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Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia

Internal ribosome entry site (IRES) sequences have become a valuable tool in the construction of gene transfer and therapeutic vectors for multi-cistronic gene expression from a single mRNA transcript. The optimal conditions for effective use of this sequence to construct a functional expression vec...

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Autores principales: Al-Allaf, Faisal A., Abduljaleel, Zainularifeen, Athar, Mohammad, Taher, Mohiuddin M., Khan, Wajahatullah, Mehmet, Huseyin, Colakogullari, Mukaddes, Apostolidou, Sophia, Bigger, Brian, Waddington, Simon, Coutelle, Charles, Themis, Michael, Al-Ahdal, Mohammed N., Al-Mohanna, Futwan A., Al-Hassnan, Zuhair N., Bouazzaoui, Abdellatif
Formato: Online Artículo Texto
Lenguaje:English
Publicado: KeAi Publishing 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6404380/
https://www.ncbi.nlm.nih.gov/pubmed/30891532
http://dx.doi.org/10.1016/j.ncrna.2018.11.005
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author Al-Allaf, Faisal A.
Abduljaleel, Zainularifeen
Athar, Mohammad
Taher, Mohiuddin M.
Khan, Wajahatullah
Mehmet, Huseyin
Colakogullari, Mukaddes
Apostolidou, Sophia
Bigger, Brian
Waddington, Simon
Coutelle, Charles
Themis, Michael
Al-Ahdal, Mohammed N.
Al-Mohanna, Futwan A.
Al-Hassnan, Zuhair N.
Bouazzaoui, Abdellatif
author_facet Al-Allaf, Faisal A.
Abduljaleel, Zainularifeen
Athar, Mohammad
Taher, Mohiuddin M.
Khan, Wajahatullah
Mehmet, Huseyin
Colakogullari, Mukaddes
Apostolidou, Sophia
Bigger, Brian
Waddington, Simon
Coutelle, Charles
Themis, Michael
Al-Ahdal, Mohammed N.
Al-Mohanna, Futwan A.
Al-Hassnan, Zuhair N.
Bouazzaoui, Abdellatif
author_sort Al-Allaf, Faisal A.
collection PubMed
description Internal ribosome entry site (IRES) sequences have become a valuable tool in the construction of gene transfer and therapeutic vectors for multi-cistronic gene expression from a single mRNA transcript. The optimal conditions for effective use of this sequence to construct a functional expression vector are not precisely defined but it is generally assumed that the internal ribosome entry site dependent expression of the second gene in such as cassette is less efficient than the cap-dependent expression of the first gene. Mainly tailoring inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector further in construction of optimised cassette for gene therapy of familial hypercholesterolemia. We tailored the size of the inter-cistronic spacer sequence at the 5′ region of the internal ribosome entry site sequence using sequential deletions and demonstrated that the expression of the 3′ gene can be significantly increased to similar levels as the cap-dependent expression of the 5’ gene. Maximum expression efficiency of the downstream gene was obtained when the spacer is composed of 18–141 base pairs. In this case a single mRNA transcriptional unit containing both the first and the second Cistron was detected. Whilst constructs with spacer sequences of 216 bp or longer generate a single transcriptional unit containing only the first Cistron. This suggests that long spacers may affect transcription termination. When the spacer is 188 bp, both transcripts were produced simultaneously in most transfected cells, while a fraction of them expressed only the first but not the second gene. Expression analyses of vectors containing optimised cassettes clearly confirm that efficiency of gene transfer and biological activity of the expressed transgenic proteins in the transduced cells can be achieved. Furthermore, Computational analysis was carried out by molecular dynamics (MD) simulation to determine the most emerges as viable containing specific binding site and bridging of 5′ and 3′ ends involving direct RNA-RNA contacts and RNA-protein interactions. These results provide a mechanistic basis for translation stimulation and RNA resembling for the synergistic stimulation of cap-dependent translation.
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spelling pubmed-64043802019-03-19 Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia Al-Allaf, Faisal A. Abduljaleel, Zainularifeen Athar, Mohammad Taher, Mohiuddin M. Khan, Wajahatullah Mehmet, Huseyin Colakogullari, Mukaddes Apostolidou, Sophia Bigger, Brian Waddington, Simon Coutelle, Charles Themis, Michael Al-Ahdal, Mohammed N. Al-Mohanna, Futwan A. Al-Hassnan, Zuhair N. Bouazzaoui, Abdellatif Noncoding RNA Res Article Internal ribosome entry site (IRES) sequences have become a valuable tool in the construction of gene transfer and therapeutic vectors for multi-cistronic gene expression from a single mRNA transcript. The optimal conditions for effective use of this sequence to construct a functional expression vector are not precisely defined but it is generally assumed that the internal ribosome entry site dependent expression of the second gene in such as cassette is less efficient than the cap-dependent expression of the first gene. Mainly tailoring inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector further in construction of optimised cassette for gene therapy of familial hypercholesterolemia. We tailored the size of the inter-cistronic spacer sequence at the 5′ region of the internal ribosome entry site sequence using sequential deletions and demonstrated that the expression of the 3′ gene can be significantly increased to similar levels as the cap-dependent expression of the 5’ gene. Maximum expression efficiency of the downstream gene was obtained when the spacer is composed of 18–141 base pairs. In this case a single mRNA transcriptional unit containing both the first and the second Cistron was detected. Whilst constructs with spacer sequences of 216 bp or longer generate a single transcriptional unit containing only the first Cistron. This suggests that long spacers may affect transcription termination. When the spacer is 188 bp, both transcripts were produced simultaneously in most transfected cells, while a fraction of them expressed only the first but not the second gene. Expression analyses of vectors containing optimised cassettes clearly confirm that efficiency of gene transfer and biological activity of the expressed transgenic proteins in the transduced cells can be achieved. Furthermore, Computational analysis was carried out by molecular dynamics (MD) simulation to determine the most emerges as viable containing specific binding site and bridging of 5′ and 3′ ends involving direct RNA-RNA contacts and RNA-protein interactions. These results provide a mechanistic basis for translation stimulation and RNA resembling for the synergistic stimulation of cap-dependent translation. KeAi Publishing 2018-11-22 /pmc/articles/PMC6404380/ /pubmed/30891532 http://dx.doi.org/10.1016/j.ncrna.2018.11.005 Text en © Research Center, Riyadh, 11211, Saudi Arabia. http://creativecommons.org/licenses/by-nc-nd/4.0/ This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).
spellingShingle Article
Al-Allaf, Faisal A.
Abduljaleel, Zainularifeen
Athar, Mohammad
Taher, Mohiuddin M.
Khan, Wajahatullah
Mehmet, Huseyin
Colakogullari, Mukaddes
Apostolidou, Sophia
Bigger, Brian
Waddington, Simon
Coutelle, Charles
Themis, Michael
Al-Ahdal, Mohammed N.
Al-Mohanna, Futwan A.
Al-Hassnan, Zuhair N.
Bouazzaoui, Abdellatif
Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia
title Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia
title_full Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia
title_fullStr Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia
title_full_unstemmed Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia
title_short Modifying inter-cistronic sequence significantly enhances IRES dependent second gene expression in bicistronic vector: Construction of optimised cassette for gene therapy of familial hypercholesterolemia
title_sort modifying inter-cistronic sequence significantly enhances ires dependent second gene expression in bicistronic vector: construction of optimised cassette for gene therapy of familial hypercholesterolemia
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6404380/
https://www.ncbi.nlm.nih.gov/pubmed/30891532
http://dx.doi.org/10.1016/j.ncrna.2018.11.005
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