Highly efficient method for isolation of total RNA from adipose tissue

Susanna Cirera Salicio

doi:10.1186/1756-0500-6-472

Highly efficient method for isolation of total RNA from adipose tissue

Susanna Cirera Salicio

35 Citations (Scopus)

304 Downloads (Pure)

Abstract

Background: RNA extraction is a crucial step for monitoring gene expression. Poor RNA quality (including degradation and remaining impurities) can result in misleading results. Isolation of RNA from animal tissues with high lipid content can be challenging. Especially, it is not trivial to isolate high quality RNA with a reasonable yield from adipose tissue. The aim of this study was to provide an optimized protocol for isolating total RNA from adipose tissue. This was achieved by combining the advantages of the two routinely used methods, TRI Reagent® and miRNeasy. Findings. The miRNeasy method results in cleaner samples but more prone to degradation while the TRI Reagent® method results in samples contaminated with salts and solvents but more intact. The new protocol combines the best of both methods resulting in RNA of high quality and suitable for downstream experiments like RT-qPCR, microarrays and high-throughput sequencing. Conclusions: The current protocol for total RNA isolation from adipose tissue yields sufficient amount of high quality total RNA free of contaminants.

Original language	English
Article number	472
Journal	BMC Research Notes
Volume	6
Number of pages	5
ISSN	1756-0500
DOIs	https://doi.org/10.1186/1756-0500-6-472
Publication status	Published - 18 Nov 2013

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title = "Highly efficient method for isolation of total RNA from adipose tissue",

abstract = "Background: RNA extraction is a crucial step for monitoring gene expression. Poor RNA quality (including degradation and remaining impurities) can result in misleading results. Isolation of RNA from animal tissues with high lipid content can be challenging. Especially, it is not trivial to isolate high quality RNA with a reasonable yield from adipose tissue. The aim of this study was to provide an optimized protocol for isolating total RNA from adipose tissue. This was achieved by combining the advantages of the two routinely used methods, TRI Reagent{\textregistered} and miRNeasy. Findings. The miRNeasy method results in cleaner samples but more prone to degradation while the TRI Reagent{\textregistered} method results in samples contaminated with salts and solvents but more intact. The new protocol combines the best of both methods resulting in RNA of high quality and suitable for downstream experiments like RT-qPCR, microarrays and high-throughput sequencing. Conclusions: The current protocol for total RNA isolation from adipose tissue yields sufficient amount of high quality total RNA free of contaminants.",

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N2 - Background: RNA extraction is a crucial step for monitoring gene expression. Poor RNA quality (including degradation and remaining impurities) can result in misleading results. Isolation of RNA from animal tissues with high lipid content can be challenging. Especially, it is not trivial to isolate high quality RNA with a reasonable yield from adipose tissue. The aim of this study was to provide an optimized protocol for isolating total RNA from adipose tissue. This was achieved by combining the advantages of the two routinely used methods, TRI Reagent® and miRNeasy. Findings. The miRNeasy method results in cleaner samples but more prone to degradation while the TRI Reagent® method results in samples contaminated with salts and solvents but more intact. The new protocol combines the best of both methods resulting in RNA of high quality and suitable for downstream experiments like RT-qPCR, microarrays and high-throughput sequencing. Conclusions: The current protocol for total RNA isolation from adipose tissue yields sufficient amount of high quality total RNA free of contaminants.

AB - Background: RNA extraction is a crucial step for monitoring gene expression. Poor RNA quality (including degradation and remaining impurities) can result in misleading results. Isolation of RNA from animal tissues with high lipid content can be challenging. Especially, it is not trivial to isolate high quality RNA with a reasonable yield from adipose tissue. The aim of this study was to provide an optimized protocol for isolating total RNA from adipose tissue. This was achieved by combining the advantages of the two routinely used methods, TRI Reagent® and miRNeasy. Findings. The miRNeasy method results in cleaner samples but more prone to degradation while the TRI Reagent® method results in samples contaminated with salts and solvents but more intact. The new protocol combines the best of both methods resulting in RNA of high quality and suitable for downstream experiments like RT-qPCR, microarrays and high-throughput sequencing. Conclusions: The current protocol for total RNA isolation from adipose tissue yields sufficient amount of high quality total RNA free of contaminants.

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Highly efficient method for isolation of total RNA from adipose tissue

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