Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes

Technical advances in the collection of clinical material, such as laser capture microdissection and cell sorting, provide the advantage of yielding more refined and homogenous populations of cells. However, these attractive advantages are counter balanced by the significant difficultly in obtaining...

Descripción completa

Detalles Bibliográficos
Autores principales: Kennedy, Laura, Pauriah, Mahesh, Godfrey, Valerie, Howie, Jacqueline, Dennis, Helen, Crowther, Daniel, Struthers, Allan, Goddard, Catharine, Feuerstein, Giora, Lang, Chim, Miele, Gino
Formato: Texto
Lenguaje:English
Publicado: Public Library of Science 2011
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3062544/
https://www.ncbi.nlm.nih.gov/pubmed/21445340
http://dx.doi.org/10.1371/journal.pone.0017625
_version_ 1782200714263527424
author Kennedy, Laura
Pauriah, Mahesh
Godfrey, Valerie
Howie, Jacqueline
Dennis, Helen
Crowther, Daniel
Struthers, Allan
Goddard, Catharine
Feuerstein, Giora
Lang, Chim
Miele, Gino
author_facet Kennedy, Laura
Pauriah, Mahesh
Godfrey, Valerie
Howie, Jacqueline
Dennis, Helen
Crowther, Daniel
Struthers, Allan
Goddard, Catharine
Feuerstein, Giora
Lang, Chim
Miele, Gino
author_sort Kennedy, Laura
collection PubMed
description Technical advances in the collection of clinical material, such as laser capture microdissection and cell sorting, provide the advantage of yielding more refined and homogenous populations of cells. However, these attractive advantages are counter balanced by the significant difficultly in obtaining adequate nucleic acid yields to allow transcriptomic analyses. Established technologies are available to carry out global transcriptomics using nanograms of input RNA, however, many clinical samples of low cell content would be expected to yield RNA within the picogram range. To fully exploit these clinical samples the challenge of isolating adequate RNA yield directly and generating sufficient microarray probes for global transcriptional profiling from this low level RNA input has been addressed in the current report. We have established an optimised RNA isolation workflow specifically designed to yield maximal RNA from minimal cell numbers. This procedure obtained RNA yield sufficient for carrying out global transcriptional profiling from vascular endothelial cell biopsies, clinical material not previously amenable to global transcriptomic approaches. In addition, by assessing the performance of two linear isothermal probe generation methods at decreasing input levels of good quality RNA we demonstrated robust detection of a class of low abundance transcripts (GPCRs) at input levels within the picogram range, a lower level of RNA input (50 pg) than previously reported for global transcriptional profiling and report the ability to interrogate the transcriptome from only 10 pg of input RNA. By exploiting an optimal RNA isolation workflow specifically for samples of low cell content, and linear isothermal RNA amplification methods for low level RNA input we were able to perform global transcriptomics on valuable and potentially informative clinically derived vascular endothelial biopsies here for the first time. These workflows provide the ability to robustly exploit ever more common clinical samples yielding extremely low cell numbers and RNA yields for global transcriptomics.
format Text
id pubmed-3062544
institution National Center for Biotechnology Information
language English
publishDate 2011
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-30625442011-03-28 Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes Kennedy, Laura Pauriah, Mahesh Godfrey, Valerie Howie, Jacqueline Dennis, Helen Crowther, Daniel Struthers, Allan Goddard, Catharine Feuerstein, Giora Lang, Chim Miele, Gino PLoS One Research Article Technical advances in the collection of clinical material, such as laser capture microdissection and cell sorting, provide the advantage of yielding more refined and homogenous populations of cells. However, these attractive advantages are counter balanced by the significant difficultly in obtaining adequate nucleic acid yields to allow transcriptomic analyses. Established technologies are available to carry out global transcriptomics using nanograms of input RNA, however, many clinical samples of low cell content would be expected to yield RNA within the picogram range. To fully exploit these clinical samples the challenge of isolating adequate RNA yield directly and generating sufficient microarray probes for global transcriptional profiling from this low level RNA input has been addressed in the current report. We have established an optimised RNA isolation workflow specifically designed to yield maximal RNA from minimal cell numbers. This procedure obtained RNA yield sufficient for carrying out global transcriptional profiling from vascular endothelial cell biopsies, clinical material not previously amenable to global transcriptomic approaches. In addition, by assessing the performance of two linear isothermal probe generation methods at decreasing input levels of good quality RNA we demonstrated robust detection of a class of low abundance transcripts (GPCRs) at input levels within the picogram range, a lower level of RNA input (50 pg) than previously reported for global transcriptional profiling and report the ability to interrogate the transcriptome from only 10 pg of input RNA. By exploiting an optimal RNA isolation workflow specifically for samples of low cell content, and linear isothermal RNA amplification methods for low level RNA input we were able to perform global transcriptomics on valuable and potentially informative clinically derived vascular endothelial biopsies here for the first time. These workflows provide the ability to robustly exploit ever more common clinical samples yielding extremely low cell numbers and RNA yields for global transcriptomics. Public Library of Science 2011-03-22 /pmc/articles/PMC3062544/ /pubmed/21445340 http://dx.doi.org/10.1371/journal.pone.0017625 Text en Kennedy et al. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Kennedy, Laura
Pauriah, Mahesh
Godfrey, Valerie
Howie, Jacqueline
Dennis, Helen
Crowther, Daniel
Struthers, Allan
Goddard, Catharine
Feuerstein, Giora
Lang, Chim
Miele, Gino
Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes
title Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes
title_full Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes
title_fullStr Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes
title_full_unstemmed Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes
title_short Global Array-Based Transcriptomics from Minimal Input RNA Utilising an Optimal RNA Isolation Process Combined with SPIA cDNA Probes
title_sort global array-based transcriptomics from minimal input rna utilising an optimal rna isolation process combined with spia cdna probes
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3062544/
https://www.ncbi.nlm.nih.gov/pubmed/21445340
http://dx.doi.org/10.1371/journal.pone.0017625
work_keys_str_mv AT kennedylaura globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT pauriahmahesh globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT godfreyvalerie globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT howiejacqueline globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT dennishelen globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT crowtherdaniel globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT struthersallan globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT goddardcatharine globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT feuersteingiora globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT langchim globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes
AT mielegino globalarraybasedtranscriptomicsfromminimalinputrnautilisinganoptimalrnaisolationprocesscombinedwithspiacdnaprobes

Ejemplares similares