Quality-Controlled Measurement Methods for Quantification of Variations in Transcript Abundance in Whole Blood Samples from Healthy Volunteers

Peters, Elizabeth H.; Rojas-Caro, Sandra; Brigell, Mitchell; Zahorchak, Robert J.; Etages, Shelley Ann des; Ruppel, Patricia L.; Knight, Charles Robert; Austermiller, Bradley; Graham, Myrna C.; Wowk, Steve; Banks, S M; Madabusi, Lakshmi V.; Turk, Patrick W.; Wilder, Donna M.; Kempfer, Carole; Osborn, Terry W.; Willey, James C.

doi:10.1373/clinchem.2006.078154

Cited by 5 publications

(7 citation statements)

References 14 publications

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“…The same conclusion was reached recently in an evaluation of QC parameters in a setting of clinical laboratory tests (19 ). Almost half (43%) of the total variation was due to interindividual variation.…”

Section: Component Of Biological Variation In Gene Expression But Insupporting

confidence: 77%

“…Recently, Peters et al examined interindividual and intraindividual variation in gene expression in blood samples (19 ). They used standardized reverse transcription-PCR analysis to measure the expression of 19 marker genes.…”

mentioning

confidence: 99%

“…Interindividual variation accounted for almost half of the total variance and was the major component of biological variation; however, the magnitude of the interindividual variation in these 19 marker genes varied over a 4-fold range, with CVs ranging from 10% to 40%. Markers with lower interindividual variation were more informative than those with high variation and had a higher individuality index (17,19 ).…”

mentioning

confidence: 99%

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Interindividual and Interethnic Variation in Genomewide Gene Expression: Insights into the Biological Variation of Gene Expression and Clinical Implications

Fan¹,

Liao²,

et al. 2009

Clinical Chemistry

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Background: Analysis of gene expression in peripheral blood samples is increasingly being applied in biomarker studies of disease diagnosis and prognosis. Although knowledge of interindividual and interethnic variation in gene expression is required to set ethnicity-specific reference intervals and to select reference genes and preferred markers from a list of candidate genes, few studies have attempted to characterize such biological variation on a genomewide scale. Methods: The genomewide expression profiles of 11 355 transcripts expressed among 210 multiethnic individuals of the HapMap project were obtained and analyzed; 4 replicates were included for each sample. The total biological CV in gene expression (CVb) was partitioned into interindividual (CVg), inter-ethnic group (CVe), and residual components by random-effects mixed models. Results: CVg was the major component of CVb, and the differences among transcripts were large (up to 38%). Distinct groups of genes were characterized by CV values and expression levels. Of the genes with lowest biological variation (CVb < 1.5%), 35 genes were highly expressed, whereas 32 had intermediate or low expression. Although CVg was almost always greater than CVe, we identified 10 genes in which ethnic variation predominated (range, 8%–18%). On the other hand, 17 annotated genes were highly variable with CVg values ranging between 15% and 38%. Conclusions: Genomewide analysis of gene expression variation demonstrated biological differences among transcripts. Transcripts with the least biological variation are better candidates for reference genes, whereas those with low interindividual variation may be good disease markers. The presence of interethnic variation suggests that ethnicity-specific reference intervals may be necessary.

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Section: Component Of Biological Variation In Gene Expression But Insupporting

confidence: 77%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Interindividual and Interethnic Variation in Genomewide Gene Expression: Insights into the Biological Variation of Gene Expression and Clinical Implications

Fan¹,

Liao²,

et al. 2009

Clinical Chemistry

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“…After incubation of PAXgene tubes at room temperature for 2 hours, the samples were stored frozen at −80 °C. The samples were shipped to Asuragen (Austin, TX) for total RNA purifi cation, similar to the recent publication (Peters et al 2007). The cDNA was then synthesized in solution by the standard protocol (Promega) using either oligo(dT) or random hexamers as primers.…”

Section: Comparison To Standard Methodsmentioning

confidence: 99%

“…The next challenge is to identify abnormal levels of mRNA that commonly exist in both normal and disease states. Although normal reference values of these mRNA were quantifi ed using healthy subject population (MAQC Consortium, 2006;Mitsuhashi et al 2006;Peters et al 2007;Zheng et al 2006), the identifi cation of disease-specifi c mRNA levels is one of the current topics in molecular diagnostics development.…”

Section: Introductionmentioning

confidence: 99%

Quantification of Drug-Induced mRNA in Human Whole Blood ex vivo

Mitsuhashi

Endo

Obara

et al. 2008

Clinical medicine. Blood disorders

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Apoptosis was induced in heparinized human whole blood by 3 different ways (radiation, bleomycin, or etoposide), and various mRNA were quantifi ed using the method we reported (Clin. Chem. 2006; 52:634-642). We found that cyclin-dependent kinase inhibitor 1A (p21) and p53 upregulated modulator of apoptosis (PUMA) were the most sensitive and universal mRNA markers of apoptosis in leukocytes. In order to defi ne positive and negative responses, a synthetic RNA was spiked into the lysis buffer and the fold increase was calculated. As a result, 837/880 (95.1%) of data points stayed between 0.75 and 1.5 fold increase, and 874/880 (99.3%) were within 0.5-2.0 fold increase. When blood samples from 40 healthy adults were stimulated with 22 different drugs, more than 75% of the samples responded to bleomycin (1 µΜ), idarubicin (2 µΜ), vincristine (1 µΜ), daunorubicin (2 µΜ), cytarabine (10 µΜ), to induce p21 and/or PUMA mRNA, and approximately 25% showed no induction. Signifi cant correlation was found between p21 and PUMA mRNA responses, and between daunorubicin and cytarabine, idarubicin, and vincristine for both p21 and PUMA. The quantifi cation of drug-induced mRNA in whole blood will be considered as ex vivo, and is a suitable platform for biomarker screening as well as a model system for drug sensitivity tests in future.

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Toxicogenomics: Applications to In Vivo Toxicology

Semizarov

Blomme

2008

Genomics in Drug Discovery and Development

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Quality-Controlled Measurement Methods for Quantification of Variations in Transcript Abundance in Whole Blood Samples from Healthy Volunteers

Cited by 5 publications

References 14 publications

Interindividual and Interethnic Variation in Genomewide Gene Expression: Insights into the Biological Variation of Gene Expression and Clinical Implications

Interindividual and Interethnic Variation in Genomewide Gene Expression: Insights into the Biological Variation of Gene Expression and Clinical Implications

Quantification of Drug-Induced mRNA in Human Whole Blood ex vivo

Toxicogenomics: Applications to In Vivo Toxicology

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