cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis

BACKGROUND: Genome-wide gene expression profiling of whole blood is an attractive method for discovery of biomarkers due to its non-invasiveness, simple clinical site processing and rich biological content. Except for a few successes, this technology has not yet matured enough to reach its full pote...

Descripción completa

Detalles Bibliográficos
Autores principales: Parrish, Mark L, Wright, Chris, Rivers, Yarek, Argilla, David, Collins, Heather, Leeson, Brendan, Loboda, Andrey, Nebozhyn, Michael, Marton, Matthew J, Lejnine, Serguei
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Research
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2954848/
https://www.ncbi.nlm.nih.gov/pubmed/20868515
http://dx.doi.org/10.1186/1479-5876-8-87
_version_ 1782187963289960448
author Parrish, Mark L
Wright, Chris
Rivers, Yarek
Argilla, David
Collins, Heather
Leeson, Brendan
Loboda, Andrey
Nebozhyn, Michael
Marton, Matthew J
Lejnine, Serguei
author_facet Parrish, Mark L
Wright, Chris
Rivers, Yarek
Argilla, David
Collins, Heather
Leeson, Brendan
Loboda, Andrey
Nebozhyn, Michael
Marton, Matthew J
Lejnine, Serguei
author_sort Parrish, Mark L
collection PubMed
description BACKGROUND: Genome-wide gene expression profiling of whole blood is an attractive method for discovery of biomarkers due to its non-invasiveness, simple clinical site processing and rich biological content. Except for a few successes, this technology has not yet matured enough to reach its full potential of identifying biomarkers useful for clinical prognostic and diagnostic applications or in monitoring patient response to therapeutic intervention. A variety of technical problems have hampered efforts to utilize this technology for identification of biomarkers. One significant hurdle has been the high and variable concentrations of globin transcripts in whole blood total RNA potentially resulting in non-specific probe binding and high background. In this study, we investigated and quantified the power of three whole blood profiling approaches to detect meaningful biological expression patterns. METHODS: To compare and quantify the impact of different mitigation technologies, we used a globin transcript spike-in strategy to synthetically generate a globin-induced signature and then mitigate it with the three different technologies. Biological differences, in globin transcript spiked samples, were modeled by supplementing with either 1% of liver or 1% brain total RNA. In order to demonstrate the biological utility of a robust globin artifact mitigation strategy in biomarker discovery, we treated whole blood ex vivo with suberoylanilide hydroxamic acid (SAHA) and compared the overlap between the obtained signatures and signatures of a known biomarker derived from SAHA-treated cell lines and PBMCs of SAHA-treated patients. RESULTS: We found cDNA hybridization targets detect at least 20 times more specific differentially expressed signatures (2597) between 1% liver and 1% brain in globin-supplemented samples than the PNA (117) or no treatment (97) method at FDR = 10% and p-value < 3x10-3. In addition, we found that the ex vivo derived gene expression profile was highly concordant with that of the previously identified SAHA pharmacodynamic biomarkers. CONCLUSIONS: We conclude that an amplification method for gene expression profiling employing cDNA targets effectively mitigates the negative impact on data of abundant globin transcripts and greatly improves the ability to identify relevant gene expression based pharmacodynamic biomarkers from whole blood.
format Text
id pubmed-2954848
institution National Center for Biotechnology Information
language English
publishDate 2010
publisher BioMed Central
record_format MEDLINE/PubMed
spelling pubmed-29548482010-10-15 cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis Parrish, Mark L Wright, Chris Rivers, Yarek Argilla, David Collins, Heather Leeson, Brendan Loboda, Andrey Nebozhyn, Michael Marton, Matthew J Lejnine, Serguei J Transl Med Research BACKGROUND: Genome-wide gene expression profiling of whole blood is an attractive method for discovery of biomarkers due to its non-invasiveness, simple clinical site processing and rich biological content. Except for a few successes, this technology has not yet matured enough to reach its full potential of identifying biomarkers useful for clinical prognostic and diagnostic applications or in monitoring patient response to therapeutic intervention. A variety of technical problems have hampered efforts to utilize this technology for identification of biomarkers. One significant hurdle has been the high and variable concentrations of globin transcripts in whole blood total RNA potentially resulting in non-specific probe binding and high background. In this study, we investigated and quantified the power of three whole blood profiling approaches to detect meaningful biological expression patterns. METHODS: To compare and quantify the impact of different mitigation technologies, we used a globin transcript spike-in strategy to synthetically generate a globin-induced signature and then mitigate it with the three different technologies. Biological differences, in globin transcript spiked samples, were modeled by supplementing with either 1% of liver or 1% brain total RNA. In order to demonstrate the biological utility of a robust globin artifact mitigation strategy in biomarker discovery, we treated whole blood ex vivo with suberoylanilide hydroxamic acid (SAHA) and compared the overlap between the obtained signatures and signatures of a known biomarker derived from SAHA-treated cell lines and PBMCs of SAHA-treated patients. RESULTS: We found cDNA hybridization targets detect at least 20 times more specific differentially expressed signatures (2597) between 1% liver and 1% brain in globin-supplemented samples than the PNA (117) or no treatment (97) method at FDR = 10% and p-value < 3x10-3. In addition, we found that the ex vivo derived gene expression profile was highly concordant with that of the previously identified SAHA pharmacodynamic biomarkers. CONCLUSIONS: We conclude that an amplification method for gene expression profiling employing cDNA targets effectively mitigates the negative impact on data of abundant globin transcripts and greatly improves the ability to identify relevant gene expression based pharmacodynamic biomarkers from whole blood. BioMed Central 2010-09-25 /pmc/articles/PMC2954848/ /pubmed/20868515 http://dx.doi.org/10.1186/1479-5876-8-87 Text en Copyright ©2010 Parrish 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 Research
Parrish, Mark L
Wright, Chris
Rivers, Yarek
Argilla, David
Collins, Heather
Leeson, Brendan
Loboda, Andrey
Nebozhyn, Michael
Marton, Matthew J
Lejnine, Serguei
cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
title cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
title_full cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
title_fullStr cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
title_full_unstemmed cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
title_short cDNA targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
title_sort cdna targets improve whole blood gene expression profiling and enhance detection of pharmocodynamic biomarkers: a quantitative platform analysis
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2954848/
https://www.ncbi.nlm.nih.gov/pubmed/20868515
http://dx.doi.org/10.1186/1479-5876-8-87
work_keys_str_mv AT parrishmarkl cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT wrightchris cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT riversyarek cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT argilladavid cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT collinsheather cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT leesonbrendan cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT lobodaandrey cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT nebozhynmichael cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT martonmatthewj cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis
AT lejnineserguei cdnatargetsimprovewholebloodgeneexpressionprofilingandenhancedetectionofpharmocodynamicbiomarkersaquantitativeplatformanalysis

Ejemplares similares