Current Practice in Bicistronic IRES Reporter Use: A Systematic Review

G.G.H. van den Akker; F. Zacchini; B.A.C. Housmans; L. van der Vloet; M.M.J. Caron; L. Montanaro; T.J.M. Welting

doi:10.3390/ijms22105193

Current Practice in Bicistronic IRES Reporter Use: A Systematic Review

G.G.H. van den Akker, F. Zacchini, B.A.C. Housmans, L. van der Vloet, M.M.J. Caron, L. Montanaro, T.J.M. Welting^*

^*Corresponding author for this work

Research output: Contribution to journal › (Systematic) Review article › peer-review

Abstract

Bicistronic reporter assays have been instrumental for transgene expression, understanding of internal ribosomal entry site (IRES) translation, and identification of novel cap-independent translational elements (CITE). We observed a large methodological variability in the use of bicistronic reporter assays and data presentation or normalization procedures. Therefore, we systematically searched the literature for bicistronic IRES reporter studies and analyzed methodological details, data visualization, and normalization procedures. Two hundred fifty-seven publications were identified using our search strategy (published 1994-2020). Experimental studies on eukaryotic adherent cell systems and the cell-free translation assay were included for further analysis. We evaluated the following methodological details for 176 full text articles: the bicistronic reporter design, the cell line or type, transfection methods, and time point of analyses post-transfection. For the cell-free translation assay, we focused on methods of in vitro transcription, type of translation lysate, and incubation times and assay temperature. Data can be presented in multiple ways: raw data from individual cistrons, a ratio of the two, or fold changes thereof. In addition, many different control experiments have been suggested when studying IRES-mediated translation. In addition, many different normalization and control experiments have been suggested when studying IRES-mediated translation. Therefore, we also categorized and summarized their use. Our unbiased analyses provide a representative overview of bicistronic IRES reporter use. We identified parameters that were reported inconsistently or incompletely, which could hamper data reproduction and interpretation. On the basis of our analyses, we encourage adhering to a number of practices that should improve transparency of bicistronic reporter data presentation and improve methodological descriptions to facilitate data replication.

Original language	English
Article number	5193
Number of pages	25
Journal	International Journal of Molecular Sciences
Volume	22
Issue number	10
DOIs	https://doi.org/10.3390/ijms22105193
Publication status	Published - 1 May 2021

Keywords

bicistronic reporter
dicistronic reporter
mRNA translation
ribosome
IRES
systematic review
INTERNAL RIBOSOME-ENTRY
HEPATITIS-C VIRUS
SITE-MEDIATED TRANSLATION
CAP-INDEPENDENT TRANSLATION
5' UNTRANSLATED REGION
MESSENGER-RNA CONTAINS
UP-REGULATES TRANSLATION
CELL-CYCLE REGULATION
TRANS-ACTING FACTORS
5'-UNTRANSLATED REGION

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Cite this

@article{a4e3c10f36214dbfa9c58669324df9f4,

title = "Current Practice in Bicistronic IRES Reporter Use: A Systematic Review",

abstract = "Bicistronic reporter assays have been instrumental for transgene expression, understanding of internal ribosomal entry site (IRES) translation, and identification of novel cap-independent translational elements (CITE). We observed a large methodological variability in the use of bicistronic reporter assays and data presentation or normalization procedures. Therefore, we systematically searched the literature for bicistronic IRES reporter studies and analyzed methodological details, data visualization, and normalization procedures. Two hundred fifty-seven publications were identified using our search strategy (published 1994-2020). Experimental studies on eukaryotic adherent cell systems and the cell-free translation assay were included for further analysis. We evaluated the following methodological details for 176 full text articles: the bicistronic reporter design, the cell line or type, transfection methods, and time point of analyses post-transfection. For the cell-free translation assay, we focused on methods of in vitro transcription, type of translation lysate, and incubation times and assay temperature. Data can be presented in multiple ways: raw data from individual cistrons, a ratio of the two, or fold changes thereof. In addition, many different control experiments have been suggested when studying IRES-mediated translation. In addition, many different normalization and control experiments have been suggested when studying IRES-mediated translation. Therefore, we also categorized and summarized their use. Our unbiased analyses provide a representative overview of bicistronic IRES reporter use. We identified parameters that were reported inconsistently or incompletely, which could hamper data reproduction and interpretation. On the basis of our analyses, we encourage adhering to a number of practices that should improve transparency of bicistronic reporter data presentation and improve methodological descriptions to facilitate data replication.",

keywords = "bicistronic reporter, dicistronic reporter, mRNA translation, ribosome, IRES, systematic review, INTERNAL RIBOSOME-ENTRY, HEPATITIS-C VIRUS, SITE-MEDIATED TRANSLATION, CAP-INDEPENDENT TRANSLATION, 5' UNTRANSLATED REGION, MESSENGER-RNA CONTAINS, UP-REGULATES TRANSLATION, CELL-CYCLE REGULATION, TRANS-ACTING FACTORS, 5'-UNTRANSLATED REGION",

author = "{van den Akker}, G.G.H. and F. Zacchini and B.A.C. Housmans and {van der Vloet}, L. and M.M.J. Caron and L. Montanaro and T.J.M. Welting",

year = "2021",

month = may,

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doi = "10.3390/ijms22105193",

language = "English",

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publisher = "Multidisciplinary Digital Publishing Institute (MDPI)",

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T1 - Current Practice in Bicistronic IRES Reporter Use: A Systematic Review

AU - van den Akker, G.G.H.

AU - Zacchini, F.

AU - Housmans, B.A.C.

AU - van der Vloet, L.

AU - Caron, M.M.J.

AU - Montanaro, L.

AU - Welting, T.J.M.

PY - 2021/5/1

Y1 - 2021/5/1

N2 - Bicistronic reporter assays have been instrumental for transgene expression, understanding of internal ribosomal entry site (IRES) translation, and identification of novel cap-independent translational elements (CITE). We observed a large methodological variability in the use of bicistronic reporter assays and data presentation or normalization procedures. Therefore, we systematically searched the literature for bicistronic IRES reporter studies and analyzed methodological details, data visualization, and normalization procedures. Two hundred fifty-seven publications were identified using our search strategy (published 1994-2020). Experimental studies on eukaryotic adherent cell systems and the cell-free translation assay were included for further analysis. We evaluated the following methodological details for 176 full text articles: the bicistronic reporter design, the cell line or type, transfection methods, and time point of analyses post-transfection. For the cell-free translation assay, we focused on methods of in vitro transcription, type of translation lysate, and incubation times and assay temperature. Data can be presented in multiple ways: raw data from individual cistrons, a ratio of the two, or fold changes thereof. In addition, many different control experiments have been suggested when studying IRES-mediated translation. In addition, many different normalization and control experiments have been suggested when studying IRES-mediated translation. Therefore, we also categorized and summarized their use. Our unbiased analyses provide a representative overview of bicistronic IRES reporter use. We identified parameters that were reported inconsistently or incompletely, which could hamper data reproduction and interpretation. On the basis of our analyses, we encourage adhering to a number of practices that should improve transparency of bicistronic reporter data presentation and improve methodological descriptions to facilitate data replication.

AB - Bicistronic reporter assays have been instrumental for transgene expression, understanding of internal ribosomal entry site (IRES) translation, and identification of novel cap-independent translational elements (CITE). We observed a large methodological variability in the use of bicistronic reporter assays and data presentation or normalization procedures. Therefore, we systematically searched the literature for bicistronic IRES reporter studies and analyzed methodological details, data visualization, and normalization procedures. Two hundred fifty-seven publications were identified using our search strategy (published 1994-2020). Experimental studies on eukaryotic adherent cell systems and the cell-free translation assay were included for further analysis. We evaluated the following methodological details for 176 full text articles: the bicistronic reporter design, the cell line or type, transfection methods, and time point of analyses post-transfection. For the cell-free translation assay, we focused on methods of in vitro transcription, type of translation lysate, and incubation times and assay temperature. Data can be presented in multiple ways: raw data from individual cistrons, a ratio of the two, or fold changes thereof. In addition, many different control experiments have been suggested when studying IRES-mediated translation. In addition, many different normalization and control experiments have been suggested when studying IRES-mediated translation. Therefore, we also categorized and summarized their use. Our unbiased analyses provide a representative overview of bicistronic IRES reporter use. We identified parameters that were reported inconsistently or incompletely, which could hamper data reproduction and interpretation. On the basis of our analyses, we encourage adhering to a number of practices that should improve transparency of bicistronic reporter data presentation and improve methodological descriptions to facilitate data replication.

KW - bicistronic reporter

KW - dicistronic reporter

KW - mRNA translation

KW - ribosome

KW - IRES

KW - systematic review

KW - INTERNAL RIBOSOME-ENTRY

KW - HEPATITIS-C VIRUS

KW - SITE-MEDIATED TRANSLATION

KW - CAP-INDEPENDENT TRANSLATION

KW - 5' UNTRANSLATED REGION

KW - MESSENGER-RNA CONTAINS

KW - UP-REGULATES TRANSLATION

KW - CELL-CYCLE REGULATION

KW - TRANS-ACTING FACTORS

KW - 5'-UNTRANSLATED REGION

U2 - 10.3390/ijms22105193

DO - 10.3390/ijms22105193

M3 - (Systematic) Review article

C2 - 34068921

SN - 1661-6596

VL - 22

JO - International Journal of Molecular Sciences

JF - International Journal of Molecular Sciences

IS - 10

M1 - 5193

ER -