Your search keyword '"Trans-splicing"' showing total 1,791 results

51. On the Function of Trans-Splicing: No Evidence for Widespread Proteome Diversification in Trypanosomes.

Author

Soulette, Cameron M, Oliverio, Oliver, and Roy, Scott W

Subjects

*TRYPANOSOMA, *RIBOSOMES, *MOLECULAR evolution, *EVIDENCE, *COMPARATIVE genomics, *RNA

Abstract

A long-standing mystery of genomic/transcriptomic structure involves spliced leader trans-splicing (SLTS), in which short RNA "tags" transcribed from a distinct genomic locus is added near the 5′ end of RNA transcripts by the spliceosome. SLTS has been observed in diverse eukaryotes in a phylogenetic pattern implying recurrent independent evolution. This striking convergence suggests important functions for SLTS, however no general novel function is known. Recent findings of frequent alternative SLTS (ALT-TS) suggest that ALT-TS could impart widespread functionality. Here, we tested the hypothesis that ALT-TS diversifies proteomes by comparing splicing patterns in orthologous genes between two deeply diverged trypanosome parasites. We also tested proteome diversification functions of ALT-TS by utilizing ribosome profiling sequence data. Finally, we investigated ALT-TS as a mechanism to regulate the expression of unproductive transcripts. Although our results indicate the functional importance of some cases of trans-splicing, we find no evidence for the hypothesis that proteome diversification is a general function of trans-splicing. [ABSTRACT FROM AUTHOR]

Published

2019

52. The Trypanosoma brucei RNA‐Binding Protein TbRRM1 is Involved in the Transcription of a Subset of RNA Pol II‐Dependent Genes.

Author

Bañuelos, Carolina P., Levy, Gabriela V., Níttolo, Analía G., Roser, Leandro G., Tekiel, Valeria, and Sánchez, Daniel O.

Subjects

*RNA-binding proteins, *TRYPANOSOMA brucei, *RNA, *DNA polymerases, *RNA polymerases, *GENES

Abstract

It has been long thought that RNA Polymerase (Pol) II transcriptional regulation does not operate in trypanosomes. However, recent reports have suggested that these organisms could regulate RNA Pol II transcription by epigenetic mechanisms. In this paper, we investigated the role of TbRRM1 in transcriptional regulation of RNA Pol II‐dependent genes by focusing both in genes located in a particular polycistronic transcription unit (PTU) and in the monocistronic units of the SL‐RNA genes. We showed that TbRRM1 is recruited throughout the PTU, with a higher presence on genes than intergenic regions. However, its depletion leads both to the decrease of nascent RNA and to chromatin compaction only of regions located distal to the main transcription start site. These findings suggest that TbRRM1 facilitates the RNA Pol II transcriptional elongation step by collaborating to maintain an open chromatin state in particular regions of the genome. Interestingly, the SL‐RNA genes do not recruit TbRRM1 and, after TbRRM1 knockdown, nascent SL‐RNAs accumulate while the chromatin state of these regions remains unchanged. Although it was previously suggested that TbRRM1 could regulate RNA Pol II‐driven genes, we provide here the first experimental evidence which involves TbRRM1 to transcriptional regulation. [ABSTRACT FROM AUTHOR]

Published

2019

53. Identified trans-splicing of YELLOW-FRUITED TOMATO 2 encoding the PHYTOENE SYNTHASE 1 protein alters fruit color by map-based cloning, functional complementation and RACE.

Author

Chen, Lulu, Li, Wenzhen, Li, Yongpeng, Feng, Xuechao, Du, Keyu, Wang, Ge, and Zhao, Lingxia

Abstract

Key message: Found a trans-splicing of PHYTOENE SYNTHASE 1 alters tomato fruit color by map-based cloning, functional complementation and RACE providing an insight into fruit color development. Color is an important fruit quality trait and a major determinant of the economic value of tomato (Solanum lycopersicum). Fruit color inheritance in a yellow-fruited cherry tomato (cv. No. 22), named yellow-fruited tomato 2 (yft2), was shown to be controlled by a single recessive gene, YFT2. The YFT2 gene was mapped in a 95.7 kb region on chromosome 3, and the candidate gene, PHYTOENE SYNTHASE 1 (PSY1), was confirmed by functional complementation analysis. Constitutive over expression of PSY1 in yft2 increased the accumulation of carotenoids and resulted in a red fruit color, while no causal mutation was detected in the YFT2 allele of yft2, compared with red-fruited SL1995 cherry tomato or cultivated variety (cv. M82). Expression of YFT2 3′ region in yft2 was significantly lower than in SL1995, and further studies revealed a difference in YFT2 post-transcriptional processing in yft2 compared with SL1995 and cv. M82, resulting in a longer YFT2 transcript. The alternatively trans-spliced allele of YFT2 in yft2 is predicted to encode a novel LT-YFT2 protein of 432 amino acid (AA) residues, compared to the 412 AA YFT2 protein of SL1995. The trans-spliced event also resulted in significantly down regulated expression of YFT2 in yft2 tomato, and the YFT2 allele suppressed expression of the downstream genes involved in the carotenoid biosynthesis pathway and carotenoids synthesis by a mechanism of the feed-forward regulation. In conclusion, we found that trans-splicing of YFT2 alters tomato fruit color, providing new insights into fruit color development. [ABSTRACT FROM AUTHOR]

Published

2019

54. New insights from Opisthorchis felineus genome: update on genomics of the epidemiologically important liver flukes.

Author

Ershov, Nikita I., Mordvinov, Viatcheslav A., Prokhortchouk, Egor B., Pakharukova, Mariya Y., Gunbin, Konstantin V., Ustyantsev, Kirill, Genaev, Mikhail A., Blinov, Alexander G., Mazur, Alexander, Boulygina, Eugenia, Tsygankova, Svetlana, Khrameeva, Ekaterina, Chekanov, Nikolay, Fan, Guangyi, Xiao, An, Zhang, He, Xu, Xun, Yang, Huanming, Solovyev, Victor, and Lee, Simon Ming-Yuen

Subjects

*OPISTHORCHIS, *OPISTHORCHIIDAE, *PARASITES, *CHOLANGIOCARCINOMA, *GENOMICS

Abstract

Background: The three epidemiologically important Opisthorchiidae liver flukes Opisthorchis felineus, O. viverrini, and Clonorchis sinensis, are believed to harbour similar potencies to provoke hepatobiliary diseases in their definitive hosts, although their populations have substantially different ecogeographical aspects including habitat, preferred hosts, population structure. Lack of O. felineus genomic data is an obstacle to the development of comparative molecular biological approaches necessary to obtain new knowledge about the biology of Opisthorchiidae trematodes, to identify essential pathways linked to parasite-host interaction, to predict genes that contribute to liver fluke pathogenesis and for the effective prevention and control of the disease. Results: Here we present the first draft genome assembly of O. felineus and its gene repertoire accompanied by a comparative analysis with that of O. viverrini and Clonorchis sinensis. We observed both noticeably high heterozygosity of the sequenced individual and substantial genetic diversity in a pooled sample. This indicates that potency of O. felineus population for rapid adaptive response to control and preventive measures of opisthorchiasis is higher than in O. viverrini and C. sinensis. We also have found that all three species are characterized by more intensive involvement of trans-splicing in RNA processing compared to other trematodes. Conclusion: All revealed peculiarities of structural organization of genomes are of extreme importance for a proper description of genes and their products in these parasitic species. This should be taken into account both in academic and applied research of epidemiologically important liver flukes. Further comparative genomics studies of liver flukes and non-carcinogenic flatworms allow for generation of well-grounded hypotheses on the mechanisms underlying development of cholangiocarcinoma associated with opisthorchiasis and clonorchiasis as well as species-specific mechanisms of these diseases. [ABSTRACT FROM AUTHOR]

Published

2019

55. Gene therapy strategies in the treatment of hypertrophic cardiomyopathy.

Author

Prondzynski, Maksymilian, Mearini, Giulia, and Carrier, Lucie

Subjects

*HYPERTROPHIC cardiomyopathy, *GENE therapy, *RNA splicing, *TREATMENT of cardiomyopathies, *PLURIPOTENT stem cells, *GENOME editing, *CARDIOMYOPATHIES

Abstract

Hypertrophic cardiomyopathy (HCM) is an inherited myocardial disease with an estimated prevalence of 1:200 caused by mutations in sarcomeric proteins. It is associated with hypertrophy of the left ventricle, increased interstitial fibrosis, and diastolic dysfunction for heterozygous mutation carriers. Carriers of double heterozygous, compound heterozygous, and homozygous mutations often display more severe forms of cardiomyopathies, ultimately leading to premature death. So far, there is no curative treatment against HCM, as current therapies are focused on symptoms relief by pharmacological intervention and not on the cause of HCM. In the last decade, several strategies have been developed to remove genetic defects, including genome editing, exon skipping, allele-specific silencing, spliceosome-mediated RNA trans-splicing, and gene replacement. Most of these technologies have already been tested for efficacy and efficiency in animal- or human-induced pluripotent stem cell models of HCM with promising results. We will summarize recent technological advances and their implication as gene therapy options in HCM with a special focus on treating MYBPC3 mutations and its potential for being a successful bench to bedside example. [ABSTRACT FROM AUTHOR]

Published

2019

56. Molecular cloning and functional characterization of two glycerol‐3‐phosphate acyltransferases from the green microalga Chlamydomonas reinhardtii.

Author

Duarte‐Coello, María E., Herrera‐Valencia, Virginia A., Echevarría‐Machado, Ileana, Casais‐Molina, Melissa L., and Peraza‐Echeverria, Santy

Subjects

*CHLAMYDOMONAS reinhardtii, *MOLECULAR cloning, *ACYLTRANSFERASES, *CHLAMYDOMONAS, *ENDOPLASMIC reticulum, *ISOENZYMES

Abstract

SUMMARY: Glycerol‐3‐phosphate acyltransferase (GPAT) catalyzes the first step of both the glycerolipid and the triacylglycerol (TAG) biosynthetic pathways. In plants, there are different isozymes for GPAT in different organelles, including the endoplasmic reticulum (ER) membrane‐bound GPAT and the soluble chloroplast (plastid) GPAT. In microalgae, studies on GPAT have been limited; only the microsomal TpGPAT from the diatom Thalassiosira pseudonana has been characterized by enzymatic assay using heterologous expression in Saccharomyces cerevisiae. In the present study, we report the cloning and sequence analysis of two genes encoding GPAT isozymes from the green microalga Chlamydomonas reinhardtii, CrGPATer and CrGPATcl. CrGPATer is a homolog to Arabidopsis thalianaAtGPAT9, which encodes an ER‐located GPAT, and CrGPATcl is a homolog to A. thalianaATS1, which encodes a chloroplast‐located GPAT. We mapped the 3′UTRs of both CrGPATer and CrGPATcl and identified three alternative splicings in CrGPATer mRNA and two in CrGPATcl mRNA. Interestingly, one of these splicings results from a trans‐splicing event in CrGPATer mRNA. The heterologous expression of the cDNAs from each gene in the S. cerevisiaegat1Δ mutant demonstrated, for the first time, that both CrGPATer and CrGPATcl show GPAT activity. Moreover, GPAT activity for CrGPATer was detected in the membrane extract, while that for CrGPATcl was detected in both the soluble and membrane extracts. Overall, these findings represent an important contribution to the better understanding of lipid metabolism in C. reinhardtii and in green microalgae in general. [ABSTRACT FROM AUTHOR]

Published

2019

57. Trans-splicing of the C. elegans let-7 primary transcript developmentally regulates let-7 microRNA biogenesis and let-7 family microRNA activity.

Author

Nelson, Charles and Ambros, Victor

Subjects

*CAENORHABDITIS elegans, *RNA splicing, *GENETIC transcription

Abstract

The sequence and roles in developmental progression of the microRNA let-7 are conserved. In general, transcription of the let-7 primary transcript ( pri-let-7) occurs early in development, whereas processing of the mature let-7 microRNA arises during cellular differentiation. In Caenorhabditis elegans and other animals, the RNA-binding protein LIN-28 post-transcriptionally inhibits let-7 biogenesis at early developmental stages, but the mechanisms by which LIN-28 does this are not fully understood. Nor is it understood how the developmental regulation of let-7 might influence the expression or activities of other microRNAs of the same seed family. Here, we show that pri-let-7 is trans-spliced to the SL1 splice leader downstream of the let-7 precursor stem-loop, which produces a short polyadenylated downstream mRNA, and that this transsplicing event negatively impacts the biogenesis of mature let-7 microRNA in cis. Moreover, this trans-spliced mRNA contains sequences that are complementary to multiple members of the let-7 seed family (let-7fam) and negatively regulates let-7fam function in trans. Thus, this study provides evidence for a mechanism by which splicing of a microRNA primary transcript can negatively regulate said microRNA in cis as well as other microRNAs in trans. [ABSTRACT FROM AUTHOR]

Published

2019

58. Reduction of non-specific toxicity of immunotoxin by intein mediated reconstitution on target cells.

Author

Wang, Jing, Han, Lei, Chen, Junsheng, Xie, Yueqing, Jiang, Hua, and Zhu, Jianwei

Subjects

*ANTIBODY-toxin conjugates, *BIOCONJUGATES, *PEPTIDES, *PROTEINS, *TUMOR antigens, *ANTIGENS

Abstract

Abstract Recombinant immunotoxins are chimeric proteins composed of a targeting peptide that binds to a specific tumor antigen and a toxin protein killing target cells. Recombinant immunotoxin exhibits potent cancer inhibiting effects both in vivo and in vitro. However, the non-specific toxicity causes severe syndromes limiting their clinical application. To reduce toxicity caused by recombinant immunotoxins in general, we divided an immunotoxin into two nontoxic segments that may restore toxic bioactivity on tumor cell surface based on the intein mediated trans-splicing reaction. Both split and reconstituted immunotoxins were tested for their biological activities. We found that the reconstituted immunotoxin retained antigen specificity and affinity toward cancer cells overexpressing HER2/neu. After being internalized into HER2/neu positive cells, the reconstituted immunotoxin showed comparable cytotoxicity as the original immunotoxin, while the split immunotoxin fragments showed no toxic activity to cells with or without HER2/neu expression. This approach can potentially be used under clinical settings to reduce non-specific toxicity by administering patients with inactive immunotoxin fragments. Cytotoxic effect only occurs at tumor sites where the inactive fragments bind, trans-splice and become active toxin. Highlights • An immunotoxin was divided to designed two-segments to eliminat toxic activity. The cytotoxicity can be recovered when they meet on cancer cell surface. • It is a facile method to prepare the split immunotoxin and to recover its cytotoxicity through intein mediated trans-splicing reaction. • This new approach can be applied to reduce non-specific toxicity of immunotoxic molecules and to expand their clinical usage. [ABSTRACT FROM AUTHOR]

Published

2019

59. Perfection of eccentricity: Mitochondrial genomes of diplonemids.

Author

Burger, Gertraud and Valach, Matus

Subjects

*MITOCHONDRIAL DNA, *GENOMES, *PROTISTA, *EUKARYOTES, *GENETIC transcription, *MESSENGER RNA

Abstract

Mitochondria are the sandbox of evolution as exemplified most particularly by the diplonemids, a group of marine microeukaryotes. These protists are uniquely characterized by their highly multipartite mitochondrial genome and systematically fragmented genes whose pieces are spread out over several dozens of chromosomes. The type species Diplonema papillatum was the first member of this group in which the expression of fragmented mitochondrial genes was investigated experimentally. We now know that gene expression involves separate transcription of gene pieces (modules), RNA editing of module transcripts, and module joining to mature mRNAs and rRNAs. The mechanism of cognate module recognition and ligation is distinct from known intron splicing and remains to be uncovered. Here, we review the current status of research on mitochondrial genome architecture, as well as gene complement, structure, and expression modes in diplonemids. Further, we discuss the potential molecular mechanisms of posttranscriptional processing, and finally reflect on the evolutionary trajectories and trends of mtDNA evolution as seen in this protist group. © 2018 IUBMB Life, 70(12):1197–1206, 2018 [ABSTRACT FROM AUTHOR]

Published

2018

60. The Chloroplast Trans-Splicing RNA–Protein Supercomplex from the Green Alga Chlamydomonas reinhardtii

Author

Ulrich Kück and Olga Schmitt

Subjects

group II intron, trans-splicing, ribonucleoprotein complex, chloroplast, Chlamydomonas reinhardtii, Cytology, QH573-671

Abstract

In eukaryotes, RNA trans-splicing is a significant RNA modification process for the end-to-end ligation of exons from separately transcribed primary transcripts to generate mature mRNA. So far, three different categories of RNA trans-splicing have been found in organisms within a diverse range. Here, we review trans-splicing of discontinuous group II introns, which occurs in chloroplasts and mitochondria of lower eukaryotes and plants. We discuss the origin of intronic sequences and the evolutionary relationship between chloroplast ribonucleoprotein complexes and the nuclear spliceosome. Finally, we focus on the ribonucleoprotein supercomplex involved in trans-splicing of chloroplast group II introns from the green alga Chlamydomonas reinhardtii. This complex has been well characterized genetically and biochemically, resulting in a detailed picture of the chloroplast ribonucleoprotein supercomplex. This information contributes substantially to our understanding of the function of RNA-processing machineries and might provide a blueprint for other splicing complexes involved in trans- as well as cis-splicing of organellar intron RNAs.

Published

2021

61. Fusion Genes and RNAs in Cancer Development

Author

Kenzui Taniue and Nobuyoshi Akimitsu

Subjects

fusion RNAs, gene fusions, chromosomal rearrangements, trans-splicing, cis-splicing, FISH, Genetics, QH426-470

Abstract

Fusion RNAs are a hallmark of some cancers. They result either from chromosomal rearrangements or from splicing mechanisms that are non-chromosomal rearrangements. Chromosomal rearrangements that result in gene fusions are particularly prevalent in sarcomas and hematopoietic malignancies; they are also common in solid tumors. The splicing process can also give rise to more complex RNA patterns in cells. Gene fusions frequently affect tyrosine kinases, chromatin regulators, or transcription factors, and can cause constitutive activation, enhancement of downstream signaling, and tumor development, as major drivers of oncogenesis. In addition, some fusion RNAs have been shown to function as noncoding RNAs and to affect cancer progression. Fusion genes and RNAs will therefore become increasingly important as diagnostic and therapeutic targets for cancer development. Here, we discuss the function, biogenesis, detection, clinical relevance, and therapeutic implications of oncogenic fusion genes and RNAs in cancer development. Further understanding the molecular mechanisms that regulate how fusion RNAs form in cancers is critical to the development of therapeutic strategies against tumorigenesis.

Published

2021

62. Counteracting the Common Shwachman–Diamond Syndrome-Causing SBDS c.258+2T>C Mutation by RNA Therapeutics and Base/Prime Editing

Author

Laura Peretto, Elena Tonetto, Iva Maestri, Valentino Bezzerri, Roberto Valli, Marco Cipolli, Mirko Pinotti, and Dario Balestra

Subjects

trans-splicing, PTM, Organic Chemistry, General Medicine, U1snRNA, base editor, Catalysis, Computer Science Applications, Inorganic Chemistry, SBDS, Shwachman–Diamond syndrome, genome editing, prime editor, Physical and Theoretical Chemistry, Molecular Biology, Spectroscopy

Abstract

Shwachman–Diamond syndrome (SDS) represents one of the most common inherited bone marrow failure syndromes and is mainly caused by SBDS gene mutations. Only supportive treatments are available, with hematopoietic cell transplantation required when marrow failure occurs. Among all causative mutations, the SBDS c.258+2T>C variant at the 5′ splice site (ss) of exon 2 is one of the most frequent. Here, we investigated the molecular mechanisms underlying aberrant SBDS splicing and showed that SBDS exon 2 is dense in splicing regulatory elements and cryptic splice sites, complicating proper 5′ss selection. Studies ex vivo and in vitro demonstrated that the mutation alters splicing, but it is also compatible with tiny amounts of correct transcripts, which would explain the survival of SDS patients. Moreover, for the first time for SDS, we explored a panel of correction approaches at the RNA and DNA levels and provided experimental evidence that the mutation effect can be partially counteracted by engineered U1snRNA, trans-splicing, and base/prime editors, ultimately leading to correctly spliced transcripts (from barely detectable to 2.5–5.5%). Among them, we propose DNA editors that, by stably reverting the mutation and potentially conferring positive selection to bone-marrow cells, could lead to the development of an innovative SDS therapy.

Published

2023

63. Characterization of Three cDNAs obtained by spliced Leader-PCR screening of a Taenia solium cDNA library

Author

Garrido, O and Ferrer, E

Subjects

trans-splicing, General Computer Science, General Mathematics, cysticercosis, General Physics and Astronomy, General Social Sciences, General Chemistry, spliced leader, PCR, recombinant proteins, General Biochemistry, Genetics and Molecular Biology, cisticercosis, líder acoplado, ou PCR, cisticercose, PCR, parasitic diseases, Taenia solium, empalme trans, General Earth and Planetary Sciences, proteínas recombinantes, spliced leader, General Agricultural and Biological Sciences, líder empalmado, acoplamento trans

Abstract

Cysticerci or metacestodes of Taenia solium cause cysticercosis, being the neurocysticercosis (NCC) the main pathology. The characterization of genes is essential for the knowledge of parasite biology, the understanding of the parasite-host relationship, and the identification of possible targets for diagnosis, treatment, and protection. The objective of this work was the molecular and bioinformatic characterization of three news cDNAs (TsTF10, TsAAP8, and TsrGAP8), obtained by spliced leader-PCR screening of a Taenia solium cDNA library. The sequences of the three cDNA were compared with the sequences in the nucleic acid and protein databases (GenBank, EMBL) and analyzed by bioinformatic programs (CDD-Search of the National Center for Biotechnology Information, Interpro of the European Bioinformatics Institute, Motif scan and Expert Protein Analysis System of the Proteomics Server from Swiss Institute of Bioinformatics). Considering the high identities with similar molecules of related helminths (Taenia asiatica, Echinococcus granulosus, Echinococcus multilocularis, and Hymenolepis diminuta) and the functional domains found, the TsTF10, TsAAP8, and TsrGAP8 genes of Taenia could act as a nuclear transcription factor gamma, a putative vacuolar ATPase membrane sector associated protein and a Rho GTPase activating protein, respectively. Although few B epitopes could be predicted in the sequences, it could be relevant to evaluate them as possible candidates for diagnosis and protection in cysticercosis. The characterization and analysis of these sequences and the prediction of their possible usefulness as antigens, vaccines, or therapeutic targetscontribute to the designing and planning of future studies. Resumen Los cisticercos de Taenia solium causan cisticercosis, y la neurocisticercosis (NCC) es la principal patología. La caracterización de genes es fundamental para el conocimiento de la biología del parásito, la relación parásitohospedador y la identificación de posibles dianas de diagnóstico, tratamiento y protección. El objetivo de este trabajo fue la caracterización molecular y bioinformática, de tres ADN complementarios (ADNc) (TsTF10, TsAAP8 y TsrGAP8), obtenidos por cribado por PCR de una genoteca de Taenia solium. Las secuencias se compararon con las de las bases de datos de ácidos nucleicos y proteínas (GenBank, EMBL) y se analizaron mediante programas bioinformáticos (CDD-Search del Centro Nacional de Información Biotecnológica, Interpro del Instituto Europeo de Bioinformática, Motif scan y Sistema de Análisis de Proteínas del Instituto Suizo de Bioinformatica). Teniendo en cuenta las altas identidades con moléculas similares de helmintos relacionados (Taenia asiatica, Echinococcus granulosus, E. multilocularis e Hymenolepis diminuta) y los dominios funcionales encontrados, los genes de Taenia, TsTF10, TsAAP8 y TsrGAP8 podrían actuar como un factor de transcripción nuclear gamma, una supuesta proteína asociada a ATPasa vacuolar de membrana y una proteína activadora de Rho GTPasa, respectivamente. Aunque pocos epítopos B pudieron predecirse en las secuencias, podría ser relevante valorarlos como posibles candidatos para diagnóstico y protección en cisticercosis. La caracterización y análisis de estas secuencias y la predicción de su posible utilidad como antígenos, vacunas o dianas terapéuticas ayudan al diseño y planificación de estudios futuros. Resumo Os cisticercos da Taenia solium causam cisticercose, e a neurocisticercose (NCC) é a principal patologia. A caracterização dos genes é fundamental para o conhecimento da biologia do parasita, da relação parasitahospedeiro e da identificação de possíveis alvos de diagnóstico, tratamento e proteção. O objetivo deste trabalho foi a caracterização molecular e bioinformática de três DNA complementar (cDNA) (TsTF10, TsAAP8 e TsrGAP8), obtidos pela triagem de PCR de uma biblioteca de DNA de Taenia solium. As sequências foram comparadas com as dos bancos de dados de ácidos nucleicos e proteína (GenBank, EMBL) e analisadas por meio de programas de bioinformática (CDD-Search do Centro Nacional de Informações Biotecnológicas, Interpro do Instituto Europeu de Bioinformática, Motif scan e Sistema de Análise de Proteínas do Instituto Suíço de Bioinformática). Considerando as altas identidades com moléculas semelhantes de helmintos relacionados (Taenia asiatica, Echinococcus granulosus, E. multilocularis e Hymenolepis diminuta) e os domínios funcionais encontrados, os genes de Taenia, TsTF10, TsAAP8 e TsrGAP8 poderiam atuar como um fator de transcrição nuclear gama, uma suposta proteína associada à ATPase vacuolar de membrana ATPase e uma proteína ativadora de Rho GTPase, respectivamente. Embora poucos epítopos B pudessem ser previstos nas sequências, poderia ser relevante avaliá-los como possíveis candidatos ao diagnóstico e à proteção em cisticercose. A caracterização e análise dessas sequências e a previsão de sua possível utilidade como antígenos, vacinas ou alvos terapêuticos ajudam no desenho e planejamento de estudos futuros.

Published

2022

64. Intein-Mediated Protein trans-Splicing of the Recombinant Streptavidin on Magnetosomes

Author

S. S. Wei, Q. L. Meng, Wei Chen, H. M. Wang, S. H. Ding, S. B. Duan, Y. J. Wang, J. J. Tian, Y. Z. Chen, and J. Chen

Subjects

Streptavidin, Magnetosome, Trans-splicing, Biophysics, law.invention, chemistry.chemical_compound, Biotin, chemistry, Biochemistry, Structural Biology, law, Protein splicing, MaMF, Recombinant DNA, Intein

Abstract

When expressing streptavidin recombinant polypeptide on magnetosomes (called bacterial magnetic nanoparticles, or BMPs), the presence of endogenous bacterial biotin might be detrimental. In the study, the streptavidin monomer fragment (SA1–116) was fused with the intein N-terminal (termed precursor SA1–116-IN), and SA1–116-IN was expressed in E. coli (BL21). Meanwhile, the SA117–160 fragment was fused with the C-terminal intein, and then this chimeric polypeptide was expressed on magnetosomes by fusion with magnetosome membrance protein MamF. In the in vitro protein splicing system, the purified engineered magnetosomes (BMP-SA117–160-IC) and the SA1–116-IN precursor were mixed. Intein-mediated trans-splicing reaction was induced to produce the functional magnetic beads BMP-SA. Our results indicate that intein-mediated protein trans-splicing may lead to efficient synthesis of the recombinant streptavidin on the magnetosomes, showing its promising potential to produce other functional magnetic nanoparticles.

Published

2021

65. In Vivo Evolution of a Trans-Splicing Group I Intron Ribozyme

Author

Behera, Ishani

Subjects

Biochemistry, Group I intron, In Vivo evolution, ribozyme, Tetrahymena, Trans-splicing

Abstract

The Tetrahymena group I intron was one of the two first catalytic RNAs (ribozymes) to be discovered. Group I introns are sequences that can exist between exons in pre-mRNAs, that are able to self-splice and remove themselves when forming mature mRNAs in the absence of the spliceosome. The Tetrahymena cis-splicing ribozyme was engineered to accept substrate RNAs in trans. The designed trans-splicing ribozyme was termed the “spliceozyme”. The spliceozyme could in principle be used in therapeutic applications. However, there are two hurdles to overcome; the delivery of the ribozyme into cells and its efficiency once delivered. The focus of this study is to improve the efficiency of the trans-splicing ribozyme in cells by evolving the ribozyme in E. coli. In a previous study, an evolution system in cells was developed for the spliceozyme which was used to generate a clone, W11, that increased product formation. However, this evolution used high ribozyme expression levels and focused on a single splice site. To improve the efficiency and sequence generality, the spliceozyme was evolved at low expression levels at two different splice sites with different flanking sequences. The results of the spliceozyme evolution in bacterial cells showed that specific mutations are able to improve spliceozyme efficiency in bacterial cells. This suggests that further analysis, and perhaps further evolution experiments, could generate spliceozymes with improved efficiency on a broad range of substrate sequences.

Published

2018

66. The YPEL5–PPP1CB fusion transcript is detected in different hematological malignancies and in normal samples

Author

Karl Vandepoele, Jan Philippé, and Barbara Denys

Subjects

Chronic lymphocytic leukemia, YPEL5–PPP1CB, Trans-splicing, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Chronic lymphocytic leukemia (CLL) is the most frequent leukemia in Western adults. It was suggested that transcripts from a reciprocal trans-splicing event between YPEL5 and PPP1CB were present exclusively in CLL patients (more than 90%). Here we show that the YPEL5–PPP1CB fusion is not specific for CLL but is also detected in other hematological malignancies such as chronic myeloid leukemia, monoclonal B cell lymphocytosis or acute leukemia and also in normal samples. As such, it is unlikely that the YPEL5–PPP1CB fusion is a good drug target in CLL or a suitable target to monitor disease.

Published

2015

67. Construction of IgG-Fab 2 bispecific antibody via intein-mediated protein trans-splicing reaction.

Author

Yamada R, Nakahara I, Kumagai I, Asano R, Nakanishi T, and Makabe K

Subjects

Trans-Splicing, Protein Splicing, Immunoglobulin G genetics, Inteins, Antibodies, Bispecific

Abstract

A bispecific antibody (bsAb) is a class of engineered antibody molecules that simultaneously binds to two different antigens by having two kinds of antigen-binding domains. One of the major obstacles for the bsAb production is the incorrect chain-pairing problem, wherein each heavy and light chain should form pairings with the correct counterpart's chains, but the structural similarity of the incorrect partners also forms the incorrect pairings. This study aimed to demonstrate a bsAb construction method using intein-mediated protein trans-splicing to create IgG-Fab 2 -type bsAbs, which is a modified antibody with a structure in which two additional Fabs are linked to the N-terminus of the heavy chain of an IgG molecule. The chain-paring problem between a heavy chain and a light chain is circumvented by separate expression and purification of the IgG part and the Fab part. We found that the deletion of a possible glycosylation residue improved the reaction yield and side-reaction cleavage in the protein ligation step. The resulting bsAb, IgG-Fab 2 (Her2/CD3), demonstrated target binding activity and cytotoxicity mediated by activated T cells. These results indicate that the use of the protein ligation to produce the IgG-Fab 2 type bsAb will expand the bsAb production method., (© 2023. Springer Nature Limited.)

Published

2023

68. High‐throughput sequencing of the chloroplast and mitochondrion of <italic>Chlamydomonas reinhardtii</italic> to generate improved <italic>de novo</italic> assemblies, analyze expression patterns and transcript speciation, and evaluate diversity among laboratory strains and wild isolates

Author

Gallaher, Sean D., Fitz‐Gibbon, Sorel T., Strenkert, Daniela, Purvine, Samuel O., Pellegrini, Matteo, and Merchant, Sabeeha S.

Subjects

*CHLAMYDOMONAS reinhardtii, *CHLOROPLASTS, *PLANT mitochondria, *GENE expression in plants, *GENETIC speciation

Abstract

Summary: Chlamydomonas reinhardtii is a unicellular chlorophyte alga that is widely studied as a reference organism for understanding photosynthesis, sensory and motile cilia, and for development of an algal‐based platform for producing biofuels and bio‐products. Its highly repetitive, ~205‐kbp circular chloroplast genome and ~15.8‐kbp linear mitochondrial genome were sequenced prior to the advent of high‐throughput sequencing technologies. Here, high coverage shotgun sequencing was used to assemble both organellar genomes de novo. These new genomes correct dozens of errors in the prior genome sequences and annotations. Genome sequencing coverage indicates that each cell contains on average 83 copies of the chloroplast genome and 130 copies of the mitochondrial genome. Using protocols and analyses optimized for organellar transcripts, RNA‐Seq was used to quantify their relative abundances across 12 different growth conditions. Forty‐six percent of total cellular mRNA is attributable to high expression from a few dozen chloroplast genes. RNA‐Seq data were used to guide gene annotation, to demonstrate polycistronic gene expression, and to quantify splicing of psaA and psbA introns. In contrast to a conclusion from a recent study, we found that chloroplast transcripts are not edited. Unexpectedly, cytosine‐rich polynucleotide tails were observed at the 3’‐end of all mitochondrial transcripts. A comparative genomics analysis of eight laboratory strains and 11 wild isolates of C. reinhardtii identified 2658 variants in the organellar genomes, which is 1/10th as much genetic diversity as is found in the nucleus. [ABSTRACT FROM AUTHOR]

Published

2018

69. Transcriptional-Readthrough RNAs Reflect the Phenomenon of "A Gene Contains Gene(s)" or "Gene(s) within a Gene" in the Human Genome, and Thus Are Not Chimeric RNAs.

Author

He, Yan, Yuan, Chengfu, Chen, Lichan, Lei, Mingjuan, Zellmer, Lucas, Huang, Hai, and Liao, Dezhong Joshua

Subjects

*HUMAN genome, *GENETIC transcription, *RIBONUCLEASES, *CHIMERISM, *NUCLEOTIDE sequence

Abstract

Tens of thousands of chimeric RNAs, i.e., RNAs with sequences of two genes, have been identified in human cells. Most of them are formed by two neighboring genes on the same chromosome and are considered to be derived via transcriptional readthrough, but a true readthrough event still awaits more evidence and trans-splicing that joins two transcripts together remains as a possible mechanism. We regard those genomic loci that are transcriptionally read through as unannotated genes, because their transcriptional and posttranscriptional regulations are the same as those of already-annotated genes, including fusion genes formed due to genetic alterations. Therefore, readthrough RNAs and fusion-gene-derived RNAs are not chimeras. Only those two-gene RNAs formed at the RNA level, likely via trans-splicing, without corresponding genes as genomic parents, should be regarded as authentic chimeric RNAs. However, since in human cells, procedural and mechanistic details of trans-splicing have never been disclosed, we doubt the existence of trans-splicing. Therefore, there are probably no authentic chimeras in humans, after readthrough and fusion-gene derived RNAs are all put back into the group of ordinary RNAs. Therefore, it should be further determined whether in human cells all two-neighboring-gene RNAs are derived from transcriptional readthrough and whether trans-splicing truly exists. [ABSTRACT FROM AUTHOR]

Published

2018

70. Absence of Correlation between Chimeric RNA and Aging.

Author

Reyna Huang, Kumar, Shailesh, and Hui Li

Subjects

*CHIMERIC enzymes, *RNA, *BIOINFORMATICS, *AGING, *HETEROCHROMATIN

Abstract

Chimeric RNAs have been recognized as a phenomenon not unique to cancer cells. They also exist in normal physiology. Aging is often characterized by deregulation of molecular and cellular mechanisms, including loss of heterochromatin, increased transcriptional noise, less tight control on alternative splicing, and more stress-induced changes. It is thus assumed that chimeric RNAs are more abundant in older people. In this study, we conducted a preliminary investigation to identify any chimeric RNAs with age-based trends in their expression levels in blood samples. A chimeric RNA candidate list generated by bioinformatic analysis indicated the possibility of both negative and positive trends in the expression of chimeric RNAs. Out of this candidate list, five novel chimeric RNAs were successfully amplified in multiple blood samples and then sequenced. Although primary smaller sample sizes displayed some weak trends with respect to age, analysis of quantitative PCR data from larger sample sizes showed essentially no relationship between expression levels and age. Altogether, these results indicate that, contradictory to the common assumption, chimeric RNAs as a group are not all higher in older individuals and that placing chimeric RNAs in the context of aging will be a much more complex task than initially anticipated. [ABSTRACT FROM AUTHOR]

Published

2017

71. Development of End-Spliced Dimeric Nanodiscs for the Improved Virucidal Activity of a Nanoperforator

Author

Dae-Hyuk Kweon, Choongjin Ban, Hyunseok Oh, Jaehyeon Hwang, Woo-Jae Chung, Younghun Jung, Jinhyo Chung, and Seokoh Moon

Subjects

Scaffold protein, Mice, Inbred BALB C, Materials science, Lipid Bilayers, Membrane Proteins, Cooperativity, Microbial Sensitivity Tests, Viral membrane, Orthomyxoviridae, Antiviral Agents, Nanostructures, Trans-Splicing, Membrane, Membrane protein, Cytoplasm, Viral Envelope, Drug delivery, Escherichia coli, Biophysics, Animals, Female, General Materials Science, Nanodisc

Abstract

Lipid-bilayer nanodiscs (NDs) wrapped in membrane scaffold proteins (MSPs) have primarily been used to study membrane proteins of interest in a physiological environment. Recently, NDs have been employed in broader applications including drug delivery, cancer immunotherapy, bio-imaging, and therapeutic virucides. Here, we developed a method to synthesize a dimeric nanodisc, whose MSPs are circularly end-spliced, with long-term thermal stability and resistance to aggregation. The end-spliced nanodiscs (esNDs) were assembled using MSPs that were self-circularized inside the cytoplasm ofEscherichia colivia highly efficient protein trans-splicing. The esNDs demonstrated a consistent size and 4-5-fold higher stability against heat and aggregation than conventional NDs. Moreover, cysteine residues on trans-spliced circularized MSPs allowed us to modulate the formation of either monomeric nanodiscs (essNDs) or dimeric nanodiscs (esdNDs) by controlling the oxidation/reduction conditions and lipid-to-protein ratios. When the esdNDs were used to prepare an antiviral nanoperforator that induced the disruption of the viral membrane upon contact, antiviral activity was dramatically increased, suggesting that the dimerization of nanodiscs led to cooperativity between linked nanodiscs. We expect that controllable structures, long-term stability, and aggregation resistance of esNDs will aid the development of novel versatile membrane-mimetic nanomaterials with flexible designs and improved therapeutic efficacy.

Published

2021

72. Optimization of trans-Splicing for Huntington's Disease RNA Therapy

Author

Hansjörg Rindt, Colton M. Tom, Christian L. Lorson, and Virginia B. Mattis

Subjects

Huntington's disease, HD, Huntingtin, HTT, trans-splicing, therapy, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571

Abstract

Huntington's disease (HD) is a devastating neurodegenerative disorder caused by a polyglutamine (polyQ) expansion in exon 1 of the Huntingtin (HTT) gene. We have previously demonstrated that spliceosome-mediated trans-splicing is a viable molecular strategy to specifically reduce and repair mutant HTT (mtHTT). Here, the targeted tethering efficacy of the pre-mRNA trans-splicing modules (PTM) in HTT was optimized. Various PTMs that targeted the 3′ end of HTT intron 1 or the intron 1 branch point were shown trans-splice into an HTT mini-gene, as well as the endogenous HTT pre-mRNA. PTMs that specifically target the endogenous intron 1 branch point increased the trans-splicing efficacy from 1–5 to 10–15%. Furthermore, lentiviral expression of PTMs in a human HD patient iPSC-derived neural culture significantly reversed two previously established polyQ-length dependent phenotypes. These results suggest that pre-mRNA repair of mtHTT could hold therapeutic benefit and it demonstrates an alternative platform to correct the mRNA product produced by the mtHTT allele in the context of HD.

Published

2017

73. Minimum free energy predicted base pairing in the 39 nt spliced leader and 5’ UTR of calmodulin mRNA from Trypanosoma cruzi: influence of the multiple trans-splicing sites

Author

FRANKLYN SAMUDIO and ADEILTON BRANDÃO

Subjects

trans-splicing, untranslated region, calmodulin, epimastigote, RNA secondary structure, minimum free energy, Science

Abstract

ABSTRACT We analyzed the compositional changes and the stable base pairs in the predicted secondary structure of the 5’ UTR calmodulin mRNA in T. cruzi. The three copies of calmodulin in T. cruzi genome display variable position of the trans splicing sites and give rise to several mRNA that differs slightly on 5’ UTR composition in the epimastigote stage. We show that the pattern of high probability base pairs in the minimum free energy predicted secondary structures of the calmodulin 5’ UTR remains unchanged despite the nucleotide composition variation. However, the 39 nt spliced leader (mini-exon, the 5’ exon sequence transferred to trypanosome mRNAs by the mechanism of trans splicing) shows a variable pattern of high and low probability base pairing as consequence of the altered composition of the 5’ UTR.

Published

2017

74. Transcriptomic analysis of diplomonad parasites reveals a trans-spliced intron in a helicase gene in Giardia

Author

Scott William Roy

Subjects

Genome complexity, Trans-splicing, Protist molecular biology, Medicine, Biology (General), QH301-705.5

Abstract

Background The mechanisms by which DNA sequences are expressed is the central preoccupation of molecular genetics. Recently, ourselves and others reported that in the diplomonad protist Giardia lamblia, the coding regions of several mRNAs are produced by ligation of independent RNA species expressed from distinct genomic loci. Such trans-splicing of introns was found to affect nearly as many genes in this organism as does classical cis-splicing of introns. These findings raised questions about the incidence of intron trans-splicing both across the G. lambliatranscriptome and across diplomonad diversity in general, however a dearth of transcriptomic data at the time prohibited systematic study of these questions. Methods I leverage newly available transcriptomic data from G. lamblia and the related diplomonad Spironucleus salmonicidato search for trans-spliced introns. My computational pipeline recovers all four previously reported trans-spliced introns in G. lamblia, suggesting good sensitivity. Results Scrutiny of thousands of potential cases revealed only a single additional trans-spliced intron in G. lamblia, in the p68 helicase gene, and no cases in S. salmonicida. The p68 intron differs from the previously reported trans-spliced introns in its high degree of streamlining: the core features of G. lamblia trans-spliced introns are closely packed together, revealing striking economy in the implementation of a seemingly inherently uneconomical molecular mechanism. Discussion These results serve to circumscribe the role of trans-splicing in diplomonads both in terms of the number of genes effected and taxonomically. Future work should focus on the molecular mechanisms, evolutionary origins and phenotypic implications of this intriguing phenomenon.

Published

2017

75. Trans-splicing facilitated by RNA pairing greatly expands sDscam isoform diversity but not homophilic binding specificity

Author

Shouqing Hou, Guo Li, Bingbing Xu, Haiyang Dong, Shixin Zhang, Ying Fu, Jilong Shi, Lei Li, Jiayan Fu, Feng Shi, Yijun Meng, and Yongfeng Jin

Subjects

Mammals, Alternative Splicing, Multidisciplinary, Animals, Drosophila Proteins, Protein Isoforms, RNA, Trans-Splicing

Abstract

The Down syndrome cell adhesion molecule 1 ( Dscam1 ) gene can generate tens of thousands of isoforms via alternative splicing, which is essential for nervous and immune functions. Chelicerates generate approximately 50 to 100 shortened Dscam (sDscam) isoforms by alternative promoters, similar to mammalian protocadherins. Here, we reveal that trans-splicing markedly increases the repository of sDscamβ isoforms in Tetranychus urticae . Unexpectedly, every variable exon cassette engages in trans-splicing with constant exons from another cluster. Moreover, we provide evidence that competing RNA pairing not only governs alternative cis-splicing but also facilitates trans-splicing. Trans-spliced sDscam isoforms mediate cell adhesion ability but exhibit the same homophilic binding specificity as their cis-spliced counterparts. Thus, we reveal a single sDscam locus that generates diverse adhesion molecules through cis- and trans-splicing coupled with alternative promoters. These findings expand understanding of the mechanism underlying molecular diversity and have implications for the molecular control of neuronal and/or immune specificity.

Published

2022

76. Circular and Fusion RNAs in Medulloblastoma Development

Author

Ani Azatyan and Peter G. Zaphiropoulos

Subjects

Cancer Research, Oncology, brain cancer, pediatric cancer, back-splicing, read-through transcription, trans-splicing

Abstract

Background. The cerebellar cancer medulloblastoma is the most common childhood cancer in the brain. Methods. RNA sequencing of 81 human biospecimens of medulloblastoma using pipelines to detect circular and fusion RNAs. Validation via PCR and Sanger sequencing. Results. 27, 56, 28 and 11 RNA circles were found to be uniquely up-regulated, while 149, 7, 20 and 15 uniquely down-regulated in the SHH, WNT, Group 3, and Group 4 medulloblastoma subtypes, respectively. Moreover, linear and circular fusion RNAs containing exons from distinct genes joined at canonical splice sites were also identified. These were generally expressed less than the circular RNAs, however the expression of both the linear and the circular fusions was comparable. Importantly, the expression of the fusions in medulloblastoma was also comparable to that of cerebellum. Conclusions. A significant number of fusions in tumor may be generated by mechanisms similar to the ones generating fusions in normal tissue. Some fusions could be rationalized by read-through transcription of two neighboring genes. However, for other fusions, e.g., a linear fusion with an exon from a downstream gene joined 5′ to 3′ with an exon from an upstream gene, more complicated splicing mechanisms, e.g., trans-splicing, have to be postulated.

Published

2022

77. LYSINE KETOGLUTARATE REDUCTASE TRANS-SPLICING RELATED 1 is involved in temperature-dependent root growth in rice

Author

Jian Feng Ma, Kanatani Asaka, En Yu, Naoki Yamaji, Keiich Mochida, and Ivan Galis

Subjects

Oryza sativa, Physiology, Chemistry, Mutant, Temperature, food and beverages, Oryza, Plant Science, Glutamic acid, Meristem, Plant Roots, Trans-Splicing, Cell biology, Complementation, Gene Expression Regulation, Plant, Mutation, Shoot, Saccharopine Dehydrogenases, Elongation, Gene, Plant Proteins

Abstract

Root length is one of the important parameters of root traits directly related to uptake of water and nutrients, however, the molecular mechanisms controlling root length are still not fully understood. Here, we isolated a mutant, dice2 (defective in cell elongation 2) of rice (Oryza sativa) showing short roots. The cell length and meristem size of the roots was decreased in the mutant, but the root function in mineral element uptake normalized by root biomass, root cell width and root anatomy was hardly altered compared with the wild-type rice (WT). Intriguingly, the root growth defect in the mutant could be partially rescued by high temperature. The mutant accumulated more H2O2 and glutamic acid, but less O2 •- in the roots at low temperature than WT, but they became similar at high temperature between two lines. A map-based cloning combined with complementation test revealed that the short-root phenotype was caused by a nucleotide substitution of a gene, which was annotated to encode Lysine Ketoglutarate Reductase Trans-Splicing related 1 (OsLKRT1). OsLKRT1 encodes a cytosol-localized protein and was expressed in both the roots and shoots. Furthermore, OsLKRT1 was expressed in all cells of the root tip and root elongation regions. RNA-seq analysis showed that there was no difference in the expression level of genes involved in root development identified so far. These results indicate that the gene identified in this study is involved in novel pathway required for cell elongation of the roots in rice although its exact role remains to be further investigated.

Published

2021

78. Trans-spliced mRNA products produced from circRNA expression vectors

Author

Jennifer Chu, Francis Robert, and Jerry Pelletier

Subjects

0303 health sciences, Messenger RNA, Expression vector, fungi, 030302 biochemistry & molecular biology, Trans-splicing, RNA, Computational biology, Biology, 03 medical and health sciences, Internal ribosome entry site, Open reading frame, Gene expression, Vector (molecular biology), Molecular Biology, 030304 developmental biology

Abstract

Circular (circ) RNA expression vectors are used as a method of identifying and characterizing RNA sequences that harbor internal ribosome entry site (IRES) activity. During the course of developing a vector series tailored for IRES discovery, we found evidence for the occurrence of trans-spliced mRNAs arising when sequences with promoter activity were embedded between the upstream CTD and downstream NTD exons of the pre-mRNA. These trans-spliced products regenerate the same open reading frame expected from a circRNA and can lead to false-positive signals in screens relying on circRNA expression vectors for IRES discovery. Our results caution against interpretations of IRES activity solely based on results obtained from circRNA expression vectors.

Published

2021

79. Real-time visualization of intratumoral necrosis using split-luciferase reconstitution by protein trans-splicing

Author

Mana Kato, Fumitaka Kawakami, Fumiaki Kojima, Ryohei Ogawa, Fuminori Hyodo, Makoto Kubo, Naoya Abe, Masanori Hatashita, Yukari Nishimura, Ayaka Sato, and Go Kagiya

Subjects

0301 basic medicine, Cancer Research, Programmed cell death, Necrosis, dnaE, Trans-splicing, intein, lcsh:RC254-282, necrosis, extein, 03 medical and health sciences, 0302 clinical medicine, split-luciferase reconstitution, medicine, Bioluminescence, Pharmacology (medical), Luciferase, bioluminescent imaging, Chemistry, Cancer, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, medicine.disease, cell death, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Cancer research, Molecular Medicine, Original Article, protein trans-splicing, medicine.symptom, Intein, necrosis imaging reporter

Abstract

Necrosis, a form of cell death, occurs not only with the development of various diseases but also with a tumor tissue response to cancer treatment. Therefore, pursuing progress for cancer therapy through induction of necrosis may be one of the most effective approaches for cancer eradication. We herein describe the development of a real-time imaging system to visualize intratumoral necrosis. The system is composed of two types of cells expressing either one of two necrosis imaging reporters that consist of a DnaE intein sequence linking to one of two split-luciferase fragments. When necrosis occurs in a tumor composed of both of the cells, the two types of leaked reporters can reconstitute the enzymatic activity as a result of protein trans-splicing and thereby emit bioluminescence in the presence of the substrate. This system, which was constructed with shrimp-derived luciferase, allowed in vitro imaging of necrosis. We further confirmed real-time imaging of intratumoral necrosis caused by physical or chemical tissue disruption, validating its application in in vivo necrosis imaging. Thus, the constructed imaging system could be a powerful tool for the optimization of the therapeutic condition for cancer therapy and for the evaluation of novel anticancer drugs targeting necrosis., Graphical Abstract, Necrosis occurs with the development of various diseases and in tumor tissue responding to cancer treatment. To evaluate the preclinical effectiveness of different anticancer drugs and radiation therapy, Kagiya and colleagues have constructed a real-time visualization system for intratumoral necrosis using split-luciferase reconstitution by protein trans-splicing.

Published

2021

80. Fugacium Spliced Leader Genes Identified from Stranded RNA-Seq Datasets

Author

Yue Song, Bahareh Zaheri, Min Liu, Sunil Kumar Sahu, Huan Liu, Wenbin Chen, Bo Song, and David Morse

Subjects

dinoflagellates, Symbiodinium, Fugacium, trans-splicing, spliced leader, Biology (General), QH301-705.5

Abstract

Trans-splicing mechanisms have been documented in many lineages that are widely distributed phylogenetically, including dinoflagellates. The spliced leader (SL) sequence itself is conserved in dinoflagellates, although its gene sequences and arrangements have diversified within or across different species. In this study, we present 18 Fugacium kawagutii SL genes identified from stranded RNA-seq reads. These genes typically have a single SL but can contain several partial SLs with lengths ranging from 103 to 292 bp. Unexpectedly, we find the SL gene transcripts contain sequences upstream of the canonical SL, suggesting that generation of mature transcripts will require additional modifications following trans-splicing. We have also identified 13 SL-like genes whose expression levels and length are comparable to Dino-SL genes. Lastly, introns in these genes were identified and a new site for Sm-protein binding was proposed. Overall, this study provides a strategy for fast identification of SL genes and identifies new sequences of F. kawagutii SL genes to supplement our understanding of trans-splicing.

Published

2019

81. Semisynthetic head-to-tail cyclized peptides obtained by combining proteintrans-splicing and intramolecular expressed protein ligation

Author

Henning D. Mootz and Shubhendu Palei

Subjects

0303 health sciences, Natural product, 010405 organic chemistry, Stereochemistry, Trypsin inhibitor, Trans-splicing, Metals and Alloys, General Chemistry, 01 natural sciences, Semisynthesis, Catalysis, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, 03 medical and health sciences, chemistry.chemical_compound, chemistry, Intramolecular force, Materials Chemistry, Ceramics and Composites, Peptide bond, Intein, Ligation, 030304 developmental biology

Abstract

A dual-intein approach for the preparation of head-to-tail macrocyclic peptides is reported, where synthetic and genetically encoded fragments are ligated by two native peptide bonds. A split intein ligates the synthetic and genetically encoded peptides via protein trans-splicing and is followed by intramolecular cyclization through an expressed protein ligation step mediated with a cis-intein. We identified a suitable pair of orthogonal inteins and optimized the conditions for a one-pot cyclization protocol. We report the semisynthesis of model macrocyles with various ring sizes and of the natural product sunflower trypsin inhibitor (SFTI) along with its ornithine analog.

Published

2021

82. Research Progress of Chimeric RNA and Health

Author

Weikai Chen, Di Cui, Wei Cui, and Ye Qiu

Subjects

Fusion gene, chemistry.chemical_compound, chemistry, Chimeric RNA, RNA splicing, Trans-splicing, Chimeric gene, Computational biology, Biology, Gene, Fusion protein, DNA

Abstract

With the development of deep sequencing and bioinformatics technology, a large number of products produced by abnormal RNA splicing, such as chimeric RNA and chimeric/fusion proteins, have been discovered. Natural chimeric/fusion genes are new genes formed by natural fusion of two or more independent genes. Chimeric RNAs can be transcribed by natural chimeric genes, and can also be formed by cis-splicing or trans-splicing of two or more precursor mRNAs. Unlike fusion genes, the production of chimeric RNAs does not involve changes in the DNA level of chromosomes. At first, chimeric RNAs were found as tumor markers. With the deepening of research, researchers also found a large number of chimeric RNAs in normal tissues. From the perspective of biological function, chimeric RNAs can play a biological role in regulating the expression of corresponding maternal genes, translating into chimeric proteins, and forming long non-coding RNAs. The objective of the present study focused on the frontiers of chimeric RNA and reviewed its role in health and tumor study to reveal research progress of chimeric RNA and health and provide a new sight of relative disease treatment. The main conclusion of this review is that chimeric RNA may serve as a biomarker for specific tumor diagnose and treatment while its role in normal physiology needs to be revealed.

Published

2021

83. The

Author

Tania, Bishola Tshitenge and Christine, Clayton

Subjects

Mammals, Trypanosoma brucei brucei, Animals, RNA-Binding Proteins, RNA, Messenger, Polyadenylation, 3' Untranslated Regions, Trans-Splicing

Abstract

The parasite

Published

2022

84. From trans-splicing discovery and onwards, trypanosomes lead the way

Author

Idálio J, Viegas and Luisa M, Figueiredo

Subjects

Trypanosoma, RNA Splicing, Trans-Splicing

Published

2022

85. Liver gene therapy with intein-mediated F8 trans-splicing corrects mouse haemophilia A

Author

Esposito, Federica, Lyubenova, Hristiana, Tornabene, Patrizia, Auricchio, Stefano, Iuliano, Antonella, Nusco, Edoardo, Merlin, Simone, Olgasi, Cristina, Manni, Giorgia, Gargaro, Marco, Fallarino, Francesca, Follenzi, Antonia, Auricchio, Alberto, Esposito, Federica, Lyubenova, Hristiana, Tornabene, Patrizia, Auricchio, Stefano, Iuliano, Antonella, Nusco, Edoardo, Merlin, Simone, Olgasi, Cristina, Manni, Giorgia, Gargaro, Marco, Fallarino, Francesca, Follenzi, Antonia, and Auricchio, Alberto

Subjects

Genetic Vectors, haemophilia A, Genetic Therapy, Dependovirus, Hemophilia A, AAV vectors, Inteins, Trans-Splicing, AAV vector, Mice, Liver, Molecular Medicine, Animals, liver gene therapy, protein trans-splicing

Abstract

Liver gene therapy with adeno-associated viral (AAV) vectors is under clinical investigation for haemophilia A (HemA), the most common inherited X-linked bleeding disorder. Major limitations are the large size of the F8 transgene, which makes packaging in a single AAV vector a challenge, as well as the development of circulating anti-F8 antibodies which neutralise F8 activity. Taking advantage of split-intein-mediated protein trans-splicing, we divided the coding sequence of the large and highly secreted F8-N6 variant in two separate AAV-intein vectors whose co-administration to HemA mice results in the expression of therapeutic levels of F8 over time. This occurred without eliciting circulating anti-F8 antibodies unlike animals treated with the single oversized AAV-F8 vector under clinical development. Therefore, liver gene therapy with AAV-F8-N6 intein should be considered as a potential therapeutic strategy for HemA.

Published

2022

86. Optimization of trans-Splicing for Huntington's Disease RNA Therapy.

Author

Rindt, Hansjörg, Tom, Colton M., Lorson, Christian L., and Mattis, Virginia B.

Subjects

HUNTINGTON disease, NEURODEGENERATION, POLYGLUTAMINE

Abstract

Huntington's disease (HD) is a devastating neurodegenerative disorder caused by a polyglutamine (polyQ) expansion in exon 1 of the Huntingtin (HTT) gene. We have previously demonstrated that spliceosome-mediated trans-splicing is a viable molecular strategy to specifically reduce and repair mutant HTT (mtHTT). Here, the targeted tethering efficacy of the pre-mRNA trans-splicing modules (PTM) in HTT was optimized. Various PTMs that targeted the 3' end of HTT intron 1 or the intron 1 branch point were shown trans-splice into an HTT mini-gene, as well as the endogenous HTT pre-mRNA. PTMs that specifically target the endogenous intron 1 branch point increased the trans-splicing efficacy from 1-5 to 10-15%. Furthermore, lentiviral expression of PTMs in a human HD patient iPSC-derived neural culture significantly reversed two previously established polyQ-length dependent phenotypes. These results suggest that pre-mRNA repair ofmtHTT could hold therapeutic benefit and it demonstrates an alternative platform to correct the mRNA product produced by the mtHTT allele in the context of HD. [ABSTRACT FROM AUTHOR]

Published

2017

87. RNA Editing for Muscular Dystrophy Therapy.

Author

Yakovlev, I., Deev, R., Rizvanov, A., and Isaev, A.

Abstract

Due to lack of effective therapies, muscular dystrophies became a focus for gene therapy. Multiple pre-clinical studies have shown successful restoration of dystrofin and dysferlin by RNA editing both in vivo and in vitro, but possibility of a clinical translation is still obscure. A number of new chemicals are being studied, and a search for new techniques is ongoing. This work is intended to give a brief overview of the current state of the RNA editing for treating muscular dystrophies. [ABSTRACT FROM AUTHOR]

Published

2017

88. It Is Imperative to Establish a Pellucid Definition of Chimeric RNA and to Clear Up a Lot of Confusion in the Relevant Research.

Author

Chengfu Yuan, Yaping Han, Zellmer, Lucas, Wenxiu Yang, Zhizhong Guan, Wenfeng Yu, Hai Huang, and Liao, D. Joshua

Subjects

*RNA analysis, *NUCLEIC acid analysis, *GENOMIC imprinting, *CHIMERISM, *ZONA pellucida

Abstract

There have been tens of thousands of RNAs deposited in different databases that contain sequences of two genes and are coined chimeric RNAs, or chimeras. However, “chimeric RNA” has never been lucidly defined, partly because “gene” itself is still ill-defined and because the means of production for many RNAs is unclear. Since the number of putative chimeras is soaring, it is imperative to establish a pellucid definition for it, in order to differentiate chimeras from regular RNAs. Otherwise, not only will chimeric RNA studies be misled but also characterization of fusion genes and unannotated genes will be hindered. We propose that only those RNAs that are formed by joining two RNA transcripts together without a fusion gene as a genomic basis should be regarded as authentic chimeras, whereas those RNAs transcribed as, and cis-spliced from, single transcripts should not be deemed as chimeras. Many RNAs containing sequences of two neighboring genes may be transcribed via a readthrough mechanism, and thus are actually RNAs of unannotated genes or RNA variants of known genes, but not chimeras. In today’s chimeric RNA research, there are still several key flaws, technical constraints and understudied tasks, which are also described in this perspective essay. [ABSTRACT FROM AUTHOR]

Published

2017

89. Detecting intragenic trans-splicing events from non-co-linearly spliced junctions by hybrid sequencing.

Author

Chen YC, Chen CY, Chiang TW, Chan MH, Hsiao M, Ke HM, Tsai IJ, and Chuang TJ

Subjects

Genome, RNA Splicing, RNA, Circular, Trans-Splicing, Sequence Analysis, RNA methods

Abstract

Trans-spliced RNAs (ts-RNAs) are a type of non-co-linear (NCL) transcripts that consist of exons in an order topologically inconsistent with the corresponding DNA template. Detecting ts-RNAs is often interfered by experimental artifacts, circular RNAs (circRNAs) and genetic rearrangements. Particularly, intragenic ts-RNAs, which are derived from separate precursor mRNA molecules of the same gene, are often mistaken for circRNAs through analyses of RNA-seq data. Here we developed a bioinformatics pipeline (NCLscan-hybrid), which integrated short and long RNA-seq reads to minimize false positives and proposed out-of-circle and rolling-circle long reads to distinguish between intragenic ts-RNAs and circRNAs. Combining NCLscan-hybrid screening and multiple experimental validation steps successfully confirmed that four NCL events, which were previously regarded as circRNAs in databases, originated from trans-splicing. CRISPR-based endogenous genome modification experiments further showed that flanking intronic complementary sequences can significantly contribute to ts-RNA formation, providing an efficient/specific method to deplete ts-RNAs. We also experimentally validated that one ts-RNA (ts-ARFGEF1) played an important role for p53-mediated apoptosis through affecting the PERK/eIF2a/ATF4/CHOP signaling pathway in breast cancer cells. This study thus described both bioinformatics procedures and experimental validation steps for rigorous characterization of ts-RNAs, expanding future studies for identification, biogenesis, and function of these important but understudied transcripts., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023

90. Extending AAV Packaging Cargo through Dual Co-Transduction: Efficient Protein Trans-Splicing at Low Vector Doses.

Author

Ferreira MV, Fernandes S, Almeida AI, Neto S, Mendes JP, Silva RJS, Peixoto C, and Coroadinha AS

Subjects

Inteins, Gene Transfer Techniques, Drug Packaging, Trans-Splicing, Protein Splicing

Abstract

Adeno-associated viral (AAV) vectors represent one of the leading platforms for gene delivery. Nevertheless, their small packaging capacity restricts their use for diseases requiring large-gene delivery. To overcome this, dual-AAV vector systems that rely on protein trans-splicing were developed, with the split-intein Npu DnaE among the most-used. However, the reconstitution efficiency of Npu DnaE is still insufficient, requiring higher vector doses. In this work, two split-inteins, Cfa and Gp41-1, with reportedly superior trans-splicing were evaluated in comparison with Npu DnaE by transient transfections and dual-AAV in vitro co-transductions. Both Cfa and Gp41-1 split-inteins enabled reconstitution rates that were over two-fold higher than Npu DnaE and 100% of protein reconstitution. The impact of different vector preparation qualities in split-intein performances was also evaluated in co-transduction assays. Higher-quality preparations increased split-inteins' performances by three-fold when compared to low-quality preparations (60-75% vs. 20-30% full particles, respectively). Low-quality vector preparations were observed to limit split-gene reconstitutions by inhibiting co-transduction. We show that combining superior split-inteins with higher-quality vector preparations allowed vector doses to be decreased while maintaining high trans-splicing rates. These results show the potential of more-efficient protein-trans-splicing strategies in dual-AAV vector co-transduction, allowing the extension of its use to the delivery of larger therapeutic genes.

Published

2023

91. Trans-amplifying RNA: Translational application in gene therapy.

Author

Lundstrom K

Subjects

Protein Processing, Post-Translational, Trans-Splicing, RNA metabolism, Genetic Therapy

Abstract

Competing Interests: Declaration of interests The author declares no conflict of interest.

Published

2023

92. Post-transcriptional mending of gene sequences: Looking under the hood of mitochondrial gene expression in diplonemids.

Author

Valach, Matus, Moreira, Sandrine, Faktorová, Drahomíra, Lukeš, Julius, and Burger, Gertraud

Published

2016

93. A directed approach for the identification of transcripts harbouring the spliced leader sequence and the effect of trans-splicing knockdown in Schistosoma mansoni

Author

Marina de Moraes Mourao, Maina Bitar, Francisco Pereira Lobo, Ana Paula Peconick, Priscila Grynberg, Francisco Prosdocimi, Michael Waisberg, Gustavo Coutinho Cerqueira, Andrea Mara Macedo, Carlos Renato Machado, Timothy Yoshino, and Gloria Regina Franco

Subjects

spliced leader, trans-splicing, RNA interference, Schistosoma mansoni, Microbiology, QR1-502, Infectious and parasitic diseases, RC109-216

Abstract

Schistosomiasis is a major neglected tropical disease caused by trematodes from the genus Schistosoma. Because schistosomes exhibit a complex life cycle and numerous mechanisms for regulating gene expression, it is believed that spliced leader (SL) trans-splicing could play an important role in the biology of these parasites. The purpose of this study was to investigate the function of trans-splicing in Schistosoma mansoni through analysis of genes that may be regulated by this mechanism and via silencing SL-containing transcripts through RNA interference. Here, we report our analysis of SL transcript-enriched cDNA libraries from different S. mansoni life stages. Our results show that the trans-splicing mechanism is apparently not associated with specific genes, subcellular localisations or life stages. In cross-species comparisons, even though the sets of genes that are subject to SL trans-splicing regulation appear to differ between organisms, several commonly shared orthologues were observed. Knockdown of trans-spliced transcripts in sporocysts resulted in a systemic reduction of the expression levels of all tested trans-spliced transcripts; however, the only phenotypic effect observed was diminished larval size. Further studies involving the findings from this work will provide new insights into the role of trans-splicing in the biology of S. mansoni and other organisms. All Expressed Sequence Tags generated in this study were submitted to dbEST as five different libraries. The accessions for each library and for the individual sequences are as follows: (i) adult worms of mixed sexes (LIBEST_027999: JZ139310 - JZ139779), (ii) female adult worms (LIBEST_028000: JZ139780 - JZ140379), (iii) male adult worms (LIBEST_028001: JZ140380 - JZ141002), (iv) eggs (LIBEST_028002: JZ141003 - JZ141497) and (v) schistosomula (LIBEST_028003: JZ141498 - JZ141974).

Published

2013

94. Group II Introns Generate Functional Chimeric Relaxase Enzymes with Modified Specificities through Exon Shuffling at Both the RNA and DNA Level

Author

Félix LaRoche-Johnston, Rafia Bosan, and Benoit Cousineau

Subjects

Recombinant Fusion Proteins, Retrotransposon, Biology, AcademicSubjects/SCI01180, Exon shuffling, Relaxase, 03 medical and health sciences, Exon, Bacterial Proteins, Enterococcus faecalis, Genetics, Molecular Biology, Gene, Discoveries, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, trans-splicing, 0303 health sciences, Endodeoxyribonucleases, molecular evolution, 030306 microbiology, AcademicSubjects/SCI01130, Intron, RNA, genetic diversity, Lactococcus lactis, Ef.PcfG, Enterococcus faecalis, conjugation, Group II intron, Introns, Lactococcus lactis, Conjugation, Genetic, bacterial genetics, Ll.LtrB

Abstract

Group II introns are large self-splicing RNA enzymes with a broad but somewhat irregular phylogenetic distribution. These ancient retromobile elements are the proposed ancestors of approximately half the human genome, including the abundant spliceosomal introns and non-long terminal repeat retrotransposons. In contrast to their eukaryotic derivatives, bacterial group II introns have largely been considered as harmful selfish mobile retroelements that parasitize the genome of their host. As a challenge to this view, we recently uncovered a new intergenic trans-splicing pathway that generates an assortment of mRNA chimeras. The ability of group II introns to combine disparate mRNA fragments was proposed to increase the genetic diversity of the bacterial host by shuffling coding sequences. Here, we show that the Ll.LtrB and Ef.PcfG group II introns from Lactococcus lactis and Enterococcus faecalis respectively can both use the intergenic trans-splicing pathway to catalyze the formation of chimeric relaxase mRNAs and functional proteins. We demonstrated that some of these compound relaxase enzymes yield gain-of-function phenotypes, being significantly more efficient than their precursor wild-type enzymes at supporting bacterial conjugation. We also found that relaxase enzymes with shuffled functional domains are produced in biologically relevant settings under natural expression levels. Finally, we uncovered examples of lactococcal chimeric relaxase genes with junctions exactly at the intron insertion site. Overall, our work demonstrates that the genetic diversity generated by group II introns, at the RNA level by intergenic trans-splicing and at the DNA level by recombination, can yield new functional enzymes with shuffled exons, which can lead to gain-of-function phenotypes.

Published

2020

95. Therapeutic applications oftrans-splicing

Author

Carin K. Ingemarsdotter, Elizabeth M Hong, and Andrew M. L. Lever

Subjects

0303 health sciences, Invited Review, Genetic enhancement, Trans-splicing, Rational design, Proteins, RNA, General Medicine, Computational biology, Biology, Inteins, Trans-Splicing, 03 medical and health sciences, Exon, 0302 clinical medicine, In vivo, 030220 oncology & carcinogenesis, RNA splicing, Humans, Gene, 030304 developmental biology

Abstract

BackgroundRNA trans-splicing joins exons from different pre-mRNA transcripts to generate a chimeric product. Trans-splicing can also occur at the protein level, with split inteins mediating the ligation of separate gene products to generate a mature protein.Sources of dataComprehensive literature search of published research papers and reviews using Pubmed.Areas of agreementTrans-splicing techniques have been used to target a wide range of diseases in both in vitro and in vivo models, resulting in RNA, protein and functional correction.Areas of controversyOff-target effects can lead to therapeutically undesirable consequences. In vivo efficacy is typically low, and delivery issues remain a challenge.Growing pointsTrans-splicing provides a promising avenue for developing novel therapeutic approaches. However, much more research needs to be done before developing towards preclinical studies.Areas timely for developing researchIncreasing trans-splicing efficacy and specificity by rational design, screening and competitive inhibition of endogenous cis-splicing.

Published

2020

96. Treatment of a Mouse Model of ALS by In Vivo Base Editing

Author

Colin K.W. Lim, Michael Gapinske, Alexandra K. Brooks, Wendy S. Woods, Jackson E. Powell, M. Alejandra Zeballos C., Jackson Winter, Pablo Perez-Pinera, and Thomas Gaj

Subjects

Male, Streptococcus pyogenes, Genetic enhancement, Genetic Vectors, Nonsense mutation, SOD1, Mice, Transgenic, Inteins, Trans-Splicing, Mice, 03 medical and health sciences, Superoxide Dismutase-1, 0302 clinical medicine, CRISPR-Associated Protein 9, Drug Discovery, Genetics, medicine, Animals, Humans, CRISPR, Amyotrophic lateral sclerosis, Molecular Biology, Injections, Spinal, 030304 developmental biology, Gene Editing, Pharmacology, 0303 health sciences, Cas9, business.industry, Amyotrophic Lateral Sclerosis, Neurodegeneration, Dependovirus, medicine.disease, Muscle atrophy, Disease Models, Animal, HEK293 Cells, Treatment Outcome, Codon, Nonsense, 030220 oncology & carcinogenesis, Cancer research, Molecular Medicine, Original Article, medicine.symptom, business

Abstract

Amyotrophic lateral sclerosis (ALS) is a debilitating and fatal disorder that can be caused by mutations in the superoxide dismutase 1 (SOD1) gene. Although ALS is currently incurable, CRISPR base editors hold the potential to treat the disease through their ability to create nonsense mutations that can permanently disable the expression of the mutant SOD1 gene. However, the restrictive carrying capacity of adeno-associated virus (AAV) vectors has limited their therapeutic application. In this study, we establish an intein-mediated trans-splicing system that enables in vivo delivery of cytidine base editors (CBEs) consisting of the widely used Cas9 protein from Streptococcus pyogenes. We show that intrathecal injection of dual AAV particles encoding a split-intein CBE engineered to trans-splice and introduce a nonsense-coding substitution into a mutant SOD1 gene prolonged survival and markedly slowed the progression of disease in the G93A-SOD1 mouse model of ALS. Adult animals treated by this split-intein CRISPR base editor had a reduced rate of muscle atrophy, decreased muscle denervation, improved neuromuscular function, and up to 40% fewer SOD1 immunoreactive inclusions at end-stage mice compared to control mice. This work expands the capabilities of single-base editors and demonstrates their potential for gene therapy.

Published

2020

97. Promiscuous Trans-splicing Activities Revealed by Next Generation Sequencing-based Analysis of 298 Split Inteins

Author

Duhee Bang and Han Na Seo

Subjects

0106 biological sciences, 0303 health sciences, dnaE, Trans-splicing, Biomedical Engineering, Bioengineering, Computational biology, Protein engineering, Biology, 01 natural sciences, Applied Microbiology and Biotechnology, DNA sequencing, 03 medical and health sciences, 010608 biotechnology, RNA splicing, splice, Intein, Gene, 030304 developmental biology, Biotechnology

Abstract

Protein trans-splicing is a naturally occurring process in which two protein fragments are ligated by a reaction between two intein domains, called split inteins. Despite their usefulness in research, the reactivity and structure of only a few split inteins have been studied. We used cell-based kanamycin selection and next-generation sequencing (NGS) to simultaneously measure the splicing reactivity of 298 N-intein–C-intein combinations derived from the DnaE gene of cyanobacteria. Additionally, we confirmed the splicing activities by measuring the growth of cells individually harboring each split intein under kanamycin selection. Overall, the N-intein–C-intein combinations were promiscuous in their trans-splicing activities, although certain combinations did not splice actively. These results and the NGS-based analysis in this research would be helpful for the development of novel split inteins and further understanding of the trans-splicing mechanism.

Published

2020

98. Small Animal PET Imaging of hTERT RNA-Targeted HSV1-tk Gene Expression withTrans-Splicing Ribozyme

Author

Ju Hui Park, Min-Jung Seo, Joo Hyun Kang, Tae Hyun Choi, Kyo Chul Lee, Yong Jin Lee, Kwang Il Kim, Tae Sup Lee, and Seong-Wook Lee

Subjects

0301 basic medicine, Pharmacology, Cancer Research, biology, Chemistry, fungi, Trans-splicing, Ribozyme, RNA, General Medicine, Pet imaging, Cell biology, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Oncology, 030220 oncology & carcinogenesis, Small animal, Gene expression, biology.protein, Radiology, Nuclear Medicine and imaging, Telomerase reverse transcriptase

Abstract

Background: Trans-splicing ribozymes (TSR) are useful anticancer agents targeting cancer-specific transcripts and replacing the RNA to induce anticancer gene expression specifically and selectively...

Published

2020

99. Can Adeno-Associated Viral Vectors Deliver Effectively Large Genes?

Author

Patrizia Tornabene and Ivana Trapani

Subjects

Acquired diseases, viruses, Genetic enhancement, Genetic Vectors, Gene Expression, Biology, Trans-Splicing, Viral vector, 03 medical and health sciences, 0302 clinical medicine, Genome Size, Genetics, Animals, Humans, RNA, Messenger, Transgenes, Molecular Biology, Gene, 030304 developmental biology, 0303 health sciences, Gene Transfer Techniques, Genetic Therapy, Dependovirus, Virology, 030220 oncology & carcinogenesis, Molecular Medicine, Genetic Engineering

Abstract

Gene therapy with adeno-associated viral (AAV) vectors has reached the clinical stage for many inherited and acquired diseases. However, due to a cargo capacity limited to5 kb, AAV-mediated treatment of diseases that require transfer of larger genes still appears elusive. This is a major drawback of a platform that has otherwise been repeatedly found to be safe and effective. Thus, great efforts have been directed toward the identification of strategies to overcome this limitation. Among the most studied approaches is the use of dual vectors, in which a transgene is split across two separate AAV vectors. Mechanisms acting at either the DNA, pre-mRNA, or protein levels have been explored to restore full-length transgene expression in infected cells. Here, we will review them as well as additional strategies developed to deliver large genes with AAV. We discuss the pros and cons of these strategies and the aspects that still need to be addressed.

Published

2020

100. Hypothesis: Trans-splicing Generates Evolutionary Novelty in the Photosynthetic Amoeba Paulinella

Author

Arwa Gabr, Timothy G. Stephens, and Debashish Bhattacharya

Subjects

RNA, Spliced Leader, Rhizaria, Plant Science, Aquatic Science, Amoeba, Biological Evolution, Trans-Splicing

Abstract

Plastid primary endosymbiosis has occurred twice, once in the Archaeplastida ancestor and once in the Paulinella (Rhizaria) lineage. Both events precipitated massive evolutionary changes, including the recruitment and activation of genes that are horizontally acquired (HGT) and the redeployment of existing genes and pathways in novel contexts. Here we address the latter aspect in Paulinella micropora KR01 (hereafter, KR01) that has independently evolved spliced leader (SL) trans-splicing (SLTS) of nuclear-derived transcripts. We investigated the role of this process in gene regulation, novel gene origination, and endosymbiont integration. Our analysis shows that 20% of KR01 genes give rise to transcripts with at least one (but in some cases, multiple) sites of SL addition. This process, which often occurs at canonical cis-splicing acceptor sites (internal introns), results in shorter transcripts that may produce 5'-truncated proteins with novel functions. SL-truncated transcripts fall into four categories that may show: (i) altered protein localization, (ii) altered protein function, structure, or regulation, (iii) loss of valid alternative start codons, preventing translation, or (iv) multiple SL addition sites at the 5'-terminus. The SL RNA genes required for SLTS are putatively absent in the heterotrophic sister lineage of photosynthetic Paulinella species. Moreover, a high proportion of transcripts derived from genes of endosymbiotic gene transfer (EGT) and HGT origin contain SL sequences. We hypothesize that truncation of transcripts by SL addition may facilitate the generation and expression of novel gene variants and that SLTS may have enhanced the activation and fixation of foreign genes in the host genome of the photosynthetic lineages, playing a key role in primary endosymbiont integration.

Published

2022