization of a soybean mosaic virus variant causing different diseases in Glycine max and Nicotiana benthamiana

Author

Daolong Dou, Hua Jiang, Jun-Yi Gai, and Kai Li

Subjects

0106 biological sciences, 0301 basic medicine, Untranslated region, food.ingredient, viruses, Potyvirus, Nicotiana benthamiana, Soybean mosaic virus, Biology, 01 natural sciences, Virus, Viral Proteins, 03 medical and health sciences, food, Species Specificity, Cistron, Virology, Plant virus, Tobacco, Watermelon mosaic virus, Phylogeny, Plant Diseases, Recombination, Genetic, Plant Stems, fungi, food and beverages, RNA, General Medicine, biology.organism_classification, Plant Leaves, 030104 developmental biology, RNA, Viral, Soybeans, 5' Untranslated Regions, Genome, Plant, 010606 plant biology & botany

Abstract

We discovered a soybean mosaic virus (SMV) variant (4278-1) that caused systemic infections in Nicotiana benthamiana plants, resulting in stem stunting and leaf shriveling. The virus had a particle morphology and incubation period similar to those of other SMV isolates but differed from them in the leaf symptoms it caused when infecting soybean and N. benthamiana. The genome of this variant consisted of a 9994-nt single-stranded RNA, which was different from most of the other known SMV isolates (approximately 9600 nt). Interestingly, we found evidence that two recombination events (nt 1-476 and nt 1145-1349) had occurred between 4278-1 and a watermelon mosaic virus analogue (WMV analogue), in the 5' untranslated region and the P1 cistron.

Published

2016

42. The Termination Phase in Protein Synthesis is not Obligatorily Followed by the RRF/EF-G-Dependent Recycling Phase

Author

Umesh Varshney, Knud H. Nierhaus, Takuya Ueda, Hiroshi Yamamoto, and Bo Qin

Subjects

Ribosomal Proteins, 0301 basic medicine, Prokaryotic Initiation Factor-3, Biology, Models, Biological, Ribosome, 03 medical and health sciences, Cistron, Genes, Reporter, Structural Biology, Escherichia coli, Protein biosynthesis, Luciferase, RNA, Messenger, Luciferases, Molecular Biology, Gene, Microbiology & Cell Biology, Messenger RNA, Peptide Chain Termination, Translational, Ribosomal RNA, Peptide Elongation Factor G, Cell biology, 030104 developmental biology, Genes, Biochemistry, Ribosomes, EF-G

Abstract

It is general wisdom that termination of bacterial protein synthesis is obligatorily followed by recycling governed by the factors ribosomal recycling factor (RRF), EF-G, and IF3, where the ribosome dissociates into its subunits. In contrast, a recently described 70S-scanning mode of initiation holds that after termination, scanning of 70S can be triggered by fMet-tRNA to the initiation site of a downstream cistron. Here, we analyze the apparent conflict. We constructed a bicistronic mRNA coding for luciferases and showed with a highly resolved in vitro system that the expression of the second cistron did not at all depend on the presence of active RRF. An in vivo analysis cannot be performed in a straightforward way, since RRF is essential for viability and therefore, the RRF gene cannot be knocked out. However, we found an experimental window, where the RRF amount could be reduced to below 2.5%, and in this situation, the expression of the second cistron of a bicistronic luciferase mRNA was only moderately reduced. Both in vitro and in vivo results suggested that RRF-dependent recycling is not an obligatory step after termination, in agreement with the previous findings concerning 70S-scanning initiation. In this view, recycling after termination is a special case of the general RRF function, which happens whenever fMet-tRNA is not available for triggering 70S scanning. (C) 2016 Elsevier Ltd. All rights reserved.

Published

2016

43. Population Analysis of Iranian Potato virus Y Isolates Using Complete Genome Sequence

Author

Shirin Farzadfar and Reza Pourrahim

Subjects

0301 basic medicine, Whole genome sequencing, education.field_of_study, biology, Phylogenetic tree, Population, lcsh:Plant culture, phylogeny, biology.organism_classification, Virology, Genome, recombination, 03 medical and health sciences, 030104 developmental biology, PVYN, Cistron, Potato virus Y, Phylogenetics, lcsh:SB1-1110, variation, education, Agronomy and Crop Science, Gene, Research Article

Abstract

In this study, the full-length nucleotide sequences of four Iranian PVY isolates belonging to PVY(N) strain were determined. The genome of Iranian PVY isolates were 9,703-9,707 nucleotides long encoding all potyviral cistrons including P1, HC-Pro, P3, 6K1, CI, 6K2, VPg, NIa-Pro, NIb and CP with coding regions of 825, 1,395, 1,095, 156, 1,902, 156, 564, 732, 1,557 and 801 nucleotides in length, respectively. The length of pipo, embedded in the P3 cistron, was 231 nucleotides. Phylogenetic analysis showed that the Iranian isolates clustered with European recombinant NTN isolates in the N lineage. Recombination analysis demonstrated that Iranian PVY(N) isolates had a typical European PVY(NTN) genome having three recombinant junctions while PVY(N) and PVY(O) were identified as the parents. We used dN/dS methods to detect candidate amino acid positions for positive selection in viral proteins. The mean ω ratio differed among different genes. Using model M0, ω values were 0.267 (P1), 0.085 (HC-Pro), 0.153 (P3), 0.050 (CI), 0.078 (VPg), 0.087 (NIa-pro), 0.079 (NIb) and 0.165 (CP). The analysis showed different sites within P1, P3 and CP were under positive selection pressure, however, the sites varied among PVY populations. To the best of our knowledge, our analysis provides the first demonstration of population structure of PVY(N) strain in mid-Eurasia Iran using complete genome sequences and highlights the importance of recombination and selection pressure in the evolution of PVY.

Published

2016

44. Viral Strain-Specific Differential Alterations in Arabidopsis Developmental Patterns

Author

Pablo González-Melendi, Carmen Mansilla, Fernando Ponz, Silvia López-González, Pablo Lunello, Guillermo Rodrigo, John A. Walsh, Carol E. Jenner, Pilar Manrique, Flora Sánchez, Santiago F. Elena, and Xiaowu Wang

Subjects

Genetics, biology, Physiology, viruses, Arabidopsis, Context (language use), Genome, Viral, General Medicine, Viral Nonstructural Proteins, Plants, Genetically Modified, biology.organism_classification, Genome, Transcriptome, RNA silencing, Cistron, Mosaic Viruses, Turnip mosaic virus, Agronomy and Crop Science, Gene

Abstract

Turnip mosaic virus (TuMV) infections affect many Arabidopsis developmental traits. This paper analyzes, at different levels, the development-related differential alterations induced by different strains of TuMV, represented by isolates UK 1 and JPN 1. The genomic sequence of JPN 1 TuMV isolate revealed highest divergence in the P1 and P3 viral cistrons, upon comparison with the UK 1 sequence. Infectious viral chimeras covering the whole viral genome uncovered the P3 cistron as a major viral determinant of development alterations, excluding the involvement of the PIPO open reading frame. However, constitutive transgenic expression of P3 in Arabidopsis did not induce developmental alterations nor modulate the strong effects induced by the transgenic RNA silencing suppressor HC-Pro from either strain. This highlights the importance of studying viral determinants within the context of actual viral infections. Transcriptomic and interactomic analyses at different stages of plant development revealed large differences in the number of genes affected by the different infections at medium infection times but no significant differences at very early times. Biological functions affected by UK 1 (the most severe strain) included mainly stress response and transport. Most cellular components affected cell-wall transport or metabolism. Hubs in the interactome were affected upon infection. © 2015 The American Phytopathological Society.

Published

2015

45. The in vivo expression of the globin genes of the β cistron in γ-, δ-, and δβ-thalassemia heterozygotes.

Author

Dimovski, A., Adekile, A., and Huisman, T.

Abstract

There is considerable evidence suggesting that the switch from γ to δ and β chain production after birth is due, in part, to silencing of the γ genes by stage-specific factors which bind to their promoters and to the competition from the adult (δ and β) genes for a common enhancer element located in the locus control region. As a consequence one can expect that the increased Hb F production in adults with hereditary persistence of fetal hemoglobin or δβ-thalassemia is directed mainly by γ-globin genes in cis to the deletion(s) responsible for these conditions. Here we review data on heterozygotes with γ-, δ-, or δβ-thalassemia, who also had anγ mutation, in cis or in trans, which was used as a marker of γ gene expression. The results show that a deletion affecting adult β genes favors the expression of γ genes in cis, while the deletion of a single γ gene does not affect the expression of the β gene in cis but leads to a faster γ→β switch postnatally. [ABSTRACT FROM AUTHOR]

Published

1994

46. Complete genome sequence of a putative novel potyvirus isolated from Platycodon grandiflorum

Author

Seungmo Lim, Su-Heon Lee, and Jae Sun Moon

Subjects

Platycodon, viruses, Potyvirus, Genome, Viral, 03 medical and health sciences, Open Reading Frames, Viral Proteins, Cistron, Virology, Peptide sequence, Phylogeny, 030304 developmental biology, Plant Diseases, 0303 health sciences, Mosaic virus, biology, Base Sequence, 030306 microbiology, Potyviridae, Nucleic acid sequence, General Medicine, biology.organism_classification, Open reading frame, GenBank

Abstract

The complete 9,556-nt genomic sequence of a putative new potyvirus, tentatively named “platycodon mild mottle virus” (PlaMMV), infecting Platycodon grandiflorum was determined (GenBank accession no. MH779625). A single large open reading frame (ORF; nt 121-9360, 3079 aa) encoding a polyprotein that was predicted to be cleaved into 10 mature proteins was detected. By comparison with other potyviruses, nine cleavage sites and conserved domains/motifs were identified. PlaMMV also has a highly conserved GA6 motif (nt 2857-2863) that could enable a small overlapping ORF (PIPO) embedded within the P3 cistron to be translated by a viral polymerase slippage mechanism. A BLAST analysis showed that the complete PlaMMV nucleotide sequence shared 70% identity (40% query coverage) with carrot thin leaf virus (JX156434) and that the complete amino acid sequence of the PlaMMV polyprotein shared 54% identity (98% query coverage) with Thunberg fritillary mosaic virus (CAI59123). These results suggest that PlaMMV is a new member of the genus Potyvirus in the family Potyviridae.

Published

2018

47. Early Ongoing Speciation of Ogataea uvarum Sp. Nov. Within the Grape Ecosystem Revealed by the Internal Variability Among the rDNA Operon Repeats

Author

Luca Roscini, Mariana Tristezza, Laura Corte, Claudia Colabella, Carla Perrotta, Patrizia Rampino, Vincent Robert, Duong Vu, Gianluigi Cardinali, Francesco Grieco, Westerdijk Fungal Biodiversity Institute, Westerdijk Fungal Biodiversity Institute - Software and Databasing, Roscini, L., Tristezza, Mariana, Corte, L., Colabella, C., Perrotta, C., Rampino, P., Robert, V., Vu, D., Cardinali, G., and Grieco, F.

Subjects

0301 basic medicine, Microbiology (medical), grape ecosystem, Operon, lcsh:QR1-502, yeast, Biology, Microbiology, lcsh:Microbiology, DNA sequencing, 03 medical and health sciences, symbols.namesake, wine yeast, Cistron, Ribosomal DNA, 2. Zero hunger, Genetics, Sanger sequencing, ribosomal DNA, Concerted evolution, Grape ecosystem, Internal variability, Wine yeast, Yeast, Ribosomal RNA, 030104 developmental biology, Metagenomics, internal variability, symbols, concerted evolution

Abstract

A yeast strain was isolated during a study on vineyard-associated yeast strains from Apulia in Southern Italy. ITS and LSU D1/D2 rDNA sequences showed this strain not to belong to any known species and was described as the type strain of Ogataea uvarum sp. nov., a close relative of O. philodendri. Several secondary peaks appeared in the sequences, suggesting internal heterogeneity among the copies of the rDNA. This hypothesis was tested by sequencing single clones of the marker region. The analyses showed different levels of variability throughout the operon with differences between the rRNA encoding genes and the internally transcribed regions. O. uvarum and O. philodendri share high frequency variants, i.e., variants frequently found in many clones, whereas there is a large variability of the low frequency polymorphisms, suggesting that the mechanism of homogenization is more active with the former than with the latter type of variation. These findings indicate that low frequency variants are detected in Sanger sequencing as secondary peaks whereas in Next Generation Sequencing (NGS) of metagenomics DNA would lead to an overestimate of the alpha diversity. For the first time in our knowledge, this investigation shed light on the variation of the copy number of the rDNA cistron during the yeast speciation process. These polymorphisms can be used to investigate on the processes occurring in these taxonomic markers during the separation of fungal species, it being a genetic process highly frequent in the complex microbial ecosystem existing in grape, must and wine.

Published

2018

48. Genes within Genes in Bacterial Genomes

Author

Nora Vázquez-Laslop, Sezen Meydan, and Alexander S. Mankin

Subjects

0301 basic medicine, Microbiology (medical), Physiology, 030106 microbiology, Codon, Initiator, Bacterial genome size, Computational biology, Biology, 03 medical and health sciences, Open Reading Frames, Cistron, Start codon, Bacterial Proteins, Genetics, Genes, Overlapping, Peptide Chain Initiation, Translational, Gene, General Immunology and Microbiology, Ecology, Bacteria, Translation (biology), Cell Biology, Gene Expression Regulation, Bacterial, Genetic code, Open reading frame, Infectious Diseases, Genetic Code, Proteome, Genome, Bacterial

Abstract

Genetic coding in bacteria largely operates via the “one gene-one protein” paradigm. However, the peculiarities of the mRNA structure, the versatility of the genetic code, and the dynamic nature of translation sometimes allow organisms to deviate from the standard rules of protein encoding. Bacteria can use several unorthodox modes of translation to express more than one protein from a single mRNA cistron. One such alternative path is the use of additional translation initiation sites within the gene. Proteins whose translation is initiated at different start sites within the same reading frame will differ in their N termini but will have identical C-terminal segments. On the other hand, alternative initiation of translation in a register different from the frame dictated by the primary start codon will yield a protein whose sequence is entirely different from the one encoded in the main frame. The use of internal mRNA codons as translation start sites is controlled by the nucleotide sequence and the mRNA folding. The proteins of the alternative proteome generated via the “genes-within-genes” strategy may carry important functions. In this review, we summarize the currently known examples of bacterial genes encoding more than one protein due to the utilization of additional translation start sites and discuss the known or proposed functions of the alternative polypeptides in relation to the main protein product of the gene. We also discuss recent proteome- and genome-wide approaches that will allow the discovery of novel translation initiation sites in a systematic fashion.

Published

2018

49. 'Therapeutic applications of the 'NPGP' family of viral 2As'

Author

Martin D. Ryan and Garry A. Luke

Subjects

0301 basic medicine, Indoles, Amino Acid Motifs, Computational biology, Biology, Genome, Ribosome, Pichia, 03 medical and health sciences, Cistron, Virology, Gene Expression Regulation, Fungal, Gene, Translation (biology), beta Carotene, Recombinant Proteins, Biosynthetic Pathways, Internal ribosome entry site, Open reading frame, 030104 developmental biology, Infectious Diseases, Genes, Metabolic Engineering, Protein Biosynthesis, Ribosomes, Biogenesis

Abstract

Oligopeptide "2A" and "2A-like" sequences ("2As"; 18-25aa) are found in a range of RNA virus genomes controlling protein biogenesis through "recoding" of the host-cell translational apparatus. Insertion of multiple 2As within a single open reading frame (ORF) produces multiple proteins; hence, 2As have been used in a very wide range of biotechnological and biomedical applications. During translation, these 2A peptide sequences mediate a eukaryote-specific, self-"cleaving" event, termed "ribosome skipping" with very high efficiency. A particular advantage of using 2As is the ability to simultaneously translate a number of proteins at an equal level in all eukaryotic systems although, naturally, final steady-state levels depend upon other factors-notably protein stability. By contrast, the use of internal ribosome entry site elements for co-expression results in an unbalanced expression due to the relative inefficiency of internal initiation. For example, a 1:1 ratio is of particular importance for the biosynthesis of the heavy-chain and light-chain components of antibodies: highly valuable as therapeutic proteins. Furthermore, each component of these "artificial polyprotein" systems can be independently targeted to different sub-cellular sites. The potential of this system was vividly demonstrated by concatenating multiple gene sequences, linked via 2A sequences, into a single, long, ORF-a polycistronic construct. Here, ORFs comprising the biosynthetic pathways for violacein (five gene sequences) and β-carotene (four gene sequences) were concatenated into a single cistron such that all components were co-expressed in the yeast Pichia pastoris. In this review, we provide useful information on 2As to serve as a guide for future utilities of this co-expression technology in basic research, biotechnology, and clinical applications.

Published

2018

50. Neocosmospora perseae sp. nov., causing trunk cankers on avocado in Italy

Author

Marcelo Sandoval-Denis, Giancarlo Polizzi, Vladimiro Guarnaccia, Dalia Aiello, Pedro W. Crous, Westerdijk Fungal Biodiversity Institute, and Westerdijk Fungal Biodiversity Institute - Evolutionary Phytopathology

Subjects

Canker, canker, Persea, biology, Phylogenetic tree, multigene phylogeny, medicine.disease, biology.organism_classification, Morphology, Multigene phylogeny, One new taxon, Pathogenicity, Agricultural and Biological Sciences (miscellaneous), Biochemistry, Genetics and Molecular Biology (miscellaneous), Microbiology, Article, Intergenic region, Cistron, Botany, morphology, medicine, pathogenicity, Taxonomy (biology), Internal transcribed spacer, one new taxon, Ribosomal DNA, Ecology, Evolution, Behavior and Systematics

Abstract

Trunk and branch cankers are among the most important diseases compromising avocado production worldwide. A novel species, Neocosmospora perseae sp. nov. is described isolated from trunk lesions on Persea americana in the main avocado producing area of Sicily, Italy. The new species is characterised using a polyphasic approach including morphological characters and a multilocus molecular phylogenetic analysis based on partial sequences of the translation elongation factor-1α, the internal transcribed spacer regions plus the large subunit of the rDNA cistron, and the RNA polymerase II second largest subunit. Pathogenicity tests and the fulfilment of Koch’s postulates confirm N. perseae as a novel canker pathogen of Persea americana.

Published

2018