Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100

BACKGROUND: Controlling and limiting the expression of short hairpin RNA (shRNA) by using constitutive or tissue-specific polymerase II (pol II) expression can be a promising strategy to avoid RNAi toxicity. However, to date detailed studies on requirements for effective pol II shRNA expression and...

Descripción completa

Detalles Bibliográficos
Autores principales: Maczuga, Piotr, Koornneef, Annemart, Borel, Florie, Petry, Harald, van Deventer, Sander, Ritsema, Tita, Konstantinova, Pavlina
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2012
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3424168/
https://www.ncbi.nlm.nih.gov/pubmed/22827812
http://dx.doi.org/10.1186/1472-6750-12-42
_version_ 1782241189649448960
author Maczuga, Piotr
Koornneef, Annemart
Borel, Florie
Petry, Harald
van Deventer, Sander
Ritsema, Tita
Konstantinova, Pavlina
author_facet Maczuga, Piotr
Koornneef, Annemart
Borel, Florie
Petry, Harald
van Deventer, Sander
Ritsema, Tita
Konstantinova, Pavlina
author_sort Maczuga, Piotr
collection PubMed
description BACKGROUND: Controlling and limiting the expression of short hairpin RNA (shRNA) by using constitutive or tissue-specific polymerase II (pol II) expression can be a promising strategy to avoid RNAi toxicity. However, to date detailed studies on requirements for effective pol II shRNA expression and processing are not available. We investigated the optimal structural configuration of shRNA molecules, namely: hairpin location, stem length and termination signal required for effective pol II expression and compared it with an alternative strategy of avoiding toxicity by using artificial microRNA (miRNA) scaffolds. RESULTS: Highly effective shRNAs targeting luciferase (shLuc) or Apolipoprotein B100 (shApoB1 and shApoB2) were placed under the control of the pol II CMV promoter and expressed at +5 or +6 nucleotides (nt) with reference to the transcription start site (TSS). Different transcription termination signals (TTS), namely minimal polyadenylation (pA), poly T (T5) and U1 were also used. All pol II- expressed shRNA variants induced mild inhibition of Luciferase reporters carrying specific targets and none of them showed comparable efficacy to their polymerase III-expressed H1-shRNA controls, regardless of hairpin position and termination signal used. Extending hairpin stem length from 20 basepairs (bp) to 21, 25 or 29 bp yielded only slight improvement in the overall efficacy. When shLuc, shApoB1 and shApoB2 were placed in an artificial miRNA scaffold, two out of three were as potent as the H1-shRNA controls. Quantification of small interfering RNA (siRNA) molecules showed that the artificial miRNA constructs expressed less molecules than H1-shRNAs and that CMV-shRNA expressed the lowest amount of siRNA molecules suggesting that RNAi processing in this case is least effective. Furthermore, CMV-miApoB1 and CMV-miApoB2 were as effective as the corresponding H1-shApoB1 and H1-shApoB2 in inhibiting endogenous ApoB mRNA. CONCLUSION: Our results demonstrate that artificial miRNA have a better efficacy profile than shRNA expressed either from H1 or CMV promoter and will be used in the future for RNAi therapeutic development.
format Online
Article
Text
id pubmed-3424168
institution National Center for Biotechnology Information
language English
publishDate 2012
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-34241682012-08-22 Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100 Maczuga, Piotr Koornneef, Annemart Borel, Florie Petry, Harald van Deventer, Sander Ritsema, Tita Konstantinova, Pavlina BMC Biotechnol Research Article BACKGROUND: Controlling and limiting the expression of short hairpin RNA (shRNA) by using constitutive or tissue-specific polymerase II (pol II) expression can be a promising strategy to avoid RNAi toxicity. However, to date detailed studies on requirements for effective pol II shRNA expression and processing are not available. We investigated the optimal structural configuration of shRNA molecules, namely: hairpin location, stem length and termination signal required for effective pol II expression and compared it with an alternative strategy of avoiding toxicity by using artificial microRNA (miRNA) scaffolds. RESULTS: Highly effective shRNAs targeting luciferase (shLuc) or Apolipoprotein B100 (shApoB1 and shApoB2) were placed under the control of the pol II CMV promoter and expressed at +5 or +6 nucleotides (nt) with reference to the transcription start site (TSS). Different transcription termination signals (TTS), namely minimal polyadenylation (pA), poly T (T5) and U1 were also used. All pol II- expressed shRNA variants induced mild inhibition of Luciferase reporters carrying specific targets and none of them showed comparable efficacy to their polymerase III-expressed H1-shRNA controls, regardless of hairpin position and termination signal used. Extending hairpin stem length from 20 basepairs (bp) to 21, 25 or 29 bp yielded only slight improvement in the overall efficacy. When shLuc, shApoB1 and shApoB2 were placed in an artificial miRNA scaffold, two out of three were as potent as the H1-shRNA controls. Quantification of small interfering RNA (siRNA) molecules showed that the artificial miRNA constructs expressed less molecules than H1-shRNAs and that CMV-shRNA expressed the lowest amount of siRNA molecules suggesting that RNAi processing in this case is least effective. Furthermore, CMV-miApoB1 and CMV-miApoB2 were as effective as the corresponding H1-shApoB1 and H1-shApoB2 in inhibiting endogenous ApoB mRNA. CONCLUSION: Our results demonstrate that artificial miRNA have a better efficacy profile than shRNA expressed either from H1 or CMV promoter and will be used in the future for RNAi therapeutic development. BioMed Central 2012-07-24 /pmc/articles/PMC3424168/ /pubmed/22827812 http://dx.doi.org/10.1186/1472-6750-12-42 Text en Copyright ©2012 Maczuga et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Maczuga, Piotr
Koornneef, Annemart
Borel, Florie
Petry, Harald
van Deventer, Sander
Ritsema, Tita
Konstantinova, Pavlina
Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100
title Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100
title_full Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100
title_fullStr Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100
title_full_unstemmed Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100
title_short Optimization and comparison of knockdown efficacy between polymerase II expressed shRNA and artificial miRNA targeting luciferase and Apolipoprotein B100
title_sort optimization and comparison of knockdown efficacy between polymerase ii expressed shrna and artificial mirna targeting luciferase and apolipoprotein b100
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3424168/
https://www.ncbi.nlm.nih.gov/pubmed/22827812
http://dx.doi.org/10.1186/1472-6750-12-42
work_keys_str_mv AT maczugapiotr optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100
AT koornneefannemart optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100
AT borelflorie optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100
AT petryharald optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100
AT vandeventersander optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100
AT ritsematita optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100
AT konstantinovapavlina optimizationandcomparisonofknockdownefficacybetweenpolymeraseiiexpressedshrnaandartificialmirnatargetingluciferaseandapolipoproteinb100

Ejemplares similares