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Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage

BACKGROUND: Simultaneous isolation of nucleic acids and proteins from a single biological sample facilitates meaningful data interpretation and reduces time, cost and sampling errors. This is particularly relevant for rare human and animal specimens, often scarce, and/or irreplaceable. TRIzol(®) and...

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Autores principales: Simões, André ES, Pereira, Diane M, Amaral, Joana D, Nunes, Ana F, Gomes, Sofia E, Rodrigues, Pedro M, Lo, Adrian C, D'Hooge, Rudi, Steer, Clifford J, Thibodeau, Stephen N, Borralho, Pedro M, Rodrigues, Cecília MP
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3620933/
https://www.ncbi.nlm.nih.gov/pubmed/23496794
http://dx.doi.org/10.1186/1471-2164-14-181
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author Simões, André ES
Pereira, Diane M
Amaral, Joana D
Nunes, Ana F
Gomes, Sofia E
Rodrigues, Pedro M
Lo, Adrian C
D'Hooge, Rudi
Steer, Clifford J
Thibodeau, Stephen N
Borralho, Pedro M
Rodrigues, Cecília MP
author_facet Simões, André ES
Pereira, Diane M
Amaral, Joana D
Nunes, Ana F
Gomes, Sofia E
Rodrigues, Pedro M
Lo, Adrian C
D'Hooge, Rudi
Steer, Clifford J
Thibodeau, Stephen N
Borralho, Pedro M
Rodrigues, Cecília MP
author_sort Simões, André ES
collection PubMed
description BACKGROUND: Simultaneous isolation of nucleic acids and proteins from a single biological sample facilitates meaningful data interpretation and reduces time, cost and sampling errors. This is particularly relevant for rare human and animal specimens, often scarce, and/or irreplaceable. TRIzol(®) and TRIzol(®)LS are suitable for simultaneous isolation of RNA, DNA and proteins from the same biological sample. These reagents are widely used for RNA and/or DNA isolation, while reports on their use for protein extraction are limited, attributable to technical difficulties in protein solubilisation. RESULTS: TRIzol(®)LS was used for RNA isolation from 284 human colon cancer samples, including normal colon mucosa, tubulovillous adenomas, and colon carcinomas with proficient and deficient mismatch repair system. TRIzol(®) was used for RNA isolation from human colon cancer cells, from brains of transgenic Alzheimer’s disease mice model, and from cultured mouse cortical neurons. Following RNA extraction, the TRIzol(®)-chloroform fractions from human colon cancer samples and from mouse hippocampus and frontal cortex were stored for 2 years and 3 months, respectively, at −80°C until used for protein isolation. Simple modifications to the TRIzol(®) manufacturer’s protocol, including Urea:SDS solubilization and sonication, allowed improved protein recovery yield compared to the TRIzol(®) manufacturer’s protocol. Following SDS-PAGE and Ponceau and Coomassie staining, recovered proteins displayed wide molecular weight range and staining pattern comparable to those obtainable with commonly used protein extraction protocols. We also show that nuclear and cytosolic proteins can be easily extracted and detected by immunoblotting, and that posttranslational modifications, such as protein phosphorylation, are detectable in proteins recovered from TRIzol(®)-chloroform fractions stored for up to 2 years at −80°C. CONCLUSIONS: We provide a novel approach to improve protein recovery from samples processed for nucleic acid extraction with TRIzol(®) and TRIzol(®)LS compared to the manufacturer`s protocol, allowing downstream immunoblotting and evaluation of steady-state relative protein expression levels. The method was validated in large sets of samples from multiple sources, including human colon cancer and brains of transgenic Alzheimer’s disease mice model, stored in TRIzol(®)-chloroform for up to two years. Collectively, we provide a faster and cheaper alternative to the TRIzol(®) manufacturer`s protein extraction protocol, illustrating the high relevance, and wide applicability, of the present protein isolation method for the immunoblot evaluation of steady-state relative protein expression levels in samples from multiple sources, and following prolonged storage.
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spelling pubmed-36209332013-04-10 Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage Simões, André ES Pereira, Diane M Amaral, Joana D Nunes, Ana F Gomes, Sofia E Rodrigues, Pedro M Lo, Adrian C D'Hooge, Rudi Steer, Clifford J Thibodeau, Stephen N Borralho, Pedro M Rodrigues, Cecília MP BMC Genomics Methodology Article BACKGROUND: Simultaneous isolation of nucleic acids and proteins from a single biological sample facilitates meaningful data interpretation and reduces time, cost and sampling errors. This is particularly relevant for rare human and animal specimens, often scarce, and/or irreplaceable. TRIzol(®) and TRIzol(®)LS are suitable for simultaneous isolation of RNA, DNA and proteins from the same biological sample. These reagents are widely used for RNA and/or DNA isolation, while reports on their use for protein extraction are limited, attributable to technical difficulties in protein solubilisation. RESULTS: TRIzol(®)LS was used for RNA isolation from 284 human colon cancer samples, including normal colon mucosa, tubulovillous adenomas, and colon carcinomas with proficient and deficient mismatch repair system. TRIzol(®) was used for RNA isolation from human colon cancer cells, from brains of transgenic Alzheimer’s disease mice model, and from cultured mouse cortical neurons. Following RNA extraction, the TRIzol(®)-chloroform fractions from human colon cancer samples and from mouse hippocampus and frontal cortex were stored for 2 years and 3 months, respectively, at −80°C until used for protein isolation. Simple modifications to the TRIzol(®) manufacturer’s protocol, including Urea:SDS solubilization and sonication, allowed improved protein recovery yield compared to the TRIzol(®) manufacturer’s protocol. Following SDS-PAGE and Ponceau and Coomassie staining, recovered proteins displayed wide molecular weight range and staining pattern comparable to those obtainable with commonly used protein extraction protocols. We also show that nuclear and cytosolic proteins can be easily extracted and detected by immunoblotting, and that posttranslational modifications, such as protein phosphorylation, are detectable in proteins recovered from TRIzol(®)-chloroform fractions stored for up to 2 years at −80°C. CONCLUSIONS: We provide a novel approach to improve protein recovery from samples processed for nucleic acid extraction with TRIzol(®) and TRIzol(®)LS compared to the manufacturer`s protocol, allowing downstream immunoblotting and evaluation of steady-state relative protein expression levels. The method was validated in large sets of samples from multiple sources, including human colon cancer and brains of transgenic Alzheimer’s disease mice model, stored in TRIzol(®)-chloroform for up to two years. Collectively, we provide a faster and cheaper alternative to the TRIzol(®) manufacturer`s protein extraction protocol, illustrating the high relevance, and wide applicability, of the present protein isolation method for the immunoblot evaluation of steady-state relative protein expression levels in samples from multiple sources, and following prolonged storage. BioMed Central 2013-03-15 /pmc/articles/PMC3620933/ /pubmed/23496794 http://dx.doi.org/10.1186/1471-2164-14-181 Text en Copyright © 2013 Simões 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 Methodology Article
Simões, André ES
Pereira, Diane M
Amaral, Joana D
Nunes, Ana F
Gomes, Sofia E
Rodrigues, Pedro M
Lo, Adrian C
D'Hooge, Rudi
Steer, Clifford J
Thibodeau, Stephen N
Borralho, Pedro M
Rodrigues, Cecília MP
Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage
title Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage
title_full Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage
title_fullStr Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage
title_full_unstemmed Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage
title_short Efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))LS RNA extraction and long-term storage
title_sort efficient recovery of proteins from multiple source samples after trizol((®)) or trizol((®))ls rna extraction and long-term storage
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3620933/
https://www.ncbi.nlm.nih.gov/pubmed/23496794
http://dx.doi.org/10.1186/1471-2164-14-181
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