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

Silvia Zucchelli; Francesca Fasolo; Roberta Russo; Laura Cimatti; Laura Patrucco; Hazuki Takahashi; Michael H. Jones; Claudio Santoro; Daniele Sblattero; Diego Cotella; Francesca Persichetti; Piero Carninci; Stefano Gustincich

doi:10.3389/fncel.2015.00174

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

Silvia Zucchelli
, Francesca Fasolo
, Roberta Russo
, Laura Cimatti
, Laura Patrucco
, Hazuki Takahashi
, Michael H. Jones
, Claudio Santoro
, Daniele Sblattero
, Diego Cotella
, Francesca Persichetti
, Piero Carninci
, Stefano Gustincich

Department of Health Sciences

Research output: Contribution to journal › Article › peer-review

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 toward 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.

Original language	English
Journal	Frontiers in Cellular Neuroscience
Volume	9
Issue number	MAY
DOIs	https://doi.org/10.3389/fncel.2015.00174
Publication status	Published - 13 May 2015

Keywords

Antisense
Cell lines
Long non-coding RNA
Protein expression
SINEUP

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10.3389/fncel.2015.00174

Cite this

Zucchelli, S., Fasolo, F., Russo, R., Cimatti, L., Patrucco, L., Takahashi, H., Jones, M. H., Santoro, C., Sblattero, D., Cotella, D., Persichetti, F., Carninci, P., & Gustincich, S. (2015). SINEUPs are modular antisense long non-coding RNAs that increase synthesis of target proteins in cells. Frontiers in Cellular Neuroscience, 9(MAY). https://doi.org/10.3389/fncel.2015.00174

@article{c92c0080d47b44babd93d9dc1315a252,

title = "SINEUPs are modular antisense long non-coding RNAs that increase synthesis of target proteins in cells",

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 toward 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.",

keywords = "Antisense, Cell lines, Long non-coding RNA, Protein expression, SINEUP",

author = "Silvia Zucchelli and Francesca Fasolo and Roberta Russo and Laura Cimatti and Laura Patrucco and Hazuki Takahashi and Jones, \{Michael H.\} and Claudio Santoro and Daniele Sblattero and Diego Cotella and Francesca Persichetti and Piero Carninci and Stefano Gustincich",

note = "Publisher Copyright: {\textcopyright} 2015 Zucchelli, Fasolo, Russo, Cimatti, Patrucco, Takahashi, Jones, Santoro, Sblattero, Cotella, Persichetti, Carninci and Gustincich.",

year = "2015",

month = may,

day = "13",

doi = "10.3389/fncel.2015.00174",

language = "English",

volume = "9",

journal = "Frontiers in Cellular Neuroscience",

issn = "1662-5102",

publisher = "Frontiers Media SA",

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Zucchelli, S, Fasolo, F, Russo, R, Cimatti, L, Patrucco, L, Takahashi, H, Jones, MH, Santoro, C, Sblattero, D, Cotella, D , Persichetti, F, Carninci, P & Gustincich, S 2015, 'SINEUPs are modular antisense long non-coding RNAs that increase synthesis of target proteins in cells', Frontiers in Cellular Neuroscience, vol. 9, no. MAY. https://doi.org/10.3389/fncel.2015.00174

TY - JOUR

T1 - SINEUPs are modular antisense long non-coding RNAs that increase synthesis of target proteins in cells

AU - Zucchelli, Silvia

AU - Fasolo, Francesca

AU - Russo, Roberta

AU - Cimatti, Laura

AU - Patrucco, Laura

AU - Takahashi, Hazuki

AU - Jones, Michael H.

AU - Santoro, Claudio

AU - Sblattero, Daniele

AU - Cotella, Diego

AU - Persichetti, Francesca

AU - Carninci, Piero

AU - Gustincich, Stefano

PY - 2015/5/13

Y1 - 2015/5/13

N2 - 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 toward 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.

AB - 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 toward 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.

KW - Antisense

KW - Cell lines

KW - Long non-coding RNA

KW - Protein expression

KW - SINEUP

UR - https://www.scopus.com/pages/publications/84929603662

U2 - 10.3389/fncel.2015.00174

DO - 10.3389/fncel.2015.00174

M3 - Article

SN - 1662-5102

VL - 9

JO - Frontiers in Cellular Neuroscience

JF - Frontiers in Cellular Neuroscience

IS - MAY

ER -

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

Abstract

Keywords

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