DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli

BACKGROUND: Manufacturing large quantities of recombinant RNAs by overexpression in a bacterial host is hampered by their instability in intracellular environment. To overcome this problem, an RNA of interest can be fused into a stable bacterial RNA for the resulting chimeric construct to accumulate...

Descripción completa

Detalles Bibliográficos
Autores principales: Liu, Yamei, Stepanov, Victor G, Strych, Ulrich, Willson, Richard C, Jackson, George W, Fox, George E
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3019158/
https://www.ncbi.nlm.nih.gov/pubmed/21134283
http://dx.doi.org/10.1186/1472-6750-10-85
_version_ 1782196173024526336
author Liu, Yamei
Stepanov, Victor G
Strych, Ulrich
Willson, Richard C
Jackson, George W
Fox, George E
author_facet Liu, Yamei
Stepanov, Victor G
Strych, Ulrich
Willson, Richard C
Jackson, George W
Fox, George E
author_sort Liu, Yamei
collection PubMed
description BACKGROUND: Manufacturing large quantities of recombinant RNAs by overexpression in a bacterial host is hampered by their instability in intracellular environment. To overcome this problem, an RNA of interest can be fused into a stable bacterial RNA for the resulting chimeric construct to accumulate in the cytoplasm to a sufficiently high level. Being supplemented with cost-effective procedures for isolation of the chimera from cells and recovery of the recombinant RNA from stabilizing scaffold, this strategy might become a viable alternative to the existing methods of chemical or enzymatic RNA synthesis. RESULTS: Sequence encoding a 71-nucleotide recombinant RNA was inserted into a plasmid-borne deletion mutant of the Vibrio proteolyticus 5S rRNA gene in place of helix III - loop C segment of the original 5S rRNA. After transformation into Escherichia coli, the chimeric RNA (3×pen aRNA) was expressed constitutively from E. coli rrnB P1 and P2 promoters. The RNA chimera accumulated to levels that exceeded those of the host's 5S rRNA. A novel method relying on liquid-solid partitioning of cellular constituents was developed for isolation of total RNA from bacterial cells. This protocol avoids toxic chemicals, and is therefore more suitable for large scale RNA purification than traditional methods. A pair of biotinylated 8-17 DNAzymes was used to bring about the quantitative excision of the 71-nt recombinant RNA from the chimera. The recombinant RNA was isolated by sequence-specific capture on beads with immobilized complementary deoxyoligonucleotide, while DNAzymes were recovered by biotin affinity chromatography for reuse. CONCLUSIONS: The feasibility of a fermentation-based approach for manufacturing large quantities of small RNAs in vivo using a "5S rRNA scaffold" strategy is demonstrated. The approach provides a route towards an economical method for the large-scale production of small RNAs including shRNAs, siRNAs and aptamers for use in clinical and biomedical research.
format Text
id pubmed-3019158
institution National Center for Biotechnology Information
language English
publishDate 2010
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-30191582011-01-12 DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli Liu, Yamei Stepanov, Victor G Strych, Ulrich Willson, Richard C Jackson, George W Fox, George E BMC Biotechnol Research Article BACKGROUND: Manufacturing large quantities of recombinant RNAs by overexpression in a bacterial host is hampered by their instability in intracellular environment. To overcome this problem, an RNA of interest can be fused into a stable bacterial RNA for the resulting chimeric construct to accumulate in the cytoplasm to a sufficiently high level. Being supplemented with cost-effective procedures for isolation of the chimera from cells and recovery of the recombinant RNA from stabilizing scaffold, this strategy might become a viable alternative to the existing methods of chemical or enzymatic RNA synthesis. RESULTS: Sequence encoding a 71-nucleotide recombinant RNA was inserted into a plasmid-borne deletion mutant of the Vibrio proteolyticus 5S rRNA gene in place of helix III - loop C segment of the original 5S rRNA. After transformation into Escherichia coli, the chimeric RNA (3×pen aRNA) was expressed constitutively from E. coli rrnB P1 and P2 promoters. The RNA chimera accumulated to levels that exceeded those of the host's 5S rRNA. A novel method relying on liquid-solid partitioning of cellular constituents was developed for isolation of total RNA from bacterial cells. This protocol avoids toxic chemicals, and is therefore more suitable for large scale RNA purification than traditional methods. A pair of biotinylated 8-17 DNAzymes was used to bring about the quantitative excision of the 71-nt recombinant RNA from the chimera. The recombinant RNA was isolated by sequence-specific capture on beads with immobilized complementary deoxyoligonucleotide, while DNAzymes were recovered by biotin affinity chromatography for reuse. CONCLUSIONS: The feasibility of a fermentation-based approach for manufacturing large quantities of small RNAs in vivo using a "5S rRNA scaffold" strategy is demonstrated. The approach provides a route towards an economical method for the large-scale production of small RNAs including shRNAs, siRNAs and aptamers for use in clinical and biomedical research. BioMed Central 2010-12-06 /pmc/articles/PMC3019158/ /pubmed/21134283 http://dx.doi.org/10.1186/1472-6750-10-85 Text en Copyright ©2010 Liu et al; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (<url>http://creativecommons.org/licenses/by/2.0</url>), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Liu, Yamei
Stepanov, Victor G
Strych, Ulrich
Willson, Richard C
Jackson, George W
Fox, George E
DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli
title DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli
title_full DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli
title_fullStr DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli
title_full_unstemmed DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli
title_short DNAzyme-mediated recovery of small recombinant RNAs from a 5S rRNA-derived chimera expressed in Escherichia coli
title_sort dnazyme-mediated recovery of small recombinant rnas from a 5s rrna-derived chimera expressed in escherichia coli
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3019158/
https://www.ncbi.nlm.nih.gov/pubmed/21134283
http://dx.doi.org/10.1186/1472-6750-10-85
work_keys_str_mv AT liuyamei dnazymemediatedrecoveryofsmallrecombinantrnasfroma5srrnaderivedchimeraexpressedinescherichiacoli
AT stepanovvictorg dnazymemediatedrecoveryofsmallrecombinantrnasfroma5srrnaderivedchimeraexpressedinescherichiacoli
AT strychulrich dnazymemediatedrecoveryofsmallrecombinantrnasfroma5srrnaderivedchimeraexpressedinescherichiacoli
AT willsonrichardc dnazymemediatedrecoveryofsmallrecombinantrnasfroma5srrnaderivedchimeraexpressedinescherichiacoli
AT jacksongeorgew dnazymemediatedrecoveryofsmallrecombinantrnasfroma5srrnaderivedchimeraexpressedinescherichiacoli
AT foxgeorgee dnazymemediatedrecoveryofsmallrecombinantrnasfroma5srrnaderivedchimeraexpressedinescherichiacoli

Ejemplares similares