Your search keyword '"SINEUP"' showing total 16 results

1. SINEUP RNA rescues molecular phenotypes associated with CHD8 suppression in autism spectrum disorder model systems

Author

Di Leva, Francesca, Arnoldi, Michele, Santarelli, Stefania, Massonot, Mathieu, Lemée, Marianne Victoria, Bon, Carlotta, Pellegrini, Miguel, Castellini, Maria Elena, Zarantonello, Giulia, Messina, Andrea, Bozzi, Yuri, Bernier, Raphael, Zucchelli, Silvia, Casarosa, Simona, Dassi, Erik, Ronzitti, Giuseppe, Golzio, Christelle, Morandell, Jasmin, Gustincich, Stefano, Espinoza, Stefano, and Biagioli, Marta

Published

2025

2. SINEUP non-coding RNA activity depends on specific N6-methyladenosine nucleotides

Author

Bianca Pierattini, Sabrina D’Agostino, Carlotta Bon, Omar Peruzzo, Andrej Alendar, Azzurra Codino, Gloria Ros, Francesca Persichetti, Remo Sanges, Piero Carninci, Claudio Santoro, Stefano Espinoza, Paola Valentini, Luca Pandolfini, and Stefano Gustincich

Subjects

MT: Non-coding RNAs, SINEUP, lncRNA, RNA therapeutics, m6A, N6-methyladenosine, Therapeutics. Pharmacology, RM1-950

Abstract

SINEUPs are natural and synthetic antisense long non-coding RNAs (lncRNAs) selectively enhancing target mRNAs translation by increasing their association with polysomes. This activity requires two RNA domains: an embedded inverted SINEB2 element acting as effector domain, and an antisense region, the binding domain, conferring target selectivity. SINEUP technology presents several advantages to treat genetic (haploinsufficiencies) and complex diseases restoring the physiological activity of diseased genes and of compensatory pathways. To streamline these applications to the clinic, a better understanding of the mechanism of action is needed. Here we show that natural mouse SINEUP AS Uchl1 and synthetic human miniSINEUP-DJ-1 are N6-methyladenosine (m6A) modified by METTL3 enzyme. Then, we map m6A-modified sites along SINEUP sequence with Nanopore direct RNA sequencing and a reverse transcription assay. We report that m6A removal from SINEUP RNA causes the depletion of endogenous target mRNA from actively translating polysomes, without altering SINEUP enrichment in ribosomal subunit-associated fractions. These results prove that SINEUP activity requires an m6A-dependent step to enhance translation of target mRNAs, providing a new mechanism for m6A translation regulation and strengthening our knowledge of SINEUP-specific mode of action. Altogether these new findings pave the way to a more effective therapeutic application of this well-defined class of lncRNAs.

Published

2023

3. Natural SINEUP RNAs in Autism Spectrum Disorders: RAB11B-AS1 Dysregulation in a Neuronal CHD8 Suppression Model Leads to RAB11B Protein Increase

Author

Giulia Zarantonello, Michele Arnoldi, Michele Filosi, Toma Tebaldi, Giovanni Spirito, Anna Barbieri, Stefano Gustincich, Remo Sanges, Enrico Domenici, Francesca Di Leva, and Marta Biagioli

Subjects

autism spectrum disorders (ASD), CHD8, lncRNA, natural antisense transcript (NAT), SINEUP, post-transcriptional regulation, Genetics, QH426-470

Abstract

CHD8 represents one of the highest confidence genetic risk factors implied in Autism Spectrum Disorders, with most mutations leading to CHD8 haploinsufficiency and the insurgence of specific phenotypes, such as macrocephaly, facial dysmorphisms, intellectual disability, and gastrointestinal complaints. While extensive studies have been conducted on the possible consequences of CHD8 suppression and protein coding RNAs dysregulation during neuronal development, the effects of transcriptional changes of long non-coding RNAs (lncRNAs) remain unclear. In this study, we focused on a peculiar class of natural antisense lncRNAs, SINEUPs, that enhance translation of a target mRNA through the activity of two RNA domains, an embedded transposable element sequence and an antisense region. By looking at dysregulated transcripts following CHD8 knock down (KD), we first identified RAB11B-AS1 as a potential SINEUP RNA for its domain configuration. Then we demonstrated that such lncRNA is able to increase endogenous RAB11B protein amounts without affecting its transcriptional levels. RAB11B has a pivotal role in vesicular trafficking, and mutations on this gene correlate with intellectual disability and microcephaly. Thus, our study discloses an additional layer of molecular regulation which is altered by CHD8 suppression. This represents the first experimental confirmation that naturally occurring SINEUP could be involved in ASD pathogenesis and underscores the importance of dysregulation of functional lncRNAs in neurodevelopment.

Published

2021

4. Natural SINEUP RNAs in Autism Spectrum Disorders: RAB11B-AS1 Dysregulation in a Neuronal CHD8 Suppression Model Leads to RAB11B Protein Increase.

Author

Zarantonello, Giulia, Arnoldi, Michele, Filosi, Michele, Tebaldi, Toma, Spirito, Giovanni, Barbieri, Anna, Gustincich, Stefano, Sanges, Remo, Domenici, Enrico, Di Leva, Francesca, and Biagioli, Marta

Subjects

AUTISM spectrum disorders, LINCRNA, RNA, PROTEINS, INTELLECTUAL disabilities

Abstract

CHD8 represents one of the highest confidence genetic risk factors implied in Autism Spectrum Disorders, with most mutations leading to CHD8 haploinsufficiency and the insurgence of specific phenotypes, such as macrocephaly, facial dysmorphisms, intellectual disability, and gastrointestinal complaints. While extensive studies have been conducted on the possible consequences of CHD8 suppression and protein coding RNAs dysregulation during neuronal development, the effects of transcriptional changes of long non-coding RNAs (lncRNAs) remain unclear. In this study, we focused on a peculiar class of natural antisense lncRNAs, SINEUPs, that enhance translation of a target mRNA through the activity of two RNA domains, an embedded transposable element sequence and an antisense region. By looking at dysregulated transcripts following CHD8 knock down (KD), we first identified RAB11B-AS1 as a potential SINEUP RNA for its domain configuration. Then we demonstrated that such lncRNA is able to increase endogenous RAB11B protein amounts without affecting its transcriptional levels. RAB11B has a pivotal role in vesicular trafficking, and mutations on this gene correlate with intellectual disability and microcephaly. Thus, our study discloses an additional layer of molecular regulation which is altered by CHD8 suppression. This represents the first experimental confirmation that naturally occurring SINEUP could be involved in ASD pathogenesis and underscores the importance of dysregulation of functional lncRNAs in neurodevelopment. [ABSTRACT FROM AUTHOR]

Published

2021

5. Long Noncoding RNAs and Their Applications: Focus on Architectural RNA (arcRNA), a Class of lncRNA

Author

Yamazaki, Tomohiro, Masuda, Seiji, editor, and Izawa, Shingo, editor

Published

2018

6. Improving the expression of anti-IL-2Rα monoclonal antibody in the CHO cells through optimization of the expression vector and translation efficiency.

Author

Hoseinpoor, Reyhaneh, Kazemi, Bahram, Rajabibazl, Masoumeh, and Rahimpour, Azam

Subjects

*CHO cell, *LINCRNA

Abstract

• UCOE element was associated with increased yield of antibody. • UCOE pools had greater number of positive clones and more stable expression. • Clones that stably co-express mAb and its specific SINEUP had more mAb titer. • Stably expressed SINEUP clones had stable long-term expression. • Combined UCOE and SINEUP provided more optimized expression conditions in CHO cells. The growing need for monoclonal antibodies (mAbs) necessitates the development of novel and efficient production approaches. Regulatory elements like ubiquitous chromatin-opening elements (UCOEs) have been employed for improvement of the mAb expression in the Chinese hamster ovary (CHO) cells. SINEUPs are a class of long non-coding RNAs, which can improve the translation of partly overlapping mRNAs. A combination of these two elements might lead to higher production of mAbs. Therefore, the current study was conducted to investigate the effects of SINEUPs and A2UCOE on the expression of an IgG1 in the CHO-K1 cells. Hence, after constructing the mAb, mAb-SINEUP, and mAb-UCOE vectors, four stable cell pools were generated through combining the above vectors. According to the expression analysis, antibody yields were higher in the mAb-SINEUP and mAb-UCOE cell pools compared to the mAb cells. In addition, the cells possessing both SINEUP and UCOE elements provided the best expression. Persistent mAb expression was observed for over 2 months in these cells, whilst the expression was decreased in the mAb pool. SINEUP and UCOE positively influenced the stable mAb expression. It can be concluded that the SINEUP and UCOE enhance the antibody stability and expression level separately and their combination improves the mAb production in the CHO cells. [ABSTRACT FROM AUTHOR]

Published

2020

7. Engineering Translation in Mammalian Cell Factories to Increase Protein Yield: The Unexpected Use of Long Non-Coding SINEUP RNAs

Author

Silvia Zucchelli, Laura Patrucco, Francesca Persichetti, Stefano Gustincich, and Diego Cotella

Subjects

Cell factory, Recombinant protein, Protein translation, Signal peptide, lncRNA, SINEUP, Biotechnology, TP248.13-248.65

Abstract

Mammalian cells are an indispensable tool for the production of recombinant proteins in contexts where function depends on post-translational modifications. Among them, Chinese Hamster Ovary (CHO) cells are the primary factories for the production of therapeutic proteins, including monoclonal antibodies (MAbs). To improve expression and stability, several methodologies have been adopted, including methods based on media formulation, selective pressure and cell- or vector engineering. This review presents current approaches aimed at improving mammalian cell factories that are based on the enhancement of translation. Among well-established techniques (codon optimization and improvement of mRNA secondary structure), we describe SINEUPs, a family of antisense long non-coding RNAs that are able to increase translation of partially overlapping protein-coding mRNAs. By exploiting their modular structure, SINEUP molecules can be designed to target virtually any mRNA of interest, and thus to increase the production of secreted proteins. Thus, synthetic SINEUPs represent a new versatile tool to improve the production of secreted proteins in biomanufacturing processes.

Published

2016

8. The Yin and Yang of nucleic acid-based therapy in the brain.

Author

Gustincich, Stefano, Zucchelli, Silvia, and Mallamaci, Antonello

Subjects

*TREATMENT of neurodegeneration, *NUCLEIC acids, *NON-coding RNA, *HOMEOSTASIS, *GENE expression, *CLINICAL trials, *THERAPEUTICS

Abstract

The post-genomic era has unveiled the existence of a large repertory of non-coding RNAs and repetitive elements that play a fundamental role in cellular homeostasis and dysfunction. These may represent unprecedented opportunities to modify gene expression at the right time in the correct space in vivo , providing an almost unlimited reservoir of new potential pharmacological agents. Hijacking their mode of actions, the druggable genome can be extended to regulatory RNAs and DNA elements in a scalable fashion. Here, we discuss the state-of-the–art of nucleic acid-based drugs to treat neurodegenerative diseases. Beneficial effects can be obtained by inhibiting (Yin) and increasing (Yang) gene expression, depending on the disease and the drug target. Together with the description of the current use of inhibitory RNAs (small inhibitory RNAs and antisense oligonucleotides) in animal models and clinical trials, we discuss the molecular basis and applications of new classes of activatory RNAs at transcriptional (RNAa) and translational (SINEUP) levels. [ABSTRACT FROM AUTHOR]

Published

2017

9. SINEUPs are modular antisense long-non coding RNAs that increase synthesis of target proteins in cells

Author

Silvia eZucchelli, Francesca eFasolo, Roberta eRusso, Laura eCimatti, Laura ePatrucco, Hazuki eTakahashi, Michael H. Jones, Claudio eSantoro, Daniele eSblattero, Diego eCotella, Francesca ePersichetti, Piero eCarninci, and Stefano eGustincich

Subjects

protein expression, long non-coding RNA, antisense, cell lines, SINEUP, Neurosciences. Biological psychiatry. Neuropsychiatry, RC321-571

Abstract

Despite recent efforts in discovering novel long non-coding RNAs (lncRNAs) and unveiling their functions in a wide range of biological processes their applications as biotechnological or therapeutic tools are still at their infancy. We have recently shown that AS Uchl1, a natural lncRNA antisense to the Parkinson’s disease-associated gene Ubiquitin carboxyl-terminal esterase L1 (Uchl1), is able to increase UchL1 protein synthesis at post-transcriptional level. Its activity requires two RNA elements: an embedded inverted SINEB2 sequence to increase translation and the overlapping region to target its sense mRNA. This functional organization is shared with several mouse lncRNAs antisense to protein coding genes. The potential use of AS Uchl1-derived lncRNAs as enhancers of target mRNA translation remains unexplored. Here we define AS Uchl1 as the representative member of a new functional class of natural and synthetic antisense lncRNAs that activate translation. We named this class of RNAs SINEUPs for their requirement of the inverted SINEB2 sequence to UP-regulate translation in a gene-specific manner. The overlapping region is indicated as the Binding Doman (BD) while the embedded inverted SINEB2 element is the Effector Domain (ED). By swapping BD, synthetic SINEUPs are designed targeting mRNAs of interest. SINEUPs function in an array of cell lines and can be efficiently directed towards N-terminally tagged proteins. Their biological activity is retained in a miniaturized version within the range of small RNAs length. Its modular structure was exploited to successfully design synthetic SINEUPs targeting endogenous Parkinson’s disease-associated DJ-1 and proved to be active in different neuronal cell lines.In summary, SINEUPs represent the first scalable tool to increase synthesis of proteins of interest. We propose SINEUPs as reagents for molecular biology experiments, in protein manufacturing as well as in therapy of haploinsufficiencies.

Published

2015

10. Engineering mammalian cell factories with SINEUP noncoding RNAs to improve translation of secreted proteins.

Author

Patrucco, Laura, Chiesa, Andrea, Soluri, Maria Felicia, Fasolo, Francesca, Takahashi, Hazuki, Carninci, Piero, Zucchelli, Silvia, Santoro, Claudio, Gustincich, Stefano, Sblattero, Daniele, and Cotella, Diego

Subjects

*GENETIC engineering, *RNA analysis, *GENETIC translation, *MONOCLONAL antibodies, *CELLULAR signal transduction, MAMMAL cytology

Abstract

Whenever the function of a recombinant protein depends on post-translational processing, mammalian cells become an indispensable tool for their production. This is particularly true for biologics and therapeutic monoclonal antibodies (MAbs). Despite some drawbacks, Chinese Hamster Ovary (CHO) cells are the workhorse for MAbs production in academia and industry. Several methodologies have been adopted to improve expression and stability, including methods based on selective pressure or cell engineering. We have previously identified SINEUPs as a new functional class of natural and synthetic long non-coding RNAs that through the activity of an inverted SINEB2 element are able to promote translation of partially overlapping sense coding mRNAs. Here we show that by taking advantage of their modular structure, synthetic SINEUPs can be designed to increase production of secreted proteins. Furthermore, by experimentally validating antisense to elastin (AS-eln) RNA as a natural SINEUP, we show that SINEUP-mediated control may target extracellular proteins. These results lead us to propose synthetic SINEUPs as new versatile tools to optimize production of secreted proteins in manufacturing pipelines and natural SINEUPs as new regulatory RNAs in the secretory pathways. [ABSTRACT FROM AUTHOR]

Published

2015

11. SINEUPs: A new class of natural and synthetic antisense long non-coding RNAs that activate translation.

Author

Zucchelli, S, Cotella, D, Takahashi, H, Carrieri, C, Cimatti, L, Fasolo, F, Jones, MH, Sblattero, D, Sanges, R, Santoro, C, Persichetti, F, Carninci, P, and Gustincich, S

Published

2015

12. A long non-coding SINEUP RNA boosts semi-stable production of fully human monoclonal antibodies in HEK293E cells

Author

Claudia De Lorenzo, Emanuele Sasso, Nicola Zambrano, Guendalina Froechlich, Alfredo Nicosia, Margherita Passariello, Mariangela Succoio, Debora Latino, Sasso, Emanuele, Latino, Debora, Froechlich, Guendalina, Succoio, Mariangela, Passariello, Margherita, De Lorenzo, Claudia, Nicosia, Alfredo, and Zambrano, Nicola

Subjects

0301 basic medicine, Glycosylation, glycosylation, medicine.drug_class, Immunology, Biology, Monoclonal antibody, scFv, 03 medical and health sciences, chemistry.chemical_compound, lncRNA, SINEUP, Peptide Library, Cell Line, Tumor, Claudin-1, medicine, Humans, Immunology and Allergy, monoclonal antibodie, antibody production, IgG4, Antibodies, Monoclonal, RNA, Virology, Antibody production, HEK293 Cells, 030104 developmental biology, Gene Expression Regulation, chemistry, CLDN1, HEK293E, Immunoglobulin Light Chains, RNA, Long Noncoding, Immunoglobulin Heavy Chains

Abstract

Use of monoclonal antibodies is emerging as a highly promising and fast-developing scenario for innovative treatment of viral, autoimmune and tumour diseases. The search for diagnostic and therapeutic antibodies currently depends on in vitro screening approaches, such as phage and yeast display technologies. Antibody production still represents a critical step for preclinical and clinical evaluations. Accordingly, improving production of monoclonal antibodies represents an opportunity, to facilitate downstream target validations. SINEUP RNAs are long non-coding transcripts, possessing the ability to enhance translation of selected mRNAs. We applied SINEUP technology to semi-stable production of monoclonal antibodies in HEK293E cells, which allows for episomal propagation of the expression vectors encoding the heavy and light chains of IgGs. Co-expression of SINEUP RNA with mRNAs encoding heavy and light chains of IgG4s was able to increase the production of different anti-CLDN1 antibodies up to three-fold. Improved production of monoclonal antibodies was achieved both in transiently transfected HEK293E cells and in cellular clones with stable expression of the SINEUP. Compared to antibody preparations obtained under standard conditions, the anti-CLDN1 IgG4s produced in the presence of the SINEUP transcript showed unaltered post-translational modifications, and retained the ability to recognize their target. We thus propose SINEUP technology as a valuable tool to enhance semi-stable antibody production in human cell lines.

Published

2018

13. SINEUP Non-coding RNA Targeting GDNF Rescues Motor Deficits and Neurodegeneration in a Mouse Model of Parkinson's Disease

Author

Stefano Espinoza, Federico Mingozzi, Piero Carninci, Giuseppe Ronzitti, Omar Peruzzo, Francesca Managò, Claudio Santoro, Francesco Papaleo, Margherita Scarpato, Devid Damiani, Stefano Gustincich, Silvia Zucchelli, Andrea Contestabile, Maddalena Mereu, CEA Le Ripault (CEA Le Ripault), Direction des Applications Militaires (DAM), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA), Dipartimento di Genetica e Biologia Molecolare, Università degli Studi di Roma 'La Sapienza' = Sapienza University [Rome] (UNIROMA), Centro di Ricerca in Neurobiologia-D. Bovet, Approches génétiques intégrées et nouvelles thérapies pour les maladies rares (INTEGRARE), Université d'Évry-Val-d'Essonne (UEVE)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Paris-Saclay-Généthon, and Università degli Studi di Roma 'La Sapienza' = Sapienza University [Rome]

Subjects

Parkinson's disease, RNA, Untranslated, animal diseases, [SDV]Life Sciences [q-bio], non-coding RNA, Pharmacology, Mice, 0302 clinical medicine, Neurotrophic factors, Drug Discovery, Sense (molecular biology), Glial cell line-derived neurotrophic factor, Motor Neurons, 0303 health sciences, Neurodegeneration, Gene Transfer Techniques, Long-term potentiation, Neurodegenerative Diseases, Parkinson Disease, AAV, Dependovirus, Immunohistochemistry, GDNF, gene therapy, 3. Good health, Phenotype, 030220 oncology & carcinogenesis, Molecular Medicine, RNA Interference, Original Article, medicine.drug, Genetic Vectors, Biology, 03 medical and health sciences, Neurochemical, SINEUP, Dopamine, Genetics, medicine, Animals, Humans, Glial Cell Line-Derived Neurotrophic Factor, Molecular Biology, 030304 developmental biology, urogenital system, Dopaminergic Neurons, medicine.disease, Corpus Striatum, Disease Models, Animal, Gene Expression Regulation, nervous system, biology.protein, Parkinson’s disease

Abstract

Glial cell-derived neurotrophic factor (GDNF) has a potent action in promoting the survival of dopamine (DA) neurons. Several studies indicate that increasing GDNF levels may be beneficial for the treatment of Parkinson’s disease (PD) by reducing neurodegeneration of DA neurons. Despite a plethora of preclinical studies showing GDNF efficacy in PD animal models, its application in humans remains questionable for its poor efficacy and side effects due to its uncontrolled, ectopic expression. Here we took advantage of SINEUPs, a new class of antisense long non-coding RNA, that promote translation of partially overlapping sense protein-coding mRNAs with no effects on their mRNA levels. By synthesizing a SINEUP targeting Gdnf mRNA, we were able to increase endogenous GDNF protein levels by about 2-fold. Adeno-associated virus (AAV)9-mediated delivery in the striatum of wild-type (WT) mice led to an increase of endogenous GDNF protein for at least 6 months and the potentiation of the DA system’s functions while showing no side effects. Furthermore, SINEUP-GDNF was able to ameliorate motor deficits and neurodegeneration of DA neurons in a PD neurochemical mouse model. Our data indicate that SINEUP-GDNF could represent a new strategy to increase endogenous GDNF protein levels in a more physiological manner for therapeutic treatments of PD., Espinoza and colleagues demonstrate that a SINEUP non-coding RNA targeting GDNF mRNA can increase GDNF protein levels in vivo for several months after viral delivery. They also show that SINEUP-GDNF ameliorates motor deficits and neurodegeneration of dopamine neurons in a mouse model of Parkinson’s disease.

Published

2020

14. Design and Delivery of SINEUP: A New Modular Tool to Increase Protein Translation.

Author

Arnoldi M, Zarantonello G, Espinoza S, Gustincich S, Di Leva F, and Biagioli M

Subjects

Animals, Mice, RNA, Antisense genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Short Interspersed Nucleotide Elements, Protein Biosynthesis, RNA, Long Noncoding genetics, RNA, Long Noncoding metabolism

Abstract

SINEUP is a new class of long non-coding RNAs (lncRNAs) which contain an inverted Short Interspersed Nuclear Element (SINE) B2 element (invSINEB2) necessary to specifically upregulate target gene translation. Originally identified in the mouse AS-Uchl1 (antisense Ubiquitin carboxyl-terminal esterase L1) locus, natural SINEUP molecules are oriented head to head to their sense protein coding, target gene (Uchl1, in this example). Peculiarly, SINEUP is able to augment, in a specific and controlled way, the expression of the target protein, with no alteration of target mRNA levels. SINEUP is characterized by a modular structure with the Binding Domain (BD) providing specificity to the target transcript and an effector domain (ED)-containing the invSINEB2 element-able to promote the loading to the heavy polysomes of the target mRNA. Since the understanding of its modular structure in the endogenous AS-Uchl1 ncRNA, synthetic SINEUP molecules have been developed by creating a specific BD for the gene of interest and placing it upstream the invSINEB2 ED. Synthetic SINEUP is thus a novel molecular tool that potentially may be used for any industrial or biomedical application to enhance protein production, also as possible therapeutic strategy in haploinsufficiency-driven disorders.Here, we describe a detailed protocol to (1) design a specific BD directed to a gene of interest and (2) assemble and clone it with the ED to obtain a functional SINEUP molecule. Then, we provide guidelines to efficiently deliver SINEUP into mammalian cells and evaluate its ability to effectively upregulate target protein translation., (© 2022. The Author(s).)

Published

2022

15. Engineering Translation in Mammalian Cell Factories to Increase Protein Yield: The Unexpected Use of Long Non-Coding SINEUP RNAs

Author

Stefano Gustincich, Francesca Persichetti, Laura Patrucco, Silvia Zucchelli, and Diego Cotella

Subjects

0301 basic medicine, Signal peptide, CHO, Cell, Biochemistry, lncRNA, long non-coding RNA, lncRNA, Structural Biology, Settore BIO/13 - Biologia Applicata, CHO, Chinese hamster ovary, Cell factory, ER, Endoplasmic reticulum, MAb, monoclonal antibody, Protein translation, Recombinant protein, SINE, short interspersed nuclear element, SINEUP, SME, small and medium-sized enterprise, SP, Signal peptide, SP, long non-coding RNA, Chinese hamster ovary cell, SME, Translation (biology), Computer Science Applications, medicine.anatomical_structure, short interspersed nuclear element, Biotechnology, MAb, lcsh:Biotechnology, Biophysics, Computational biology, Biology, 03 medical and health sciences, lcsh:TP248.13-248.65, Genetics, medicine, Biomanufacturing, Messenger RNA, small and medium-sized enterprise, Molecular biology, Chinese hamster ovary, SINE, 030104 developmental biology, Secretory protein, ER, monoclonal antibody, Short Survey, Function (biology), Endoplasmic reticulum

Abstract

Mammalian cells are an indispensable tool for the production of recombinant proteins in contexts where function depends on post-translational modifications. Among them, Chinese Hamster Ovary (CHO) cells are the primary factories for the production of therapeutic proteins, including monoclonal antibodies (MAbs). To improve expression and stability, several methodologies have been adopted, including methods based on media formulation, selective pressure and cell- or vector engineering. This review presents current approaches aimed at improving mammalian cell factories that are based on the enhancement of translation. Among well-established techniques (codon optimization and improvement of mRNA secondary structure), we describe SINEUPs, a family of antisense long non-coding RNAs that are able to increase translation of partially overlapping protein-coding mRNAs. By exploiting their modular structure, SINEUP molecules can be designed to target virtually any mRNA of interest, and thus to increase the production of secreted proteins. Thus, synthetic SINEUPs represent a new versatile tool to improve the production of secreted proteins in biomanufacturing processes.

Published

2016

16. SINEUP Non-coding RNA Targeting GDNF Rescues Motor Deficits and Neurodegeneration in a Mouse Model of Parkinson's Disease.

Author

Espinoza S, Scarpato M, Damiani D, Managò F, Mereu M, Contestabile A, Peruzzo O, Carninci P, Santoro C, Papaleo F, Mingozzi F, Ronzitti G, Zucchelli S, and Gustincich S

Subjects

Animals, Corpus Striatum metabolism, Corpus Striatum pathology, Dependovirus genetics, Disease Models, Animal, Dopaminergic Neurons metabolism, Gene Expression Regulation, Gene Transfer Techniques, Genetic Vectors genetics, Glial Cell Line-Derived Neurotrophic Factor metabolism, Humans, Immunohistochemistry, Mice, Motor Neurons pathology, Neurodegenerative Diseases genetics, Neurodegenerative Diseases metabolism, Neurodegenerative Diseases pathology, Parkinson Disease metabolism, Parkinson Disease pathology, Phenotype, Glial Cell Line-Derived Neurotrophic Factor genetics, Motor Neurons metabolism, Parkinson Disease genetics, RNA Interference, RNA, Untranslated genetics

Abstract

Glial cell-derived neurotrophic factor (GDNF) has a potent action in promoting the survival of dopamine (DA) neurons. Several studies indicate that increasing GDNF levels may be beneficial for the treatment of Parkinson's disease (PD) by reducing neurodegeneration of DA neurons. Despite a plethora of preclinical studies showing GDNF efficacy in PD animal models, its application in humans remains questionable for its poor efficacy and side effects due to its uncontrolled, ectopic expression. Here we took advantage of SINEUPs, a new class of antisense long non-coding RNA, that promote translation of partially overlapping sense protein-coding mRNAs with no effects on their mRNA levels. By synthesizing a SINEUP targeting Gdnf mRNA, we were able to increase endogenous GDNF protein levels by about 2-fold. Adeno-associated virus (AAV)9-mediated delivery in the striatum of wild-type (WT) mice led to an increase of endogenous GDNF protein for at least 6 months and the potentiation of the DA system's functions while showing no side effects. Furthermore, SINEUP-GDNF was able to ameliorate motor deficits and neurodegeneration of DA neurons in a PD neurochemical mouse model. Our data indicate that SINEUP-GDNF could represent a new strategy to increase endogenous GDNF protein levels in a more physiological manner for therapeutic treatments of PD., (Copyright © 2019 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2020